CA2301082C - Anti-cancer compounds - Google Patents
Anti-cancer compounds Download PDFInfo
- Publication number
- CA2301082C CA2301082C CA002301082A CA2301082A CA2301082C CA 2301082 C CA2301082 C CA 2301082C CA 002301082 A CA002301082 A CA 002301082A CA 2301082 A CA2301082 A CA 2301082A CA 2301082 C CA2301082 C CA 2301082C
- Authority
- CA
- Canada
- Prior art keywords
- cells
- sap
- peplus
- euphorbia
- cell
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired - Lifetime
Links
Classifications
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K36/00—Medicinal preparations of undetermined constitution containing material from algae, lichens, fungi or plants, or derivatives thereof, e.g. traditional herbal medicines
- A61K36/18—Magnoliophyta (angiosperms)
- A61K36/185—Magnoliopsida (dicotyledons)
- A61K36/47—Euphorbiaceae (Spurge family), e.g. Ricinus (castorbean)
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/21—Esters, e.g. nitroglycerine, selenocyanates
- A61K31/215—Esters, e.g. nitroglycerine, selenocyanates of carboxylic acids
- A61K31/22—Esters, e.g. nitroglycerine, selenocyanates of carboxylic acids of acyclic acids, e.g. pravastatin
- A61K31/225—Polycarboxylic acids
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P1/00—Drugs for disorders of the alimentary tract or the digestive system
- A61P1/04—Drugs for disorders of the alimentary tract or the digestive system for ulcers, gastritis or reflux esophagitis, e.g. antacids, inhibitors of acid secretion, mucosal protectants
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P11/00—Drugs for disorders of the respiratory system
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P13/00—Drugs for disorders of the urinary system
- A61P13/08—Drugs for disorders of the urinary system of the prostate
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P15/00—Drugs for genital or sexual disorders; Contraceptives
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P17/00—Drugs for dermatological disorders
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P17/00—Drugs for dermatological disorders
- A61P17/02—Drugs for dermatological disorders for treating wounds, ulcers, burns, scars, keloids, or the like
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P17/00—Drugs for dermatological disorders
- A61P17/12—Keratolytics, e.g. wart or anti-corn preparations
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P17/00—Drugs for dermatological disorders
- A61P17/16—Emollients or protectives, e.g. against radiation
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P25/00—Drugs for disorders of the nervous system
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P35/00—Antineoplastic agents
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P37/00—Drugs for immunological or allergic disorders
- A61P37/02—Immunomodulators
- A61P37/04—Immunostimulants
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P43/00—Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
Abstract
This invention relates to a compound or group of compounds present in an active principle derived from plants of the species Euphorbia peplus, Euphorbia hirta and Euphorbia drummondii, and to pharmaceutical compositions comprising these compounds. Extracts from these plants have been found to show selective cytotoxicity against several different cancer cell lines. The compounds are useful in effective treatment of cancers, particularly malignant melanomas and squamous cell carcinomas (SCCs). In a preferred embodiment of the invention, the compound is selected from the group consisting of jatrophanes, pepluanes , paralianes and ingenanes, and pharmaceutically-acceptable salts or esters thereof, and more particularly jatrophanes of Conformation I I.
Description
ANTI-CANCER COMPOUNDS
This invention relates to a compound or group of compounds present in an active principle derived from the family Euphorbiaceae, and in particular in plants of the species Euphorbia peplus, Euphorbia hirta and Euphorbia drummondii. Extracts from these plants have been found to show selective cytotoxicity against several different cancer cell lines. Compounds present in the sap of Euphorbia spp. are useful in effective treatment of cancers, particularly malignant melanomas and squamous cell carcinomas (SCCs).
Background of the Invention There is a strong association between exposure of the skin to the ultraviolet light component of sunlight and the development of skin cancers, such as malignant melanoma and the non-melanoma skin cancers, mainly basal cell carcinomas (BCCs) and squamous cell carcinomas (SCCs). The incidence of these cancers has been rapidly increasing world wide. In Britain, there were 4000 newly-diagnosed cases of malignant melanoma in 1994, an 80% increase over the past 10 years (Wessex Cancer Trust, 1996). in the United States, approximately 34,100 new cases were expected, an increase of 4% per year. Queensland, Australia, has the highest incidence of melanoma in the world, but early detection and widespread public health campaigns and the promotion of the use of sunscreens and reduction of ultraviolet exposure have helped to reduce the number of deaths. BCCs currently affect one in 1,000 in the U.K. population, and the incidence has more than doubled in the last 20 years (Imperial Cancer Research Fund, U.K., 1997). One million new cases of BCCs and SCCs are expected to be diagnosed in the USA in 1997, compared to 600,000 in 1990 and 400,000 in 1980 (National Oceanic and Atmospheric Administration U.S.A., 1997). In Australia, there is no reason to suspect that a similarly *rB
This invention relates to a compound or group of compounds present in an active principle derived from the family Euphorbiaceae, and in particular in plants of the species Euphorbia peplus, Euphorbia hirta and Euphorbia drummondii. Extracts from these plants have been found to show selective cytotoxicity against several different cancer cell lines. Compounds present in the sap of Euphorbia spp. are useful in effective treatment of cancers, particularly malignant melanomas and squamous cell carcinomas (SCCs).
Background of the Invention There is a strong association between exposure of the skin to the ultraviolet light component of sunlight and the development of skin cancers, such as malignant melanoma and the non-melanoma skin cancers, mainly basal cell carcinomas (BCCs) and squamous cell carcinomas (SCCs). The incidence of these cancers has been rapidly increasing world wide. In Britain, there were 4000 newly-diagnosed cases of malignant melanoma in 1994, an 80% increase over the past 10 years (Wessex Cancer Trust, 1996). in the United States, approximately 34,100 new cases were expected, an increase of 4% per year. Queensland, Australia, has the highest incidence of melanoma in the world, but early detection and widespread public health campaigns and the promotion of the use of sunscreens and reduction of ultraviolet exposure have helped to reduce the number of deaths. BCCs currently affect one in 1,000 in the U.K. population, and the incidence has more than doubled in the last 20 years (Imperial Cancer Research Fund, U.K., 1997). One million new cases of BCCs and SCCs are expected to be diagnosed in the USA in 1997, compared to 600,000 in 1990 and 400,000 in 1980 (National Oceanic and Atmospheric Administration U.S.A., 1997). In Australia, there is no reason to suspect that a similarly *rB
increasing incidence would not also apply, despite extensive publicising of the dangers of solar and UV
radiation, with the Queensland population being at the greatest risk.
Over 90% of all skin cancers occur on areas of the skin that have been regularly exposed to sunlight or other ultraviolet radiation, with U.V.B. responsible for burning the skin and associated with malignant melanomas, and U.V.A. associated with premature skin aging and the development of BCCs and SCCs (Wessex Cancer Trust, 1996).
Childhood sun exposure has been linked to the development of malignant melanoma in younger adults. Other risk factors include a genetic predisposition (fair complexion, many skin moles), chemical pollution, over-exposure to X-rays, and exposure to some drugs and pesticides.
Depletion of the ozone layer of the stratosphere is considered to contribute to long-term increases in skin cancer.
Surgical removal is by far the most common treatment for malignant melanomas, BCCs and SCCs. This can take the form of electrodesiccation arid curettage, cryosurgery, simple wide excision, micrographic surgery or laser therapy. Other treatments, used when the cancers are detected at a later stage of development, are external radiation therapy, chemotherapy or to a lesser extent bio-immunotherapy or photodynamic therapy. The choice of treatment is dependent on the type and stage of the disease and the age and health of the patient (National Cancer Institute, U.S.A., 1997).
All of the present treatments suffer from severe limitations. The major concern is the poor recognition of cancerous cells at the site of excision and the high likelihood of recurrence, necessitating follow-up surgery and treatment, with the risk of further disfigurement and scarring. In one publication, the reported rates for incompletely-excised BCCs was 30-67% (Sussman and Liggins, 1996). Immune suppression associated with surgery may =y` WO 99/08994 PCT/AU98/00656 . . I L .M
radiation, with the Queensland population being at the greatest risk.
Over 90% of all skin cancers occur on areas of the skin that have been regularly exposed to sunlight or other ultraviolet radiation, with U.V.B. responsible for burning the skin and associated with malignant melanomas, and U.V.A. associated with premature skin aging and the development of BCCs and SCCs (Wessex Cancer Trust, 1996).
Childhood sun exposure has been linked to the development of malignant melanoma in younger adults. Other risk factors include a genetic predisposition (fair complexion, many skin moles), chemical pollution, over-exposure to X-rays, and exposure to some drugs and pesticides.
Depletion of the ozone layer of the stratosphere is considered to contribute to long-term increases in skin cancer.
Surgical removal is by far the most common treatment for malignant melanomas, BCCs and SCCs. This can take the form of electrodesiccation arid curettage, cryosurgery, simple wide excision, micrographic surgery or laser therapy. Other treatments, used when the cancers are detected at a later stage of development, are external radiation therapy, chemotherapy or to a lesser extent bio-immunotherapy or photodynamic therapy. The choice of treatment is dependent on the type and stage of the disease and the age and health of the patient (National Cancer Institute, U.S.A., 1997).
All of the present treatments suffer from severe limitations. The major concern is the poor recognition of cancerous cells at the site of excision and the high likelihood of recurrence, necessitating follow-up surgery and treatment, with the risk of further disfigurement and scarring. In one publication, the reported rates for incompletely-excised BCCs was 30-67% (Sussman and Liggins, 1996). Immune suppression associated with surgery may =y` WO 99/08994 PCT/AU98/00656 . . I L .M
cause any remaining cells to proliferate, and increase the risk of metastases. In melanoma patients there is a high risk that the cancer has already metastasized at the time of initial surgery, and late recurrence leading to death is common. Present alternatives to surgery, such as radiation therapy and chemotherapy, also carry risks of immune suppression and poor specificity. Immunotherapy and gene therapy hold the greatest promise, but the rational application of these is likely to be still decades away.
When the tumour is past the stage amenable to surgery, the most common treatment for melanoma or metastatic skin cancer of all types is chemotherapy, which has been largely unsuccessful (Beljanski and Crochet, 1996) In theory, an ideal drug would be one that when applied topically to an exposed melanoma, BCC or SCC, selectively necrotises the tumour cells or induces them to und'ergo apoptosis, without causing damage to the surrounding healthy skin cells. In practice, this has yet to be achieved. The drugs currently available are neither selective nor penetrative..
The lay public is also enamoured of the concept of topical chemotherapy. There have been many documented "home remedies" for skin cancer, which have had disastrous consequences, eg the use of boot polish (Adele Green,-Queensland Institute of Medical Research, pers. Comm.) The major danger is the production of scar tissue, underneath which the tumour cells continue to grow. An extract derived from plants of the genus Solanum (kangaroo apple or devil's apple) and purportedly containing solasodine glycosides has been available in Australia as a non-prescription preparation treatment of sunspots and solar keratoses, under'the name "Curaderm"T'. However the preparation was shown in a small clinical trial against BCCs to be ineffective, with 14/20 patients showing persisting tumour on histological examination of tissue from the treated site. in some cases, histological examination of the site of treatment revealed malignant tissue embedded in scar tissue. The authors warned against self-diagnosis and treatment, particularly with irritant substances (Francis et al, 1989).
However, anecdotal reports suggest that plant sap extracts are still being used by the general public for the treatment of sunspots or solar keratoses, with some success being claimed.
The sap of plants of the family Euphorbiaceae, particularly the genus Euphorbia, has been used in the folk medicine of many countries. The genus was named after an early Greek physician in deference to its purported medicinal properties (Pearn, 1987). Only recently have some of these claims been investigated scientifically. The genus is enormously diverse, ranging from small, low-growing herbaceous plants to shrubs and trees. Nearly all reports of activity of these plants and their extracts are anecdotal or derived from traditional medicine, and the nature of the preparations used is frequently either unknown or very poorly described. Activity has been claimed against a huge variety of conditions, ranging from warts, "excrescences", calluses, "cheloid tumours", corns, whitlows or felons, "superfluous flesh" and the like, to a variety of cancers (see, for example, Hartwell: Lloydia 1969 32 153).
As part of the screening program for anti-cancer activity carried out on 114,000 extracts from 35,000 terrestrial plant species carried out by the United States National Cancer Institute, a number of species of Euphor.bia were tested. An aqueous suspension, an olive-oil suspension, an alcohol extract and an acid extract were screened for activity against the transplantable tumour cell line sarcoma 37. Four species were tested. Of these, Euphorbia peplus showed no activity in any of the extracts;
Euphorbia drummondii, Euphorbia pilulifera, and Euphorbia resinifera showed weak activity of an acid extract, an alcohol extract, and an olive-oil suspension respectively (Belkin and Fitzgerald, 1953). A review of the scientific and medical literature of the past five years revealed a diversity of powerful active principles such as di- and tetra-terpenes, flavonoids, sterols and proteins in this genus, and many bioactive effects have been reported, with both positive and adverse effects noted. These reports are summarized in Table 1. In particular the genus Euphorbia is well known to produce tumour promoters such as phorbol esters (Hecker, E.: "Cocarcinogens from Euphorbiaceae and Thymeleaceae" in "Symposium on Pharmacognosy and Phytochemistry" (Wagner et al, eds., Springer Verlag 1970 147-165)).
When the tumour is past the stage amenable to surgery, the most common treatment for melanoma or metastatic skin cancer of all types is chemotherapy, which has been largely unsuccessful (Beljanski and Crochet, 1996) In theory, an ideal drug would be one that when applied topically to an exposed melanoma, BCC or SCC, selectively necrotises the tumour cells or induces them to und'ergo apoptosis, without causing damage to the surrounding healthy skin cells. In practice, this has yet to be achieved. The drugs currently available are neither selective nor penetrative..
The lay public is also enamoured of the concept of topical chemotherapy. There have been many documented "home remedies" for skin cancer, which have had disastrous consequences, eg the use of boot polish (Adele Green,-Queensland Institute of Medical Research, pers. Comm.) The major danger is the production of scar tissue, underneath which the tumour cells continue to grow. An extract derived from plants of the genus Solanum (kangaroo apple or devil's apple) and purportedly containing solasodine glycosides has been available in Australia as a non-prescription preparation treatment of sunspots and solar keratoses, under'the name "Curaderm"T'. However the preparation was shown in a small clinical trial against BCCs to be ineffective, with 14/20 patients showing persisting tumour on histological examination of tissue from the treated site. in some cases, histological examination of the site of treatment revealed malignant tissue embedded in scar tissue. The authors warned against self-diagnosis and treatment, particularly with irritant substances (Francis et al, 1989).
However, anecdotal reports suggest that plant sap extracts are still being used by the general public for the treatment of sunspots or solar keratoses, with some success being claimed.
The sap of plants of the family Euphorbiaceae, particularly the genus Euphorbia, has been used in the folk medicine of many countries. The genus was named after an early Greek physician in deference to its purported medicinal properties (Pearn, 1987). Only recently have some of these claims been investigated scientifically. The genus is enormously diverse, ranging from small, low-growing herbaceous plants to shrubs and trees. Nearly all reports of activity of these plants and their extracts are anecdotal or derived from traditional medicine, and the nature of the preparations used is frequently either unknown or very poorly described. Activity has been claimed against a huge variety of conditions, ranging from warts, "excrescences", calluses, "cheloid tumours", corns, whitlows or felons, "superfluous flesh" and the like, to a variety of cancers (see, for example, Hartwell: Lloydia 1969 32 153).
As part of the screening program for anti-cancer activity carried out on 114,000 extracts from 35,000 terrestrial plant species carried out by the United States National Cancer Institute, a number of species of Euphor.bia were tested. An aqueous suspension, an olive-oil suspension, an alcohol extract and an acid extract were screened for activity against the transplantable tumour cell line sarcoma 37. Four species were tested. Of these, Euphorbia peplus showed no activity in any of the extracts;
Euphorbia drummondii, Euphorbia pilulifera, and Euphorbia resinifera showed weak activity of an acid extract, an alcohol extract, and an olive-oil suspension respectively (Belkin and Fitzgerald, 1953). A review of the scientific and medical literature of the past five years revealed a diversity of powerful active principles such as di- and tetra-terpenes, flavonoids, sterols and proteins in this genus, and many bioactive effects have been reported, with both positive and adverse effects noted. These reports are summarized in Table 1. In particular the genus Euphorbia is well known to produce tumour promoters such as phorbol esters (Hecker, E.: "Cocarcinogens from Euphorbiaceae and Thymeleaceae" in "Symposium on Pharmacognosy and Phytochemistry" (Wagner et al, eds., Springer Verlag 1970 147-165)).
41 -u ro ~s a) ~ v -u u 41 a~ ~ v a) a~ ~ rts ri !/] fa < 1 d+ d N N Lfl $1 N "O 0 d~ ~ rl -~ ~ ,Y~ d+ >+ r-i m 01 0 Q1 ra 'o ~ 01 fo 44 U1 01 r1 rn C: ~.' ~ rn =n m .~G -1 c~ H ::I " O ti :J =r1 H =ri h I
x o-- w-- OM ro c~ ro a-- ro ~4 aa ~
~ >1 m ~4 ~ .~ Q. a) rn a) 4J
0 'o r-i U
p t) -1I cd cz ~ ~ r. a 'zJ L-, = =~ ~ 4-4 ui w rn U S:j 44 0 cd r~ N ==-1 cz 0 4f 1 ~ -- ~-1 1J ^I
U u~ t t7t == I .0 0 j..3 ts }-~ =~ ts O -t v 41 b~
cS b 0 =~, 4j 0 =14 5 =ri 4.1 ~ ~O O O =~=i O ~ ~ =r-I
V 1~ N -114 f=a 0 4 1~4 Y=~ r, 44 04 Z c" U) 04 4 U cn O
r 4 N ~ =~
E Q tOi ~ ~
C) i4 r-i U 0 .0 cd 0 (Z A
=r=I 0 P. S-r ~-I ro r-i 0 U U =~ 4 U
?, m 0 04 cfS
=e~ (A U N N
o a) U) .~ ~z vi a-+ A~ a ~ aXi a ~1 RS J ~ S-I r'i 0 'y =rl -r-i f[S fCj 0, ~ 0, ~ c ~i .~ ~, ai o 0 `~
m rt m ~4 4-+ F., 34 =.~
a) 04 aN a) S~ 't~ A X X N~, r+ a~
=rl r-I CL >', ~ ~ >1 a) c1) 41 r-~ N (~ --~
4.1 O O r-i =H NX: S4 .t-) 41 O 41 aG 0 D .-I 0 i4 Ri I Q) rd cd .~ U1 r i .q fo a -W -Y
~ z RS = N R7 ='1 RS
U 'ZS =ri =H N -N
i N U ~4 ~4 v ~s ~ ro Q) o ~ ~
w"
~ ro ~ ~ ro ~ ro m ~ ~ .R ~ -Q A 4 =0 ri o 0 0 0 0 0 0 a~ a v a a a~4 a a ~n w w q 41 w 41 w w w .u Q) 4J
v ~s H -- ro o 0 N C. Ql E-+ u 01 (0 0) O rn -1 u GL, M ~ 4-1 r-I b) M
Ol ~ 01 O v .". v N O) N 01 b 01 N --E =.=1 UI 11 C- N M
4) r i ri e-1 LC) 7 ^i r=1 -rl (0 Q' 04 e-i O Ol 4J ro a+ ~ - r =-r~-1 v UI ` ~
rl1 '-I O ~J rl (d 41 ~ rt3 Ul 01 .tJ ^t c~ ro ~+ u c7 -- Xv 0a ~Dd+ MM
>1 v ~ z ~4 =rl rI 0 > U .U
rl -=-~ ~+
41 'ZS v U
=H rti O w U U
o ~ 4' v ~
.~ v 0 r. v rcs 31 .~ I O 01 -~ U
b 1 0 l-~ -ri m U =
rtS v =H cd U1 I,. =ri ~', =.~ ~n ~ r' ro v o r ~
a~ U r 4J -rq `~ =~ a ~ b +1 r. 4 (~= .u x 0 0 =.~
O cd ~`= U n= tn N ~ S-i U
.- I
~ = r-1 >1 U) A 0 ~ '~ ~ i p 0 =~ =ri 0) cd 0 F' ~ ~ 0 w u ::j E =H 0 N bi o Z3 == 0, .-i I =H
~ ~ ~ ~ m~ ~ ~
~ "-i 04 t2' ,~ ~~ I =~ ~ R' .~ =~
r ~ ~ ,r cd O ~ ~ N a) 0 0 ro r=q 0 M H 41 0 r+ .u ~
>t o o - ~ =.~ ,n a~ (d ~
3 3~ f~, S-t cn 04 r:; T+
~
EJ) 4J =rl O ~ v C ~ -~ f .~ ^RSi ~
cfS ~S ~ ~S cC~ ~f O O O O O
.C =~ -C fi -~ .~
Oa W W W W W W
x o-- w-- OM ro c~ ro a-- ro ~4 aa ~
~ >1 m ~4 ~ .~ Q. a) rn a) 4J
0 'o r-i U
p t) -1I cd cz ~ ~ r. a 'zJ L-, = =~ ~ 4-4 ui w rn U S:j 44 0 cd r~ N ==-1 cz 0 4f 1 ~ -- ~-1 1J ^I
U u~ t t7t == I .0 0 j..3 ts }-~ =~ ts O -t v 41 b~
cS b 0 =~, 4j 0 =14 5 =ri 4.1 ~ ~O O O =~=i O ~ ~ =r-I
V 1~ N -114 f=a 0 4 1~4 Y=~ r, 44 04 Z c" U) 04 4 U cn O
r 4 N ~ =~
E Q tOi ~ ~
C) i4 r-i U 0 .0 cd 0 (Z A
=r=I 0 P. S-r ~-I ro r-i 0 U U =~ 4 U
?, m 0 04 cfS
=e~ (A U N N
o a) U) .~ ~z vi a-+ A~ a ~ aXi a ~1 RS J ~ S-I r'i 0 'y =rl -r-i f[S fCj 0, ~ 0, ~ c ~i .~ ~, ai o 0 `~
m rt m ~4 4-+ F., 34 =.~
a) 04 aN a) S~ 't~ A X X N~, r+ a~
=rl r-I CL >', ~ ~ >1 a) c1) 41 r-~ N (~ --~
4.1 O O r-i =H NX: S4 .t-) 41 O 41 aG 0 D .-I 0 i4 Ri I Q) rd cd .~ U1 r i .q fo a -W -Y
~ z RS = N R7 ='1 RS
U 'ZS =ri =H N -N
i N U ~4 ~4 v ~s ~ ro Q) o ~ ~
w"
~ ro ~ ~ ro ~ ro m ~ ~ .R ~ -Q A 4 =0 ri o 0 0 0 0 0 0 a~ a v a a a~4 a a ~n w w q 41 w 41 w w w .u Q) 4J
v ~s H -- ro o 0 N C. Ql E-+ u 01 (0 0) O rn -1 u GL, M ~ 4-1 r-I b) M
Ol ~ 01 O v .". v N O) N 01 b 01 N --E =.=1 UI 11 C- N M
4) r i ri e-1 LC) 7 ^i r=1 -rl (0 Q' 04 e-i O Ol 4J ro a+ ~ - r =-r~-1 v UI ` ~
rl1 '-I O ~J rl (d 41 ~ rt3 Ul 01 .tJ ^t c~ ro ~+ u c7 -- Xv 0a ~Dd+ MM
>1 v ~ z ~4 =rl rI 0 > U .U
rl -=-~ ~+
41 'ZS v U
=H rti O w U U
o ~ 4' v ~
.~ v 0 r. v rcs 31 .~ I O 01 -~ U
b 1 0 l-~ -ri m U =
rtS v =H cd U1 I,. =ri ~', =.~ ~n ~ r' ro v o r ~
a~ U r 4J -rq `~ =~ a ~ b +1 r. 4 (~= .u x 0 0 =.~
O cd ~`= U n= tn N ~ S-i U
.- I
~ = r-1 >1 U) A 0 ~ '~ ~ i p 0 =~ =ri 0) cd 0 F' ~ ~ 0 w u ::j E =H 0 N bi o Z3 == 0, .-i I =H
~ ~ ~ ~ m~ ~ ~
~ "-i 04 t2' ,~ ~~ I =~ ~ R' .~ =~
r ~ ~ ,r cd O ~ ~ N a) 0 0 ro r=q 0 M H 41 0 r+ .u ~
>t o o - ~ =.~ ,n a~ (d ~
3 3~ f~, S-t cn 04 r:; T+
~
EJ) 4J =rl O ~ v C ~ -~ f .~ ^RSi ~
cfS ~S ~ ~S cC~ ~f O O O O O
.C =~ -C fi -~ .~
Oa W W W W W W
~
x ro ~ U U =
p = r+
ro 'o U) a ~
W N O rn .R m N ~ ~ ~ ~ ~-1 M ~ ~
N 4-) W
~ 44 ~-I ~ U ~i U 43 RS ~ O tn -Lj U
b O=~ L+-i cd ~4 0 .u U -+ A -+ ?, E
~ 0 ~ co 0 ~ u aU ~
i ~+ ,~
~ VI ~
Ul RS U U cr tt -I
=r1 .-= r-, TS ~ U r-i z ~A O =; PQ
N v1 U N roN O rti O W
11 ~ (tj (Y1 'J - rl (." - r-I r`i (A V7 ~4 z v =~ x =~ A-, ro ~4 0 Cn (a 4-) o ~4 ~ =~ .c o -1.1 a) r, 41 U u2 S-I U C: A ~ U) U =r-I
~ ~ U O ~ 4 '=O 14 .-I 0 0 "1 U d) N ~
[r 4 U Cp ~ U -r=I f L1 V U) ~-I U W
N
r-I
ro ~
E b a) =1+
u-w 0 x c~
4-) =~ ai r--i ~n u~
~ ro 0 a) a) 4f =,I ~-4 ro Z r-t U U] 4) =ri (L) p+
f4 O .W U) Q4 N i-t U) 0 f-+ ~C N
A ~ ?, (1) ~u O
>, ~ =.~ rti c%= 'o ~
v (a =~ .~ =~ .q a~i . i ~
O O O O p O U
W W R, 04 W+~-~
x ro ~ U U =
p = r+
ro 'o U) a ~
W N O rn .R m N ~ ~ ~ ~ ~-1 M ~ ~
N 4-) W
~ 44 ~-I ~ U ~i U 43 RS ~ O tn -Lj U
b O=~ L+-i cd ~4 0 .u U -+ A -+ ?, E
~ 0 ~ co 0 ~ u aU ~
i ~+ ,~
~ VI ~
Ul RS U U cr tt -I
=r1 .-= r-, TS ~ U r-i z ~A O =; PQ
N v1 U N roN O rti O W
11 ~ (tj (Y1 'J - rl (." - r-I r`i (A V7 ~4 z v =~ x =~ A-, ro ~4 0 Cn (a 4-) o ~4 ~ =~ .c o -1.1 a) r, 41 U u2 S-I U C: A ~ U) U =r-I
~ ~ U O ~ 4 '=O 14 .-I 0 0 "1 U d) N ~
[r 4 U Cp ~ U -r=I f L1 V U) ~-I U W
N
r-I
ro ~
E b a) =1+
u-w 0 x c~
4-) =~ ai r--i ~n u~
~ ro 0 a) a) 4f =,I ~-4 ro Z r-t U U] 4) =ri (L) p+
f4 O .W U) Q4 N i-t U) 0 f-+ ~C N
A ~ ?, (1) ~u O
>, ~ =.~ rti c%= 'o ~
v (a =~ .~ =~ .q a~i . i ~
O O O O p O U
W W R, 04 W+~-~
The most intensively studied species of this group is Euphorbia pilulifera L (synonyms E. hirta L.;
E. capitata Lam.), whose common names include pill-bearing spurge, snake-weed, cat's hair, Queensland asthma weed and flowery-headed spurge. The plant is widely distributed in tropical countries, including India, and in Northern Australia, including Queensland. According to the "Encyclopedia of Common Natural Ingredients Used in Food, Drugs and Cosmetics" (Leung and Foster, 1996), the whole flowering or fruiting plant is used in herbal remedies, principally for cough preparations, and in traditional medicine for treatment of respiratory conditions such as asthma, bronchitis, coughs and hayfever. This reference reports the active constituents of Euphorbia pilulifera to be choline and shikimic acid, and that other compounds present include triterpenes, sterols, flavonoids, n-alkanes, phenolic acids, L-inositol, sugars and resins.
Of these components, shikimic acid is an essential intermediate in the synthesis of aromatic amino acids, and has been reported to have carcinogenic activity in mice (Evans and Osman, 1974; Stavric and Stoltz, 1976).
Jatrophanes, ingenanes, and a tetracyclic diterpene designated pepluane were identified in the sap of Euphorbia peplus by Jakupovic et al (1998a). The jatrophanes were stated to have a different conformation from those of previously-known jatrophanes. Jatrophanes are also stated to belong to a group of non-irritant diterpenes, which could have accounted to their being overlooked in previous studies. There is no disclosure or suggestion at all of any biological activity of the jatrophanes or of the new pepluane compound; nor is it suggested that any of these compounds might be useful for any pharmaceutical purpose.
A recent report describes selective cytotoxicity of a number of tigliane diterpene esters from the latex of Euphorbia poisonii, a highly-toxic plant found in Northern Nigeria, which is used as a garden pesticide and reputed to be used in homicides. One of these compounds has a selective cytotoxicity for the human kidney carcinoma cell line A-498 more than 10,000 times greater than that of adriamycin (Fatope et al, 1996).
In a series of patent applications, Tamas has claimed use of Euphorbia hirta plants and extracts thereof for a variety of purposes, including tumour therapy (EP 330094), AIDS-related complex and AIDS (HU-208790) and increasing immunity and as an antifungoid agent for treatment of open wounds (DE-4102054).
Thus, while there are isolated reports of anti-cancer activity of various Euphorbia preparations (see Fatope et al, 1996; Oksuz et al, 1996), not only are the compounds present in at least one Euphorbia species reported to be carcinogenic (Evans and Osman, 1974; Stavric and Stolz, 1976; Hecker, 1970; 1977), but at least one species has a skin-irritant and tumour-promoting effect (Gundidza et al, 1993), and another species reduces EBV-specific cellular immunity in Burkitt's lymphoma (Imai, 1994).
To our knowledge, there has been no reliable or reproducible report of the use of any extract from Euphorbia species for the treatment of malignant melanoma or SCCs. An anecdotal report of home treatment of a BCC
with the latex of Euphorbia peplus (petty spurge or milk weed) was the publication of Weedon, D. and Chick, J., entitled "Home treatment of basal cell carcinoma" (1976).
The authors stated that medicinal propeties have been claimed for the milky juice of this plant since the time.of Galen, and it was widely used as a home remedy for corns, warts, and asthma. At the turn of the century it was used by some physicians in Sydney for the treatment of rodent ulcers. The author's patient claimed to have treated himself over many years for multiple BCCs.
"The patient, a 54 year old male, had been seen sporadically at the Royal Brisbane Hospital since 1971. On one visit he was noted to have a clinical basal cell carcinoma on the anterior part of his chest which was confirmed by biopsy- of a tiny specimen taken from one edge.
Some days later when the biopsy site had healed the patient applied the sap of Euphorbia peplus every day for 5 days.
The area became erythematous and then pustular, after which the lesion sloughed off. On his return 6 weeks after treatment, the patient agreed to let us surgically excise the small area of residual scarring. Multiple sections showed dermal scar tissue which contained a few chronic inflammatory cells, but showed no evidence of residual tumour."
The authors stated that "this communication'-should in no way be taken as a recommendation of the fbrm of therapy". There are a few reports cautioning on the corrosive nature of the sap, and minor eye damage that has resulted from the home treatment of warts using Euphorbia peplus (Eke, T., 1994). It appears likely that the effect reported by Weedon and Chick resulted,from the irritant activity of the Euphorbia peplus sap, and that, as in the case of the Solanum extract "Curaderm"TM reported by Francis et al (1989), there is a high risk of residual.tumour cells surviving in or under the scar tissue that results from such treatment.
The inventor has now surprisingly found that sap of plants from three different Euphorbia species, Euphorbia peplus, Euphorbia hirta and Euphorbia drummondii, specifically inhibits growth of three different human tumour cell lines, including malignant melanoma. Moreover, at very low concentrations, sap from Euphorbia peplus and Euphorbia hirta induced differentiation of malignant melanoma cells so that they adopted the morphological appearance of normal melanocytes. At similar or even lower concentrations an extract stimulated activation of the metallothionein gene promoter and expression of a reporter gene in MM96L malignant melanoma cells. The results were particularly striking, since the melanoma cell line which was used is refractory to inhibition by all of the conventional chemotherapeutic agents which have been tested against it (Maynard and Parsons, 1986).
Summary Of The Invention In a first aspect, the invention provides a compound or compounds present in plants of the genus Euphorbia, and in particular in sap of Euphorbia peplus, Euphorbia hirta and/or Euphorbia drumrnondii, which:
(a) is able to kill or inhibit the growth of cancer cells, but does not significantly affect normal neonatal fibroblasts, or spontaneously transformed keratinocytes;
(b) has activity which is not destroyed by heating at 95% for 15 minutes;
(c) has activity which is not destroyed by treatment with acetone;
(d) has activity which can be extracted with 95% ethanol; and (e) stimulates metallothionein gene activation.
Preferably, the compound(s) is able to inhibit the growth of at least one cell line selected from the group consisting of MM96L, MM229, MM220, MM237, MM2058, B16, LIM1215, HeLa, A549, MCF7, MCC16 and Colo16 as herein defined. More preferably, the compound(s) is able to inhibit growth of or to induce differentiation in MM96L
cells.
Even more preferably the compound is also able to induce normal melanocytes to proliferate.
Preferably, the compound is present in sap of E. peplus or E. hirta.
It will be clearly understood that while the invention is described in detail with reference to compounds detected in sap or sap extracts, these compounds, when present in or extracted from whole plants or parts thereof, are still within the scope of the invention.
In a second aspect, the invention provides a composition comprising an active compound as described above, together with a pharmaceutically-suitable carrier or diluent.
More preferably the compound is selected from the group consisting of jatrophanes, pepluanes, paralianes and ingenanes.
Where the compound is a jatrophane, it is preferably of Conformation II as defined by Jakupovic et al (1998a). It will be clearly understood that the substitutions observed in naturally-occurring jatrophane, pepluane and paraliane skeletons are within the scope of the invention. These include the following substitutions and analogues.
Compounds of this type have been found in a variety of plants of the genus Euphobia (Jakupovic et al, 1998a, b, c; Marco et al, 1998).
E. capitata Lam.), whose common names include pill-bearing spurge, snake-weed, cat's hair, Queensland asthma weed and flowery-headed spurge. The plant is widely distributed in tropical countries, including India, and in Northern Australia, including Queensland. According to the "Encyclopedia of Common Natural Ingredients Used in Food, Drugs and Cosmetics" (Leung and Foster, 1996), the whole flowering or fruiting plant is used in herbal remedies, principally for cough preparations, and in traditional medicine for treatment of respiratory conditions such as asthma, bronchitis, coughs and hayfever. This reference reports the active constituents of Euphorbia pilulifera to be choline and shikimic acid, and that other compounds present include triterpenes, sterols, flavonoids, n-alkanes, phenolic acids, L-inositol, sugars and resins.
Of these components, shikimic acid is an essential intermediate in the synthesis of aromatic amino acids, and has been reported to have carcinogenic activity in mice (Evans and Osman, 1974; Stavric and Stoltz, 1976).
Jatrophanes, ingenanes, and a tetracyclic diterpene designated pepluane were identified in the sap of Euphorbia peplus by Jakupovic et al (1998a). The jatrophanes were stated to have a different conformation from those of previously-known jatrophanes. Jatrophanes are also stated to belong to a group of non-irritant diterpenes, which could have accounted to their being overlooked in previous studies. There is no disclosure or suggestion at all of any biological activity of the jatrophanes or of the new pepluane compound; nor is it suggested that any of these compounds might be useful for any pharmaceutical purpose.
A recent report describes selective cytotoxicity of a number of tigliane diterpene esters from the latex of Euphorbia poisonii, a highly-toxic plant found in Northern Nigeria, which is used as a garden pesticide and reputed to be used in homicides. One of these compounds has a selective cytotoxicity for the human kidney carcinoma cell line A-498 more than 10,000 times greater than that of adriamycin (Fatope et al, 1996).
In a series of patent applications, Tamas has claimed use of Euphorbia hirta plants and extracts thereof for a variety of purposes, including tumour therapy (EP 330094), AIDS-related complex and AIDS (HU-208790) and increasing immunity and as an antifungoid agent for treatment of open wounds (DE-4102054).
Thus, while there are isolated reports of anti-cancer activity of various Euphorbia preparations (see Fatope et al, 1996; Oksuz et al, 1996), not only are the compounds present in at least one Euphorbia species reported to be carcinogenic (Evans and Osman, 1974; Stavric and Stolz, 1976; Hecker, 1970; 1977), but at least one species has a skin-irritant and tumour-promoting effect (Gundidza et al, 1993), and another species reduces EBV-specific cellular immunity in Burkitt's lymphoma (Imai, 1994).
To our knowledge, there has been no reliable or reproducible report of the use of any extract from Euphorbia species for the treatment of malignant melanoma or SCCs. An anecdotal report of home treatment of a BCC
with the latex of Euphorbia peplus (petty spurge or milk weed) was the publication of Weedon, D. and Chick, J., entitled "Home treatment of basal cell carcinoma" (1976).
The authors stated that medicinal propeties have been claimed for the milky juice of this plant since the time.of Galen, and it was widely used as a home remedy for corns, warts, and asthma. At the turn of the century it was used by some physicians in Sydney for the treatment of rodent ulcers. The author's patient claimed to have treated himself over many years for multiple BCCs.
"The patient, a 54 year old male, had been seen sporadically at the Royal Brisbane Hospital since 1971. On one visit he was noted to have a clinical basal cell carcinoma on the anterior part of his chest which was confirmed by biopsy- of a tiny specimen taken from one edge.
Some days later when the biopsy site had healed the patient applied the sap of Euphorbia peplus every day for 5 days.
The area became erythematous and then pustular, after which the lesion sloughed off. On his return 6 weeks after treatment, the patient agreed to let us surgically excise the small area of residual scarring. Multiple sections showed dermal scar tissue which contained a few chronic inflammatory cells, but showed no evidence of residual tumour."
The authors stated that "this communication'-should in no way be taken as a recommendation of the fbrm of therapy". There are a few reports cautioning on the corrosive nature of the sap, and minor eye damage that has resulted from the home treatment of warts using Euphorbia peplus (Eke, T., 1994). It appears likely that the effect reported by Weedon and Chick resulted,from the irritant activity of the Euphorbia peplus sap, and that, as in the case of the Solanum extract "Curaderm"TM reported by Francis et al (1989), there is a high risk of residual.tumour cells surviving in or under the scar tissue that results from such treatment.
The inventor has now surprisingly found that sap of plants from three different Euphorbia species, Euphorbia peplus, Euphorbia hirta and Euphorbia drummondii, specifically inhibits growth of three different human tumour cell lines, including malignant melanoma. Moreover, at very low concentrations, sap from Euphorbia peplus and Euphorbia hirta induced differentiation of malignant melanoma cells so that they adopted the morphological appearance of normal melanocytes. At similar or even lower concentrations an extract stimulated activation of the metallothionein gene promoter and expression of a reporter gene in MM96L malignant melanoma cells. The results were particularly striking, since the melanoma cell line which was used is refractory to inhibition by all of the conventional chemotherapeutic agents which have been tested against it (Maynard and Parsons, 1986).
Summary Of The Invention In a first aspect, the invention provides a compound or compounds present in plants of the genus Euphorbia, and in particular in sap of Euphorbia peplus, Euphorbia hirta and/or Euphorbia drumrnondii, which:
(a) is able to kill or inhibit the growth of cancer cells, but does not significantly affect normal neonatal fibroblasts, or spontaneously transformed keratinocytes;
(b) has activity which is not destroyed by heating at 95% for 15 minutes;
(c) has activity which is not destroyed by treatment with acetone;
(d) has activity which can be extracted with 95% ethanol; and (e) stimulates metallothionein gene activation.
Preferably, the compound(s) is able to inhibit the growth of at least one cell line selected from the group consisting of MM96L, MM229, MM220, MM237, MM2058, B16, LIM1215, HeLa, A549, MCF7, MCC16 and Colo16 as herein defined. More preferably, the compound(s) is able to inhibit growth of or to induce differentiation in MM96L
cells.
Even more preferably the compound is also able to induce normal melanocytes to proliferate.
Preferably, the compound is present in sap of E. peplus or E. hirta.
It will be clearly understood that while the invention is described in detail with reference to compounds detected in sap or sap extracts, these compounds, when present in or extracted from whole plants or parts thereof, are still within the scope of the invention.
In a second aspect, the invention provides a composition comprising an active compound as described above, together with a pharmaceutically-suitable carrier or diluent.
More preferably the compound is selected from the group consisting of jatrophanes, pepluanes, paralianes and ingenanes.
Where the compound is a jatrophane, it is preferably of Conformation II as defined by Jakupovic et al (1998a). It will be clearly understood that the substitutions observed in naturally-occurring jatrophane, pepluane and paraliane skeletons are within the scope of the invention. These include the following substitutions and analogues.
Compounds of this type have been found in a variety of plants of the genus Euphobia (Jakupovic et al, 1998a, b, c; Marco et al, 1998).
0 u ~
a~ a cl) U
0 x U O
=~ td U x x ,--I =rl r~ U U N
la 0 w ~s ~ N u x a O1 a u o o u x x 0 u a' rH
~d r.~
U r~ ~ ` ~ n Lj 0 A U ~ ,~ ~ .Q u v x ro o, a~ 0 a, r-i ~ 0 r-0I ~O Ls U 'o r-+
~4 a m N U r1 U " U
x u o x o u x o,~ o u ~
t N a e-1 N
N o x 0 's a 0 o 0 0 N U ro ~ u z i-- N A W
.u r, V U 0 ~ a) 0 p O 4 ~ p fA
~ ~ 4 ro 0 o x m a ~ m o~ u U
a 0 UIri , =~ U,.< O
o0 o o :ZU O O, O
+d U ?Q W U V Mi o U U S-1' ^V N
o 4 ~s 4 U >, 4 a 0 --~ 14 0 V O O U O O 0 11 ~
af - < x a! 4 5C N U N~ U
H h x O O O O (1) x O x O O
1.) m tl) 0 =~
~ 4.) rt3 "~
~
~4 a ~ N M ~M t.C) l0 L- 00 01 0 ~
z 0 ~
U
a~ a cl) U
0 x U O
=~ td U x x ,--I =rl r~ U U N
la 0 w ~s ~ N u x a O1 a u o o u x x 0 u a' rH
~d r.~
U r~ ~ ` ~ n Lj 0 A U ~ ,~ ~ .Q u v x ro o, a~ 0 a, r-i ~ 0 r-0I ~O Ls U 'o r-+
~4 a m N U r1 U " U
x u o x o u x o,~ o u ~
t N a e-1 N
N o x 0 's a 0 o 0 0 N U ro ~ u z i-- N A W
.u r, V U 0 ~ a) 0 p O 4 ~ p fA
~ ~ 4 ro 0 o x m a ~ m o~ u U
a 0 UIri , =~ U,.< O
o0 o o :ZU O O, O
+d U ?Q W U V Mi o U U S-1' ^V N
o 4 ~s 4 U >, 4 a 0 --~ 14 0 V O O U O O 0 11 ~
af - < x a! 4 5C N U N~ U
H h x O O O O (1) x O x O O
1.) m tl) 0 =~
~ 4.) rt3 "~
~
~4 a ~ N M ~M t.C) l0 L- 00 01 0 ~
z 0 ~
U
N
f1 U
O II
x ~+
U a -, U U N
x x u o o x N
o a) co U U
~
II
0 ,q 0 o x s~
b ro ~ ro x a . -ri m U
O 0 x N
0 x.R 0 x x.12 U x ~ ~ 0 o ~ o x "- U ^
x u N N II
~ ~ U
C~ U 0 cV ~- I I~I
r-I r-i N r 4-3 JU~ fc~ N U
u x x A 0 u U
0 O .u 0 .C~
~ ~ r, ~2! U ! ~ i I
ro ro 0 u x o U ~ 0 OO
0 ~
~ N M dI L() Op O uin C.) r-{ '-1 rl c-I -q rl U ~11 U U U
!I II
I!
N ~1 U W f~
Ln -' = PCT/AU98/00656 Received 24 June 1999 Even more preferably, the compound is selected from the group consisting of:
5,8,9,10,14-pentaacetoxy-3-benzoyloxy-15-hydroxypepluane (pepluane);
15-pentaacetoxy-9-nicotinoyloxy-14-oxojatropha-6(1),11E-diene (jatrophane 1);
2,5,7,9,14-hexaacetoxy-3-benzoyloxy-15-hydroxy-jatropha-6(17),11E-diene (jatrophane 2);
2,5,14-triacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 3);
2,5,9,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxyjatropha-6(17),11E-diene) (jatrophane 4);
2,5,7,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 5);
2,5,7,9,14-pentaacetoxy-3-benzoyloxy-8,15-dihydroxyjatropha-6(17),11E-diene (jatrophane 6);
20-acetyl-ingenol-3-angelate;
and pharmaceutically-acceptable salts or esters thereof.
In one preferred embodiment of the invention, the composition additionally comprises (3-alanine betaine hydrochloride or t-4-hydroxy-N,N-dimethyl proline.
In a third aspect, the invention provides a method of treatment of a cancer, comprising the step of administering an anti-cancer effective amount of a compound of the invention to a mammal in need of such treatment.
Preferably, the cancer is a solid tumour. More preferably, the cancer is selected from the group consisting of malignant melanoma, other skin cancers including Merkel cell carcinoma, squamous cell carcinoma and basal cell carcinoma, lung cancer, colon cancer, prostate cancer, cervical cancer and breast cancer.
In a fourth aspect, the invention provides a method of inhibiting proliferative activity of neoplastic H:\PClarke\Keep\Retypea\PCT-00656.doc 24/06/99 AMENDED SHEET (Article 34) (IPEA/AU1 cells, comprising the step of exposing the cells to an anti-proliferative amount of a compound of the invention.
The cells may be treated either ex vivo or in vivo.
In a fifth aspect, the invention provides a method of preventing or alleviating damage to skin, caused by ultraviolet irradiation, ionizing radiation, microwave radiation, exposure to ozone, or the like, comprising the step of topically administering an effective amount of a compound of the invention to a subject in need of such treatment. This aspect of the invention may be used in the treatment of solar keratosis, skin damage occurring during radiotherapy, and the like.
In a sixth aspect the invention provides a method of stimulating proliferation of non-neoplastic cells comprising the step of exposing the cells to a proliferation-inducing amount of a compound or a composition of the invention. This is useful in inducing regeneration of tissues and, because T-lymphocytes proliferate in response to the compositions of the invention,.is useful in promoting the immune response to disease states.
The mammal may be a human, or may be a domestic or companion animal. While it is particularly contemplated that the compounds of the invention are suitable for use in medical treatment of humans, it is also applicable to veterinary treatment, including treatment of companion animals such as dogs and cats, and domestic animals such 'as horses, cattle and sheep, or zoo animals such as felids, canids, bovids, and ungulates.
The compounds and compositions of the invention may be administered by any suitable route, and the person skilled in the art will readily be able to determine the most suitable route and dose for the condition to be treated. Dosage will be at the discretion of the attendant physician or veterinarian, and will depend on the nature and state of the condition to be treated, the age and general state of health of the subject to be treated, the route of administration, and any previous treatment which may have been administered.
The carrier or diluent, and other excipients, will depend on the route of administration, and again the person skilled in the art will readily be able to determine the most suitable formulation for each particular case. It is contemplated that compounds of the invention may be .administered orally, topically, and/or by parenteral injection, including intravenous injection.
Methods and pharmaceutical carriers for preparation of pharmaceutical compositions are well known in the art, as set out in textbooks such as Remington's Pharmaceutical Sciences, 17th Edition, Mack Publishing Company, Easton, Pennsylvania, USA.
For the purposes of this specification it will be clearly understood that the word "comprising" means "including but not limited to", and that the word "comprises" has a corresponding meaning.
Brief Description of the Figures Figure 1 shows the eifect of E. peplus sap on metallothionein gene activation, measured by detecting the activity of (3-galactosidase using a chromogenic substrate.
Figure 2 shows the proliferation of MCF7 breast cancer cells grown in microtitre wells in the presence of E. peplus sap for 7 days (expressed as a percentage of control values).
Figure 3 shows the absorbance profile at 195 nm, following RP-HPLC sub-fractionation of an ethanol-soluble extract of E. peplus sap.
Figure 4 shows the results of repeated RP-HPLC
chromatography of fraction 14 from Figure 3.
Figure 5 shows the constant diode array spectrum of the peak from Figure 4.
f1 U
O II
x ~+
U a -, U U N
x x u o o x N
o a) co U U
~
II
0 ,q 0 o x s~
b ro ~ ro x a . -ri m U
O 0 x N
0 x.R 0 x x.12 U x ~ ~ 0 o ~ o x "- U ^
x u N N II
~ ~ U
C~ U 0 cV ~- I I~I
r-I r-i N r 4-3 JU~ fc~ N U
u x x A 0 u U
0 O .u 0 .C~
~ ~ r, ~2! U ! ~ i I
ro ro 0 u x o U ~ 0 OO
0 ~
~ N M dI L() Op O uin C.) r-{ '-1 rl c-I -q rl U ~11 U U U
!I II
I!
N ~1 U W f~
Ln -' = PCT/AU98/00656 Received 24 June 1999 Even more preferably, the compound is selected from the group consisting of:
5,8,9,10,14-pentaacetoxy-3-benzoyloxy-15-hydroxypepluane (pepluane);
15-pentaacetoxy-9-nicotinoyloxy-14-oxojatropha-6(1),11E-diene (jatrophane 1);
2,5,7,9,14-hexaacetoxy-3-benzoyloxy-15-hydroxy-jatropha-6(17),11E-diene (jatrophane 2);
2,5,14-triacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 3);
2,5,9,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxyjatropha-6(17),11E-diene) (jatrophane 4);
2,5,7,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 5);
2,5,7,9,14-pentaacetoxy-3-benzoyloxy-8,15-dihydroxyjatropha-6(17),11E-diene (jatrophane 6);
20-acetyl-ingenol-3-angelate;
and pharmaceutically-acceptable salts or esters thereof.
In one preferred embodiment of the invention, the composition additionally comprises (3-alanine betaine hydrochloride or t-4-hydroxy-N,N-dimethyl proline.
In a third aspect, the invention provides a method of treatment of a cancer, comprising the step of administering an anti-cancer effective amount of a compound of the invention to a mammal in need of such treatment.
Preferably, the cancer is a solid tumour. More preferably, the cancer is selected from the group consisting of malignant melanoma, other skin cancers including Merkel cell carcinoma, squamous cell carcinoma and basal cell carcinoma, lung cancer, colon cancer, prostate cancer, cervical cancer and breast cancer.
In a fourth aspect, the invention provides a method of inhibiting proliferative activity of neoplastic H:\PClarke\Keep\Retypea\PCT-00656.doc 24/06/99 AMENDED SHEET (Article 34) (IPEA/AU1 cells, comprising the step of exposing the cells to an anti-proliferative amount of a compound of the invention.
The cells may be treated either ex vivo or in vivo.
In a fifth aspect, the invention provides a method of preventing or alleviating damage to skin, caused by ultraviolet irradiation, ionizing radiation, microwave radiation, exposure to ozone, or the like, comprising the step of topically administering an effective amount of a compound of the invention to a subject in need of such treatment. This aspect of the invention may be used in the treatment of solar keratosis, skin damage occurring during radiotherapy, and the like.
In a sixth aspect the invention provides a method of stimulating proliferation of non-neoplastic cells comprising the step of exposing the cells to a proliferation-inducing amount of a compound or a composition of the invention. This is useful in inducing regeneration of tissues and, because T-lymphocytes proliferate in response to the compositions of the invention,.is useful in promoting the immune response to disease states.
The mammal may be a human, or may be a domestic or companion animal. While it is particularly contemplated that the compounds of the invention are suitable for use in medical treatment of humans, it is also applicable to veterinary treatment, including treatment of companion animals such as dogs and cats, and domestic animals such 'as horses, cattle and sheep, or zoo animals such as felids, canids, bovids, and ungulates.
The compounds and compositions of the invention may be administered by any suitable route, and the person skilled in the art will readily be able to determine the most suitable route and dose for the condition to be treated. Dosage will be at the discretion of the attendant physician or veterinarian, and will depend on the nature and state of the condition to be treated, the age and general state of health of the subject to be treated, the route of administration, and any previous treatment which may have been administered.
The carrier or diluent, and other excipients, will depend on the route of administration, and again the person skilled in the art will readily be able to determine the most suitable formulation for each particular case. It is contemplated that compounds of the invention may be .administered orally, topically, and/or by parenteral injection, including intravenous injection.
Methods and pharmaceutical carriers for preparation of pharmaceutical compositions are well known in the art, as set out in textbooks such as Remington's Pharmaceutical Sciences, 17th Edition, Mack Publishing Company, Easton, Pennsylvania, USA.
For the purposes of this specification it will be clearly understood that the word "comprising" means "including but not limited to", and that the word "comprises" has a corresponding meaning.
Brief Description of the Figures Figure 1 shows the eifect of E. peplus sap on metallothionein gene activation, measured by detecting the activity of (3-galactosidase using a chromogenic substrate.
Figure 2 shows the proliferation of MCF7 breast cancer cells grown in microtitre wells in the presence of E. peplus sap for 7 days (expressed as a percentage of control values).
Figure 3 shows the absorbance profile at 195 nm, following RP-HPLC sub-fractionation of an ethanol-soluble extract of E. peplus sap.
Figure 4 shows the results of repeated RP-HPLC
chromatography of fraction 14 from Figure 3.
Figure 5 shows the constant diode array spectrum of the peak from Figure 4.
Figure 6 shows the results of treatment of MM96L
melanoma cells with Fraction 15 from Example 7. Cells are stained with antibody TRP-1, directed against the cytoskeleton A,B: 4 days, C,D: 21 days Figure 7 shows the results of thin layer chromatography of the ether-soluble fraction from Example 6 using chloroform:ethyl acetate (82:18) as the developing solvent.
Figure 8 shows the results of further purification by 2-dimensional TLC on silica gel, using hexane:ethyl acetate (1:1) in the first dimension, and toluene:acetone (9:1) in the second dimension.
A: Spots 34-45 were visualised on a UV light box. Activities were scored towards MM96L at a 1 in 500 dilution (+++ = no effect, -= complete cell death, d 100% reversion of cells to a dendritic appearance.
B: Spots 14-20 were visualised on a UV light box. Activities were scored towards iMM96L at a 1 in 500 dilution (+++ = no effect, - = complete cell death, d 100% reversion of cells to a dendritic appearance.
C: Spots 21-27 were visualised on a W light box. Activities were scored towards MM96L at a 1 in 500 dilution (+++ = no effect, - = complete cell death, d 100% reversion of cells to a dendritic appearance.
Figure 9 shows results of ascending chromatography of crude sap on HPTLC using a toluene:acetone (9:1) solvent system. Opaque bands 1 -7 were visualised on a W light box Figure 10 shows results of ascending chromatography of fraction 1 from Figure 9 on HPTLC using a hexane:ethyl acetate (4:1) solvent system. Bands A-G were visualised on a UV light box. (Side strip stained with 0.1%
iodine in chloroform revealed Fraction G - inactive against NIIM96L).
Figure 11 shows results of ascending chromatography of fraction 1 from Figure 9 on HPTLC using a *rB
melanoma cells with Fraction 15 from Example 7. Cells are stained with antibody TRP-1, directed against the cytoskeleton A,B: 4 days, C,D: 21 days Figure 7 shows the results of thin layer chromatography of the ether-soluble fraction from Example 6 using chloroform:ethyl acetate (82:18) as the developing solvent.
Figure 8 shows the results of further purification by 2-dimensional TLC on silica gel, using hexane:ethyl acetate (1:1) in the first dimension, and toluene:acetone (9:1) in the second dimension.
A: Spots 34-45 were visualised on a UV light box. Activities were scored towards MM96L at a 1 in 500 dilution (+++ = no effect, -= complete cell death, d 100% reversion of cells to a dendritic appearance.
B: Spots 14-20 were visualised on a UV light box. Activities were scored towards iMM96L at a 1 in 500 dilution (+++ = no effect, - = complete cell death, d 100% reversion of cells to a dendritic appearance.
C: Spots 21-27 were visualised on a W light box. Activities were scored towards MM96L at a 1 in 500 dilution (+++ = no effect, - = complete cell death, d 100% reversion of cells to a dendritic appearance.
Figure 9 shows results of ascending chromatography of crude sap on HPTLC using a toluene:acetone (9:1) solvent system. Opaque bands 1 -7 were visualised on a W light box Figure 10 shows results of ascending chromatography of fraction 1 from Figure 9 on HPTLC using a hexane:ethyl acetate (4:1) solvent system. Bands A-G were visualised on a UV light box. (Side strip stained with 0.1%
iodine in chloroform revealed Fraction G - inactive against NIIM96L).
Figure 11 shows results of ascending chromatography of fraction 1 from Figure 9 on HPTLC using a *rB
hexane:ethyl acetate (4:1) solvent system. Band H was visualised on a W light box.
Figure 12 shows the results of ascending chromatography of diethyl ether soluble fraction prepared from crude sap on preparative thin layer chromatography (PLC, Merck) using hexane : ethyl acetate (4:1) solvent system. Zones H and A-F were visualised on a UV light box, extracted, and used for in vivo studies.
Figure 13 shows the results of treatment of subcutaneous human melanoma MM96L xenografts in nude mice with a partially purified fraction prepared as described in Example 11. Arrows denote the position of topical treatments for a tumour (right-hand side) and for normal skin (top of back). There was no evidence of residual tumour growth or lasting damage to the normal skin 32 days after the treatment regimen began, and 20 days after the first topical application.
DETAILED DESCRIPTION OF THE INVENTION
The invention will be described in detail by reference only to the following non-limiting examples and to the figures.
Example 1 Inhibitory Activity of Euphorbia Sap Against Tumour Cell Lines The ability of sap of three Euphorbia species, Euphorbia peplus, Euphorbia hirta and Euphorbia druznmondii to inhibit the growth of three different human tumour cell lines was tested. The activity against normal skin fibroblasts was tested as a control.
The cell lines were maintained in RPMI medium containing 5% foetal calf serum (FCS), and assays were performed in the same medium.
Sap was collected from plants growing randomly on cultivated soil on a farm at Palmwoods, in the Sunshine Coast hinterland, South-East Queensland. The plant stem surface was briefly washed with 70% ethanol, and scissors washed in ethanol were used to cut the stem and release the milky latex sap. The sap was collected into 10 ml sterile plastic centrifuge tubes, transported at 4 C to Brisbane and stored frozen at -20 C. Prior to use, the sap was serially diluted five-fold up to 1 in 3125 into sterile 1.5 ml Eppendorf tubes using sterile MilliQ water. 10 uL
aliquots of each dilution were added to each two of microtitre plate wells containing 100 ul of the cell lines.
Assays were performed in duplicate.
After 5 days, cells were examined blind, for inhibition of growth compared to control untreated cell samples. The results are summarized in Tables 3 to 6, in which the cell lines tested were NFF normal skin fibroblasts MM96L malignant melanoma, brain metastasis HeLa cervical cancer HACat spontaneously-transformed human keratinocytes and the scale is 0 = no effect to 5= complete cell death The dilution in the table heading refers to the dilution of the sample before addition to the culture.
Thus, the dilution in the final culture is approximately 10-fold greater.
Figure 12 shows the results of ascending chromatography of diethyl ether soluble fraction prepared from crude sap on preparative thin layer chromatography (PLC, Merck) using hexane : ethyl acetate (4:1) solvent system. Zones H and A-F were visualised on a UV light box, extracted, and used for in vivo studies.
Figure 13 shows the results of treatment of subcutaneous human melanoma MM96L xenografts in nude mice with a partially purified fraction prepared as described in Example 11. Arrows denote the position of topical treatments for a tumour (right-hand side) and for normal skin (top of back). There was no evidence of residual tumour growth or lasting damage to the normal skin 32 days after the treatment regimen began, and 20 days after the first topical application.
DETAILED DESCRIPTION OF THE INVENTION
The invention will be described in detail by reference only to the following non-limiting examples and to the figures.
Example 1 Inhibitory Activity of Euphorbia Sap Against Tumour Cell Lines The ability of sap of three Euphorbia species, Euphorbia peplus, Euphorbia hirta and Euphorbia druznmondii to inhibit the growth of three different human tumour cell lines was tested. The activity against normal skin fibroblasts was tested as a control.
The cell lines were maintained in RPMI medium containing 5% foetal calf serum (FCS), and assays were performed in the same medium.
Sap was collected from plants growing randomly on cultivated soil on a farm at Palmwoods, in the Sunshine Coast hinterland, South-East Queensland. The plant stem surface was briefly washed with 70% ethanol, and scissors washed in ethanol were used to cut the stem and release the milky latex sap. The sap was collected into 10 ml sterile plastic centrifuge tubes, transported at 4 C to Brisbane and stored frozen at -20 C. Prior to use, the sap was serially diluted five-fold up to 1 in 3125 into sterile 1.5 ml Eppendorf tubes using sterile MilliQ water. 10 uL
aliquots of each dilution were added to each two of microtitre plate wells containing 100 ul of the cell lines.
Assays were performed in duplicate.
After 5 days, cells were examined blind, for inhibition of growth compared to control untreated cell samples. The results are summarized in Tables 3 to 6, in which the cell lines tested were NFF normal skin fibroblasts MM96L malignant melanoma, brain metastasis HeLa cervical cancer HACat spontaneously-transformed human keratinocytes and the scale is 0 = no effect to 5= complete cell death The dilution in the table heading refers to the dilution of the sample before addition to the culture.
Thus, the dilution in the final culture is approximately 10-fold greater.
-- 'n N
lfl r-A
~y M
~~ i-I O O O O
~-1 O O O O
Ln N
N
O O O
r--l O O O O
Lf1 L!1 N
N ~
,-{ \
O
r-I O O O O
LC) Ln N N
N \ N \
--I O O O O
E
4-) 0 S2, N
c[S
~ ~ ~
td r'+ cn .-1 O O O O ~ v2 r-I m Ln O
A a~
O
rn ~4 ,n Ln CN
v w r-'1 M r--I M
O O O O
O O O O E .~ r1 ~4 ~
0 Z Lfl ~ lfI
N N
"0 a LO
[z4 \ ~o \
2 ~l O O O o r-i O O O O
Ln Lo N N
\ + \
r-~ O O O O;
N N
O -i N O O O' d~ CM N O
=~ a~ !~ =~ a~
~ r-i Ln Ln v) -4 M Ln -,r o q cn .~ Ln in in o =y H
O ~ ~1 O =~
ji 4J
u H ~
b ~
ti ra =q 'U rtS ~ ~ 9 'u a i r~d w w w z , n w w w z Ln Table 5 Hela Cells Sample Dilution E. peplus 5 3.5 3 1 1 E. hirta 5 5 5 5 0 E. drumrnondii 5 0 0 0 0 No addition 0 0 0 0 0 Table 6 HACat keratinocytes Sample Dilution E. peplus 4 0 0 0 0 E. hirta 5 0 0 0 0 E. drummondii 5 0 0 0 0 No addition 0 0 0 0 0 From these results it can be seen that:
a) E. peplus was active against HeLa cells, and to a lesser extent against MM96L cells.
b) E. hirta was active against MM96L cells and very strongly active against HeLa cells.
c) E. drummondii had a lesser effect against NIlM96L than the other two szmples, and inhibited HeLa cells only at the highest concentration tested.
d) NFF normal fibroblasts were severely affected at the 1/5 dilution, but only mildly affected at the other dilutions. For example, at a dilution of 1/25, there was mild inhibition of NFF cells (rating 2), but severe inhibition of MM96L cells (rating 4). At a dilution of 1/125, no effect was observed against NFF cells (rating .0), but severe inhibition of KM96L cells (rating 4) was observed for one sample, and milder inhibition (rating 1) *rB
lfl r-A
~y M
~~ i-I O O O O
~-1 O O O O
Ln N
N
O O O
r--l O O O O
Lf1 L!1 N
N ~
,-{ \
O
r-I O O O O
LC) Ln N N
N \ N \
--I O O O O
E
4-) 0 S2, N
c[S
~ ~ ~
td r'+ cn .-1 O O O O ~ v2 r-I m Ln O
A a~
O
rn ~4 ,n Ln CN
v w r-'1 M r--I M
O O O O
O O O O E .~ r1 ~4 ~
0 Z Lfl ~ lfI
N N
"0 a LO
[z4 \ ~o \
2 ~l O O O o r-i O O O O
Ln Lo N N
\ + \
r-~ O O O O;
N N
O -i N O O O' d~ CM N O
=~ a~ !~ =~ a~
~ r-i Ln Ln v) -4 M Ln -,r o q cn .~ Ln in in o =y H
O ~ ~1 O =~
ji 4J
u H ~
b ~
ti ra =q 'U rtS ~ ~ 9 'u a i r~d w w w z , n w w w z Ln Table 5 Hela Cells Sample Dilution E. peplus 5 3.5 3 1 1 E. hirta 5 5 5 5 0 E. drumrnondii 5 0 0 0 0 No addition 0 0 0 0 0 Table 6 HACat keratinocytes Sample Dilution E. peplus 4 0 0 0 0 E. hirta 5 0 0 0 0 E. drummondii 5 0 0 0 0 No addition 0 0 0 0 0 From these results it can be seen that:
a) E. peplus was active against HeLa cells, and to a lesser extent against MM96L cells.
b) E. hirta was active against MM96L cells and very strongly active against HeLa cells.
c) E. drummondii had a lesser effect against NIlM96L than the other two szmples, and inhibited HeLa cells only at the highest concentration tested.
d) NFF normal fibroblasts were severely affected at the 1/5 dilution, but only mildly affected at the other dilutions. For example, at a dilution of 1/25, there was mild inhibition of NFF cells (rating 2), but severe inhibition of MM96L cells (rating 4). At a dilution of 1/125, no effect was observed against NFF cells (rating .0), but severe inhibition of KM96L cells (rating 4) was observed for one sample, and milder inhibition (rating 1) *rB
with the duplicate sample). HACat cells, which could be considered as representative of normal keratinocytes, were only inhibited at the highest concentration.
At high concentrations of E. peplus sap, it appeared that there was direct killing of MM96 cells.
However, at lower concentrations (down to a dilution of 1/625), although no growth inhibition was observed, the surviving cells were dendritic, and had the appearance of normal melanocytes. Without wishing to be limited to any proposed mechanism, it appears that E. peplus sap may contain at least one agent which promotes differentiation, rather than directly cytotoxic agents which damage DNA.
Example 2 Effect of Heat or Acetone Treatment on Activity of Euphorbia Sap The experiment described in Example 1 was repeated for E. peplus and E. hirta by a different person, using different cell line preparations, different plant samples and a different rating scale.
The samples were either prepared as described in Example 1, or were subjected to treatment with heat or acetone. Undiluted extracts of plant sap were heated at 95 C for 15 minutes. For the acetone treatment, 40 }zl extract was suspended in 400 ul acetone, and the tube shaken on a vortex mixer. Contents were centrifuged at 10,000 g for 3 minutes and the supernatant (acetone-soluble fraction) removed to a separate tube. Both the pellet and supernatant were left in open tubes at room temperature in the fume hood overnight with exhaust fan operating to evaporate the residual acetone.
The results are shown in Tables 7 to 9, in which +++ indicates no effect, and - indicates 100% cell death.
"C" indicates that the culture was contaminated. Using this rating scale the results were even more striking than in Example 1, with strong inhibitory activity being observed up to a dilution of 1:3125. However, some growth inhibition of NFF cells was seen in this experiment.
At high concentrations of E. peplus sap, it appeared that there was direct killing of MM96 cells.
However, at lower concentrations (down to a dilution of 1/625), although no growth inhibition was observed, the surviving cells were dendritic, and had the appearance of normal melanocytes. Without wishing to be limited to any proposed mechanism, it appears that E. peplus sap may contain at least one agent which promotes differentiation, rather than directly cytotoxic agents which damage DNA.
Example 2 Effect of Heat or Acetone Treatment on Activity of Euphorbia Sap The experiment described in Example 1 was repeated for E. peplus and E. hirta by a different person, using different cell line preparations, different plant samples and a different rating scale.
The samples were either prepared as described in Example 1, or were subjected to treatment with heat or acetone. Undiluted extracts of plant sap were heated at 95 C for 15 minutes. For the acetone treatment, 40 }zl extract was suspended in 400 ul acetone, and the tube shaken on a vortex mixer. Contents were centrifuged at 10,000 g for 3 minutes and the supernatant (acetone-soluble fraction) removed to a separate tube. Both the pellet and supernatant were left in open tubes at room temperature in the fume hood overnight with exhaust fan operating to evaporate the residual acetone.
The results are shown in Tables 7 to 9, in which +++ indicates no effect, and - indicates 100% cell death.
"C" indicates that the culture was contaminated. Using this rating scale the results were even more striking than in Example 1, with strong inhibitory activity being observed up to a dilution of 1:3125. However, some growth inhibition of NFF cells was seen in this experiment.
Neither heat nor acetone affected the anti-tumour activity significantly. With acetone treatment, most activity was found in the pellet, particularly in the case of E. hirta, though some activity was also present in the soluble fraction. This suggests that the compounds responsible are not protein in nature, and that at least one component may be a lipid.
Ln N
r-i M +
~ + +
r-1 + + +
Ln N
+
~ + +
.-I + + +
U'1 r-I
~ + +
+ +
Ln CV
N ~
+
N
~
~ Ln C!~ rl Ln ~
+ + + + + + +
~ + + + + + + 11 ~ ~ rl +I + + + + + + +
N
w +
+ + + + + + +
~ + + + + + + ~
+ + + +
L(1 N
+
~ + +
+ + + -1 -i +1 + + + + + + +
L(1 N
+ + +1 Q ~ i + + + + + i +
=rl N
Ln .,a rtS
+{ +1 +1 1-4 Q) N
Ic: 0 o 4-J 4-) ~ (d ~
^i 1J ,J a) a) u a) - rl a) ~ a ~4 ~+ r-a ~ ~+ r a ~n ~ a a r + a) a .~ ~ o v o=~+ o-~+ z o=~ ro a .c q D' ~ q ~ ~ a a a ~
~ L w w ~ w~ w~~ a~ a 9 w N
r-t \ + +
r-i + +
N
lp + +
'-1 + +
+
-i + +
Lr) N
N \
(L) r'1 U +
~
Ln Cn 0-1 I
Lf co N
~ z ~ + + +I + + + + +
H
+
+ + + + +
r+,~ + + + + + + + +
U-) it \ + + + +
-+ U +1 +1 + + + + +
N !~
t,' ~ \ ! + +
0 + + + + + + -H +
~ ~ ~
r4 tv + +1 + +1 d) r-1 r1 N 4) .~', t~ t~
U' ~f U) , ~ ~ a ~n ~ a a , ~' ~-[ ~ 0 a~ 0 H 1 O O~~s Q) i, Q, J'j =~ 4J U~4J U4J
11 a v av W a W v~-4 ~d ! U U U ~ I Q) U ~+
~i w w w b w ~o w~ a a ~ a.~ w Table 9 HeLa cells Sample 1/5 11/25 1/125 j 1/625 1/3125 E. peplus + +++ +++ +++
E. hirta - +++ +++ +++ +++
E. hirta heat + ++ +++ +++ +++
acetone +++ +++ +++ +++ +++
soluble E. peplus acetone +++ +++ +++ +++ +++
soluble E. hirta acetone ppte ++ ++ +++ +++ +++
E. peplus acetone ppte +++ +++ +++ +++
E. hirta E. peplus - +++ +++ +++ +++
heat Example 3 Further Tests Using E. peplus Since E. peplus is the most abundant of the three plants tested in these studies, further experiments utilised extracts from this species. This is not to be taken to imply that activity is not present in the other two species.
Example 2 was repeated, using MM229 and NIlM220 human malignant melanoma cells and B16 mouse malignant melanoma cell lines, in addition to NFF and MM96L cells.
Assays were performed in duplicate, using addition of an equivalent amount of water as a control, and dilutions of the pellet and supernatant fractions after acetone treatment from 1/20 to 1/12500. The results are summarised in Table 10.
r-i M +
~ + +
r-1 + + +
Ln N
+
~ + +
.-I + + +
U'1 r-I
~ + +
+ +
Ln CV
N ~
+
N
~
~ Ln C!~ rl Ln ~
+ + + + + + +
~ + + + + + + 11 ~ ~ rl +I + + + + + + +
N
w +
+ + + + + + +
~ + + + + + + ~
+ + + +
L(1 N
+
~ + +
+ + + -1 -i +1 + + + + + + +
L(1 N
+ + +1 Q ~ i + + + + + i +
=rl N
Ln .,a rtS
+{ +1 +1 1-4 Q) N
Ic: 0 o 4-J 4-) ~ (d ~
^i 1J ,J a) a) u a) - rl a) ~ a ~4 ~+ r-a ~ ~+ r a ~n ~ a a r + a) a .~ ~ o v o=~+ o-~+ z o=~ ro a .c q D' ~ q ~ ~ a a a ~
~ L w w ~ w~ w~~ a~ a 9 w N
r-t \ + +
r-i + +
N
lp + +
'-1 + +
+
-i + +
Lr) N
N \
(L) r'1 U +
~
Ln Cn 0-1 I
Lf co N
~ z ~ + + +I + + + + +
H
+
+ + + + +
r+,~ + + + + + + + +
U-) it \ + + + +
-+ U +1 +1 + + + + +
N !~
t,' ~ \ ! + +
0 + + + + + + -H +
~ ~ ~
r4 tv + +1 + +1 d) r-1 r1 N 4) .~', t~ t~
U' ~f U) , ~ ~ a ~n ~ a a , ~' ~-[ ~ 0 a~ 0 H 1 O O~~s Q) i, Q, J'j =~ 4J U~4J U4J
11 a v av W a W v~-4 ~d ! U U U ~ I Q) U ~+
~i w w w b w ~o w~ a a ~ a.~ w Table 9 HeLa cells Sample 1/5 11/25 1/125 j 1/625 1/3125 E. peplus + +++ +++ +++
E. hirta - +++ +++ +++ +++
E. hirta heat + ++ +++ +++ +++
acetone +++ +++ +++ +++ +++
soluble E. peplus acetone +++ +++ +++ +++ +++
soluble E. hirta acetone ppte ++ ++ +++ +++ +++
E. peplus acetone ppte +++ +++ +++ +++
E. hirta E. peplus - +++ +++ +++ +++
heat Example 3 Further Tests Using E. peplus Since E. peplus is the most abundant of the three plants tested in these studies, further experiments utilised extracts from this species. This is not to be taken to imply that activity is not present in the other two species.
Example 2 was repeated, using MM229 and NIlM220 human malignant melanoma cells and B16 mouse malignant melanoma cell lines, in addition to NFF and MM96L cells.
Assays were performed in duplicate, using addition of an equivalent amount of water as a control, and dilutions of the pellet and supernatant fractions after acetone treatment from 1/20 to 1/12500. The results are summarised in Table 10.
Ln N
~ + + + + + +
+ + + + i- + + + + + +
+ + + + 4- + + + + + + +
O
O
tn N + + + + + +
+ + + + + + + + + +
~-I + + + + + + + + + + + +
O
O
tf1 + + +
t + + + + + + + + + +
.1 + + + + + + +f + + + + +
O
O
+ + + + + +
~-i + + + + + +I + + ~ + + + +
O +
N + + +
~ + + I I I I I + + I +
C) UI
N
r{ + + + +
+ + + + + + + + +
+ + + + + + + + 1 +
~ O ( r"I O
Ln ~ =
+ + + +
+ + + + T + + + + + +
~-{ + + + + + + + + + + + +
+
O +
O + + +
Ln + + + \ +
+ + \ + + + -1 + + + +
~-{ + + + + + + + + + + + +
~
~
~ + +
+ + + + +
0 -4 + + + + + +! + + + + +
N +
-q + + +
~4 L
r. + + + + + +
O + + + + + + + + + + + +
U + + + + + + + + + + + +
yL L
tJ tJ .!J L L
4J C -4 c m 0 ,-~ r~ ~ a L a (1) ~4 ~ ro 4 (o ~ ro ~ It 41) w ~ N N L -1 4-) N L N 41 ,-i N
ca a co a u~+ a a Q vi a a ~ k, rn m ~4 o l o ~4 (~ \p \p N. i(} N N N N N N N
~ ', Ls+ Cta O~ Ol ~a v r-4 a N N GL N N QE ~o ~
V] 7.. 2 2: 2~ UI ~ x N ~ tA 2~ t~l) C4 W
~ + + + + + +
+ + + + i- + + + + + +
+ + + + 4- + + + + + + +
O
O
tn N + + + + + +
+ + + + + + + + + +
~-I + + + + + + + + + + + +
O
O
tf1 + + +
t + + + + + + + + + +
.1 + + + + + + +f + + + + +
O
O
+ + + + + +
~-i + + + + + +I + + ~ + + + +
O +
N + + +
~ + + I I I I I + + I +
C) UI
N
r{ + + + +
+ + + + + + + + +
+ + + + + + + + 1 +
~ O ( r"I O
Ln ~ =
+ + + +
+ + + + T + + + + + +
~-{ + + + + + + + + + + + +
+
O +
O + + +
Ln + + + \ +
+ + \ + + + -1 + + + +
~-{ + + + + + + + + + + + +
~
~
~ + +
+ + + + +
0 -4 + + + + + +! + + + + +
N +
-q + + +
~4 L
r. + + + + + +
O + + + + + + + + + + + +
U + + + + + + + + + + + +
yL L
tJ tJ .!J L L
4J C -4 c m 0 ,-~ r~ ~ a L a (1) ~4 ~ ro 4 (o ~ ro ~ It 41) w ~ N N L -1 4-) N L N 41 ,-i N
ca a co a u~+ a a Q vi a a ~ k, rn m ~4 o l o ~4 (~ \p \p N. i(} N N N N N N N
~ ', Ls+ Cta O~ Ol ~a v r-4 a N N GL N N QE ~o ~
V] 7.. 2 2: 2~ UI ~ x N ~ tA 2~ t~l) C4 W
The results confirm those obtained in Example 2.
At a dilution of 1/100 to 1/50 there was no effect on NFF
cells, but significant inhibition of MM96L cells was observed. The melanoma cells surviving at these dilutions had the appearance of normal melanocytes. Inhibition of the other two human melanoma cell lines and of the mouse melanoma cell line was also observE:d.
Similar results were obtained using Merkel cell carcinoma (MCC 16) or squamous cell carcinoma (Coio 6) cells. The results are shown in Table 11.
Dendritic cell morphology was displayed by squamous cell carcinoma, even at 1 in 500,000 dilution.
This extreme potency of the crude extract was also evident for Merkel cell inhibition, which was also still evident at 1 in 500,000 dilution.
At a dilution of 1/100 to 1/50 there was no effect on NFF
cells, but significant inhibition of MM96L cells was observed. The melanoma cells surviving at these dilutions had the appearance of normal melanocytes. Inhibition of the other two human melanoma cell lines and of the mouse melanoma cell line was also observE:d.
Similar results were obtained using Merkel cell carcinoma (MCC 16) or squamous cell carcinoma (Coio 6) cells. The results are shown in Table 11.
Dendritic cell morphology was displayed by squamous cell carcinoma, even at 1 in 500,000 dilution.
This extreme potency of the crude extract was also evident for Merkel cell inhibition, which was also still evident at 1 in 500,000 dilution.
o *
o 'L3 Ln + + +
~ + + + +
+ + + +
~
~
U o T~= 0 O
'c5 O ~ + + +
+ + + +
=,~ VI
o U
ri ~ ~p ic 0) rl .
N U tt~ + + + ~
U ~ + + +
c I + + + + 0 44 O
O
14 r-i O 0 ~
U
0 U~
~-i O Lr1 + ~ +
0 0 ~-\i + + + +I ~ ~
=~
U
U ~ U
W .~ o b ~ ~ U') + + y4 O 1~ + + ro 0 y4 q + i + v+
w ~ ~ 0.1 *O
0 b N r0 a v7 1 O, bi N
z7 :j O Ul 0 U1 ~ U U
~
U 3-1 Z~ ~7 cd r O, r a v ~ N 0 O 44 (1) 4-3 44 O ~ 0 R, U ?1 d.l ~ = ri J-1 ~ 4J W f 1> w 0 OU rO =U
N ~ >~
ri 4) QJ N O ~ r E
w 44 , II II ~-1 W I ~~ O ro O ~ + II C$.' I U2 U) U; Ul U + t ZS ro s~!
-r-I
r-I tD 4) r~ O ~-1 r=I
U U ~
~l Ln o ~
o 'L3 Ln + + +
~ + + + +
+ + + +
~
~
U o T~= 0 O
'c5 O ~ + + +
+ + + +
=,~ VI
o U
ri ~ ~p ic 0) rl .
N U tt~ + + + ~
U ~ + + +
c I + + + + 0 44 O
O
14 r-i O 0 ~
U
0 U~
~-i O Lr1 + ~ +
0 0 ~-\i + + + +I ~ ~
=~
U
U ~ U
W .~ o b ~ ~ U') + + y4 O 1~ + + ro 0 y4 q + i + v+
w ~ ~ 0.1 *O
0 b N r0 a v7 1 O, bi N
z7 :j O Ul 0 U1 ~ U U
~
U 3-1 Z~ ~7 cd r O, r a v ~ N 0 O 44 (1) 4-3 44 O ~ 0 R, U ?1 d.l ~ = ri J-1 ~ 4J W f 1> w 0 OU rO =U
N ~ >~
ri 4) QJ N O ~ r E
w 44 , II II ~-1 W I ~~ O ro O ~ + II C$.' I U2 U) U; Ul U + t ZS ro s~!
-r-I
r-I tD 4) r~ O ~-1 r=I
U U ~
~l Ln o ~
Example 4 Ethanol Extract of E. peplus A fresh preparation of sap from E. peplus was subjected to extraction with 95% aqueous ethanol. Ethanol was removed from the soluble fraction after extraction by vacuum centrifugation, and the fraction was reconstituted to its original volume in tissue culture medium (RPMI1640) containing 5% foetal calf serum and antibiotics. The .pellet remaining after ethanol extraction was dried by vacuum centrifugation and reconstituted to its original volume in tissue culture medium as described above. The crude sap (C), the soluble fraction (S) and the pellet (P) were tested as described above against NFF cells, the melanoma cell lines MM96L, MM537, MM229 and MM2058, and also against the colon cancer cell line LIM1215 and the lung cancer cell line A549. Assays were performed in triplicate, and were assessed after four days culture following additiorl of the sample. The results are shown in Table 12, in which + indicates normal appearance of cells, ++ indicates a possible increase in cell numbers, and -indicates cell death.
+
a + + + + + + + +
o cn + + + + + + + +
Ln N ! I
.-1 U + + + + + + + +
Ac + + + + + + + +
c!~ + + + + + + + +
O
in t !
,1 U + + + + + + + +
N
G.i + + + + + + + +
r ~
G~ + + + + + + + 1 O
O
ri I I I ! I
e-I U + + + + + + +
! ! !
a + + + + + + +'I
t ! ! t !
u~ + + + + ! i N I
r{ U I t I I I ! I I' ~
o 00 t !
=rl [- tllN
ri l a~ cn 4) M N O r-I Cl 0) Lfl N N ~ X Ln A ~! zEE x aftc The results obtained were consistent with those of the previous experiments. Again at low doses the MM96L
cells had a dendritic appearance. All of the tumour cell lines as well as the normal fibroblast cell line NFF were killed by the crude sap and by the soluble fraction obtained by ethanol extraction at a dilution of 1/20. It appeared that the majority of the activity partitioned to the ethanol-soluble fraction. The lung cancer cell line A459 appeared to be particularly susceptible, being affected at a dilution of up to 1/2500 by both the crude sap and by the soluble fraction.
Example 5 Reporter Assay for Gene Expression in Transfected MM96L Malignant Melanoma Cell Line E. peplus sap in phosphate-buffered saline diluent was added to wells containing MM96L cells or the breast cancer cell line MCF7 transfected with a construct consisting of the sheep metallothionein promoter, upstream of a 9-galactosidase reporter gene which had been substituted for the metallothionein gene. The assay thus becomes a measure of gene expression and in particular, of potential transcription, translation and expression of the metallothionein gene. Cells were treated with 4extract in microtitre plates for 20 hr, 100 M ZnSO4 was added and the plates incubated for a further 5 hr, and the medium was removed. i3-galactosidase activity was then measured by incubation of the cells for 1-2 h at 37 C with a chromogenic substrate. This assay is used as a sensitive test for transcriptional activation of genes.
The results are shown in Figure 1.
This shows that there was a marked stimulation of metallothionein gene activation, as measured by increased 9-galactosidase reporter gene expression, which surprisingly became more evident as the sample further was diluted. The mechanism by which E. peplus sap mediates this effect is not understood. Whereas known drugs specific for inhibition of histone deacetylase activity demonstrate increasing expression of the reporter gene with increasing concentration of drug, E. peplus exhibits an inverse dose response. However, the results indicate that this assay can be used to monitor purification of the active agents(s) in E. peplus sap or the plant itself.
The metallothionein protein has antioxidant activity, and is implicated in a protective role against heavy metal-induced cancers. Activation of the metallothionein promoter occurred at concentrations of E. peplus sap too low to effect direct cell killing, except for the extremely sensitive breast cancer cell line MCF7 (Figure 2). The change in appearance of MM96L melanoma cells to the dendritic morphology of normal melanocytes at these dilutions possibly implicates the metallothionein gene in these effects.
.Example 6 Subfractionation of Ethanol-Soluble Extract The soluble fraction obtained by extraction with 95% ethanol, performed as in Example 4, was subjected to isocratic reverse-phase high-performance liquid chromatography (RP-HPLC).
100 ul of crude extract was dissolved in lml 95%
ethanol and periodically shaken at 4 C overnight. The extract was centrifuged at 10,000 x g for 4 minutes, and the supernatant was removed and dried by vacuum centrifugation. The solids were reconstituted in 100 ul running buffer centrifuged briefly, and the soluble material applied to a Brownlee Aquapore RP-300 column (C8), 220 x 4 mm, with a 30 x 4 mm RP-300 guard column.
The running buffer was acetonitrile:water 50:50 (V/V), and the flow rate was 0.75 mi/mn. Fractions were collected at 0.5 mi.n intervals, and the absorbance profile at 195 mn was monitored. The absorbance profile is shown in Figure 3.
Fractions were dried by vacuum centrifugation, reconstituted in 500 l PBS, and assayed against MM96L
*rB
a + + + + + + + +
o cn + + + + + + + +
Ln N ! I
.-1 U + + + + + + + +
Ac + + + + + + + +
c!~ + + + + + + + +
O
in t !
,1 U + + + + + + + +
N
G.i + + + + + + + +
r ~
G~ + + + + + + + 1 O
O
ri I I I ! I
e-I U + + + + + + +
! ! !
a + + + + + + +'I
t ! ! t !
u~ + + + + ! i N I
r{ U I t I I I ! I I' ~
o 00 t !
=rl [- tllN
ri l a~ cn 4) M N O r-I Cl 0) Lfl N N ~ X Ln A ~! zEE x aftc The results obtained were consistent with those of the previous experiments. Again at low doses the MM96L
cells had a dendritic appearance. All of the tumour cell lines as well as the normal fibroblast cell line NFF were killed by the crude sap and by the soluble fraction obtained by ethanol extraction at a dilution of 1/20. It appeared that the majority of the activity partitioned to the ethanol-soluble fraction. The lung cancer cell line A459 appeared to be particularly susceptible, being affected at a dilution of up to 1/2500 by both the crude sap and by the soluble fraction.
Example 5 Reporter Assay for Gene Expression in Transfected MM96L Malignant Melanoma Cell Line E. peplus sap in phosphate-buffered saline diluent was added to wells containing MM96L cells or the breast cancer cell line MCF7 transfected with a construct consisting of the sheep metallothionein promoter, upstream of a 9-galactosidase reporter gene which had been substituted for the metallothionein gene. The assay thus becomes a measure of gene expression and in particular, of potential transcription, translation and expression of the metallothionein gene. Cells were treated with 4extract in microtitre plates for 20 hr, 100 M ZnSO4 was added and the plates incubated for a further 5 hr, and the medium was removed. i3-galactosidase activity was then measured by incubation of the cells for 1-2 h at 37 C with a chromogenic substrate. This assay is used as a sensitive test for transcriptional activation of genes.
The results are shown in Figure 1.
This shows that there was a marked stimulation of metallothionein gene activation, as measured by increased 9-galactosidase reporter gene expression, which surprisingly became more evident as the sample further was diluted. The mechanism by which E. peplus sap mediates this effect is not understood. Whereas known drugs specific for inhibition of histone deacetylase activity demonstrate increasing expression of the reporter gene with increasing concentration of drug, E. peplus exhibits an inverse dose response. However, the results indicate that this assay can be used to monitor purification of the active agents(s) in E. peplus sap or the plant itself.
The metallothionein protein has antioxidant activity, and is implicated in a protective role against heavy metal-induced cancers. Activation of the metallothionein promoter occurred at concentrations of E. peplus sap too low to effect direct cell killing, except for the extremely sensitive breast cancer cell line MCF7 (Figure 2). The change in appearance of MM96L melanoma cells to the dendritic morphology of normal melanocytes at these dilutions possibly implicates the metallothionein gene in these effects.
.Example 6 Subfractionation of Ethanol-Soluble Extract The soluble fraction obtained by extraction with 95% ethanol, performed as in Example 4, was subjected to isocratic reverse-phase high-performance liquid chromatography (RP-HPLC).
100 ul of crude extract was dissolved in lml 95%
ethanol and periodically shaken at 4 C overnight. The extract was centrifuged at 10,000 x g for 4 minutes, and the supernatant was removed and dried by vacuum centrifugation. The solids were reconstituted in 100 ul running buffer centrifuged briefly, and the soluble material applied to a Brownlee Aquapore RP-300 column (C8), 220 x 4 mm, with a 30 x 4 mm RP-300 guard column.
The running buffer was acetonitrile:water 50:50 (V/V), and the flow rate was 0.75 mi/mn. Fractions were collected at 0.5 mi.n intervals, and the absorbance profile at 195 mn was monitored. The absorbance profile is shown in Figure 3.
Fractions were dried by vacuum centrifugation, reconstituted in 500 l PBS, and assayed against MM96L
*rB
cells and in the metallothionein reporter assay as described above. Fractions 13 to 28 all induced complete reversion of MM96L cells to a dendritic appearance, but cell death was not observed. The effect was much more striking in the reporter assay, in which activity was still observed at a dilution of 1/10,000 (ie. at a final concentration in the culture of 1/100,000).
in addition to the foregoing results, the inventor has found that following ultracentrifugation, activity against MM96L cells is found both in the supernatant and in the pellet, and that activity cannot be removed by passing a sample through a molecular weight cut-off membrane. In addition to the cell lines tested above, proliferation of cells of the MCF7 breast cancer cell line was inhibited by E. peplus sap at a final dilution of up to 1/100,000. Cell numbers were assessed using the bicinchoninic acid reagent (Pierce). Results are shown in Figure 2.
Example 7 Solvent fractionation Further solvent fractionation of the crude latex of E. peplus was effected by a series of solvents of increasing polarity. To 1 ml crude latex was added 20 ml diethyl ether in a centrifuge tube. The tube was shaken and centrifuged at 5000g for 5 minutes to partition the layers. The diethyl ether upper layer was removed and the procedure repeated twice. The ether fractions were combined, concentrated to dryness on a rotary evaporator and reconstituted in 1 ml DME for bioassay. In a similar manner, the residue was extracted with ethyl acetate, followed by methylene chloride. The initial ether extract obtained the majority of the activity as measured by decrease in cell numbers of MCF7 breast cancer cells and reversion to a dendritic appearance. However, activity was also demonstrated from the fractions derived from the ethyl acetate and methylene chloride layers. No activity was seen in the final water - soluble (aqueous) fraction. The results are summarised in Table 13.
in addition to the foregoing results, the inventor has found that following ultracentrifugation, activity against MM96L cells is found both in the supernatant and in the pellet, and that activity cannot be removed by passing a sample through a molecular weight cut-off membrane. In addition to the cell lines tested above, proliferation of cells of the MCF7 breast cancer cell line was inhibited by E. peplus sap at a final dilution of up to 1/100,000. Cell numbers were assessed using the bicinchoninic acid reagent (Pierce). Results are shown in Figure 2.
Example 7 Solvent fractionation Further solvent fractionation of the crude latex of E. peplus was effected by a series of solvents of increasing polarity. To 1 ml crude latex was added 20 ml diethyl ether in a centrifuge tube. The tube was shaken and centrifuged at 5000g for 5 minutes to partition the layers. The diethyl ether upper layer was removed and the procedure repeated twice. The ether fractions were combined, concentrated to dryness on a rotary evaporator and reconstituted in 1 ml DME for bioassay. In a similar manner, the residue was extracted with ethyl acetate, followed by methylene chloride. The initial ether extract obtained the majority of the activity as measured by decrease in cell numbers of MCF7 breast cancer cells and reversion to a dendritic appearance. However, activity was also demonstrated from the fractions derived from the ethyl acetate and methylene chloride layers. No activity was seen in the final water - soluble (aqueous) fraction. The results are summarised in Table 13.
Ln e`I + + + + + + + + + + +I +I +I + +
O
O U
O z = ~
o U
Ln + + +
.-1 + + + + + + + + + + +I +i +I + + U) c~
4l u o o c~
=
+ + + + + + + + + + +i +I +i +I +
r-M [z4 ~ U
O o ~
~4 o 4 Ln fd e-I +1 +1 + +1 + +1 + + + +1 +1 +
E~ 0 rt o ~
Ln v 1- ~
+I + + I i +1 + + +I +
td ~
O 0 r-i r-i -1-1 41 4-) 41 ~
X~ O~ X~ O~ XZ O~
(L) O-ri w a) O=r-i 4.+ v 0 -4 4-4 N
õ -r, 41 a, =ri .u .u -r+ 4J 4, t(f .U U N RS 41 U Q) c15 4-1 U (L) N
r-i U (15 'o r-i U RS 'L'3 r--1 U RS ZS (d U1 S4 w S4 0 u) S4 S-a O 0 ~4 4-~4+ P 0 ZS w O -~ ZI 4-4 O =~ :~ 44 0 ~ 0 '-I a1 r-i 41 ~'~I N r-i ~ ^I N ~
04 ~4 4J x U a~~'r, U ~4 4J
~ 4) td U ~f ri Q! 4) ZU RS 4) 0) rtl U (d 41 ~4 a .r. 4-J ~4 a .~ li ~4 ,W
t~ ~) v y-, 4J v v44 A-) N v 4=+
W,~ ~ c ~d ai ra W r- ~ + u rai u~ r' W
r-i >1 >1 >1 7y O N.~ ~--i >r O 4) r- i ~ O
p~ b O T3 41 4 N Ro 71 41 O 0 !8d :j a) :~ :~ a) ~3 71 a) cj 4.) ::s;
U'U N F ~ U'LS U E ~ U'L3 N I; rti Ga Ga z ~ ml ~ ~
~ c! , t~
G1 =rl C14 E-+ ~
() rl 2 ++
O
O U
O z = ~
o U
Ln + + +
.-1 + + + + + + + + + + +I +i +I + + U) c~
4l u o o c~
=
+ + + + + + + + + + +i +I +i +I +
r-M [z4 ~ U
O o ~
~4 o 4 Ln fd e-I +1 +1 + +1 + +1 + + + +1 +1 +
E~ 0 rt o ~
Ln v 1- ~
+I + + I i +1 + + +I +
td ~
O 0 r-i r-i -1-1 41 4-) 41 ~
X~ O~ X~ O~ XZ O~
(L) O-ri w a) O=r-i 4.+ v 0 -4 4-4 N
õ -r, 41 a, =ri .u .u -r+ 4J 4, t(f .U U N RS 41 U Q) c15 4-1 U (L) N
r-i U (15 'o r-i U RS 'L'3 r--1 U RS ZS (d U1 S4 w S4 0 u) S4 S-a O 0 ~4 4-~4+ P 0 ZS w O -~ ZI 4-4 O =~ :~ 44 0 ~ 0 '-I a1 r-i 41 ~'~I N r-i ~ ^I N ~
04 ~4 4J x U a~~'r, U ~4 4J
~ 4) td U ~f ri Q! 4) ZU RS 4) 0) rtl U (d 41 ~4 a .r. 4-J ~4 a .~ li ~4 ,W
t~ ~) v y-, 4J v v44 A-) N v 4=+
W,~ ~ c ~d ai ra W r- ~ + u rai u~ r' W
r-i >1 >1 >1 7y O N.~ ~--i >r O 4) r- i ~ O
p~ b O T3 41 4 N Ro 71 41 O 0 !8d :j a) :~ :~ a) ~3 71 a) cj 4.) ::s;
U'U N F ~ U'LS U E ~ U'L3 N I; rti Ga Ga z ~ ml ~ ~
~ c! , t~
G1 =rl C14 E-+ ~
() rl 2 ++
CMV promoter activity was assayed in HeLa cells infected with a replication-deficient adenovirus construct, in which the Ela gene had been replaced by the CMV promoter driving 9-galactosidase. The results, shown in Table 14, are expressed as a percentage of the control values of infected, untreated cells.
O o tf) O o O O
O df \O [- O O
L!1 d~ m M
~
.r{ O
4) O 1-1 Ln O O O O X
e~ O LCl I~ t.[) Lf) N o 0 =r~ ~ H N Ltl 0 ~1 ~i v r-i ~
0 o O o~,o 0 o ~ ~ d~ M d~ CO CD H N l0 r- ri --I v J~
v r~l k r. o lc:
v O =~+
~ =H .u v ~ U m 'U
td i-I =4 f,- * 'o ff1 ~ { 44 ~-1 O r-i ~-1 ry 4-4 v~ 1.) ~4 0 ~ ~ (U ctS U (0 Z >r +.) ~4 O ! `-i y t~ v v 4-i U~ 0) I W ~, ~ i = ~ ~
4 .-4 >, 4-) O v ~
~ ~ ~ (141 ) ~ ~ o vIF.2 44 ll~ (n ~
Ln The results obtained are qualitatively similar to those seen with other differentiation-inducing agents, such as histone deacetylase inhibitors or butyrate, albeit with more potent activity than seen with these agents. The lower promoter activity observed with the crude and the diethylether extracts at higher concentrations probably reflects cell killing effects against HeLa cells seen at those concentrations.
In a further solvent fractionation experiment, the crude sap was partitioned between methanol:water (17:3) and n-hexane, a solvent partition expected on the basis of previous reports to separate diterpenes (polar phase) from the triterpenes (heptane phase) (Evans and Kinghorn 1977).
Unexpectedly, however, activicy was detected in both phases, suggesting that the active principles behave anomalously in this system.
Another solvent fractionation approach was suggested by the need to clarify samples prior to HPLC
analysis. The crude latex was mixed with ethanol to 70-95%
and shaken overnight at 4 C. The mixture was centrifuged at 1,000 g for 10 min, and the supernatant was removed and concentrated to approx one third the original volume of crude sap. To the concentrate was added 100% acetonitrile to 30-60%. The resulting white precipitate was removed by centrifugation at 12,000 g for 10 minutes. The supernatant .was enriched in macrocyclic diterperies (jatrophanes and pepluane), as determined by TLC and mass spectroscopy.
This observation points the way to a suitable large scale process for enrichment of the active principles Example 8 Further activity-guided subfractionation of the ethanol-soluble extract Fractions 14 and 15 from the HPLC
subfractionation described in Example 7 and Figure 3 were further purified by repeated chromatography, selecting the dominant symmetrical peak with constant diode array spectra (eg. fractions 14 and 15; results for fraction 14 are shown in Figures 4 and 5). Activity of the purified fractions in causing reversion of MM96L to the dendritic appearance was confirmed by cell assay.
The features of the change to MM96L cells after the addition of Fraction 15 are shown in Figure 6. Cells were visualised as photomicrographs, using an antibody coupling procedure. The first antibody, a mouse monoclonal directed towards tyrosinase-related protein 1(TRP-1), was detected with a second antibody, sheep anti-mouse -alkaline phosphatase conjugate, using bromo-chloro-indolyl phosphate and nitroblue tetrazolium (BCIP/NBT) as developing substrates. After four days of incubation (Figures 6A and 6B) there was a marked reduction in the number of melanoma cells and a pronounced change in their morphology. The cells had reverted to a long, spindly (dendritic) appearance, characteristic of normal mature melanocytes. All cells in the field appeared to have adopted this altered morphology, which is surprising given the heterogeneous nature of the MM96L cell population.
After 21 days of incubation, the treated cells were seen to align somewhat parallel to one another in clusters, as shown in Figures 6C and 6D, a characteristic of normal, mature melanocytes. Similar features have been observed with all dendritic cell-inducing fractions from E. peplus, including the crude sap.
Electrospray mass spectroscopic analyses for fractions 14 and 15 indicated the presence of 2,5,7,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 5, Jakupovic et al, 1998a) with an m/a of 780 (calculated 779.315). Nuclear magnetic resonance (1~'MR) analysis, using 1D NMR, on fraction 14 gave down-field signals between 7 and 9.4 ppm which are consistent with a pyridine-like moiety, as is present in the nicotinoate group at ring position 9. Also, a trans double bond was evidenced by the large coupling constant at 5-6 ppm, in agreement with the 11, 12 internal double bond in the jatrophane ring structure. Also identified in fraction 14 by electrospray in the negative ion mode was 2,5,7,9,14-pentaacetoxy-3-benzoyloxy-8,15-dihydroxy-jatropha-6(17),11E-diene (jatrophane 6, Jakupovic et al, 1998a), with m/z 716 (calculated 716.304), 673 (M - ketene), 656 (M - AcOH).
Fraction 15 contained 2,3,5,7,15-pentaacetoxy-9-nicotinoyloxy-l4-oxojatropha-6(17),11E-diene (jatrophane 1, Jakupovic et al, 1998a) with m/z 597 (M - ketene - AcOH).
Thus, by spectroscopic analysis, the early-eluting fractions at 7-7.5 minutes on HPLC with cell killing and dendritic activity contained a mixture of jatrophanes 5, 6, and 1. This result is consistent with the behaviour of HPLC fractions 14 and 15 when chromatographed on HPTLC, using toluene:acetone 9:1 as uhe developing solvent. UV-positive spots did not move from the origin, Rf 0.0 (approx), in contrast to later-eluting fractions (eg fractions 20-22, Rf 0.3-0.5). This indicates the relatively polar behaviour of jatrophanes 5, 6, and 1, in comparison to jatrophanes 3, 2 and 4, as demonstrated by chromatography on HPTLC, using either toluene:acetone 9:1 or hexane:ethyl acetate 4:1 as developing solvents. These results are similar to those obtained by Jakupovic et al, 1998a, using petrol: methyl-tert-butyl ether (1:1) as the developing solvent, eg: jatrophane 5: Rf 0.04, jatrophane 6: Rf 0.10 (3X), and jatrophane 1: Rf 0.11. There was no evidence in the mass spectroscopic data from the early HPLC
fractions of the presence o'L ingenarie derivatives (see later), or other cotnponents reported from the literature and presented in Table 1, in E. peplus crude extracts.
Example 9 Biological Activity-Guided Purification of Crude and Ether-Soluble Extracts on Thin Layer Chromatography (TLC) and High Performance Thin Layer Chromatography (HPTLC) (a) The ether-soluble fraction, prepared as in Example 7, was reconstituted in ethylene glycol dimethyl ether (DME) and chromatographed on 20 x 20 cm silica gel plates, using chloroform:ethyl acetate (82:18) as the developing solvent (Figure 7). The plate was viewed on a W light box and the UV positive bands were identified, excised from the gel, eluted with DME, and tested for inhibitory activity and morphology reversal against MM96L
melanoma cell line. By slicing the whole gel into W and non-W absorbing fractions, it was demonstrated in preliminary experiments that activity was associated with the UV-absorbing bands. Stainirig the side strips of the gel with 0.1% iodine in chloroform revealed other iodine strongly positive bands. However, these were found to possess negligible activity. UV-absorbing bands at Rf 0.0 (A), Rf 0.16-0.18 (B1), Rf 0.22-0.24 (B2), Rf 0.73-0.80 (C), Rf 0.80-0.96 (D) were biologically active, with observable decrease in cell numbers and complete reversion to dendritic cell appearance at 1/5,000 dilution.
Zones B1, C and D were further purified by chromatography on silica gel 60 plates, using a two-dimensional solvent system with hexane:ethyl acetate (1:1) in the first dimension and toluene:acetone (9:1) in the second dimension (Figures 8A to 8C respectively). W-absorbing spots with inhibitol:y activity towards MM96L of greater than 30% of cell number5 and with complete reversion to dendritic cell appearance at 1/50C dilution are indicated on the figures.
The strongly Lv-absorbing spots 22 and 23 derived from zone D (see Figure 8C) were excised from the gel, eluted with DME and dried by vacuum centrifugation. Mass spectroscopic analysis of fractions 22 and 23 revealed the presence of 5,8,9,10,14-pentaacetoxy-3-benzoyloxy-15-hydroxypepluane, m/z 639.5 (V! - AcOH)+, ie pepluane.
(b) Whole crude sap was chromatographed on 10 x 10 cm HPTLC silica gel 60 plates with concentrating zones (Merck Cat No. 013748.1000), using toluene:acetone (9:1) as the developing solvent, as shown in Figure 9. The UV-positive zones (1, Rf 0.14; 2, Rf 0.23; 3, Rf 0.49; 4, Rf 0.54; 5, Rf 0.57; 6, Rf 0.63; and 7, Rf 0.73) were excised from the gel and eluted with DME / diethyl ether. The fractions were tested against MM96L as described above, and fractions 1, 3, 4, 5 and 6 were demonstrated to possess cell inhibitory activity and cell reversion activity.
These fractions were separately chromatographed on HPTLC
plates using hexane : ethyl ~icetate (4:1) as the developing solvent, yielding Uv positive bands A, Rf 0.17; B, Rf 0.24;
C, Rf 0.42; D, Rf 0.48; E, Rf 0.52; F, Rf 0.58; G, Rf 0.62 (Figure 10) and H, R 0.02 (Figure 11). All fractions except G (iodine positive, see Figure 10) were active against MM96L cells, in terms of cell growth inhibition and reversion to complete dendritic morphology, at 1 in 5000 dilution.
Mass spectroscopic analyses of fractions A-F (B
missing) and H are shown in Table 15, with a tentative assignment of compounds from the known molecular mass ions of the published constituen~.s o-.L' E. peplus:
O df \O [- O O
L!1 d~ m M
~
.r{ O
4) O 1-1 Ln O O O O X
e~ O LCl I~ t.[) Lf) N o 0 =r~ ~ H N Ltl 0 ~1 ~i v r-i ~
0 o O o~,o 0 o ~ ~ d~ M d~ CO CD H N l0 r- ri --I v J~
v r~l k r. o lc:
v O =~+
~ =H .u v ~ U m 'U
td i-I =4 f,- * 'o ff1 ~ { 44 ~-1 O r-i ~-1 ry 4-4 v~ 1.) ~4 0 ~ ~ (U ctS U (0 Z >r +.) ~4 O ! `-i y t~ v v 4-i U~ 0) I W ~, ~ i = ~ ~
4 .-4 >, 4-) O v ~
~ ~ ~ (141 ) ~ ~ o vIF.2 44 ll~ (n ~
Ln The results obtained are qualitatively similar to those seen with other differentiation-inducing agents, such as histone deacetylase inhibitors or butyrate, albeit with more potent activity than seen with these agents. The lower promoter activity observed with the crude and the diethylether extracts at higher concentrations probably reflects cell killing effects against HeLa cells seen at those concentrations.
In a further solvent fractionation experiment, the crude sap was partitioned between methanol:water (17:3) and n-hexane, a solvent partition expected on the basis of previous reports to separate diterpenes (polar phase) from the triterpenes (heptane phase) (Evans and Kinghorn 1977).
Unexpectedly, however, activicy was detected in both phases, suggesting that the active principles behave anomalously in this system.
Another solvent fractionation approach was suggested by the need to clarify samples prior to HPLC
analysis. The crude latex was mixed with ethanol to 70-95%
and shaken overnight at 4 C. The mixture was centrifuged at 1,000 g for 10 min, and the supernatant was removed and concentrated to approx one third the original volume of crude sap. To the concentrate was added 100% acetonitrile to 30-60%. The resulting white precipitate was removed by centrifugation at 12,000 g for 10 minutes. The supernatant .was enriched in macrocyclic diterperies (jatrophanes and pepluane), as determined by TLC and mass spectroscopy.
This observation points the way to a suitable large scale process for enrichment of the active principles Example 8 Further activity-guided subfractionation of the ethanol-soluble extract Fractions 14 and 15 from the HPLC
subfractionation described in Example 7 and Figure 3 were further purified by repeated chromatography, selecting the dominant symmetrical peak with constant diode array spectra (eg. fractions 14 and 15; results for fraction 14 are shown in Figures 4 and 5). Activity of the purified fractions in causing reversion of MM96L to the dendritic appearance was confirmed by cell assay.
The features of the change to MM96L cells after the addition of Fraction 15 are shown in Figure 6. Cells were visualised as photomicrographs, using an antibody coupling procedure. The first antibody, a mouse monoclonal directed towards tyrosinase-related protein 1(TRP-1), was detected with a second antibody, sheep anti-mouse -alkaline phosphatase conjugate, using bromo-chloro-indolyl phosphate and nitroblue tetrazolium (BCIP/NBT) as developing substrates. After four days of incubation (Figures 6A and 6B) there was a marked reduction in the number of melanoma cells and a pronounced change in their morphology. The cells had reverted to a long, spindly (dendritic) appearance, characteristic of normal mature melanocytes. All cells in the field appeared to have adopted this altered morphology, which is surprising given the heterogeneous nature of the MM96L cell population.
After 21 days of incubation, the treated cells were seen to align somewhat parallel to one another in clusters, as shown in Figures 6C and 6D, a characteristic of normal, mature melanocytes. Similar features have been observed with all dendritic cell-inducing fractions from E. peplus, including the crude sap.
Electrospray mass spectroscopic analyses for fractions 14 and 15 indicated the presence of 2,5,7,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-9-nicotinoyloxyjatropha-6(17),11E-diene (jatrophane 5, Jakupovic et al, 1998a) with an m/a of 780 (calculated 779.315). Nuclear magnetic resonance (1~'MR) analysis, using 1D NMR, on fraction 14 gave down-field signals between 7 and 9.4 ppm which are consistent with a pyridine-like moiety, as is present in the nicotinoate group at ring position 9. Also, a trans double bond was evidenced by the large coupling constant at 5-6 ppm, in agreement with the 11, 12 internal double bond in the jatrophane ring structure. Also identified in fraction 14 by electrospray in the negative ion mode was 2,5,7,9,14-pentaacetoxy-3-benzoyloxy-8,15-dihydroxy-jatropha-6(17),11E-diene (jatrophane 6, Jakupovic et al, 1998a), with m/z 716 (calculated 716.304), 673 (M - ketene), 656 (M - AcOH).
Fraction 15 contained 2,3,5,7,15-pentaacetoxy-9-nicotinoyloxy-l4-oxojatropha-6(17),11E-diene (jatrophane 1, Jakupovic et al, 1998a) with m/z 597 (M - ketene - AcOH).
Thus, by spectroscopic analysis, the early-eluting fractions at 7-7.5 minutes on HPLC with cell killing and dendritic activity contained a mixture of jatrophanes 5, 6, and 1. This result is consistent with the behaviour of HPLC fractions 14 and 15 when chromatographed on HPTLC, using toluene:acetone 9:1 as uhe developing solvent. UV-positive spots did not move from the origin, Rf 0.0 (approx), in contrast to later-eluting fractions (eg fractions 20-22, Rf 0.3-0.5). This indicates the relatively polar behaviour of jatrophanes 5, 6, and 1, in comparison to jatrophanes 3, 2 and 4, as demonstrated by chromatography on HPTLC, using either toluene:acetone 9:1 or hexane:ethyl acetate 4:1 as developing solvents. These results are similar to those obtained by Jakupovic et al, 1998a, using petrol: methyl-tert-butyl ether (1:1) as the developing solvent, eg: jatrophane 5: Rf 0.04, jatrophane 6: Rf 0.10 (3X), and jatrophane 1: Rf 0.11. There was no evidence in the mass spectroscopic data from the early HPLC
fractions of the presence o'L ingenarie derivatives (see later), or other cotnponents reported from the literature and presented in Table 1, in E. peplus crude extracts.
Example 9 Biological Activity-Guided Purification of Crude and Ether-Soluble Extracts on Thin Layer Chromatography (TLC) and High Performance Thin Layer Chromatography (HPTLC) (a) The ether-soluble fraction, prepared as in Example 7, was reconstituted in ethylene glycol dimethyl ether (DME) and chromatographed on 20 x 20 cm silica gel plates, using chloroform:ethyl acetate (82:18) as the developing solvent (Figure 7). The plate was viewed on a W light box and the UV positive bands were identified, excised from the gel, eluted with DME, and tested for inhibitory activity and morphology reversal against MM96L
melanoma cell line. By slicing the whole gel into W and non-W absorbing fractions, it was demonstrated in preliminary experiments that activity was associated with the UV-absorbing bands. Stainirig the side strips of the gel with 0.1% iodine in chloroform revealed other iodine strongly positive bands. However, these were found to possess negligible activity. UV-absorbing bands at Rf 0.0 (A), Rf 0.16-0.18 (B1), Rf 0.22-0.24 (B2), Rf 0.73-0.80 (C), Rf 0.80-0.96 (D) were biologically active, with observable decrease in cell numbers and complete reversion to dendritic cell appearance at 1/5,000 dilution.
Zones B1, C and D were further purified by chromatography on silica gel 60 plates, using a two-dimensional solvent system with hexane:ethyl acetate (1:1) in the first dimension and toluene:acetone (9:1) in the second dimension (Figures 8A to 8C respectively). W-absorbing spots with inhibitol:y activity towards MM96L of greater than 30% of cell number5 and with complete reversion to dendritic cell appearance at 1/50C dilution are indicated on the figures.
The strongly Lv-absorbing spots 22 and 23 derived from zone D (see Figure 8C) were excised from the gel, eluted with DME and dried by vacuum centrifugation. Mass spectroscopic analysis of fractions 22 and 23 revealed the presence of 5,8,9,10,14-pentaacetoxy-3-benzoyloxy-15-hydroxypepluane, m/z 639.5 (V! - AcOH)+, ie pepluane.
(b) Whole crude sap was chromatographed on 10 x 10 cm HPTLC silica gel 60 plates with concentrating zones (Merck Cat No. 013748.1000), using toluene:acetone (9:1) as the developing solvent, as shown in Figure 9. The UV-positive zones (1, Rf 0.14; 2, Rf 0.23; 3, Rf 0.49; 4, Rf 0.54; 5, Rf 0.57; 6, Rf 0.63; and 7, Rf 0.73) were excised from the gel and eluted with DME / diethyl ether. The fractions were tested against MM96L as described above, and fractions 1, 3, 4, 5 and 6 were demonstrated to possess cell inhibitory activity and cell reversion activity.
These fractions were separately chromatographed on HPTLC
plates using hexane : ethyl ~icetate (4:1) as the developing solvent, yielding Uv positive bands A, Rf 0.17; B, Rf 0.24;
C, Rf 0.42; D, Rf 0.48; E, Rf 0.52; F, Rf 0.58; G, Rf 0.62 (Figure 10) and H, R 0.02 (Figure 11). All fractions except G (iodine positive, see Figure 10) were active against MM96L cells, in terms of cell growth inhibition and reversion to complete dendritic morphology, at 1 in 5000 dilution.
Mass spectroscopic analyses of fractions A-F (B
missing) and H are shown in Table 15, with a tentative assignment of compounds from the known molecular mass ions of the published constituen~.s o-.L' E. peplus:
tn M U ri LI1 a) RS lfl 110 ~ U") ~
t.0 Q4 O lD ":Zv ~ 0 u to ~ N ~1 m r- z Ln z +
ul M~
o i0 tn ~ ~ ~ `r to 3 N -Lj D rn 9 r~ "~ ~
U =r1 Ql ~ [` ~ ~
1 d M
G~ 4J = . Op m M co ^tl U ~ M, C .- rn ~, +J tfl ~, N
M v ~ M
id w v lD C- L(1 CO
O lzzp O N ttl f~ ~
o\o f !d O d! C) r (~
~
.ri ~ ...
v 1 =r1 (' N 4 o~l ,.,~ Op 04 M Ul ~~~ U o1 l0 Ol ~4 0 N >1 U rd kp tio 1' ~' ri rl ro .) +
r-i O + + ` ry ^ (0 E-4 c0 0 0 u+~ z zl U U U -- Z
=rl r:l, rti 00 -F q ~= m 0 ~ -- Ci N ~ O ~-I O
0 .-= Z N Co !cc Ol ~ 9.' 0 p (0) ~(~ RS N N al N Qa .tJ r-I 'D r- U-. N 0 u 0,i ul 1 ~=I
{2, ~ 04 c~ 4..) Ll, N+~ rn cri o N = U QI ~ 0I { Ui r-i n 0 ~.j NI tU N~
(A !
RS O FC ( O Ln O'L,-' C) CV O = O C) r! i ( r 1 M '-f r-1 U' ~ 0 rl ~ ~ ~; H -z E- + t-D Z "Ol tf1 (tf N ^ l.f) =n~ Cr. -nl 1i rn CO + ~ 00 N N -- ! M ,' N
N r-{ N N C', N d! M
i.n N rn 0 a~i 4.J
rn C?, h U i~ N M r-I rn l~ - cY1 d' `-' z Ln ~C tf) ~ ~2 -~ t 1 CO, _=
r!
!
~
t.0 Q4 O lD ":Zv ~ 0 u to ~ N ~1 m r- z Ln z +
ul M~
o i0 tn ~ ~ ~ `r to 3 N -Lj D rn 9 r~ "~ ~
U =r1 Ql ~ [` ~ ~
1 d M
G~ 4J = . Op m M co ^tl U ~ M, C .- rn ~, +J tfl ~, N
M v ~ M
id w v lD C- L(1 CO
O lzzp O N ttl f~ ~
o\o f !d O d! C) r (~
~
.ri ~ ...
v 1 =r1 (' N 4 o~l ,.,~ Op 04 M Ul ~~~ U o1 l0 Ol ~4 0 N >1 U rd kp tio 1' ~' ri rl ro .) +
r-i O + + ` ry ^ (0 E-4 c0 0 0 u+~ z zl U U U -- Z
=rl r:l, rti 00 -F q ~= m 0 ~ -- Ci N ~ O ~-I O
0 .-= Z N Co !cc Ol ~ 9.' 0 p (0) ~(~ RS N N al N Qa .tJ r-I 'D r- U-. N 0 u 0,i ul 1 ~=I
{2, ~ 04 c~ 4..) Ll, N+~ rn cri o N = U QI ~ 0I { Ui r-i n 0 ~.j NI tU N~
(A !
RS O FC ( O Ln O'L,-' C) CV O = O C) r! i ( r 1 M '-f r-1 U' ~ 0 rl ~ ~ ~; H -z E- + t-D Z "Ol tf1 (tf N ^ l.f) =n~ Cr. -nl 1i rn CO + ~ 00 N N -- ! M ,' N
N r-{ N N C', N d! M
i.n N rn 0 a~i 4.J
rn C?, h U i~ N M r-I rn l~ - cY1 d' `-' z Ln ~C tf) ~ ~2 -~ t 1 CO, _=
r!
!
~
pepluane = 5,8,9,10,14-pentaacetoxy-3-benzoyloxy-15-hydroxypepluane jatrophane 2 = 2,5,7,9,14-hexaacetoxy-3-benzoyloxy-15-hydroxy-jatropha-6(17),11E-diene jatrophane 3 = 2,5,14-triacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxy-9-nicotinoyloxyjatropha-6(17),11E-diene jatrophane 4 = 2,5,9,14-tetraacetoxy-3-benzoyloxy-8,15-dihydroxy-7-isobutyroyloxyjatropha-6(17),11E-diene) Thus, mass spectroscopy revealed a mixture of 20-acetyl-ingenol-3-angelate (fraction A), pepluane (fractions A, C & D) and jatroptianes 2(fractiUn D) 3(fractions C&H), and 4 (fractions E & F). 'H chemical shift data for fraction H are shown in Table 16.
Table 16 'H Chemical Shift* Data for Fraction H
H ppm Mu2tiplicity Indicative Jatrophane Ring Backbone Signals la 2.816 brd 1f3 2.056 d 3 5.918 d 4 3.731 brd 5 5.730 brd 7 5.390 d 8 (OH) 2 . 948 _ d 9 4.971 ~ s 11 6.145 d 12 5.640 dd 13 2.840 cm 14 5.110 s 15(OH) 3.645 s 16 i 1.489 s 17 4.438 d 17' 4.788 d 18 1.052 s 19 1.152 s 20 1.353 d Ester Substituent Signals 9.290 brd Onic 8.340 ddd 8.805 brdd 7.390 brd 9.079 brd Onic 8.202 !ddd 8.767 1brdd 7.327 brd 8.040 AA' OBz 7.403 1BB' ~ 7.541 iC
~ 1.972 qq OiBu 0 . 912 Id 10.449 d 0.450 d * Chemical shifts are measured at 295K relative to chloroform at 7.24 ppm.
These assigrunents indicated the presence of a jatrophane ring structure as determined from DQF-COSY, NOESY and TOCSY two--dimensional spectra. The spectrum of Fraction H was cons:stent with the preserce of Jatrophane 3 in two diastereomeric conformations (considered most likely), a mixture of two or more similarly substituted jatrophanes, or a new jatrophane with two nicotinate, one benzoate, and an isc-butyrate moiety. The likely ring confirmation was II, as per Jakupovic et al (1998a), with a J4,5 of approxintately 6 Hz and strong NOE's between 5 and 8, and 4 and 7; with J7,8 and tT8,9 practically zero - as evidenced by tocal lack of cross peaks in the DQF COSY
Table 16 'H Chemical Shift* Data for Fraction H
H ppm Mu2tiplicity Indicative Jatrophane Ring Backbone Signals la 2.816 brd 1f3 2.056 d 3 5.918 d 4 3.731 brd 5 5.730 brd 7 5.390 d 8 (OH) 2 . 948 _ d 9 4.971 ~ s 11 6.145 d 12 5.640 dd 13 2.840 cm 14 5.110 s 15(OH) 3.645 s 16 i 1.489 s 17 4.438 d 17' 4.788 d 18 1.052 s 19 1.152 s 20 1.353 d Ester Substituent Signals 9.290 brd Onic 8.340 ddd 8.805 brdd 7.390 brd 9.079 brd Onic 8.202 !ddd 8.767 1brdd 7.327 brd 8.040 AA' OBz 7.403 1BB' ~ 7.541 iC
~ 1.972 qq OiBu 0 . 912 Id 10.449 d 0.450 d * Chemical shifts are measured at 295K relative to chloroform at 7.24 ppm.
These assigrunents indicated the presence of a jatrophane ring structure as determined from DQF-COSY, NOESY and TOCSY two--dimensional spectra. The spectrum of Fraction H was cons:stent with the preserce of Jatrophane 3 in two diastereomeric conformations (considered most likely), a mixture of two or more similarly substituted jatrophanes, or a new jatrophane with two nicotinate, one benzoate, and an isc-butyrate moiety. The likely ring confirmation was II, as per Jakupovic et al (1998a), with a J4,5 of approxintately 6 Hz and strong NOE's between 5 and 8, and 4 and 7; with J7,8 and tT8,9 practically zero - as evidenced by tocal lack of cross peaks in the DQF COSY
spectrum. There were no signals consistent with the presence of any ingenol structure. The sample was retrieved from the magnet, and an aliquot demonstrated potent activity against MM96L, evidenced by complete cell death at 20ug/ml, and complete reversion to a dendritic appearance at less than 20 pg/ml.
Example 10 NMR analysis Fraction A was further purified by chromatography on HPTLC using hexane:ethyl acezate (4:1) as the developing solvent. As an adjunct to absorbance on a UV light box, a side strip was stained by spraying che gel with 70%
phosphoric acid in metharioi, and development by heating the gel with a hair drier revealed an intense blue band under W light, separable from the r.tajor UV absorbing band. The unstained region equivalent to this band was excised, eluted with ether and dried by -vacuum centrifugation.
Approx. 1 mg of this material was accumulated from 4 ml latex. The material was subjecLed to NN~R analysis, and subsequently bioassayed and demonstrated to be active in terms of reversion to complete dendritic morphology at 1 in 5 x 106 dilution, representing a 1 ng/ml final concentration. This material was identified by NMR as C27H3607, 20-acetyl-ingenol-3-angelate as shown in Table 17.
This finding is consistent with the mass spectroscopic evidence presented in Table i5.
Example 10 NMR analysis Fraction A was further purified by chromatography on HPTLC using hexane:ethyl acezate (4:1) as the developing solvent. As an adjunct to absorbance on a UV light box, a side strip was stained by spraying che gel with 70%
phosphoric acid in metharioi, and development by heating the gel with a hair drier revealed an intense blue band under W light, separable from the r.tajor UV absorbing band. The unstained region equivalent to this band was excised, eluted with ether and dried by -vacuum centrifugation.
Approx. 1 mg of this material was accumulated from 4 ml latex. The material was subjecLed to NN~R analysis, and subsequently bioassayed and demonstrated to be active in terms of reversion to complete dendritic morphology at 1 in 5 x 106 dilution, representing a 1 ng/ml final concentration. This material was identified by NMR as C27H3607, 20-acetyl-ingenol-3-angelate as shown in Table 17.
This finding is consistent with the mass spectroscopic evidence presented in Table i5.
Table 17 NMR data obtained on bioactive fraction A2 to support 20-acetyl-ingenol-3-angelate chemical structure:
lxNMR 13cNMR
H Jppm/multiplicity # C [Hz [PPM]
1 6.106 1 9 25933.898 206.2210 3 5.396 s 2 26 21513.854 171.0737 3.875 d 3 21 21165.912 168.3070 7 6.024 d 4 23 17626.074 140.1589 8 4.076 5 2 17086.838 135.8710 11 2.4783 m 6 6 17082.062 135.8330 12 2.222 ddd 7 1 16614.730 132.1169 12' 1.743 ddd 8~ 7 16301.014 129.6223 13 0.681 m 9 22 15976.620 127.0428 14 0.936 m 10 4 10668.691 84.8352 16 1.033 s 11 3 10395.504 82.6629 17 1.062 s 12 5 9411.686 74.8398 18 0.952 d 13 10 9059.148 72.0365 19 1.785 brs 14 20 8404.062 66.8274 20 4.745 d 15 8 5481.686 43.5892 20' 4.467 d 16 11 4841.115 38.4955 23 6.153 qq 17 12 3911.906 31.1067 24 1.906 brs 18 ? 3735.577 29.7045 ---,-25 1.996 brdd ~ 19 16 3535.756 28.5132 27 2.042 20 115 3018.427 24.001.9 - -----~
40H 3.4308 21 13 2524.308 23.2535 50H 3.514 d 22 14 2692.863 23.0035 23 27 2655.734 31.1179 24 24 2612.189 20.7716 25 18 21"7:1- . 91.3 17 . 2706 ~ -26 25 2007.760 15.9653 27 19 16.98.690 15.6546 28 17 1.951.377 15.5169 - -- - -s~s.. _ However, the absence of 20-acetyl-ingenol-3-angelate from the mass spectra of the activity-guided purifications by HPLC, and in other TLC fractions apart from fraction A, indicates that this is not the only active fraction. Rather, jatrophanes 1-6 and-pepluane are also implicated by deduction from the NMR and mass spectroscopic data. This is particularly true of fractions H as prepared by TLC (jatrophane 3 Na+ m/z 830; see also 1D NMR results in Table 16) and fractions 13 and 14 as prepared by HPLC
(jatrophane 5, m/z 779 and 1D NMR; jatrophane 6, m/z 716;
jatrophane 1 or jatrophane 6 derivative, m/z 597.
Jakupovic et a1 (1998a) have proposed that the paraliane class of compounds are intermediates in the pathway between jatrophanes and pepluane. Since anti-cancer cell activity and dendritic cell reversal by both jatrophanes and pepluane have been demonstrated in this invention, it seems reasonable to conclude that the paralianes will also exhibit these properties.
Example 11 Preparation of Material for t-he Mouse Experiments by Preparative Thin Layer Chromatography.
15 ml crude sap in 70% ethanol was extracted with diethyl ether as described in Example 6. The extract was concentrated by vacuum centr~fugation and resuspended in approx 5 ml DME. The DME extract was chromatographed on preparative TLC plates (Merck PLC, Silica gel 60, Cat no.
005745.1000) using hexane:ethyi acetate (4:1) as the developing solvent. Zones corresponding to regions "H" and "A-F" as shown in Figure 12 were excised and combined, eluted with ether/DME, and dried by vacuum centrifugation.
The extract was enriched in jaLrophanes 2, 3 and 4, pepluane, and the ingenane acetate. The pellet was suspended in 95% ethanol and centrifuged at 10,000 g for 10 minutes. The supernatant (6.0 ml, 10 mg/ml) was distributed into 0.2 ml aliqquots anft 5tored at -20 C. This extract was assayed against MM96L melanoma cell line, and showed high potency, with dendritic cell morphology still evident at 1 in 5 x 106 dilution; this replicated the potency of the crude sap. The extract so prepared was enriched in jatrophanes 2, 3 and 4, pepluane, and the ingenane acetate. Just prior to injection, 20 ul was diluted to 1 ml with RPMI 1640 tissue culture medium containing 5% foetal calf serum for injection of 0.1-0.2 ml. The ethanol solution (10 mg/ml) was absorbed on a cotton bud (0.2-0.4 ml) and used for topical application in mice.
Example 12 Inhibition of Growth of Subcutaneous Implants of Tumour Cells (a) Five 4 week old nude mice were injected s.c. at 4 different sites wit.z 0.1 ml of tissue culture medium containing 2 x 106 MM96L human melanoma cells. The three treated mice were injected on days 1, 2, 3, 5, 6, 7, and 8 with 0.1 ml RPMI medium containing 5% foetal calf serum and 20 pg ethanol extract. In addition, the treated mice received up to four topical applications of approx 5-10 ul of 10 mg/ml ethanol extract or crude undiluted sap.
Two separate sites on each treated mouse received topical treatment with either ethanol extract or crude sap. One mouse received topical treatment on days 12, 13 and 14, and the other two treated mice received topical treatment on days 15, 19, 20 and 22. Tumour volume was measured on day 32.
Prior to the topical applications, injection of' extract had no apparent effect on tumour volume. Following topical application of ethanoi extract there was an overnight change in tumour appearance. The tumours became greyish-black in colour, then developed a hard, lumpy black appearance followed by scab formation. Tumours treated with crude sap showed similar changes a day later. With time, the overall effects of ethanol extract and crude sap were similar, so measurements for r:he topically treated lesions have been combined. On the mice given injection plus topical treatment, tumour volume was reduced by 76%
(p<0.2). One tumour which had been treated with the ethanol extract had completely disappeared, as shown in Figure 13, and eight others were reduced to flat black scabs. The other three treated tumours initially showed similar colour changes and tumour regression, but had regrown following cessation of topical treatment 10 days before the measurements were taken.
(b) Six 4 week old C57 Black (C57B1) mice were injected with 0.1 ml of tissue culture rrLedium containing 105 B16 melanoma cancer cells at two sites on the underbelly. The tumours were allowed to develop for 4 days, and then were subjecced to a regimen oi three injections (20 ug ethanol extract in 0.1 ml RPMI medium containing 5% foetal calf serum (days 1, 2 and 4) and 1 topical treatment (5-10 ul of 10 mg/ml ethanol extract on day 4). 8 days after the first injection the areas of the tumours were measured using a ruler. Treatment reduced the size of the B16 melanoma tumours by 64% (p<0.05) on the three treated mice by comparison with the size of tumours on the three control mice.
The results are sumraarised in Table 18.
lxNMR 13cNMR
H Jppm/multiplicity # C [Hz [PPM]
1 6.106 1 9 25933.898 206.2210 3 5.396 s 2 26 21513.854 171.0737 3.875 d 3 21 21165.912 168.3070 7 6.024 d 4 23 17626.074 140.1589 8 4.076 5 2 17086.838 135.8710 11 2.4783 m 6 6 17082.062 135.8330 12 2.222 ddd 7 1 16614.730 132.1169 12' 1.743 ddd 8~ 7 16301.014 129.6223 13 0.681 m 9 22 15976.620 127.0428 14 0.936 m 10 4 10668.691 84.8352 16 1.033 s 11 3 10395.504 82.6629 17 1.062 s 12 5 9411.686 74.8398 18 0.952 d 13 10 9059.148 72.0365 19 1.785 brs 14 20 8404.062 66.8274 20 4.745 d 15 8 5481.686 43.5892 20' 4.467 d 16 11 4841.115 38.4955 23 6.153 qq 17 12 3911.906 31.1067 24 1.906 brs 18 ? 3735.577 29.7045 ---,-25 1.996 brdd ~ 19 16 3535.756 28.5132 27 2.042 20 115 3018.427 24.001.9 - -----~
40H 3.4308 21 13 2524.308 23.2535 50H 3.514 d 22 14 2692.863 23.0035 23 27 2655.734 31.1179 24 24 2612.189 20.7716 25 18 21"7:1- . 91.3 17 . 2706 ~ -26 25 2007.760 15.9653 27 19 16.98.690 15.6546 28 17 1.951.377 15.5169 - -- - -s~s.. _ However, the absence of 20-acetyl-ingenol-3-angelate from the mass spectra of the activity-guided purifications by HPLC, and in other TLC fractions apart from fraction A, indicates that this is not the only active fraction. Rather, jatrophanes 1-6 and-pepluane are also implicated by deduction from the NMR and mass spectroscopic data. This is particularly true of fractions H as prepared by TLC (jatrophane 3 Na+ m/z 830; see also 1D NMR results in Table 16) and fractions 13 and 14 as prepared by HPLC
(jatrophane 5, m/z 779 and 1D NMR; jatrophane 6, m/z 716;
jatrophane 1 or jatrophane 6 derivative, m/z 597.
Jakupovic et a1 (1998a) have proposed that the paraliane class of compounds are intermediates in the pathway between jatrophanes and pepluane. Since anti-cancer cell activity and dendritic cell reversal by both jatrophanes and pepluane have been demonstrated in this invention, it seems reasonable to conclude that the paralianes will also exhibit these properties.
Example 11 Preparation of Material for t-he Mouse Experiments by Preparative Thin Layer Chromatography.
15 ml crude sap in 70% ethanol was extracted with diethyl ether as described in Example 6. The extract was concentrated by vacuum centr~fugation and resuspended in approx 5 ml DME. The DME extract was chromatographed on preparative TLC plates (Merck PLC, Silica gel 60, Cat no.
005745.1000) using hexane:ethyi acetate (4:1) as the developing solvent. Zones corresponding to regions "H" and "A-F" as shown in Figure 12 were excised and combined, eluted with ether/DME, and dried by vacuum centrifugation.
The extract was enriched in jaLrophanes 2, 3 and 4, pepluane, and the ingenane acetate. The pellet was suspended in 95% ethanol and centrifuged at 10,000 g for 10 minutes. The supernatant (6.0 ml, 10 mg/ml) was distributed into 0.2 ml aliqquots anft 5tored at -20 C. This extract was assayed against MM96L melanoma cell line, and showed high potency, with dendritic cell morphology still evident at 1 in 5 x 106 dilution; this replicated the potency of the crude sap. The extract so prepared was enriched in jatrophanes 2, 3 and 4, pepluane, and the ingenane acetate. Just prior to injection, 20 ul was diluted to 1 ml with RPMI 1640 tissue culture medium containing 5% foetal calf serum for injection of 0.1-0.2 ml. The ethanol solution (10 mg/ml) was absorbed on a cotton bud (0.2-0.4 ml) and used for topical application in mice.
Example 12 Inhibition of Growth of Subcutaneous Implants of Tumour Cells (a) Five 4 week old nude mice were injected s.c. at 4 different sites wit.z 0.1 ml of tissue culture medium containing 2 x 106 MM96L human melanoma cells. The three treated mice were injected on days 1, 2, 3, 5, 6, 7, and 8 with 0.1 ml RPMI medium containing 5% foetal calf serum and 20 pg ethanol extract. In addition, the treated mice received up to four topical applications of approx 5-10 ul of 10 mg/ml ethanol extract or crude undiluted sap.
Two separate sites on each treated mouse received topical treatment with either ethanol extract or crude sap. One mouse received topical treatment on days 12, 13 and 14, and the other two treated mice received topical treatment on days 15, 19, 20 and 22. Tumour volume was measured on day 32.
Prior to the topical applications, injection of' extract had no apparent effect on tumour volume. Following topical application of ethanoi extract there was an overnight change in tumour appearance. The tumours became greyish-black in colour, then developed a hard, lumpy black appearance followed by scab formation. Tumours treated with crude sap showed similar changes a day later. With time, the overall effects of ethanol extract and crude sap were similar, so measurements for r:he topically treated lesions have been combined. On the mice given injection plus topical treatment, tumour volume was reduced by 76%
(p<0.2). One tumour which had been treated with the ethanol extract had completely disappeared, as shown in Figure 13, and eight others were reduced to flat black scabs. The other three treated tumours initially showed similar colour changes and tumour regression, but had regrown following cessation of topical treatment 10 days before the measurements were taken.
(b) Six 4 week old C57 Black (C57B1) mice were injected with 0.1 ml of tissue culture rrLedium containing 105 B16 melanoma cancer cells at two sites on the underbelly. The tumours were allowed to develop for 4 days, and then were subjecced to a regimen oi three injections (20 ug ethanol extract in 0.1 ml RPMI medium containing 5% foetal calf serum (days 1, 2 and 4) and 1 topical treatment (5-10 ul of 10 mg/ml ethanol extract on day 4). 8 days after the first injection the areas of the tumours were measured using a ruler. Treatment reduced the size of the B16 melanoma tumours by 64% (p<0.05) on the three treated mice by comparison with the size of tumours on the three control mice.
The results are sumraarised in Table 18.
~ o =rl O
=~ C- O l0 V V
=,~ 0' 04 o\0 J.~
U
~-o M
+1 +1 N
Ln =N
R~ iA N C=~
~
0 Ln rn co 0 co LO
~ +1 ~ , ~I rn co co Ln F 3 m H
~ 0 a 0 ~ ~-I
O
Ei F
LI-4 ~ tl ~I {i O m m rl i.i 0 m 0 A H
.,~
~="~ Q~ `^ ~
F_: `n N cd aC
0 ai ~ ~
~ `
~r O ~ ..rtiS .Q
lD ri Q) U
O1 -i U tc~
L[1 Example 13 Changes in Gene Expression Induced in a Human Melanoma Cell Line (MM96L) by Purified Extract Human me:_anoma cells of the MM96L cell line, cultured in 150 cm2 plates in RPMI 1640 medium containing 10% foetal calf serum, were incubated with purified extract for 4 hr at 37 C in 5% C02/air. Cells were washed with phosphate buffered saline (PBS), scraped in PBS, pelleted, resuspended in 1 ml PBS, pelleted and taken up in 300 ul NP-40 lysis buffer, left on ice for 15 min, pelleted and the supernatant traated with proteinase K and SDS at 37 C
for 15 min, extrac7-ed with phenol chloroform and the total RNA precipitated by ammonium acetate/ethanol at -20 C
overnight. The Promega mRNA isolation kit was used to isolate mRNA, which was then reverse transcribed in the presence of 33P-labelled dCTP to generate cDNA. The latter was hybridised on a Genome Syscems humarl Gene Discovery Array 1.2 (GDA) according to the manufacturer's instructions. The array was quantitated with a Molecular Dynamics PhosphorImager, and analysed with ImageQant and Excel software.
The ratio of- duplicate spot volumes from treated and untreated cells was calculated, and used to define the level of gene activation (ratio >1) or inhibition (<1).
Backgrounds were typically 500-1000 counts, but were not subtracted; thus the stated ratios will tend to be underestimates of the actual changes.
The array contained cDNA spots from over 18,000 unique sequences, so-called expressed sequence tags (ESTs), of which approximately 3000 were from identifiable expressed genes of human cells. Many EST sequences in the human melanoma cells tested were either up- or down-regulated by the extract treatment. Only changes based on duplicates which had standard deviatioris <30% of the ratio were considered to be biologa.caily significant at this stage. It should also be noted that a relatively short treatment time of 4 hr was used in order to identify the earliest and most critical targets for the agent. It is likely that further, major changes in gene expression, dependent upon the primary response, will occur after this time.
Results from the changes in level of the transcripts of some relevant known genes, considered to be beneficial either directly or indirectly for the control of cancer cells, are summarized in Table 19.
The changes in cell morphology observed in the Examples can be expected to result from the major down-regulation of a number of proteins that birid to actin, a major cytoskeletal protein. An increase in the retinol binding protein may also be involved here, as well as in induction of the differentiated phenotype through increasing the intracellular level of retinoids.
Repair of current and future DNA damage induced by solar UV irradiation may be enhanced by the observed induction of XP repair proteins. In addition, the decrease in GADD45 and ionising radiation resistance protein (DAP3) may be useful in sensitising tumour tissue to radiotherapy.
The latter change is also notable because it is strongly upregulated in MM96L cells by UVB, the cause of skin cancer and melanoma.
A number of molecules relevant to enhancing the immune response were induced, particu:Larly G-CSF. Some of these, such as proteins of the major histocompatability complex (MHC), are considered to be useful attributes for immunotherapy, enhancing killer T-cell activity.
The changes ntost significant for control of cell growth relate to the detected alterations of the G-protein and PKC pathways, and enhancement of proteosome activity.
Intracellular signalling is critical for many cell processes, including proliferation and aiterations in the normal equilibrium of pathways and pathway interactions, such as those mediated by Ras signalling,are likely to have adverse consequences for the cell. The level of induction of the proteosome component LAMP'7-El was among the highest W(? 99/08994 PCT/AU98/00656 found for any gene in the experiment, and would be expected to greatly alter the processing of many proteins via the ubiquitin pathway.
On the basis of the gene expression array data, the compounds of this invention are expected to have activity:
1. In modulating gene expression in the G-protein, PKC and Ras signalling pathways, in a manner that leads to anticancer activity in vivo.
2. In ameliorating damage from solar UV and like agents, by enhancing DNA repair and the immune response, either in the target or effector cells.
3. As an adjuvant to radiotherapy or to therapy with other DNA-damaging agents, on the basis of down-regulation of protective proteins (GADD45 and DAP3).
=~ C- O l0 V V
=,~ 0' 04 o\0 J.~
U
~-o M
+1 +1 N
Ln =N
R~ iA N C=~
~
0 Ln rn co 0 co LO
~ +1 ~ , ~I rn co co Ln F 3 m H
~ 0 a 0 ~ ~-I
O
Ei F
LI-4 ~ tl ~I {i O m m rl i.i 0 m 0 A H
.,~
~="~ Q~ `^ ~
F_: `n N cd aC
0 ai ~ ~
~ `
~r O ~ ..rtiS .Q
lD ri Q) U
O1 -i U tc~
L[1 Example 13 Changes in Gene Expression Induced in a Human Melanoma Cell Line (MM96L) by Purified Extract Human me:_anoma cells of the MM96L cell line, cultured in 150 cm2 plates in RPMI 1640 medium containing 10% foetal calf serum, were incubated with purified extract for 4 hr at 37 C in 5% C02/air. Cells were washed with phosphate buffered saline (PBS), scraped in PBS, pelleted, resuspended in 1 ml PBS, pelleted and taken up in 300 ul NP-40 lysis buffer, left on ice for 15 min, pelleted and the supernatant traated with proteinase K and SDS at 37 C
for 15 min, extrac7-ed with phenol chloroform and the total RNA precipitated by ammonium acetate/ethanol at -20 C
overnight. The Promega mRNA isolation kit was used to isolate mRNA, which was then reverse transcribed in the presence of 33P-labelled dCTP to generate cDNA. The latter was hybridised on a Genome Syscems humarl Gene Discovery Array 1.2 (GDA) according to the manufacturer's instructions. The array was quantitated with a Molecular Dynamics PhosphorImager, and analysed with ImageQant and Excel software.
The ratio of- duplicate spot volumes from treated and untreated cells was calculated, and used to define the level of gene activation (ratio >1) or inhibition (<1).
Backgrounds were typically 500-1000 counts, but were not subtracted; thus the stated ratios will tend to be underestimates of the actual changes.
The array contained cDNA spots from over 18,000 unique sequences, so-called expressed sequence tags (ESTs), of which approximately 3000 were from identifiable expressed genes of human cells. Many EST sequences in the human melanoma cells tested were either up- or down-regulated by the extract treatment. Only changes based on duplicates which had standard deviatioris <30% of the ratio were considered to be biologa.caily significant at this stage. It should also be noted that a relatively short treatment time of 4 hr was used in order to identify the earliest and most critical targets for the agent. It is likely that further, major changes in gene expression, dependent upon the primary response, will occur after this time.
Results from the changes in level of the transcripts of some relevant known genes, considered to be beneficial either directly or indirectly for the control of cancer cells, are summarized in Table 19.
The changes in cell morphology observed in the Examples can be expected to result from the major down-regulation of a number of proteins that birid to actin, a major cytoskeletal protein. An increase in the retinol binding protein may also be involved here, as well as in induction of the differentiated phenotype through increasing the intracellular level of retinoids.
Repair of current and future DNA damage induced by solar UV irradiation may be enhanced by the observed induction of XP repair proteins. In addition, the decrease in GADD45 and ionising radiation resistance protein (DAP3) may be useful in sensitising tumour tissue to radiotherapy.
The latter change is also notable because it is strongly upregulated in MM96L cells by UVB, the cause of skin cancer and melanoma.
A number of molecules relevant to enhancing the immune response were induced, particu:Larly G-CSF. Some of these, such as proteins of the major histocompatability complex (MHC), are considered to be useful attributes for immunotherapy, enhancing killer T-cell activity.
The changes ntost significant for control of cell growth relate to the detected alterations of the G-protein and PKC pathways, and enhancement of proteosome activity.
Intracellular signalling is critical for many cell processes, including proliferation and aiterations in the normal equilibrium of pathways and pathway interactions, such as those mediated by Ras signalling,are likely to have adverse consequences for the cell. The level of induction of the proteosome component LAMP'7-El was among the highest W(? 99/08994 PCT/AU98/00656 found for any gene in the experiment, and would be expected to greatly alter the processing of many proteins via the ubiquitin pathway.
On the basis of the gene expression array data, the compounds of this invention are expected to have activity:
1. In modulating gene expression in the G-protein, PKC and Ras signalling pathways, in a manner that leads to anticancer activity in vivo.
2. In ameliorating damage from solar UV and like agents, by enhancing DNA repair and the immune response, either in the target or effector cells.
3. As an adjuvant to radiotherapy or to therapy with other DNA-damaging agents, on the basis of down-regulation of protective proteins (GADD45 and DAP3).
rn r-;
m a~
14 ro ~
Gl N
1.1 m ~ ai r O ao W O rn ~4 rn 0 a ~ ~~
ro Ai co %,o rn rn c- en r c-1 D M ~--i Lf1 lp N M 10 '1 . . r~ . =
N CV r-I v-i N O N ( N O O
00 01 C) M O N lD
l- U) CO r--I [- N d+ t.C1 r-I
01 C) \D rn I- Lfl CO r- O
N U7 t A rd U ro ~+-+
~ sI M O E[~+
cn .u ~4 r o u ~
w O ( ~ u 0 N
4 tn ~ aQ'i R
u ~4 ~4 ~ ~ ~ a ~ ~ rO ~
x o ~.~ co =~ ~
Q1 ~ 0 ~i o~ m 0 ~ A rti C'1 CA 04 C7 0o Cr- U R4 CA C7 C~
~ 0 ~4 0 ^ ~ Oy-~ y ~ Ul ~ ; a) 0 3 y-'. ?4 U C4 41 ou .~ I (U
~4 C C7 f~, . ~~_ .u -, v ~i 4J 0 ro a~ v U) 'CS H
4.j ~ t31 N !~ Q1 ,c: rts fu cp co f!~ 01 al RS 0) U1 o oi ri rn n rn =.I
d} l~ fT l0 lD 01 l0 m N l0 tD r-1 N
O ~ Ol M rM O ~.O "zv = tD LC) M l0 M
= . . . .
,::r O. c-~ N N N O= O N CD O O O C) w M m '-1 Ql [- t- lf) 00 C) C~ M M O
r'= .-1 Lll CD Ol d+ r^ lD tI'1 CfJ Il=1 Ln '-i lfl q:r ri [- N 01 N .--I r=1 m N l0 01 00 M
N N M It zv N ::I' M ldl m M -I --I H M
E=i E+ E-1 E+ E-+ E-1 E- E+ E-i E~ E+ E+ E-+ E+
õ ~C x' x x x]C x x x x x x x x 0 U ~ v ~ =~ U
v r G1 41 v a ~
ul A 'U C. v E-~ ~ 0 v -i i~ oo ~ ~ -- ~
v ~=t u) =,i M W rtf b a a 0 c~ ~ u ~ Q H ~~
0 a'Ji U) o ~ 0 un =~ =~ r-; =~ ~, .~
(1, N J-1 N ~-I -zli U1 v, C- ri r=I O r-i E0 . t)) tfT a=r-i .u L?: f 4-1 -r-1 r-i O U r-i 04 (1. 0 O 44 U A
{ a a ~ ~ x~~~ + a a t ~ u HE-1 ~
~
to 0 ~ 0 U) ~ ~ ~ s~ ` ~ ~
a ~ a) '~ =~ 0 ` a o 0 - 9, a () i a F Q ~ ~a c~.~ o Example 14 Treatment of a Solar Keratosis in a Human Volunteer Ethics committee approval was obtained from the Queensland Institute of Medical Research for a clinician -supervised trial of use of crude sap of E. peplus for treatment of a facial solar keratosis in a human subject.
Crude extract obtair.ed from Australian-grown plants and stored in 50% glycerol for 2 weeks at -20 C was applied with a cotton bud applicator to the surface of a clinically diagnosed solar keratosis, approximately 5 mm in diameter, on the left temple of the face of a male human volunteer. Approximately 50 ul was delivered to the surface. One day later, a second application was made to the same site. After the first application, no reaction was noted for 4-5 h, whereafter an inflammation reaction occurred at the site and extended to an area of 80-100 mm in diameter. One day later, there was localised swelling, and blister formation at the site of application and on localised patches distal to the area of application, as if new premalignant sites were also targeted. After four days following the first treatment, the swelling subsided and scab formation was evident at the affected sites. After fourteen days, the scabs had sloughed off, leaving new skin underneath. After six weeks, the treated areas still had a pinkish tinge, but there was no sig:a of the original solar keratosis. As a control, a 1 cm' patch of normal skin on the forearm of the same volunteer was similarly treated.
There was localised mild inflammar.ion, which disappeared 7-10 days after treatment.
The strong inflammatory reaction associated with treatment of the solar keratosis could reflect recruitment and proliferation of killer-T cells, as suggested by the results for immurie response obtained from the gene array screen in Example 13, and the observation of in vitro proliferation of T-cells by E. peplus crude sap in Example 15 below. Enhancement of killer-T cell activity is considered to be a key step in destruction of cancer cells by the immune system and may help to explain the recognition and attack of premalignant lesions distal to the site of original treatment.
Example 15 Effect of Crude Sap and Purified Fractions "A" and "H" from TLC on Normal Melanocyte Cell Numbers 12-0-tetradecanoylphorbol-13-acetate (TPA) is essential for the culture of normal melasiocytes in vitro, since these cells grow very poorly without TPA. In a preliminary experiment, E. peplus fractions were added to .medium without added TPA from the start of the experiment.
E. peplus fractions were added to fresh medium, and the cell numbers scored compared co fresh media without E. peplus fractions or TPA. Under this regimen, higher numbers of melanocytes were obtained thari with the "control"cells grown in TPA-deficient rnedium.
Interestingly, the cells in the medium with E. peplus fractions looked healthier than those cells grown in so-called "standard" medium with TPA. Thus E. peplus-derived compounds may provide a supcrior alcerr,ative to the use of TPA as a tool in cell culture.
In a second experiment, normal melanocytes were plated at 5000 cells per well, in RPMI 1640 medium containing 10% foecal calf serum, cholera toxin, antibiotics, and TPA. After 24 hours, che medium was removed from the cells by suction, and rep-laced with fresh medium without added TPA, but with the additions as specified. Cells were scored after a further 10 days of incubation. The results are shown in Table 20. It is evident that even at a 1 in 5,000,000 dilution a cell proliferation effect was noted with crude and purified fractions, in contrast to cell inhibitory effects observed at these concentrations against cancer cell lines as shown in earlier examples. In a separate tesc, in vitro proliferation of T cells was also obtained following treatment of T cells with crude E. peplus sap.
m a~
14 ro ~
Gl N
1.1 m ~ ai r O ao W O rn ~4 rn 0 a ~ ~~
ro Ai co %,o rn rn c- en r c-1 D M ~--i Lf1 lp N M 10 '1 . . r~ . =
N CV r-I v-i N O N ( N O O
00 01 C) M O N lD
l- U) CO r--I [- N d+ t.C1 r-I
01 C) \D rn I- Lfl CO r- O
N U7 t A rd U ro ~+-+
~ sI M O E[~+
cn .u ~4 r o u ~
w O ( ~ u 0 N
4 tn ~ aQ'i R
u ~4 ~4 ~ ~ ~ a ~ ~ rO ~
x o ~.~ co =~ ~
Q1 ~ 0 ~i o~ m 0 ~ A rti C'1 CA 04 C7 0o Cr- U R4 CA C7 C~
~ 0 ~4 0 ^ ~ Oy-~ y ~ Ul ~ ; a) 0 3 y-'. ?4 U C4 41 ou .~ I (U
~4 C C7 f~, . ~~_ .u -, v ~i 4J 0 ro a~ v U) 'CS H
4.j ~ t31 N !~ Q1 ,c: rts fu cp co f!~ 01 al RS 0) U1 o oi ri rn n rn =.I
d} l~ fT l0 lD 01 l0 m N l0 tD r-1 N
O ~ Ol M rM O ~.O "zv = tD LC) M l0 M
= . . . .
,::r O. c-~ N N N O= O N CD O O O C) w M m '-1 Ql [- t- lf) 00 C) C~ M M O
r'= .-1 Lll CD Ol d+ r^ lD tI'1 CfJ Il=1 Ln '-i lfl q:r ri [- N 01 N .--I r=1 m N l0 01 00 M
N N M It zv N ::I' M ldl m M -I --I H M
E=i E+ E-1 E+ E-+ E-1 E- E+ E-i E~ E+ E+ E-+ E+
õ ~C x' x x x]C x x x x x x x x 0 U ~ v ~ =~ U
v r G1 41 v a ~
ul A 'U C. v E-~ ~ 0 v -i i~ oo ~ ~ -- ~
v ~=t u) =,i M W rtf b a a 0 c~ ~ u ~ Q H ~~
0 a'Ji U) o ~ 0 un =~ =~ r-; =~ ~, .~
(1, N J-1 N ~-I -zli U1 v, C- ri r=I O r-i E0 . t)) tfT a=r-i .u L?: f 4-1 -r-1 r-i O U r-i 04 (1. 0 O 44 U A
{ a a ~ ~ x~~~ + a a t ~ u HE-1 ~
~
to 0 ~ 0 U) ~ ~ ~ s~ ` ~ ~
a ~ a) '~ =~ 0 ` a o 0 - 9, a () i a F Q ~ ~a c~.~ o Example 14 Treatment of a Solar Keratosis in a Human Volunteer Ethics committee approval was obtained from the Queensland Institute of Medical Research for a clinician -supervised trial of use of crude sap of E. peplus for treatment of a facial solar keratosis in a human subject.
Crude extract obtair.ed from Australian-grown plants and stored in 50% glycerol for 2 weeks at -20 C was applied with a cotton bud applicator to the surface of a clinically diagnosed solar keratosis, approximately 5 mm in diameter, on the left temple of the face of a male human volunteer. Approximately 50 ul was delivered to the surface. One day later, a second application was made to the same site. After the first application, no reaction was noted for 4-5 h, whereafter an inflammation reaction occurred at the site and extended to an area of 80-100 mm in diameter. One day later, there was localised swelling, and blister formation at the site of application and on localised patches distal to the area of application, as if new premalignant sites were also targeted. After four days following the first treatment, the swelling subsided and scab formation was evident at the affected sites. After fourteen days, the scabs had sloughed off, leaving new skin underneath. After six weeks, the treated areas still had a pinkish tinge, but there was no sig:a of the original solar keratosis. As a control, a 1 cm' patch of normal skin on the forearm of the same volunteer was similarly treated.
There was localised mild inflammar.ion, which disappeared 7-10 days after treatment.
The strong inflammatory reaction associated with treatment of the solar keratosis could reflect recruitment and proliferation of killer-T cells, as suggested by the results for immurie response obtained from the gene array screen in Example 13, and the observation of in vitro proliferation of T-cells by E. peplus crude sap in Example 15 below. Enhancement of killer-T cell activity is considered to be a key step in destruction of cancer cells by the immune system and may help to explain the recognition and attack of premalignant lesions distal to the site of original treatment.
Example 15 Effect of Crude Sap and Purified Fractions "A" and "H" from TLC on Normal Melanocyte Cell Numbers 12-0-tetradecanoylphorbol-13-acetate (TPA) is essential for the culture of normal melasiocytes in vitro, since these cells grow very poorly without TPA. In a preliminary experiment, E. peplus fractions were added to .medium without added TPA from the start of the experiment.
E. peplus fractions were added to fresh medium, and the cell numbers scored compared co fresh media without E. peplus fractions or TPA. Under this regimen, higher numbers of melanocytes were obtained thari with the "control"cells grown in TPA-deficient rnedium.
Interestingly, the cells in the medium with E. peplus fractions looked healthier than those cells grown in so-called "standard" medium with TPA. Thus E. peplus-derived compounds may provide a supcrior alcerr,ative to the use of TPA as a tool in cell culture.
In a second experiment, normal melanocytes were plated at 5000 cells per well, in RPMI 1640 medium containing 10% foecal calf serum, cholera toxin, antibiotics, and TPA. After 24 hours, che medium was removed from the cells by suction, and rep-laced with fresh medium without added TPA, but with the additions as specified. Cells were scored after a further 10 days of incubation. The results are shown in Table 20. It is evident that even at a 1 in 5,000,000 dilution a cell proliferation effect was noted with crude and purified fractions, in contrast to cell inhibitory effects observed at these concentrations against cancer cell lines as shown in earlier examples. In a separate tesc, in vitro proliferation of T cells was also obtained following treatment of T cells with crude E. peplus sap.
+ + + +
o ;{
O + + + +
0 + + +
rq o + + +
O + + + +
Ln ~ If o N
+' +
H ~ + +
rq ~4 O
} +
1l1 + + + +
~4 ~
+ +1 ..~, ~ ~o t7, Ln ~
(a o 1 _ cn Q) o o ? I'; S1! -rl I) 11 1,J ! ^1 ( +
U r `L rl + +
~
a~ W~ O ~ N O.C
4j. =~ U ¾=
e- N. N 41 -.-I rff 1 N=~-! O Q!
rO U s4 JJ u s4 ~4 ~; r-+
75 . ~ T ~! -, ) ro o; s4s4 a, 0 >4 (1) rt~ U
vt cn V~ tt, . T ~.
Lr, Since both normal melanocytes and T-cells were induced to proliferate by fractions from E. peplus sap, this agent may have wide application as a cell proliferation agent for normal cells, either in vivo or in vitro, in any medical condition where regeneration of normal cells would be advantageous, including but not limited to a) multiplication of skin cells (keratinocytes) for rapid wound healing in trauma cases and after surgery, and in recovery from burns.
b) multiplication of pancreatic islet cells for implantation c) multiplication of T-cells and other cells of the immune system. It is interesting to note that the expansion of action past the point of application in the human volunteer trial on treatment of solar keratosis may be explained by a recruitment of natural killer-T cells to the regiorl of application.
d) regeneration of aged or necrotic tissue from liver, ki(Lzey, colon, lung and eye.
e) multiplication of hosc tissue as an alternative to organ transplantation Example 16 Effect of betaines on nialignant melanoma MM96L cell numbers Betaiiies of different types were solubilised in sterile Mi11iQTM water to a final concentration of 1 mg/ml, and diluted into 0.1 ml tissue culture medium containing 5000 MM96L cells as described previously. Cells were scored after 4 days incubation. The results are shown in Table 21.
Whereas most betaines tested had no effect on cell numbers, !3-alanine beta:ine hydrochloride (homobetaine) depressed cell numbers at a iinal concentration of 20 pg/ml, and the ceils had a dendritic appearance. t-4 hydroxy N,N-dimethyl proline also irihibited cell numbers at a final concentration of 20 ug/ml; however, the cell morphology changed to that of polydendritic forms, the significance of which is unknown.
It is envisaged that f3-alanine betaine hydrochloride (homobetaine) may be a suitable formulation agent for E. peplus crude sap or its purified active principles, including ingenol, pepluane, and jatrophanes 1-6, either separately or in -ombination. This could be used for topical application against premalignant skin lesions at low dilutions of F. peplus principle(s), or formulated as an ariticancer drug with higher concentrations of E. peplus principle(s). It has been suggested that betaines per= se are useful as anti-cancer agents; see for example U.S. Patent No. 5,545,667 by Wiersema et al.
Because of their surfactant properties,.betaines are widely used as formulatiozl ingredients in cosmetics.
Due to their zwitterion properties, betaines could also assist transport of other ingredients into the deeper layers of the skin. A betaine to be used in a skin cosmetic preparation along with very dilute extracts of E.
peplus sap or purified fractions derived therefrom, such as jatrophanes, pepluane, paraliane, or irigenane, separately or in combination, should desirably have complementary properties. Of all the betaines tested, including glycine betaine, only fs-alanine betaine hydrochloride (homobetaine) had a phenotype reversal effect, albeit modest, as compared to E. peplus sap and fractioals.
o ;{
O + + + +
0 + + +
rq o + + +
O + + + +
Ln ~ If o N
+' +
H ~ + +
rq ~4 O
} +
1l1 + + + +
~4 ~
+ +1 ..~, ~ ~o t7, Ln ~
(a o 1 _ cn Q) o o ? I'; S1! -rl I) 11 1,J ! ^1 ( +
U r `L rl + +
~
a~ W~ O ~ N O.C
4j. =~ U ¾=
e- N. N 41 -.-I rff 1 N=~-! O Q!
rO U s4 JJ u s4 ~4 ~; r-+
75 . ~ T ~! -, ) ro o; s4s4 a, 0 >4 (1) rt~ U
vt cn V~ tt, . T ~.
Lr, Since both normal melanocytes and T-cells were induced to proliferate by fractions from E. peplus sap, this agent may have wide application as a cell proliferation agent for normal cells, either in vivo or in vitro, in any medical condition where regeneration of normal cells would be advantageous, including but not limited to a) multiplication of skin cells (keratinocytes) for rapid wound healing in trauma cases and after surgery, and in recovery from burns.
b) multiplication of pancreatic islet cells for implantation c) multiplication of T-cells and other cells of the immune system. It is interesting to note that the expansion of action past the point of application in the human volunteer trial on treatment of solar keratosis may be explained by a recruitment of natural killer-T cells to the regiorl of application.
d) regeneration of aged or necrotic tissue from liver, ki(Lzey, colon, lung and eye.
e) multiplication of hosc tissue as an alternative to organ transplantation Example 16 Effect of betaines on nialignant melanoma MM96L cell numbers Betaiiies of different types were solubilised in sterile Mi11iQTM water to a final concentration of 1 mg/ml, and diluted into 0.1 ml tissue culture medium containing 5000 MM96L cells as described previously. Cells were scored after 4 days incubation. The results are shown in Table 21.
Whereas most betaines tested had no effect on cell numbers, !3-alanine beta:ine hydrochloride (homobetaine) depressed cell numbers at a iinal concentration of 20 pg/ml, and the ceils had a dendritic appearance. t-4 hydroxy N,N-dimethyl proline also irihibited cell numbers at a final concentration of 20 ug/ml; however, the cell morphology changed to that of polydendritic forms, the significance of which is unknown.
It is envisaged that f3-alanine betaine hydrochloride (homobetaine) may be a suitable formulation agent for E. peplus crude sap or its purified active principles, including ingenol, pepluane, and jatrophanes 1-6, either separately or in -ombination. This could be used for topical application against premalignant skin lesions at low dilutions of F. peplus principle(s), or formulated as an ariticancer drug with higher concentrations of E. peplus principle(s). It has been suggested that betaines per= se are useful as anti-cancer agents; see for example U.S. Patent No. 5,545,667 by Wiersema et al.
Because of their surfactant properties,.betaines are widely used as formulatiozl ingredients in cosmetics.
Due to their zwitterion properties, betaines could also assist transport of other ingredients into the deeper layers of the skin. A betaine to be used in a skin cosmetic preparation along with very dilute extracts of E.
peplus sap or purified fractions derived therefrom, such as jatrophanes, pepluane, paraliane, or irigenane, separately or in combination, should desirably have complementary properties. Of all the betaines tested, including glycine betaine, only fs-alanine betaine hydrochloride (homobetaine) had a phenotype reversal effect, albeit modest, as compared to E. peplus sap and fractioals.
O + + + + + + +
= + + + + + + +
Il1 + + + + + + +
+ + + + + + +
lCl + + + t + t +
\ + + t + t ~=i 0 (N In + + + + 7~ Iro +I + + + + + +
E
4-+ 44 -ri H
! v! ~ o 0 o -'"4 r-! =rI ,-q $04 r-i ,-=~
ry r; rti ~ - 0 .-i A I O ~ O u ~- >+ .c: (1) Ik ! O ~ f~N a ~ O Q+ ~ U
rC7 O U ~
~4 41 44 ~ ~ O
-i Q) ~ r('1 I = ~-I Q) Pa tll y~ f:
~4 O O
04 '~ r U
co 0 J O? ~ II p z1 a 0 =~ a) 0 ~11 Rf Oa~ S-! ~+
~ ~-l k 0 L4 !--3 4J 4 tn ro r+ +
N >t Z7 'o ciS ''O ?S (t 0 4 ?, ;~ A ?, ,, ,L~
.uI c c 4 T O' C TJ N
( D 1 a) U v w >r, ~ v U1 , Ci N M Ul 1~ O d' Q) ;4 r I ! ! ~! 1 ~I td 4: ! ~.I! `o U
v1 '! bi iJ i~ 4-4 .u Q ~? J. J 4-4 'ti U. v1 ~
~
WO 99/08994 PCT/AU98/0065,f`^.
= + + + + + + +
Il1 + + + + + + +
+ + + + + + +
lCl + + + t + t +
\ + + t + t ~=i 0 (N In + + + + 7~ Iro +I + + + + + +
E
4-+ 44 -ri H
! v! ~ o 0 o -'"4 r-! =rI ,-q $04 r-i ,-=~
ry r; rti ~ - 0 .-i A I O ~ O u ~- >+ .c: (1) Ik ! O ~ f~N a ~ O Q+ ~ U
rC7 O U ~
~4 41 44 ~ ~ O
-i Q) ~ r('1 I = ~-I Q) Pa tll y~ f:
~4 O O
04 '~ r U
co 0 J O? ~ II p z1 a 0 =~ a) 0 ~11 Rf Oa~ S-! ~+
~ ~-l k 0 L4 !--3 4J 4 tn ro r+ +
N >t Z7 'o ciS ''O ?S (t 0 4 ?, ;~ A ?, ,, ,L~
.uI c c 4 T O' C TJ N
( D 1 a) U v w >r, ~ v U1 , Ci N M Ul 1~ O d' Q) ;4 r I ! ! ~! 1 ~I td 4: ! ~.I! `o U
v1 '! bi iJ i~ 4-4 .u Q ~? J. J 4-4 'ti U. v1 ~
~
WO 99/08994 PCT/AU98/0065,f`^.
It :vill be aonarent to t.~e oerson skill ed in the art that while the invent_on has bc= : descr=:bed ir_ some detail for the pur-poses o= clarity a~_-~d znderstandir_g, vari ous modifications and alterations zo the embod_mer_ts and methods described here_n may be made without denarzing from the scope of the inventive conc=z>t disclosed in this snecification.
References cited herein are li sted on the following pages.
, --- -REFERENCES
Beljanski M and Crochet, S.
Int. J. Oncol., 1996 8 1143-1148 Belkin, M. and Fitzgerald, D.B.
J. Natl. Cancer Inst., 1952 :.> 139 Bosch, R.R., Patel, A.M., Van Emst-de Vries, S.E., Smeets, R.L., De Pont, J.J., Willems, P.H., Pont, J.J.
Eur J Pharmacol 1998 346 345-351 Djafarzadeh, S.
Exp Cell Res. 1997 Nov 1; 236(2) 1997, 236 427-435 Eke, T.
Eye, 1994 8 694-696 Evans, F.J. and Kinghorn, A,D.
Botanical Journal of the Linnean Society, 1977 74 23-35 Evans, I.A. and Osman, M.A.
Nature, 1974 250 348 Falsone G et ai, Farmaco., 1994 49 167-174 Fatope, M.O. et al J. Med. Chem., 1996 39 1005-1008 Francis, D.B., Hart, L.V., Wilson, P.R. and Beardmore, G.L.
Med J. Aust., 1989 6 541-542 Galvez, J. et a1 Planta Med., 1993 59 333-336 Gundidza, M. et al Cent. Afr. J. Med., 1992 38 444-447 Guo, Z. et al Chung Kuo Chung Yao Tsa Chih, 1995 20 744-745 Hartwell, J.L.
Lloydia 1969 32 153 Hecker, "Cocarcinogens from Euphorbiaceae and Thymeleaceae"
in "Symposium on Pharmacognosy and Phytochemistry", 147-165 (Wagner et al, eds., Springer Verlag 1970).
Imai, S.
Anticancer Research, 1994 14 933-936 Jakupovic, J., Morgenstern, T., Bitner, M. and Silva, M.
Phytochemistry, 1998a 47 1601-1609 Jakupovic, J., Jeske, F., Morgenstern, T., Tsichritzis, F., Marco, J.A. and Berendsohn, W.
Phytochemistry, 1998b 47 1583-1600 Jakupovic, J., Morgenstern, T., Marco, J.A. and Berendsohn, W.
Phytochemistry, 1998c 47 1611-10619 Jurberg, P. et al Mem. Inst. Oswaldo Cruz, 1995 90 191-194 Kanai, M., Goke, M., Tsunekawa, S. and Podolsky, D.K.
J Biol Chem 1997 272 6621-6628 Leung, A.Y. and Foster, A.
Encyclopedia of Common Natural Ingredients Used Food, Drugs and Cosmetics, John Wiley & Sons, inc. 2nd edition, 1996 Li, M., Vemulapalli, R., Ullah, A., Izu, L., Duffey, M.E.
and Lance, P.
Am. J. Physiol., 1998 274 G599-G606 Liu. Y et al Chung Kuo Chung His Chieh Ho Tsa Chih, 1994 14 282-284 Marco, J. A., Sanz-Cervera, J. F., Yuste, A., Jakupovic, J.
and Jeske, F.
Phytochemistry, 1998 47 1621-1630 Matsumoto, T. et al Planta Med., 1992 58 255-258 Maynard, K. and Parsons, P.G.
Cancer Res, 1986 46 5009-5013 Mimnaugh, E.G., Chen, H.Y., Davie, J.R., Celis, J.E. and Neckers, L.
Biochemistry 1997 36 14418-14429 Moulin, A. et al Proc. Natl. Acad. Sci. USA, 1994 91 11328-11332 Oksuz, S. et a1.
Phytochemistry, 1996 42 473-478 Pearn, J.
Med. J. Aust., 1987 147 568-572 Perozzi, G., Barila, D., Plateroti, M., Sarabuy, Y., Nobili, F. and Gaetani, S.
Z. Ernahrungsw-iss, 1998 37 29-34 Pise-Masison, C.A., Radonovich, M., Sakaguchi, K., Appella, E. and Brady, J.N.
J. Virol., 1998 72 6348-6355 Stavric, B. and Stoltz, D.R.
Food Cosmet. Toxicol., 1976 14 141 Stirpe, F. et al Biochim. Biophys. Acta, 1993 1158 33-39 Sussman, L.A.E. and Liggins, D.F.
Australian and New Zealand Journal of Surgery, 1996 66 Vijaya, K. et al J. Ethnopharmacol., 1995 49 115-118 Weedon, D. and Chick, J.
Med. J. Aust., 1976 928 1-24 Yoshida, T. et al Chem. Pharm. Bull. (Tokyo), 1994 42 1803-1807
References cited herein are li sted on the following pages.
, --- -REFERENCES
Beljanski M and Crochet, S.
Int. J. Oncol., 1996 8 1143-1148 Belkin, M. and Fitzgerald, D.B.
J. Natl. Cancer Inst., 1952 :.> 139 Bosch, R.R., Patel, A.M., Van Emst-de Vries, S.E., Smeets, R.L., De Pont, J.J., Willems, P.H., Pont, J.J.
Eur J Pharmacol 1998 346 345-351 Djafarzadeh, S.
Exp Cell Res. 1997 Nov 1; 236(2) 1997, 236 427-435 Eke, T.
Eye, 1994 8 694-696 Evans, F.J. and Kinghorn, A,D.
Botanical Journal of the Linnean Society, 1977 74 23-35 Evans, I.A. and Osman, M.A.
Nature, 1974 250 348 Falsone G et ai, Farmaco., 1994 49 167-174 Fatope, M.O. et al J. Med. Chem., 1996 39 1005-1008 Francis, D.B., Hart, L.V., Wilson, P.R. and Beardmore, G.L.
Med J. Aust., 1989 6 541-542 Galvez, J. et a1 Planta Med., 1993 59 333-336 Gundidza, M. et al Cent. Afr. J. Med., 1992 38 444-447 Guo, Z. et al Chung Kuo Chung Yao Tsa Chih, 1995 20 744-745 Hartwell, J.L.
Lloydia 1969 32 153 Hecker, "Cocarcinogens from Euphorbiaceae and Thymeleaceae"
in "Symposium on Pharmacognosy and Phytochemistry", 147-165 (Wagner et al, eds., Springer Verlag 1970).
Imai, S.
Anticancer Research, 1994 14 933-936 Jakupovic, J., Morgenstern, T., Bitner, M. and Silva, M.
Phytochemistry, 1998a 47 1601-1609 Jakupovic, J., Jeske, F., Morgenstern, T., Tsichritzis, F., Marco, J.A. and Berendsohn, W.
Phytochemistry, 1998b 47 1583-1600 Jakupovic, J., Morgenstern, T., Marco, J.A. and Berendsohn, W.
Phytochemistry, 1998c 47 1611-10619 Jurberg, P. et al Mem. Inst. Oswaldo Cruz, 1995 90 191-194 Kanai, M., Goke, M., Tsunekawa, S. and Podolsky, D.K.
J Biol Chem 1997 272 6621-6628 Leung, A.Y. and Foster, A.
Encyclopedia of Common Natural Ingredients Used Food, Drugs and Cosmetics, John Wiley & Sons, inc. 2nd edition, 1996 Li, M., Vemulapalli, R., Ullah, A., Izu, L., Duffey, M.E.
and Lance, P.
Am. J. Physiol., 1998 274 G599-G606 Liu. Y et al Chung Kuo Chung His Chieh Ho Tsa Chih, 1994 14 282-284 Marco, J. A., Sanz-Cervera, J. F., Yuste, A., Jakupovic, J.
and Jeske, F.
Phytochemistry, 1998 47 1621-1630 Matsumoto, T. et al Planta Med., 1992 58 255-258 Maynard, K. and Parsons, P.G.
Cancer Res, 1986 46 5009-5013 Mimnaugh, E.G., Chen, H.Y., Davie, J.R., Celis, J.E. and Neckers, L.
Biochemistry 1997 36 14418-14429 Moulin, A. et al Proc. Natl. Acad. Sci. USA, 1994 91 11328-11332 Oksuz, S. et a1.
Phytochemistry, 1996 42 473-478 Pearn, J.
Med. J. Aust., 1987 147 568-572 Perozzi, G., Barila, D., Plateroti, M., Sarabuy, Y., Nobili, F. and Gaetani, S.
Z. Ernahrungsw-iss, 1998 37 29-34 Pise-Masison, C.A., Radonovich, M., Sakaguchi, K., Appella, E. and Brady, J.N.
J. Virol., 1998 72 6348-6355 Stavric, B. and Stoltz, D.R.
Food Cosmet. Toxicol., 1976 14 141 Stirpe, F. et al Biochim. Biophys. Acta, 1993 1158 33-39 Sussman, L.A.E. and Liggins, D.F.
Australian and New Zealand Journal of Surgery, 1996 66 Vijaya, K. et al J. Ethnopharmacol., 1995 49 115-118 Weedon, D. and Chick, J.
Med. J. Aust., 1976 928 1-24 Yoshida, T. et al Chem. Pharm. Bull. (Tokyo), 1994 42 1803-1807
Claims (12)
1. The use of at least one compound selected from the group consisting of an angeloyl-substituted ingenane obtained from the sap of Euphorbia peplus and an active derivative of an angeloyl-substituted ingenane obtained from the sap of Euphorbia peplus, and pharmaceutically acceptable salts thereof, wherein said active derivative exhibits the same activity as said angeloyl-substituted ingenane, for treating a subject with skin cancer.
2. The use of claim 1, wherein the derivative of an angeloyl-substituted ingenane obtained from the sap of Euphorbia peplus is an acetylated derivative.
3. The use of claim 1, wherein the at least one compound is selected from the group consisting of a 20-O-acetyl-ingenol-3-angelate and an ester derivative of a 20-O-acetyl-ingenol-3-angelate.
4. The use of claim 1, wherein the at least one compound is selected from a group consisting of a pharmaceutically acceptable salt of a 20-O-acetyl-ingenol-3-angelate or a 20-O-acetyl-ingenol-3-angelate ester derivative.
5. The use of claim 1, wherein the at least one compound is obtained from the sap of Euphorbia peplus by subjecting the sap to aqueous extraction and collecting the aqueous fraction.
6. The use of claim 1, wherein the compound is obtained from the sap of Euphorbia peplus by the process of extracting said sap with 95% v/v ethanol, discarding a soluble fraction and retaining a solid fraction.
7. The use of any one of claims 1 through 6, wherein the skin cancer is a malignant melanoma.
8. The use of any one of claims 1 through 6, wherein the skin cancer is a Merkel cell carcinoma.
9. The use of any one of claims 1 through 6, wherein the skin cancer is a squamous cell carcinoma.
10. The use of any one of claims 1 through 6, wherein the skin cancer is a basal cell carcinoma.
11. The use of any one of claims 1 through 6, wherein the skin cancer is a solar keratosis.
12. The use of any one of claims 1 through 6, wherein the subject is human.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| AUPO8640 | 1997-08-19 | ||
| AUPO8640A AUPO864097A0 (en) | 1997-08-19 | 1997-08-19 | Anti-cancer compounds |
| PCT/AU1998/000656 WO1999008994A1 (en) | 1997-08-19 | 1998-08-19 | Anti-cancer compounds |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CA2301082A1 CA2301082A1 (en) | 1999-02-25 |
| CA2301082C true CA2301082C (en) | 2009-02-03 |
Family
ID=3802927
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002301082A Expired - Lifetime CA2301082C (en) | 1997-08-19 | 1998-08-19 | Anti-cancer compounds |
Country Status (17)
| Country | Link |
|---|---|
| US (4) | US6432452B1 (en) |
| EP (1) | EP1015413B1 (en) |
| JP (3) | JP2001515059A (en) |
| CN (1) | CN1266421B (en) |
| AT (1) | ATE397580T1 (en) |
| AU (1) | AUPO864097A0 (en) |
| BE (1) | BE2013C026I2 (en) |
| BR (1) | BR9811327A (en) |
| CA (1) | CA2301082C (en) |
| CY (2) | CY1108303T1 (en) |
| DE (1) | DE69839586D1 (en) |
| DK (1) | DK1015413T3 (en) |
| ES (1) | ES2308810T3 (en) |
| HU (2) | HU228862B1 (en) |
| LU (1) | LU92185I2 (en) |
| PT (1) | PT1015413E (en) |
| WO (1) | WO1999008994A1 (en) |
Families Citing this family (52)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| AUPO864097A0 (en) * | 1997-08-19 | 1997-09-11 | Peplin Pty Ltd | Anti-cancer compounds |
| US6822267B1 (en) * | 1997-08-20 | 2004-11-23 | Advantest Corporation | Signal transmission circuit, CMOS semiconductor device, and circuit board |
| US7078434B1 (en) * | 1999-08-12 | 2006-07-18 | Societe De Conseils De Recherches Et D'applications Scientifiques Sas | Use of Ginkgo extract |
| AU748542B2 (en) * | 2000-06-07 | 2002-06-06 | Leo Laboratories Limited | Therapeutic agents - III |
| AUPQ801700A0 (en) * | 2000-06-07 | 2000-06-29 | Peplin Research Pty Ltd | Enzyme and viral activation |
| AUPQ923100A0 (en) * | 2000-08-07 | 2000-08-31 | Peplin Research Pty Ltd | Treatment of prostate cancer |
| US6923993B2 (en) * | 2001-12-12 | 2005-08-02 | Nicholas J. Donato | Process of isolating extract from the Euphorbia obesa plant and methods for using the same |
| MY139563A (en) * | 2002-09-04 | 2009-10-30 | Bristol Myers Squibb Co | Heterocyclic aromatic compounds useful as growth hormone secretagogues |
| US7154002B1 (en) | 2002-10-08 | 2006-12-26 | Takeda San Diego, Inc. | Histone deacetylase inhibitors |
| US7250514B1 (en) | 2002-10-21 | 2007-07-31 | Takeda San Diego, Inc. | Histone deacetylase inhibitors |
| JP2006520796A (en) | 2003-03-17 | 2006-09-14 | タケダ サン ディエゴ インコーポレイテッド | Histone deacetylase inhibitor |
| EP1673450B1 (en) | 2003-10-14 | 2010-04-28 | Baxter International Inc. | Vitamin k epoxide recycling polypeptide vkorc1, a therapeutic target of coumarin and their derivatives |
| US20050137234A1 (en) * | 2003-12-19 | 2005-06-23 | Syrrx, Inc. | Histone deacetylase inhibitors |
| AU2005214979B2 (en) * | 2004-02-17 | 2009-09-10 | The Uab Research Foundation | Cytotoxin compound and method of isolation |
| WO2005084712A2 (en) * | 2004-02-27 | 2005-09-15 | Antisense Pharma Gmbh | Use of an oligonucleotide or its active derivative for the preparation of a pharmaceutical composition for inhibiting the formation of metastases in cancer treatment |
| DE102004044428A1 (en) * | 2004-09-14 | 2006-03-30 | Toximed Gmbh | Process and pharmaceutical agent for the control of plasmodia |
| US8106092B2 (en) | 2004-12-13 | 2012-01-31 | Leo Laboratories Limited | Treatment of solid cancers |
| AU2005316185B2 (en) * | 2004-12-13 | 2012-04-12 | Leo Laboratories Limited | Treatment of solid cancers |
| WO2006066133A2 (en) | 2004-12-16 | 2006-06-22 | Takeda San Diego, Inc. | Histone deacetylase inhibitors |
| WO2006122319A2 (en) | 2005-05-11 | 2006-11-16 | Takeda San Diego, Inc. | Histone deacetylase inhibitors |
| US20090035403A2 (en) * | 2005-06-16 | 2009-02-05 | Mmi Corporation | Novel anticancer agent, methods for obtaining the same and pharmaceutical compositions thereof |
| US7655620B2 (en) * | 2005-07-07 | 2010-02-02 | Cancure Laboratories, Llc | Use of one or more metal carriers to selectively kill mammalian cells |
| WO2007011626A2 (en) | 2005-07-14 | 2007-01-25 | Takeda San Diego, Inc. | Histone deacetylase inhibitors |
| US9597311B2 (en) * | 2005-09-27 | 2017-03-21 | Robert Benson Aylor | Suppression and prevention of tumors |
| CA2629899A1 (en) * | 2005-11-25 | 2007-05-31 | Peplin Research Pty Ltd | Methods for wound healing |
| WO2007065925A2 (en) * | 2005-12-07 | 2007-06-14 | Toximed Gmbh | Composition for treatment of melanomas and skin disorders and cosmetic care product |
| GB0525680D0 (en) | 2005-12-16 | 2006-01-25 | Peplin Ltd | Therapeutic compositions |
| JP2009525955A (en) * | 2006-01-13 | 2009-07-16 | タケダ サン ディエゴ インコーポレイテッド | Histone deacetylase inhibitor |
| US20080069809A1 (en) * | 2006-04-20 | 2008-03-20 | Ogbourne Steven M | Compositions and methods for the diagnosis and treatment of cancer |
| US20080207738A1 (en) * | 2007-02-28 | 2008-08-28 | Cancure Laboratories, Llc | Drug combinations to treat drug resistant tumors |
| TWI389699B (en) * | 2009-02-13 | 2013-03-21 | Univ Kaohsiung Medical | Ethanol extract of antrodia camphorata for inducing apoptosis and preparation method thereof |
| RU2491050C2 (en) * | 2009-02-13 | 2013-08-27 | Лео Лэборетериз Лимитед | Skin treatment |
| PT2558435T (en) | 2010-04-16 | 2017-07-24 | Leo Pharma As | Orthorhombic crystalline ingenol mebutate |
| WO2011139172A1 (en) * | 2010-05-06 | 2011-11-10 | Goran Milosavljevic | Diterpene compounds with antineoplastic activities and pharmaceutical compositions comprising same |
| EP2632459B1 (en) * | 2010-10-25 | 2017-08-16 | Niiki Pharma Inc. | Method of treating neuroendocrine tumors |
| US9402823B2 (en) | 2010-12-17 | 2016-08-02 | Leo Laboratories Limited | Ingenols for treating seborrheic keratosis |
| CN103402977B (en) | 2010-12-22 | 2016-01-20 | 利奥实验室有限公司 | Ingenol-3-acylate III and ingenol-3-carbamate |
| EP2655311A1 (en) | 2010-12-22 | 2013-10-30 | Leo Laboratories Limited | Ingenol-3-acylates i |
| BR112013015859A2 (en) | 2010-12-22 | 2018-11-21 | Leo Laboratories Ltd | compound, use of a compound, methods of prevention, treatment, amelioration or prophylaxis of physiological disorders or diseases, and treatment or amelioration of cosmetic indications, and, pharmaceutical composition |
| US8858953B2 (en) | 2011-05-09 | 2014-10-14 | Yu-Hwa Peter Sheng | Herbal composition for treating cancer |
| WO2012176015A1 (en) | 2011-06-24 | 2012-12-27 | Leo Pharma A/S | Methods for treating uv-damaged skin and scc tumors and for removing tattoos with topical ingenol mebutate |
| KR101374760B1 (en) * | 2011-10-26 | 2014-03-17 | 한국생명공학연구원 | Phorbol type diterpene compound and a pharmaceutical composition for treatment and prevention of virus infection comprising the same |
| CN104411685B (en) | 2012-06-26 | 2017-03-29 | 利奥实验室有限公司 | 3 O heteroaryl ingenols |
| CN103655674A (en) * | 2012-09-11 | 2014-03-26 | 清华大学深圳研究生院 | Euphorbia esula extract as well as preparation method and application thereof |
| KR101578404B1 (en) | 2014-03-18 | 2015-12-18 | 원광대학교 산학협력단 | Composition for prevention or treatment of cancer containing extract or fraction of Euphorbia L. |
| US9948261B2 (en) * | 2014-11-20 | 2018-04-17 | Tymphany Hk Limited | Method and apparatus to equalize acoustic response of a speaker system using multi-rate FIR and all-pass IIR filters |
| CN105255476B (en) * | 2015-10-01 | 2017-10-13 | 申俊 | Based on biological color development technology to serve the storage tank of Internet of Things |
| CN107101998A (en) * | 2015-10-01 | 2017-08-29 | 钱秀英 | Biological color development agent for judging the time |
| US9758786B2 (en) | 2016-02-09 | 2017-09-12 | Autotelic, Llc | Compositions and methods for treating pancreatic cancer |
| US10722484B2 (en) | 2016-03-09 | 2020-07-28 | K-Gen, Inc. | Methods of cancer treatment |
| EP3510052A4 (en) | 2016-09-02 | 2020-06-17 | Thailand Center of Excellence for Life Sciences | Method for preparing an extract of hevea latex and composition thereof |
| CN110663685B (en) * | 2019-10-23 | 2021-10-12 | 扬州大学 | Mesoporous silica supported PPTE nano pesticide preparation |
Family Cites Families (32)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| DE2902506A1 (en) | 1979-01-23 | 1980-07-24 | Deutsches Krebsforsch | USE OF DITERPENAL ALCOHOLS AND DERIVATIVES THEREOF AS AN ANTINEOPLASTIC AGENT, OR ONLY LITTLE IRRITATING AND / OR PROMOVING |
| JPS5813571A (en) * | 1981-07-14 | 1983-01-26 | Sagami Chem Res Center | Dihydrofuran derivative and its preparation |
| US4418064A (en) * | 1982-09-29 | 1983-11-29 | The United States Of America As Represented By The Secretary Of Agriculture | Chemotherapeutically active maytansinoids: treflorine, trenudine, and N-methyltrenudone |
| US4560774A (en) | 1982-11-17 | 1985-12-24 | Arizona State University | Macrocyclic lactones |
| US5886019A (en) | 1986-06-11 | 1999-03-23 | Procyon Pharmaceuticals, Inc. | Protein kinase C modulators. F. |
| US5891870A (en) | 1986-06-11 | 1999-04-06 | Procyon Pharmaceuticals, Inc. | Protein kinase C modulators Q |
| US5750568A (en) | 1986-06-11 | 1998-05-12 | Procyon Pharmaceuticals, Inc. | Protein kinase C Modulators. L. |
| US5886017A (en) | 1986-06-11 | 1999-03-23 | Procyon Pharmaceuticals, Inc. | Protein kinase C modulators. E. |
| US5145842A (en) | 1986-06-11 | 1992-09-08 | Alder Research Center Limited Partnership | Protein kinase c. modulators. d. |
| US5891906A (en) | 1986-06-11 | 1999-04-06 | Procyon Pharmaceuticals, Inc. | Polyacetate-derived phorboids having anti-inflammatory and other uses |
| US5643948A (en) | 1986-06-11 | 1997-07-01 | Procyon Pharmaceuticals, Inc. | Protein kinase C modulators. K. |
| IL82811A0 (en) | 1986-06-11 | 1987-12-20 | Alder Res Center Corp | Anti-inflammatory compositions containing methanol derivatives and novel compounds contained therein |
| US5716968A (en) | 1986-06-11 | 1998-02-10 | Procyon Pharmaceuticals, Inc. | Protein kinase C modulators. H. |
| DE3805965A1 (en) * | 1988-02-25 | 1989-09-07 | Tamas Geb Szenasi Eszter | USE OF THE EUPHORBIA HIRTA L. PLANT AND ITS EXTRACTS AND ITS ACTIVE SUBSTANCES |
| DE4102054A1 (en) * | 1991-01-24 | 1992-07-30 | Geb Szenasi Tamas | Euphorbia hirta L. to increase immunity - e.g. against influenza, winter colds and AIDS and as antifungal agent to treat open wounds |
| CN1047084C (en) | 1993-03-30 | 1999-12-08 | 刘振宪 | Oral liquid for treatment of esophagus disease and its preparing method |
| US6593371B1 (en) | 1993-05-19 | 2003-07-15 | Jeff J. Staggs | Treatment for wart and related disorders |
| CN1048164C (en) | 1993-08-24 | 2000-01-12 | 吴雪姣 | Oral liquid |
| JP2913451B2 (en) | 1994-06-22 | 1999-06-28 | 株式会社イナックス | Height adjustment structure of waterproof pan |
| JPH08245505A (en) * | 1994-09-09 | 1996-09-24 | Tosoh Corp | Diterpene derivative, its production and antitumor agent containing the same as active ingredient |
| JPH08176002A (en) * | 1994-12-27 | 1996-07-09 | Kao Corp | Cell-anchoring inhibitor |
| CN1070372C (en) | 1995-02-15 | 2001-09-05 | 赵国强 | Powerful anticancer plaster and its preparing method |
| WO1997015575A1 (en) | 1995-10-27 | 1997-05-01 | Procyon Pharmaceuticals, Inc. | Protein kinase c modulators. y. |
| CN1058620C (en) * | 1995-11-12 | 2000-11-22 | 卢颖 | Yingfengaidi medicine and its production process |
| JPH08268961A (en) * | 1996-02-28 | 1996-10-15 | Procyon Pharmaceut Inc | Anti-inflammatory composition |
| US5932613A (en) * | 1996-07-03 | 1999-08-03 | Millennium Pharmaceuticals, Inc. | Anticancer agents |
| AUPO864097A0 (en) * | 1997-08-19 | 1997-09-11 | Peplin Pty Ltd | Anti-cancer compounds |
| JP2001139468A (en) | 1999-11-11 | 2001-05-22 | Lead Chemical Co Ltd | Phorbol derivative having antiviral action |
| US6444555B2 (en) * | 1999-12-07 | 2002-09-03 | Advanced Micro Devices, Inc. | Method for establishing ultra-thin gate insulator using anneal in ammonia |
| AUPQ801700A0 (en) | 2000-06-07 | 2000-06-29 | Peplin Research Pty Ltd | Enzyme and viral activation |
| AUPQ923100A0 (en) | 2000-08-07 | 2000-08-31 | Peplin Research Pty Ltd | Treatment of prostate cancer |
| US20030185168A1 (en) * | 2002-03-28 | 2003-10-02 | Yu-Wei Tung | Topology of frequency converting blocks of wireless lan access point |
-
1997
- 1997-08-19 AU AUPO8640A patent/AUPO864097A0/en not_active Abandoned
-
1998
- 1998-08-19 BR BR9811327-5A patent/BR9811327A/en not_active Application Discontinuation
- 1998-08-19 CA CA002301082A patent/CA2301082C/en not_active Expired - Lifetime
- 1998-08-19 AT AT98938534T patent/ATE397580T1/en active
- 1998-08-19 ES ES98938534T patent/ES2308810T3/en not_active Expired - Lifetime
- 1998-08-19 US US09/486,199 patent/US6432452B1/en not_active Expired - Lifetime
- 1998-08-19 CN CN98807751.5A patent/CN1266421B/en not_active Expired - Lifetime
- 1998-08-19 WO PCT/AU1998/000656 patent/WO1999008994A1/en active IP Right Grant
- 1998-08-19 DK DK98938534T patent/DK1015413T3/en active
- 1998-08-19 HU HU0004262A patent/HU228862B1/en active Protection Beyond IP Right Term
- 1998-08-19 DE DE69839586T patent/DE69839586D1/en not_active Expired - Lifetime
- 1998-08-19 PT PT98938534T patent/PT1015413E/en unknown
- 1998-08-19 JP JP2000509681A patent/JP2001515059A/en not_active Withdrawn
- 1998-08-19 EP EP98938534A patent/EP1015413B1/en not_active Expired - Lifetime
-
2001
- 2001-06-21 US US09/888,178 patent/US6787161B2/en not_active Expired - Lifetime
- 2001-06-21 US US09/888,997 patent/US6844013B2/en not_active Expired - Lifetime
-
2004
- 2004-07-22 US US10/896,811 patent/US7410656B2/en not_active Expired - Lifetime
-
2008
- 2008-08-29 CY CY20081100929T patent/CY1108303T1/en unknown
-
2011
- 2011-11-14 JP JP2011249091A patent/JP2012031212A/en active Pending
-
2013
- 2013-04-23 BE BE2013C026C patent/BE2013C026I2/en unknown
- 2013-04-23 LU LU92185C patent/LU92185I2/en unknown
- 2013-05-13 CY CY2013020C patent/CY2013020I1/en unknown
- 2013-10-30 HU HUS1300063 patent/HUS1300063I1/en unknown
-
2014
- 2014-10-09 JP JP2014207764A patent/JP2015007130A/en active Pending
Also Published As
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| CA2301082C (en) | Anti-cancer compounds | |
| Akdemir et al. | Bioassay-guided isolation of anti-inflammatory, antinociceptive and wound healer glycosides from the flowers of Verbascum mucronatum Lam. | |
| Güvenç et al. | Biological activities of Pseudevernia furfuracea (L.) Zopf extracts and isolation of the active compounds | |
| Süntar et al. | Comparative evaluation of traditional prescriptions from Cichorium intybus L. for wound healing: stepwise isolation of an active component by in vivo bioassay and its mode of activity | |
| Ghosh et al. | Evaluation of the wound healing activity of methanol extract of Pedilanthus tithymaloides (L.) Poit leaf and its isolated active constituents in topical formulation | |
| Süntar et al. | Exploration of the wound healing potential of Helichrysum graveolens (Bieb.) Sweet: Isolation of apigenin as an active component | |
| Kumar et al. | A review on pharmacological and phytochemical profile of Calotropis gigantea Linn | |
| Arévalo-Lopéz et al. | Leishmanicidal and cytotoxic activity from plants used in Tacana traditional medicine (Bolivia) | |
| Mishra et al. | A brief review on phytoconstituents and ethnopharmacology of Scoparia dulcis Linn.(Scrophulariaceae) | |
| Tosun et al. | Wound healing potential of selected Liverworts | |
| Giri et al. | Traditional Uses, Phytochemistry and Pharmacological Activities of Woodfordia fruticosa (L) Kurz: A Comprehensive Review. | |
| Oz et al. | Effects of Alchemilla mollis and Alchemilla persica on the wound healing process | |
| AU750624B2 (en) | Anti-cancer compounds-I | |
| Tessema et al. | Evaluation of in vivo wound healing and anti-inflammatory activity of crude extract of the fruits of Brucea antidysentrica in mice | |
| Sreekumar et al. | Wound healing potency of Hemigraphis alternata (Burm. f) T. Anderson leaf extract (HALE) with molecular evidence | |
| AU748545B2 (en) | Anti-cancer compounds-III | |
| AU750628B2 (en) | Anti-cancer compounds-II | |
| Deepa et al. | Wound healing activity of hydro-alcoholic extract of Cinnamomum nitidum Blume (Lauraceae) in wistar albino rats | |
| Saravanan et al. | Evaluation of wound healing and anti microbial activity of the Argemone mexicana linn (Papavraceae) | |
| Hassan et al. | A review on the pharmacological and traditional properties of Mimosa pudica | |
| Ullah et al. | Medicinal benefits of lemon balm (Melissa officinalis) for human health | |
| Devi et al. | Emerging Therapeutic properties of Terminalia Arjuna: A Review | |
| Song et al. | Natural products-Dawn of keloid treatment | |
| Panduranga Murthy et al. | Evaluation of ethno-medicinal plant drugs for wound healing practiced by tribal healers of Biligirirangana Hills (Karnataka), India | |
| Shehab et al. | Chemical composition, docking simulations and burn wound healing effect of Micromeria fruticosa extract and its isolated flavonoidal compound. |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| EEER | Examination request | ||
| MKEX | Expiry |
Effective date: 20180820 |