CA2345205A1 - Polyvinyl alcohol microspheres, and methods for making and therapeutic uses of the same - Google Patents
Polyvinyl alcohol microspheres, and methods for making and therapeutic uses of the same Download PDFInfo
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- CA2345205A1 CA2345205A1 CA002345205A CA2345205A CA2345205A1 CA 2345205 A1 CA2345205 A1 CA 2345205A1 CA 002345205 A CA002345205 A CA 002345205A CA 2345205 A CA2345205 A CA 2345205A CA 2345205 A1 CA2345205 A1 CA 2345205A1
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- microspheres
- polyvinylalcohol
- agent
- cell adhesion
- crosslinked
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/14—Particulate form, e.g. powders, Processes for size reducing of pure drugs or the resulting products, Pure drug nanoparticles
- A61K9/16—Agglomerates; Granulates; Microbeadlets ; Microspheres; Pellets; Solid products obtained by spray drying, spray freeze drying, spray congealing,(multiple) emulsion solvent evaporation or extraction
- A61K9/1605—Excipients; Inactive ingredients
- A61K9/1629—Organic macromolecular compounds
- A61K9/1635—Organic macromolecular compounds obtained by reactions only involving carbon-to-carbon unsaturated bonds, e.g. polyvinyl pyrrolidone, poly(meth)acrylates
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K47/00—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
- A61K47/50—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates
- A61K47/69—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the conjugate being characterised by physical or galenical forms, e.g. emulsion, particle, inclusion complex, stent or kit
- A61K47/6921—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the conjugate being characterised by physical or galenical forms, e.g. emulsion, particle, inclusion complex, stent or kit the form being a particulate, a powder, an adsorbate, a bead or a sphere
- A61K47/6927—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient the non-active ingredient being chemically bound to the active ingredient, e.g. polymer-drug conjugates the conjugate being characterised by physical or galenical forms, e.g. emulsion, particle, inclusion complex, stent or kit the form being a particulate, a powder, an adsorbate, a bead or a sphere the form being a solid microparticle having no hollow or gas-filled cores
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P35/00—Antineoplastic agents
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P9/00—Drugs for disorders of the cardiovascular system
Abstract
The present invention relates to microspheres useful for embolization which comprises polyvinylalcohol. The present invention also relates to an injectable suspension suitable for embolization which comprises the polyvinylalcohol microspheres and a suitable liquid carrier. The present invention further relates to a method for prophylactic or therapeutic embolization which comprises administering to a mammal an injectable suspension containing the polyvinylalcohol microspheres and a suitable liquid carrier. Finally, the present invention relates to a process for producing the polyvinylalcohol microspheres.
Description
BOLYVrrtYL ALCO$oL M=CROSFxEREB, AND METRODS FoR HARINO AND TRERApEpTZC OSES OF THE sAME
1. FIELD OF INVENTION
The present invention relates to materials useful for embolization, methods for using the same for embolization and processes for producing such materials.
1. FIELD OF INVENTION
The present invention relates to materials useful for embolization, methods for using the same for embolization and processes for producing such materials.
2. BAC'RaROUND OF THE INVENTION
Therapeutic 'vascular occlusions (embolizations) are l0 used to prevent or treat certain pathological conditions in situ. Generally they are employed using catheters, under imagery control, to position particulate occlusion agents (emboli) in the circulatory system. Embolizations can be used in a variety of vessels and organs whether healthy or diseased; however, the!~r are more commonly used in conditions i5 such as, e.g., tumors, vascular malformations, hemorrhagic processes, etc. Notab:Ly, in the case of tumors, vascular occlusion can suppress pain, limit blood loss during surgical intervention following embolization or even bring on tumoral necrosis and avoid the necessity for surgical intervention.
In the case of vascular malformations, embolization enables 20 the blood flow to the "normal" tissues to be normalized, aids in surgery and limits t:he risk of hemorrhage. In hemorrhagic events or processes, vascular occlusion produces a reduction of blood flow, which promotes cicatrization of the arterial opening ( s ) .
Furthermore, depending on the pathological 2s conditions treated, emr>olization can be used for temporary as well as permanent ob~ecaives.
Embolization has been performed with a variety of solid materials such as, small pieces of dura mater, irregular polyvinylalcohol particles, irregular gelatin particles, and more recently with crosslinked spherical hydrogel made from a 30 polyacrylamide derivative and a crosslinked gelatin.
U.S. Patent No. 5,635,215 discloses microspheres, comprising a hydrophilic acrylic copolymer coated with a cell adhesion promoter and a marking agent which are useful for embolization. U.S. Patent No. 5,648,100 discloses an injectable solution for therapeutic embolization, comprising S mi.crospheres comprising a hydrophilic acrylic copolymer coated With a cell adhesion promoter and a marking agent.
U.S. Patent No. 5,648,100 also discloses a method for therapeutic embolizat.ion which comprises administering to a mammal the above inje~ctable solution.
The most common material used to date in a variety l0 of embolization applications is irregular polyvinylaleohol particles. However, these irregular polyvinylalcohol particles have numerous drawbacks, and can in certain circumstances even led to deaths. For example, Repa et al., gadioloav, 1987, 170:,395-399 discloses that two infants with symptomatic hepatic arteriovenous malformation (AVM) were 1S treated with catheter embolization using commercially available polyvinyla:lcohol (IVALON particle suspensions from Laboratory Ingenor (I?aris)). Both infants died soon after the AVM embolization.. Further examination demonstrates that marked heterogeneity of particle size very probably contributed to the d~aath of the infants. Indeed, these and 20 other problems are a:~sociated with irregular polyvinylalcohol particles mostly due to their particle shapes. These problems make it dif:Eicult, or even dangerous in certain cases, to use irregu:Lar polyvinylalcohol particles in embolization.
Polyvinylalcohol products are commercially 25 available from Target Therapeutics/Boston Scientific (CONTOUR), from Nyco:med (IVALON, ULTRA-DRIVALON, and ULTRA-IVALON), from Cordis (TRUFILL) and from Cook (PVA). These poly~inylalcohol particles are known to be irregularly shaped particles. Generally, these polyvinylalcohol particles are sold as dry powders or saline suspensions. Despite their 30 potential damage, irregular polyvinylalcohol particles have been used extensively. Examples of the use of irregular polyvinylalcohol particles are discussed below.
Kusano et al., Invest. Radiol_._, 1987, 22:388-392, discloses low-dose particulate polyvinylalcohol embolization in animal and clinical studies. Polyvinylalcohol particles used in Kusano were IVALON obtained from Unipoint Labaratory, High Point, NC, in the radiopaque form. xusano discloses that low-dose large polyvinylalcohol particles (diameter at 590-1000 um) are suitable as an embolic material for trans-catheter occlusion of small intestinal hemorrhage in patients with certain diseases such as stress ulcer, surgical drain, ~ anastomosis, tubercul.ous ulcer and nonspecific ulcer.
Rump et al., Gen. Pharmac., 1996, 27(4):669-671, discloses pharmacokinetics of intraarterial Mitomycin C (MMC) in the chemo-emboliza~tion treatment of liver metastases. In Rump, hepatic branchea of patients with primary colorectal cancer and liver metastases were embolized using irregular 15 polyvinylalcohol particles (150-250 ~tm) before applying t~IC.
Barton et al., 0~1IR, 1996, 7:81-88, discloses embolization of patients with bone metastases to prevent major blood loss during surgery, to reduce bone metastases, to reduce pain and to control heavy bleeding.
Polyvinylalcohol foam particles (VALON; DRIVALON 300-600 ~Sm;
2o Nycomed-Ingenor, Paris) were used in eight cases in Barton.
Wakhloo et al., AJNR, 1993, 14:571-582, discloses extended preoperativ~a micro-embolization of intracranial meningiomas using 50~-150 ~m and 150-300 ~tm polyvinylalcohol particles. Wakhloo concluded from their study that embolization with 50~-150 um irregular polyvinylalcohol 25 particles led to a higher percentage of effective tumor devascularization and tumor necrosis for intracranial meningiomas.
Given the interest in the use of polyvinylalcohol particles for embolization, there is a great need for a safe and effective method for its application. The present 30 invention addresses these and other needs in the art.
Therapeutic 'vascular occlusions (embolizations) are l0 used to prevent or treat certain pathological conditions in situ. Generally they are employed using catheters, under imagery control, to position particulate occlusion agents (emboli) in the circulatory system. Embolizations can be used in a variety of vessels and organs whether healthy or diseased; however, the!~r are more commonly used in conditions i5 such as, e.g., tumors, vascular malformations, hemorrhagic processes, etc. Notab:Ly, in the case of tumors, vascular occlusion can suppress pain, limit blood loss during surgical intervention following embolization or even bring on tumoral necrosis and avoid the necessity for surgical intervention.
In the case of vascular malformations, embolization enables 20 the blood flow to the "normal" tissues to be normalized, aids in surgery and limits t:he risk of hemorrhage. In hemorrhagic events or processes, vascular occlusion produces a reduction of blood flow, which promotes cicatrization of the arterial opening ( s ) .
Furthermore, depending on the pathological 2s conditions treated, emr>olization can be used for temporary as well as permanent ob~ecaives.
Embolization has been performed with a variety of solid materials such as, small pieces of dura mater, irregular polyvinylalcohol particles, irregular gelatin particles, and more recently with crosslinked spherical hydrogel made from a 30 polyacrylamide derivative and a crosslinked gelatin.
U.S. Patent No. 5,635,215 discloses microspheres, comprising a hydrophilic acrylic copolymer coated with a cell adhesion promoter and a marking agent which are useful for embolization. U.S. Patent No. 5,648,100 discloses an injectable solution for therapeutic embolization, comprising S mi.crospheres comprising a hydrophilic acrylic copolymer coated With a cell adhesion promoter and a marking agent.
U.S. Patent No. 5,648,100 also discloses a method for therapeutic embolizat.ion which comprises administering to a mammal the above inje~ctable solution.
The most common material used to date in a variety l0 of embolization applications is irregular polyvinylaleohol particles. However, these irregular polyvinylalcohol particles have numerous drawbacks, and can in certain circumstances even led to deaths. For example, Repa et al., gadioloav, 1987, 170:,395-399 discloses that two infants with symptomatic hepatic arteriovenous malformation (AVM) were 1S treated with catheter embolization using commercially available polyvinyla:lcohol (IVALON particle suspensions from Laboratory Ingenor (I?aris)). Both infants died soon after the AVM embolization.. Further examination demonstrates that marked heterogeneity of particle size very probably contributed to the d~aath of the infants. Indeed, these and 20 other problems are a:~sociated with irregular polyvinylalcohol particles mostly due to their particle shapes. These problems make it dif:Eicult, or even dangerous in certain cases, to use irregu:Lar polyvinylalcohol particles in embolization.
Polyvinylalcohol products are commercially 25 available from Target Therapeutics/Boston Scientific (CONTOUR), from Nyco:med (IVALON, ULTRA-DRIVALON, and ULTRA-IVALON), from Cordis (TRUFILL) and from Cook (PVA). These poly~inylalcohol particles are known to be irregularly shaped particles. Generally, these polyvinylalcohol particles are sold as dry powders or saline suspensions. Despite their 30 potential damage, irregular polyvinylalcohol particles have been used extensively. Examples of the use of irregular polyvinylalcohol particles are discussed below.
Kusano et al., Invest. Radiol_._, 1987, 22:388-392, discloses low-dose particulate polyvinylalcohol embolization in animal and clinical studies. Polyvinylalcohol particles used in Kusano were IVALON obtained from Unipoint Labaratory, High Point, NC, in the radiopaque form. xusano discloses that low-dose large polyvinylalcohol particles (diameter at 590-1000 um) are suitable as an embolic material for trans-catheter occlusion of small intestinal hemorrhage in patients with certain diseases such as stress ulcer, surgical drain, ~ anastomosis, tubercul.ous ulcer and nonspecific ulcer.
Rump et al., Gen. Pharmac., 1996, 27(4):669-671, discloses pharmacokinetics of intraarterial Mitomycin C (MMC) in the chemo-emboliza~tion treatment of liver metastases. In Rump, hepatic branchea of patients with primary colorectal cancer and liver metastases were embolized using irregular 15 polyvinylalcohol particles (150-250 ~tm) before applying t~IC.
Barton et al., 0~1IR, 1996, 7:81-88, discloses embolization of patients with bone metastases to prevent major blood loss during surgery, to reduce bone metastases, to reduce pain and to control heavy bleeding.
Polyvinylalcohol foam particles (VALON; DRIVALON 300-600 ~Sm;
2o Nycomed-Ingenor, Paris) were used in eight cases in Barton.
Wakhloo et al., AJNR, 1993, 14:571-582, discloses extended preoperativ~a micro-embolization of intracranial meningiomas using 50~-150 ~m and 150-300 ~tm polyvinylalcohol particles. Wakhloo concluded from their study that embolization with 50~-150 um irregular polyvinylalcohol 25 particles led to a higher percentage of effective tumor devascularization and tumor necrosis for intracranial meningiomas.
Given the interest in the use of polyvinylalcohol particles for embolization, there is a great need for a safe and effective method for its application. The present 30 invention addresses these and other needs in the art.
3. 81~1I~ Y OF THE INVENTION
Despite the: risks and difficulties associated with the use of polyvinyla.lcohol particles in embolization, applicant has discovered surprisingly that microspheres made from crosslinked polyvinylalcohol are biocompatible, non-toxic and safe in embolization procedures. Accordingly, the present invention encompasses microspheres useful for embolization which comprise crosslinked polyvinylalcohol microspheres, injectable suspensions suitable for embolization which comprise the crosslinked polyvinylalcohol microspheres and a suitable liquid carrier, methods for l0 prophylactic or therapeutic embolization using such injectable suspensions, and processes for producing the crosslinked polyvinylalcohol microspheres.
The invention described herein encompasses microspheres, having diameters ranging from about 10 ~cm to about 2,000 ~m usefu:l for embolization, which comprise ZS crosslinked polyviny:Lalcohol. The microspheres of the present invention can be in the form of dry powder or hydrogel. In one embodiment, the present invention encompasses microspheres which comprise, in crosslinked and hydrogel form, about 0.5% to about 20% polyvinylalcohol by weight. In another ~ambodiment, the present invention 20 encompasses crvsslinked polyvinylalcohol microspheres which further comprise a cell adhesion promoter, a marking agent, or both. In still another embodiment, the present invention encompasses polyvinylalcohol microspheres further comprising an anti-angiogenic agent.
The present invention also encompasses an 25 injectable suspension suitable for prophylactic or therapeutic embolization, which comprises microspheres, having diameters ranging from about to ~cm to about 2,000 ~,m which comprise crosslinked polyvinylalcohol and a suitable liquid carrier. Tn a preferred embodiment, the present invention encompasses an injectable suspension wherein the 3o microspheres comprise, in crosslinked and hydrogel form, ~ 4 -about 0.5% to about 20% polyvinylalcohol by weight. In one embodiment, the microspheres in said injectable suspension have a uniform or narrow size range, wherein the difference in diameter between the microspheres is from about 0 ~m to about 150 Vim, preferably from about 0 um to about 100 um. In another embodiment, the present invention encompasses an injectable suspension wherein the crosslinked polyvinylalcohol microspheres further comprise a cell adhesion promoter, a marking agent or both. In still another embodiment, the present invention encompasses an injectable suspension wherein the polyvinylalcohol microspheres further comprise an anti-angiogenic agent.
The present invention additionally encompasses a method for prophylactic or therapeutic embolization in a mammal which comprises administering to said mammal an injectable suspension comprising an effective amount of microspheres, having diameters ranging from about 10 ~cm to about 2,000 um, which comprise crosslinked polyvinylalcohol.
An effective amount o~f said microspheres is generally the amount Buff icient to occlude the vessel in question. In general, this amount is between a few dozen to a few hundred microspheres. In a preferred embodiment, the present invention encompasses. a method for embolization wherein the 2o crosslinked polyvinylalcohol microspheres being administered in the i.njectable suspension comprise from about 0.5% to about ZO% crosslinked. polyvinylalcohol by weight in the hydrogel form. In another embodiment, the present invention encompasses a method for emboli2ation wherein the crosslinked polyvinylalcohol microspheres being administered further comprise a cell adhesion promoter, a marking agent, or both.
In still another embodiment, the present invention encompasses a method for embolization wherein the polyvinylalcohol microspheres being administered further comprise an anti-angi.ogenic agent.
The present: invention further encompasses a process for producing crossli.nked polyvinylalcohol microspheres, having a diameter ranging from about 10 ~m to about 2,000 ~cm, which comprises: a) dissolving polyvinylalcohol in an acidic solution; b) adding an aldehyde to said polyvinylalcohol-containing solution, or vice verse, to form a mixture; c) adding said mixture, with agitation, to an oil containing from about 0.1% to about 10% of an emulsifier having Hydrophilic-Hydrophobic Balance ("HLB") less than 5, or vice verse, to form an emulsion with droplets of polyvinylalcohol suspended in said oil; d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming spherical particles of crosslinked polyvinylalcohol; e) l0 removing said oil from said spherical particles of crosslinked poiyvinylalcohol; f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinylalcohol; g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with physiological aqueous buffers; and preferably h) sterilizing said washed i5 spherical particles of crosslinked polyvinylalcohol. The polyvinylalcohol-containing solution used in this process preferable has a polyvinylalcohol concentration from about 0.5% to about 20% (w/v).
4. DETAILED DE&CRIPTION OF THE INVENTION
20 Microspheres useful for embolization which comprise polyvinylalcohol, injectable suspensions suitable for embolization which comprise the polyvinylalcohol microspheres, methods for prophylactic or therapeutic embolization using such injectable suspensions, and processes for producing the polyvinylalcohol microspheres are described 25 herein.
As used herein, "microspheres" means solid insoluble particles which may be suspended in biological or biologically-compatible liquids, and which have, under microscopic examination, substantially a sphere or a spheroidal shape (ell.ipsis). A sphere is defined as a volume 30 that presents the lowest external surface area, The surface of microspheres appear smooth under less than 1000-fold magnifications.
As used herein, "irregular particles" means solid insoluble particles, under microscopic examination, have a shape that is not a substantially sphere or spheroidal (ellipsis . The shape of irregular particles is often the result of a larger solid particle that has been crushed.
Each irregular particle appears non-uniform in shape as compared to microspheres. Also in contrast to microspheres, irregular particles have rough surface. The length, thickness and depth o~f irregular particles are not uniform;
l0 they show angles and protuberances on the surface. These particles also appear irregular in their ability to transmit light under microscopic examination, depending on the thickness of the particles at particular locations.
The use of irregular particles in emboliaation has certain drawbacks. first, spheres are defined by their i5 diameter. Irregular particles can not be defined geometrically except by their whole volume and do not have real dimensions. Therefore, irregular particles can not be accurately sieved to achieve a uniform or even narrow range size distribution. ~,s a result, it is difficult to properly and completely occluale artery lumen using irregular particles 20 because they can not establish complete contact with all the surface of the artery which is cylindrical. In addition, irregular particles ~~ametimes block the catheter lumen depending on their space orientation inside the lumen of a catheter. Moreover, as a result of the rough surface of irregular particles and the possibility that such particles 25 may break as a consequence of attrition phenomena, very small-sized particles. can be generated from the irregular particles. When such very small-sized particles are generated during handling or administration in vivo, inadvertent pulmonary embolization, a potentially fatal complication, can occur. Furthermore, irregular particles 30 have large surface area in comparison to their volume. They tend to for~a clumps or aggregations, which are responsible for catheter clogging and undesired proximal embolization.
In contrast, use of microspheres described herein in embolization has ~aertain advantages. For example, due to their spherical shape or substantially spherical shape, microspheres can properly and completely occlude artezy lumen because they can establish complete contact with all the surface of the artery which is cylindrical. In addition, the microspheres of the ;present invention can be easily calibrated, and samples or suspensions containing these microspheres will not block or clog catheters because they always have the same dimension regardless of their space orientation in the catheter. Moreover, due to their smooth surface, no attrition will occur and small-sized particles will not be generated from the microspheres; thus avoiding the potentially fatal complications, such as pulmonary embolization. Furthermore, microspheres can only interact with each other on a single point and such contact is not enough to induce aggregation by surface interaction.
The invention described herein encompasses microspheres, having a diameter ranging from about l0 ~m to about 2,000 Vim, useful for embolization which comprises crosslinked polyvinylalcohol. Preferred diameters for the present invention will depend on the type of embolization and can be readily determined by the skilled artisans. The microspheres of the 'present invention can be in the form of dry powder or hydrogel. In a preferred embodiment, the present invention encompasses microspheres, which comprise in crosslinked and hydrogel form, from about 0.5% to about 20%
~ crosslinked polyvinylalcohol by weight. In other embodiments, the crosslinked polyvinylalcohol microspheres may further comprise one or more of a cell adhesion promoter, a marking agent, or an anti-angiogenic agent.
The present invention also encompasses an injectable suspension suitable f or embolization, which comprises crosslinked polyvinylalcohol microspheres, having a diameter ranging from about 10 ytm to about 2,000 um and a suitable liquid carrier. In a preferred embodiment, the crosslinked polyvinylalcohol microspheres in said injectable suspension have a uniform or narrow size range, wherein the difference in diameter between the microspheres is from about 0 ~m to about 150 ~Cm, preferably from about 0 ~m to about 100 Vim. In other embodiments, the present invention encompasses an injectable suspension wherein the microspheres are comprised of from about 0.5% to about 20% crosslinked polyvinylalcohol by weight in the hydrogel form; an injectable suspension wherein the crosslinked polyvinylalcohol microspheres may further comprise a cell adhesion promoter, a marking agent, and an injectable solution wherein the polyvinylalcohol microspheres and an anti-angiogenic agent:.
The present: invention additionally encompasses a method for prophylactic or therapeutic embolization in a manunal which comprises administering to said mammal in need of such embolization an injectable suspension comprising an effective amount of c:rosslinked polyvinylalcohol microspheres, having diameters ranging from about l0 ~m to about 2,000 ~cm, and a suitable liquid carrier. In a preferred embodiment,, the present invention encompasses a method for therapeut:i.c embolization wherein the 2o polyvinylalcohol microspheres in the injectable suspension being administered comprise from about 0.5% to about 20%
crosslinked polyvinyaalcohol by weight in the hydrogel form.
In other embodiments., the crosslinked polyvinylalcohol microspheres being administered in said method for prophylactic or therapeutic embolization may further comprise one or more of a cell adhesion promoter, a marking agent and an anti-angiogenic agent.
The present invention further encompasses a process for producing crosslinked polyvinylalcohol microspheres, having diameters ranging from about 10 ~.m to about 2,000 ~sm.
Various acidic solutions, aldehydes, oils, emulsifiers, agitation speeds, heating conditions and oil removing methods can be used in the process as described below. In other - g ..
wo oon3osa embodiments, the present invention encompasses a process for producing crosslinked polyvinylalcohol microspheres further comprising adding a cell adhesion promoter to the acidic polyvinylalcohol solution before adding the aldehyde; a process further comprising absorbing a marking agent into the crosslinked polyvinylalcohol microspheres; and a process further comprising absorbing an anti-angiogenic agent into the crosslinked polyvinylalcohol microspheres.
For clarity of disclosure, and not by way of limitation, the detailed description of the present invention is divided into the subsections which follow.
4.1. POLYVINYIrALCOHOL MICR06PHEREB
Polyvinylalcohol is a polymer prepared from polyvinyl acetates by replacement of the acetate groups with hydroxyl groups. Examples of other names for is p°lyvinylalcohol include, but are not limited to, Akwa Tears, Elvanol, Gelvatol, Lipuifilm, Mowiol, Polyviol, Sno Tears, Vinarol and Vinol (tee Merck Index, 12th Ed., Merck ~ Co., Inc., 1996, p 1308). such synonyms are encompassed by the present invention. Polyvinylalcohol can be synthesized according to the procedures disclosed in Hermann, Haehnel, ~ 60:1658 (1927); Schildknecht, yinyl and Related Polymers (Wiley, New York, 1952); Staudinger et al., Ber. 60:1?82 (1927); Prakt, ChQ~, 155:261 (1940); Marvel, J. Am. Sog_L, 60:1045 (1938); McDowell, J-Am. Soc., 62:415 (1940); Marvel, J. Am. Soc., 65:1710 (1943); Leeds, Enc~rclopedia o~~~hemical Technoloav (KirkOthmer ed.), 21:353-368 (Wiley-Interscience, New York, 2nd ed., 1970); Polvvinyl Alcohol (Finch Ed.), p640 (Wiley, New York, 1973); and Dunn, Chem & Ind. (London), pp8o1-806 (1980). Polyvinylalcohol can also be obtained from commercial chemical suppliers such as Aldrich, Fluka and Sigma.
The present invention provides polyvinylalcohol microspheres having one or more of the following characteristics: 1) substantially spherical; 2) substantially uniform in size and ~:hape; 3) will not aggregate by surface interaction: and 4) t:he diameter of which can easily be calibrated.
Polyvinylalcohol microspheres having a diameter ranging from about 10 um to about 2,000 ~m are also provided in the present invention. The microspheres of the present invention can be in t:he form of dry powder or hydrogel. In one embodiment, cross linked hydrogel microspheres of the present invention comprise about 0.5% to about 20%
crosslinked polyvinyl~alcohol by weight.
The present: invention also provides crosslinked polyvinylalcohol microspheres which further comprise a cell adhesion promoter, a marking agent or both. Such cell adhesion promoter in<:lude, but are not limited to, CM
dextran, collagen, DhAE dextran, gelatin. glucosaminoglycans, fibronectin, lectins, polycations, natural biological cell adhesion agents or synthetic biological cell adhesion agents.
In a preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM dextran, collagen and DEAF dextran.
The marking agents useful within the present invention include, but are not limited to, dyes, imaging agents and contrasting agents. Examples of chemical dyes that can be used in i:he present invention, which make possible a direct visualization of the microspheres, include, but are not limited i~o, Cibacron Blue and Procion Red HE-3B.
Examples of imaging <3gents that can be used in the present invention include, but are not limited to, magnetic resonance imaging agents such as erbium, gadolinium and magnetite. In a preferred embodiment, a magnetite imaging agent, such as ferrofluid, is used. Examples of contrasting agents that can be used in the present invention include, but are not limited to, barium or iodine salts and amino-3-triiodo-2,4,6-benzoic acid. The use and p~:eparation of the above dyes, imaging agents and contrasting agents are disclosed in U.S. Patent Nos. 5,635,215; 5,6413,100; Hoschetti, Biochem-Biophys. Meth.
19: 21-36 (1989); and Boschetti et al., Bull. Sec. Chim.
France. 1986 No. 4), the contents of which are incorporated herein by reference.
In the case. of barium or magnetite salts, they can be directly introduced in powdered form in the initial polyvinylalcohol solution in the process of preparing S polyvinylalcohol microspheres according to the present invention. It is also possible to incorporate such marking agents into the micre~spheres after their synthesis. This can be done, for example, by grafting of fluorescent markers such as erythrosine or flu:orescein or their derivatives (FITC, EITC, and the like).
1o In another embodiment, the present invention provides crosslinked polyvinylalcohol microspheres further comprising an anti-ar~giogenic agent.
The anti-ar~giogenic agents useful within the present invention include, but are not limited to, AGM-1470 (TNP-4'70), angiostati.c steroids, angiostatin, antibodies 15 against avG3, antibodies against bFGF, antibodies against IL-1, antibodies against: TNF-a, antibodies against VEGF, auranofin, azathiopri.ne, BB-94 and BB-2516, basic FGF-soluble receptor, carboxyamialo-trizole (CAI), cartilage-derived inhibitor (CDI), chitin, chioroquine, CM 101, cortisone/heparin, cortisone/hyaluroflan, 20 oortexolone/heparin, cT-2584, cyclophosphamide, cyclosporin A, dexamethasone, dic:lofenac/hyaluronan, eosinophilic major basic protein, fibronectin peptides, Glioma-derived angiogenesis inhibitory factor (GD-AIF), GM 1474, gold chloride, gold thiomalate, heparinases, hyaluronan (high and low molecular-weight species), hydrocortisonelbeta-25 cyclodextran, ibuprofen, indomethacin, interferon-alpha, interferon gamma-inducible protein 10, interferon-gamma, IL-1, IL-2, IL-4, IL-12, laminin, levamisole, linomide, LM609, martmastat (HB-2516), medroxyprogesterone, methvtrexate, minocycline, nitric oxide, octreotide (somatostatin analogue), D-penicil7.amine, pentosan polysulfate, placental 3o proliferin-related protein, placental RNase inhibitor, plasminogen activator- inhibitor (PAIs), platelet factor-4 (PF4), prednisolone, prolactin (16-kDa fragment), proliferin-related protein, prostaglandin synthase inhibitor, protamine, retinoids, somatostat;in, substance P, suramin, SU101, tecogalan sodium (05-4152), tetrahydrocortisol-sthrombospondins (TSP;s), tissue inhibitor of metalloproteinases (T:IMP 1, 2, 3), thalidomide, 3-aminothalidomide, 3-hydroxythalidomide, metabolites or hydrolysis products of thalidomide, 3-aminothalidomide, 3-hydroxythalidomide, vitamin A and vitreous fluids. In another preferred embodiment, the anti-angiogenic agent is selected from the group consisting of thalidomide, s-aminothalidomide, 3-hydroxythalidomide and metabolites or hydrolysis products of thalidomide, 3-aminothalidomide, 3-hydroxythalidomide. In a preferred embodiment, the anti-angiogenic agent is thalidomide. The above anti-angiogenic agents are disclosed in U.S. Patent Nos. 5,593,990;
5,629,327; and 5,712,291; Norrby, A S, 1997, 105:417-437;
p ~ Reilly, nve~t,~aational New D,~-uqs, 1997 , 15 : 5-13 ; and .T~.
Nat'1 Cancer I~.sz ti., 1996, 88(12):786-788, the contents of which are incorporated herein by reference.
The crosslinked polyvinylalcohol microspheres of the present invention can be stored and maintained in the form of dry powders, or as hydrogel suspended in a suitable liquid carrier.
4.2. INJECTABLE SOSPEN8ION8 COMPRISING POLYVINYLALCOHOL MICROSPHEREB
The present. invention provides an injectable suspension suitable for emboliaation, Which comprises microspheres, having diameters ranging from about 10 ~.m to about 2,000 Vim, useful for embolization, and a suitable carrier. Preferably, the injectable suspension is sterile.
The various. specific and preferred polyvinylalcohol microspheres that are: described in ~ a.l. can be used in the injectable suspension.
Kits containing a ready made injectable suspension, or the polyvinylalcohol microspheres described in ~ 4.1.
above in powder form, and physiologically acceptable carrier liquids) or solutions) that can solubilize the polyvinylalcohol microspheres powders, are included within the present invention. Suitable liquid carriers for use in the injectable suspensions of the present invention include biological liquids or solutions and liquids or solutions which are biologically compatible or physiologically acceptable. Examples of such liquids or solutions include, but are not limited t.o, aqueous solutions, saline, l0 physiological solutions which contain sugars, and the like.
such kits can also contain cell adhesion promoters, marking agents, or anti-angic>genic agents, or mixtures thereof. Such kits can further contain injection means such as a needle, a catheter, guides, contrast agents, and physiological dyes, such as methylene blue.
4.3. METHODS FOR EH80LIZATION QSING THE INJECTABLE
SU6PENSION8 COMF~RI8ING PO~YVINYLALCOIiOL MICRO8PHERE8 The present: invention provides a method for prophylactic or therapeutic, transient or permanent, embolization in a mazamal which comprises administering to 2o said mammal in need of such embolization an injectable suspension comprisinc; an effective amount of microspheres, having diameters ranging from about 10 ~m to about 2,000 ~,m, useful for embolizat:ion, wherein said microspheres comprise crosslinked polyviny:lalcohol. In a preferred embodiment, the mammal being emboliz~_d is a human.
The varioua specific and preferred injectable suspensions comprising the polyvinylalcohol microspheres that are described in ~ 4.1 and ~ 4.2 can be used in the embolization methods of the present invention.
Conditions and disease states that can be prevented or treated by the present embolization methods include, but are not limited to, olid tumors, vascular malformations, and hemorrhagic events or processes. Regarding tumors, the present embolization methods can be used to suppress pain, to limit blood loss occurring during surgical intervention following embolization, or to bring on tumoral necrosis and to either avoid or minimize the necessity of surgical intervention. With respect to vascular malformations, the present embolization methods can be used to normalize the blood flow to "normal''' tissues, to aid in surgery and to limit the risk of hemorrhage. For hemorrhagic events or processes, the present embolization methods can be used to reduce blood f low and to promote cicatrization of the arterial opening(s). In addition, the present embolization methods can be used a;5 a pre-surgical treatment in order to decrease the blood flow in blood rich organs (e.g., the liver) prior to surgical intervention. Examples of specific conditions that can b~e prevented or treated by the present embolization methods include, but are not limited to: uterine tumors or fibroids; small intestinal hemorrhage, such as that associated with stress ulcer; surgical drain; anastomosis;
tuberculous ulcer and nonspecific ulcer; symptomatic hepatic arteriovenous malformation (AVM); primary colorectal cancer;
hepatocellular carcinomas; liver metastases; bone metastases;
melanomas; cancers of the head or neck; and intracranial meningiomas.
The magnitude of a prophylactic or therapeutic dose of the polyvinylalcohol microspheres of the present invention, of course, vary with the nature of the type, location and severity of the condition to be treated and the route of administration. It will also vary according to the age, weight and response of the individual patient.
Effective amounts of the polyvinylalcohol microspheres to be used in the embolization methods of the present invention are based on the recommended doses known to those skilled in the art for the various conditions, diseases or disorders.
An effective amount refers to that amount of polyvinylalcohol microspheres sufficient to result in amelioration of symptoms or a prolongation of survival in a patient. Toxicity and therapeutic efficacy of such polyvinylalcohol microspheres can be determined by standard embolization procedures in experimental animals, or that is sufficient to permanently or temporarily occlude the vascular lumen in question.
Any suitable route of administration may be employed for providing the patient with an effective dosage of polyvinylalcohol microspheres of the present invention at the desired target oz' location. For example, parenteral, subcutaneous, intrarnuscular, and the like may be employed. A
~ preferred mode of administration is delivery inside targeted arteries via a catheter.
4.4. PROCESSES FOR PR~DUCIt~IG POLYVINYLALCOHOL MICR08PHEREB
The present: invention provides a process for producing crosslinked polyvinylalcohol microspheres, having a 15 diameter ranging from about l0 ~cm to about 2,000 ;cm, which comprises: a) dissolving polyvinylalcohol in an acidic solution; b) adding 2~n aldehyde to said polyvinylalcohol-containing solution t:o form a mixture, or vice verse; c) adding said mixture, with agitation, to an oil containing 20 from about 0.1% to ak>out 10% of an emulsifier having HLB less than 5, or vice verge, to form an emulsion with droplets of polyvinylalcohol suspended in said ail; d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming sapherical particles of crosslinked polyvinylalcohol; e) removing said oil from said spherical 25 Particles of crosslinked polyvinylalcohol; f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinyl_alcohol; g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with physiological aqueou:y buffers; and optionally h) sterilizing said washed spherical particles of crosslinked 30 Polyvinylalcohol. various acidic solutions, aldehydes, amino-containing agents, oils, emulsifiers, agitation speeds, heating conditions and oil removing methods can be used in the process.
various preferred reagents and reaction conditions can be used in the process for producing crosslinked polyvinylalcohol microspheres, as skilled artisans will be aware. For example, in step (a), preferred acidic solutions are 0. 5 M H~SO~-NaCl and 1. M HC1. In step (b) , the preferred aldehyde is selected from the group consisting of formaldehyde, glyoxal, glutaraldehyde and terephalaldehyde.
More preferably, the .aldehyde is glutaraldehyde. In step (c): 1) the preferred oil is selected from the group consisting of vegetal oils (e.g., olive oil, corn oil and sunflower oil), mineral oils (e. g., paraffin oil and silicone oil) and non-polar solvents, and more preferably, the oil is a mineral oil such as paraffin oil; and the preferred emulsifier having HLB less than 5 are preferably used in i5 o°ncentrations from about o.05% to 5%, and can be selected from the group consisting of sorbitan sesquioleate, sorbitan trioleate, sorbitan tristearate, polyethylene sorbitan monostearate, cellulose acetate butyrate and tetradecanol.
The agitation speed used in the process of the present invention will depend upon type of agitation equipment being used and the desired site for the microspheres being produced. In step (d) the heating is preferably conducted at about 80°C for about G hours. In step {e) said oil is removed from said spherical particles of crosslinked polyvinylalcohol using extraction agents such as light non-polar solvents, chlorinated solvents, ethyl-ether, and supercritical carbon dioxide, and preferably by extraction with light non-polar solvent or chlorinated solvent, and more preferably, by extraction with methylene chloride. In step (f) said active aldehyde on said spherical particles of crosslinked polyvinylalcohol is preferably neutralized by an amino-containing agent, such as aminoalcohols, e,g., Tris, 2-aminoethanol, aminosorbitol and glucosamine, and more preferably, by a 0.5 M Tris-HC1 buffer (pH 9).
In still another embodiment, the present invention provides a process f o:r producing crosslinked poly~inylalcohol microspheres further comprising adding a cell adhesion promoter to the acidic polyvinylalcohol solution before adding the aldehyde. In a preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen, DEAF dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, natural biological cell adhesion agents or synthetic biological cell adhesion agents.
In a more preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM dextran, collagen, and DEAE dextran.
In another embodiment, the present invention provides a process for producing crosslinked polyvinylalcohol microspheres further comprising absorbing a marking agent into the crosslinked polyvinylalcohol microspheres.
Preferably, the marking agent is selected from the group Consisting of a dye, an imaging agent and a contrasting.
agent, and more prefs~rably, the marking agent is an imaging agent such as ferrof7.uid.
In still another embodiment, the present invention provides a process for producing crosslinked polyvinylalcohol microspheres furtrier comprising absorbing an anti-angiogenic agent into the crossainked polyvinylalcohol microspheres.
More preferably, the anti-angiogenic agents described in ~
4.1 above can be used.
This inveni:.ion will be more completely described by means of the following examples, which are to be considered illustrative and not limitative.
5. EXAHPLEB
Haterials:
All chemical reagents including polyvinylalcohol are from Aldrich, Europe. All biological reagents such as 3~ dextran derivatives, cell adhesion factor, etc. are from ~ 18 -Sigma, U.S.A. The agitation system and the sieving machine are from Prolabo, France.
Example 1: Preparation of crosslinked microspheres com r'sing 5% polyyinylalcohol Five grams of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring.
The suspension is agitated until a clear solution forms and then 25 ml of formalaldehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraff in oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of formaldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size is managed by the speed of agitation of the emulsion. For' example, in order to obtain microspheres with diameter around 300 um (average dimension), the agitation speed i.s kept at about 250 rpm.
Hydrogel mi,crospheres of polyvinylalcohol are then collected by filtration. Alternatively, hydrogel microspheres of pvlyvinylalcohol may be collected by centrifugation or by simple decanting. Residue oil is extracted by non-polar solvents or chlorinated solvents such as methylene chloride. The resulting oil-free microspheres are then treated with a 0.5 M Tris-HC1 buffer (pH 9) overnight at room temperature to neutralize excess aldehydes.
Finally, the polyvinylalcohol microspheres are washed with physiological aqueous buffers, sieved to desired diameter, sterilized and stored as liquid suspensions. This material can be used for embolization procedure.
Example 2: Prepar,atioa of crosslinked microspheres com~risinQ Zo% aolyvinylalcohol Twenty grams of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring.
The suspension is agitated until a clear solution forms and then 25 ml of formaialdehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation to of formaldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 3: Preparation of crosslinked microspheras comprisinc 10% ~clyvinylalcohol Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M HMSO,-0.1 M NaCl solution under stirring. The Suspension is agitated until a clear solution forms and then ml of a 25% aqueous solution of glutaraldehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension 25 oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of glutaraldehyde on polyvinylaicohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, micrvspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 4: preparation of crosslinked microspheres comcrisina 1o% pol~winvlaiaohol Ten gram o1: polyvinylalcohol are dissolved in 85 ml of a 0.5 M HZSO,-0.1 1K NaCl solution under stirring. The suspension is agitatE:d until a clear solution forms and then 15 ml of a 25% aqueous solution of glyoxal are added to the solution. The resuli;ing mixture is rapidly poured into 500 ml of agitated paraff in oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated a1. about 80°C for at least 6 hours to l0 obtain the condensation of glyoxal on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutrali;aation of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 5: Prepa:catioa of polyvinylalcohol microspheres conta:inina collaaen Ten gram o:E polyvinylalcvhol are dissolved in 75 ml ~ of a 0.5 M H=SO,-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this solution 10 ml of 2% collagen in water are added under stirring and then 15 ml of a 50: aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesguioleat~e. Under these conditions, an emulsion is formed With droplets of polyvinylalcohol in suspension oil. The emulsion i;s heated at about 80°C fvr at least 6 hours to obtain the condensation of glutaraldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle sire control, micrvspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, - zi -sieve and sterilization are conducted as described in Exa~aple 1.
Example 6: Preparation of polyvinyl alcohol microspheres contnining~ DEAF Qextran Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this solution 10 ml of 1% DEAF dextran in water are added under stirring and then 15 ml of a 50a aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly l0 poured into 50o ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of glutaraldehyde on 15 polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutrali2ation of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
20 Example 7: preparation of polyvinylalcohol microspheres conta~.ning~ CM dextran Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SOq-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this 25 Solution 10 ml of 1% CM dextran in water are added under stirring and then 15 ml of a 50% aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing Z% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension 30 oil. The emulsion is heated at about 80°C f or at least 6 hours to obtain the condensation of glutaraldehyde on WO 00/23054 PCT/EP99~07846 polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcahol.
Particle size control, micraspheres collection, oil extraction, neutralization of aldehydes, micrvspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 8: Preparation of polyvinylalcohol microspheres containing colla en and DEAF Qextran Ten gram of polyvinylalcohol are dissolved in 65 ml of a 0.5 M H2SO,-0.1 M NaCl solution under stirring. The 1o Suspension is agitated until a clear solution forms. To this solution 10 ml of 1% DEAE dextran in water and 10 ml of 2%
collagen in water are. added under vigorous stirring and then ml of a 50% aqueous solution of glutaraldehyde are added.
The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate.
15 Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of gluta.raldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked Za polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 9: Preparation of polyvinylalcohol microspberes 2s containing magnetite Fifty ml of polyvinylalcohol microspheres obtained according to Examples 1 to 8 are each packed into a 16 mm diameter chromatographic column and washed with a physiological buffer. The column is then loaded with a 3o colloidal suspension of ferrofluid (very small particles of magnetite) at a flow rate of l0 ml/hour. Particles of wo oonsos4 magnetite are adsorbs:d by the polyvinylalcohol hydrogel network and permanently trapped. Resulting microspheres are used f or regular embolization procedure and can be monitored by MRI.
Example 10: Impregnated polyvinylalcohol mierospheres with ancio5renesie inhibitors Polyvinylal.cohol microspheres obtained according to Examples 1 to 8 are ciehydrated by sequential washing with ethanol to eliminate water. Ethanol is eliminated by washing with acetone and finally the polyvinylalcohol microspheres are dehydrated under dry nitrogen. An aqueous solution of 10 mg/ml of thalidomide is prepared and 1 gram of dry polyvinylalcohol microspheres is mixed with 12 ml of drug solution. The suspension is gently agitated for 2 hours.
Dry microspheres swell while adsorbing the drug in solution.
The resulting microspheres impregnated with the i5 drug are used for a normal embolization procedure.
Example 11: Absorption of drugs by ion exchange on op 1yv_i.nylalcohol micros~heres Polyvinyla7.cohol microspheres obtained according to Examples 6 and 8 containing about 80 ~mol of cationic groups can adsorb anionic molecules by ion exchange. Microspheres are equilibrated with a 10 mM Tris-HCl buffer (pH 7.5) in which the molecule of interest, such as anti-angiogenic or anti-inflammatory agents, are previously dissolved. Under these conditions the molecule of interest is adsorbed by ion ZS exchange effect, and the resulting microspheres can be used for regular embolizat:ion procedures.
The present: invention is not to be limited in scope by the specif is embodliments described herein. Indeed, various modifications. of the invention in addition to those described herein will. become apparent to those skilled in the 3o art from the foregoing description. Such modifications are intended to fall within the scope of the appended claims.
Despite the: risks and difficulties associated with the use of polyvinyla.lcohol particles in embolization, applicant has discovered surprisingly that microspheres made from crosslinked polyvinylalcohol are biocompatible, non-toxic and safe in embolization procedures. Accordingly, the present invention encompasses microspheres useful for embolization which comprise crosslinked polyvinylalcohol microspheres, injectable suspensions suitable for embolization which comprise the crosslinked polyvinylalcohol microspheres and a suitable liquid carrier, methods for l0 prophylactic or therapeutic embolization using such injectable suspensions, and processes for producing the crosslinked polyvinylalcohol microspheres.
The invention described herein encompasses microspheres, having diameters ranging from about 10 ~cm to about 2,000 ~m usefu:l for embolization, which comprise ZS crosslinked polyviny:Lalcohol. The microspheres of the present invention can be in the form of dry powder or hydrogel. In one embodiment, the present invention encompasses microspheres which comprise, in crosslinked and hydrogel form, about 0.5% to about 20% polyvinylalcohol by weight. In another ~ambodiment, the present invention 20 encompasses crvsslinked polyvinylalcohol microspheres which further comprise a cell adhesion promoter, a marking agent, or both. In still another embodiment, the present invention encompasses polyvinylalcohol microspheres further comprising an anti-angiogenic agent.
The present invention also encompasses an 25 injectable suspension suitable for prophylactic or therapeutic embolization, which comprises microspheres, having diameters ranging from about to ~cm to about 2,000 ~,m which comprise crosslinked polyvinylalcohol and a suitable liquid carrier. Tn a preferred embodiment, the present invention encompasses an injectable suspension wherein the 3o microspheres comprise, in crosslinked and hydrogel form, ~ 4 -about 0.5% to about 20% polyvinylalcohol by weight. In one embodiment, the microspheres in said injectable suspension have a uniform or narrow size range, wherein the difference in diameter between the microspheres is from about 0 ~m to about 150 Vim, preferably from about 0 um to about 100 um. In another embodiment, the present invention encompasses an injectable suspension wherein the crosslinked polyvinylalcohol microspheres further comprise a cell adhesion promoter, a marking agent or both. In still another embodiment, the present invention encompasses an injectable suspension wherein the polyvinylalcohol microspheres further comprise an anti-angiogenic agent.
The present invention additionally encompasses a method for prophylactic or therapeutic embolization in a mammal which comprises administering to said mammal an injectable suspension comprising an effective amount of microspheres, having diameters ranging from about 10 ~cm to about 2,000 um, which comprise crosslinked polyvinylalcohol.
An effective amount o~f said microspheres is generally the amount Buff icient to occlude the vessel in question. In general, this amount is between a few dozen to a few hundred microspheres. In a preferred embodiment, the present invention encompasses. a method for embolization wherein the 2o crosslinked polyvinylalcohol microspheres being administered in the i.njectable suspension comprise from about 0.5% to about ZO% crosslinked. polyvinylalcohol by weight in the hydrogel form. In another embodiment, the present invention encompasses a method for emboli2ation wherein the crosslinked polyvinylalcohol microspheres being administered further comprise a cell adhesion promoter, a marking agent, or both.
In still another embodiment, the present invention encompasses a method for embolization wherein the polyvinylalcohol microspheres being administered further comprise an anti-angi.ogenic agent.
The present: invention further encompasses a process for producing crossli.nked polyvinylalcohol microspheres, having a diameter ranging from about 10 ~m to about 2,000 ~cm, which comprises: a) dissolving polyvinylalcohol in an acidic solution; b) adding an aldehyde to said polyvinylalcohol-containing solution, or vice verse, to form a mixture; c) adding said mixture, with agitation, to an oil containing from about 0.1% to about 10% of an emulsifier having Hydrophilic-Hydrophobic Balance ("HLB") less than 5, or vice verse, to form an emulsion with droplets of polyvinylalcohol suspended in said oil; d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming spherical particles of crosslinked polyvinylalcohol; e) l0 removing said oil from said spherical particles of crosslinked poiyvinylalcohol; f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinylalcohol; g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with physiological aqueous buffers; and preferably h) sterilizing said washed i5 spherical particles of crosslinked polyvinylalcohol. The polyvinylalcohol-containing solution used in this process preferable has a polyvinylalcohol concentration from about 0.5% to about 20% (w/v).
4. DETAILED DE&CRIPTION OF THE INVENTION
20 Microspheres useful for embolization which comprise polyvinylalcohol, injectable suspensions suitable for embolization which comprise the polyvinylalcohol microspheres, methods for prophylactic or therapeutic embolization using such injectable suspensions, and processes for producing the polyvinylalcohol microspheres are described 25 herein.
As used herein, "microspheres" means solid insoluble particles which may be suspended in biological or biologically-compatible liquids, and which have, under microscopic examination, substantially a sphere or a spheroidal shape (ell.ipsis). A sphere is defined as a volume 30 that presents the lowest external surface area, The surface of microspheres appear smooth under less than 1000-fold magnifications.
As used herein, "irregular particles" means solid insoluble particles, under microscopic examination, have a shape that is not a substantially sphere or spheroidal (ellipsis . The shape of irregular particles is often the result of a larger solid particle that has been crushed.
Each irregular particle appears non-uniform in shape as compared to microspheres. Also in contrast to microspheres, irregular particles have rough surface. The length, thickness and depth o~f irregular particles are not uniform;
l0 they show angles and protuberances on the surface. These particles also appear irregular in their ability to transmit light under microscopic examination, depending on the thickness of the particles at particular locations.
The use of irregular particles in emboliaation has certain drawbacks. first, spheres are defined by their i5 diameter. Irregular particles can not be defined geometrically except by their whole volume and do not have real dimensions. Therefore, irregular particles can not be accurately sieved to achieve a uniform or even narrow range size distribution. ~,s a result, it is difficult to properly and completely occluale artery lumen using irregular particles 20 because they can not establish complete contact with all the surface of the artery which is cylindrical. In addition, irregular particles ~~ametimes block the catheter lumen depending on their space orientation inside the lumen of a catheter. Moreover, as a result of the rough surface of irregular particles and the possibility that such particles 25 may break as a consequence of attrition phenomena, very small-sized particles. can be generated from the irregular particles. When such very small-sized particles are generated during handling or administration in vivo, inadvertent pulmonary embolization, a potentially fatal complication, can occur. Furthermore, irregular particles 30 have large surface area in comparison to their volume. They tend to for~a clumps or aggregations, which are responsible for catheter clogging and undesired proximal embolization.
In contrast, use of microspheres described herein in embolization has ~aertain advantages. For example, due to their spherical shape or substantially spherical shape, microspheres can properly and completely occlude artezy lumen because they can establish complete contact with all the surface of the artery which is cylindrical. In addition, the microspheres of the ;present invention can be easily calibrated, and samples or suspensions containing these microspheres will not block or clog catheters because they always have the same dimension regardless of their space orientation in the catheter. Moreover, due to their smooth surface, no attrition will occur and small-sized particles will not be generated from the microspheres; thus avoiding the potentially fatal complications, such as pulmonary embolization. Furthermore, microspheres can only interact with each other on a single point and such contact is not enough to induce aggregation by surface interaction.
The invention described herein encompasses microspheres, having a diameter ranging from about l0 ~m to about 2,000 Vim, useful for embolization which comprises crosslinked polyvinylalcohol. Preferred diameters for the present invention will depend on the type of embolization and can be readily determined by the skilled artisans. The microspheres of the 'present invention can be in the form of dry powder or hydrogel. In a preferred embodiment, the present invention encompasses microspheres, which comprise in crosslinked and hydrogel form, from about 0.5% to about 20%
~ crosslinked polyvinylalcohol by weight. In other embodiments, the crosslinked polyvinylalcohol microspheres may further comprise one or more of a cell adhesion promoter, a marking agent, or an anti-angiogenic agent.
The present invention also encompasses an injectable suspension suitable f or embolization, which comprises crosslinked polyvinylalcohol microspheres, having a diameter ranging from about 10 ytm to about 2,000 um and a suitable liquid carrier. In a preferred embodiment, the crosslinked polyvinylalcohol microspheres in said injectable suspension have a uniform or narrow size range, wherein the difference in diameter between the microspheres is from about 0 ~m to about 150 ~Cm, preferably from about 0 ~m to about 100 Vim. In other embodiments, the present invention encompasses an injectable suspension wherein the microspheres are comprised of from about 0.5% to about 20% crosslinked polyvinylalcohol by weight in the hydrogel form; an injectable suspension wherein the crosslinked polyvinylalcohol microspheres may further comprise a cell adhesion promoter, a marking agent, and an injectable solution wherein the polyvinylalcohol microspheres and an anti-angiogenic agent:.
The present: invention additionally encompasses a method for prophylactic or therapeutic embolization in a manunal which comprises administering to said mammal in need of such embolization an injectable suspension comprising an effective amount of c:rosslinked polyvinylalcohol microspheres, having diameters ranging from about l0 ~m to about 2,000 ~cm, and a suitable liquid carrier. In a preferred embodiment,, the present invention encompasses a method for therapeut:i.c embolization wherein the 2o polyvinylalcohol microspheres in the injectable suspension being administered comprise from about 0.5% to about 20%
crosslinked polyvinyaalcohol by weight in the hydrogel form.
In other embodiments., the crosslinked polyvinylalcohol microspheres being administered in said method for prophylactic or therapeutic embolization may further comprise one or more of a cell adhesion promoter, a marking agent and an anti-angiogenic agent.
The present invention further encompasses a process for producing crosslinked polyvinylalcohol microspheres, having diameters ranging from about 10 ~.m to about 2,000 ~sm.
Various acidic solutions, aldehydes, oils, emulsifiers, agitation speeds, heating conditions and oil removing methods can be used in the process as described below. In other - g ..
wo oon3osa embodiments, the present invention encompasses a process for producing crosslinked polyvinylalcohol microspheres further comprising adding a cell adhesion promoter to the acidic polyvinylalcohol solution before adding the aldehyde; a process further comprising absorbing a marking agent into the crosslinked polyvinylalcohol microspheres; and a process further comprising absorbing an anti-angiogenic agent into the crosslinked polyvinylalcohol microspheres.
For clarity of disclosure, and not by way of limitation, the detailed description of the present invention is divided into the subsections which follow.
4.1. POLYVINYIrALCOHOL MICR06PHEREB
Polyvinylalcohol is a polymer prepared from polyvinyl acetates by replacement of the acetate groups with hydroxyl groups. Examples of other names for is p°lyvinylalcohol include, but are not limited to, Akwa Tears, Elvanol, Gelvatol, Lipuifilm, Mowiol, Polyviol, Sno Tears, Vinarol and Vinol (tee Merck Index, 12th Ed., Merck ~ Co., Inc., 1996, p 1308). such synonyms are encompassed by the present invention. Polyvinylalcohol can be synthesized according to the procedures disclosed in Hermann, Haehnel, ~ 60:1658 (1927); Schildknecht, yinyl and Related Polymers (Wiley, New York, 1952); Staudinger et al., Ber. 60:1?82 (1927); Prakt, ChQ~, 155:261 (1940); Marvel, J. Am. Sog_L, 60:1045 (1938); McDowell, J-Am. Soc., 62:415 (1940); Marvel, J. Am. Soc., 65:1710 (1943); Leeds, Enc~rclopedia o~~~hemical Technoloav (KirkOthmer ed.), 21:353-368 (Wiley-Interscience, New York, 2nd ed., 1970); Polvvinyl Alcohol (Finch Ed.), p640 (Wiley, New York, 1973); and Dunn, Chem & Ind. (London), pp8o1-806 (1980). Polyvinylalcohol can also be obtained from commercial chemical suppliers such as Aldrich, Fluka and Sigma.
The present invention provides polyvinylalcohol microspheres having one or more of the following characteristics: 1) substantially spherical; 2) substantially uniform in size and ~:hape; 3) will not aggregate by surface interaction: and 4) t:he diameter of which can easily be calibrated.
Polyvinylalcohol microspheres having a diameter ranging from about 10 um to about 2,000 ~m are also provided in the present invention. The microspheres of the present invention can be in t:he form of dry powder or hydrogel. In one embodiment, cross linked hydrogel microspheres of the present invention comprise about 0.5% to about 20%
crosslinked polyvinyl~alcohol by weight.
The present: invention also provides crosslinked polyvinylalcohol microspheres which further comprise a cell adhesion promoter, a marking agent or both. Such cell adhesion promoter in<:lude, but are not limited to, CM
dextran, collagen, DhAE dextran, gelatin. glucosaminoglycans, fibronectin, lectins, polycations, natural biological cell adhesion agents or synthetic biological cell adhesion agents.
In a preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM dextran, collagen and DEAF dextran.
The marking agents useful within the present invention include, but are not limited to, dyes, imaging agents and contrasting agents. Examples of chemical dyes that can be used in i:he present invention, which make possible a direct visualization of the microspheres, include, but are not limited i~o, Cibacron Blue and Procion Red HE-3B.
Examples of imaging <3gents that can be used in the present invention include, but are not limited to, magnetic resonance imaging agents such as erbium, gadolinium and magnetite. In a preferred embodiment, a magnetite imaging agent, such as ferrofluid, is used. Examples of contrasting agents that can be used in the present invention include, but are not limited to, barium or iodine salts and amino-3-triiodo-2,4,6-benzoic acid. The use and p~:eparation of the above dyes, imaging agents and contrasting agents are disclosed in U.S. Patent Nos. 5,635,215; 5,6413,100; Hoschetti, Biochem-Biophys. Meth.
19: 21-36 (1989); and Boschetti et al., Bull. Sec. Chim.
France. 1986 No. 4), the contents of which are incorporated herein by reference.
In the case. of barium or magnetite salts, they can be directly introduced in powdered form in the initial polyvinylalcohol solution in the process of preparing S polyvinylalcohol microspheres according to the present invention. It is also possible to incorporate such marking agents into the micre~spheres after their synthesis. This can be done, for example, by grafting of fluorescent markers such as erythrosine or flu:orescein or their derivatives (FITC, EITC, and the like).
1o In another embodiment, the present invention provides crosslinked polyvinylalcohol microspheres further comprising an anti-ar~giogenic agent.
The anti-ar~giogenic agents useful within the present invention include, but are not limited to, AGM-1470 (TNP-4'70), angiostati.c steroids, angiostatin, antibodies 15 against avG3, antibodies against bFGF, antibodies against IL-1, antibodies against: TNF-a, antibodies against VEGF, auranofin, azathiopri.ne, BB-94 and BB-2516, basic FGF-soluble receptor, carboxyamialo-trizole (CAI), cartilage-derived inhibitor (CDI), chitin, chioroquine, CM 101, cortisone/heparin, cortisone/hyaluroflan, 20 oortexolone/heparin, cT-2584, cyclophosphamide, cyclosporin A, dexamethasone, dic:lofenac/hyaluronan, eosinophilic major basic protein, fibronectin peptides, Glioma-derived angiogenesis inhibitory factor (GD-AIF), GM 1474, gold chloride, gold thiomalate, heparinases, hyaluronan (high and low molecular-weight species), hydrocortisonelbeta-25 cyclodextran, ibuprofen, indomethacin, interferon-alpha, interferon gamma-inducible protein 10, interferon-gamma, IL-1, IL-2, IL-4, IL-12, laminin, levamisole, linomide, LM609, martmastat (HB-2516), medroxyprogesterone, methvtrexate, minocycline, nitric oxide, octreotide (somatostatin analogue), D-penicil7.amine, pentosan polysulfate, placental 3o proliferin-related protein, placental RNase inhibitor, plasminogen activator- inhibitor (PAIs), platelet factor-4 (PF4), prednisolone, prolactin (16-kDa fragment), proliferin-related protein, prostaglandin synthase inhibitor, protamine, retinoids, somatostat;in, substance P, suramin, SU101, tecogalan sodium (05-4152), tetrahydrocortisol-sthrombospondins (TSP;s), tissue inhibitor of metalloproteinases (T:IMP 1, 2, 3), thalidomide, 3-aminothalidomide, 3-hydroxythalidomide, metabolites or hydrolysis products of thalidomide, 3-aminothalidomide, 3-hydroxythalidomide, vitamin A and vitreous fluids. In another preferred embodiment, the anti-angiogenic agent is selected from the group consisting of thalidomide, s-aminothalidomide, 3-hydroxythalidomide and metabolites or hydrolysis products of thalidomide, 3-aminothalidomide, 3-hydroxythalidomide. In a preferred embodiment, the anti-angiogenic agent is thalidomide. The above anti-angiogenic agents are disclosed in U.S. Patent Nos. 5,593,990;
5,629,327; and 5,712,291; Norrby, A S, 1997, 105:417-437;
p ~ Reilly, nve~t,~aational New D,~-uqs, 1997 , 15 : 5-13 ; and .T~.
Nat'1 Cancer I~.sz ti., 1996, 88(12):786-788, the contents of which are incorporated herein by reference.
The crosslinked polyvinylalcohol microspheres of the present invention can be stored and maintained in the form of dry powders, or as hydrogel suspended in a suitable liquid carrier.
4.2. INJECTABLE SOSPEN8ION8 COMPRISING POLYVINYLALCOHOL MICROSPHEREB
The present. invention provides an injectable suspension suitable for emboliaation, Which comprises microspheres, having diameters ranging from about 10 ~.m to about 2,000 Vim, useful for embolization, and a suitable carrier. Preferably, the injectable suspension is sterile.
The various. specific and preferred polyvinylalcohol microspheres that are: described in ~ a.l. can be used in the injectable suspension.
Kits containing a ready made injectable suspension, or the polyvinylalcohol microspheres described in ~ 4.1.
above in powder form, and physiologically acceptable carrier liquids) or solutions) that can solubilize the polyvinylalcohol microspheres powders, are included within the present invention. Suitable liquid carriers for use in the injectable suspensions of the present invention include biological liquids or solutions and liquids or solutions which are biologically compatible or physiologically acceptable. Examples of such liquids or solutions include, but are not limited t.o, aqueous solutions, saline, l0 physiological solutions which contain sugars, and the like.
such kits can also contain cell adhesion promoters, marking agents, or anti-angic>genic agents, or mixtures thereof. Such kits can further contain injection means such as a needle, a catheter, guides, contrast agents, and physiological dyes, such as methylene blue.
4.3. METHODS FOR EH80LIZATION QSING THE INJECTABLE
SU6PENSION8 COMF~RI8ING PO~YVINYLALCOIiOL MICRO8PHERE8 The present: invention provides a method for prophylactic or therapeutic, transient or permanent, embolization in a mazamal which comprises administering to 2o said mammal in need of such embolization an injectable suspension comprisinc; an effective amount of microspheres, having diameters ranging from about 10 ~m to about 2,000 ~,m, useful for embolizat:ion, wherein said microspheres comprise crosslinked polyviny:lalcohol. In a preferred embodiment, the mammal being emboliz~_d is a human.
The varioua specific and preferred injectable suspensions comprising the polyvinylalcohol microspheres that are described in ~ 4.1 and ~ 4.2 can be used in the embolization methods of the present invention.
Conditions and disease states that can be prevented or treated by the present embolization methods include, but are not limited to, olid tumors, vascular malformations, and hemorrhagic events or processes. Regarding tumors, the present embolization methods can be used to suppress pain, to limit blood loss occurring during surgical intervention following embolization, or to bring on tumoral necrosis and to either avoid or minimize the necessity of surgical intervention. With respect to vascular malformations, the present embolization methods can be used to normalize the blood flow to "normal''' tissues, to aid in surgery and to limit the risk of hemorrhage. For hemorrhagic events or processes, the present embolization methods can be used to reduce blood f low and to promote cicatrization of the arterial opening(s). In addition, the present embolization methods can be used a;5 a pre-surgical treatment in order to decrease the blood flow in blood rich organs (e.g., the liver) prior to surgical intervention. Examples of specific conditions that can b~e prevented or treated by the present embolization methods include, but are not limited to: uterine tumors or fibroids; small intestinal hemorrhage, such as that associated with stress ulcer; surgical drain; anastomosis;
tuberculous ulcer and nonspecific ulcer; symptomatic hepatic arteriovenous malformation (AVM); primary colorectal cancer;
hepatocellular carcinomas; liver metastases; bone metastases;
melanomas; cancers of the head or neck; and intracranial meningiomas.
The magnitude of a prophylactic or therapeutic dose of the polyvinylalcohol microspheres of the present invention, of course, vary with the nature of the type, location and severity of the condition to be treated and the route of administration. It will also vary according to the age, weight and response of the individual patient.
Effective amounts of the polyvinylalcohol microspheres to be used in the embolization methods of the present invention are based on the recommended doses known to those skilled in the art for the various conditions, diseases or disorders.
An effective amount refers to that amount of polyvinylalcohol microspheres sufficient to result in amelioration of symptoms or a prolongation of survival in a patient. Toxicity and therapeutic efficacy of such polyvinylalcohol microspheres can be determined by standard embolization procedures in experimental animals, or that is sufficient to permanently or temporarily occlude the vascular lumen in question.
Any suitable route of administration may be employed for providing the patient with an effective dosage of polyvinylalcohol microspheres of the present invention at the desired target oz' location. For example, parenteral, subcutaneous, intrarnuscular, and the like may be employed. A
~ preferred mode of administration is delivery inside targeted arteries via a catheter.
4.4. PROCESSES FOR PR~DUCIt~IG POLYVINYLALCOHOL MICR08PHEREB
The present: invention provides a process for producing crosslinked polyvinylalcohol microspheres, having a 15 diameter ranging from about l0 ~cm to about 2,000 ;cm, which comprises: a) dissolving polyvinylalcohol in an acidic solution; b) adding 2~n aldehyde to said polyvinylalcohol-containing solution t:o form a mixture, or vice verse; c) adding said mixture, with agitation, to an oil containing 20 from about 0.1% to ak>out 10% of an emulsifier having HLB less than 5, or vice verge, to form an emulsion with droplets of polyvinylalcohol suspended in said ail; d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming sapherical particles of crosslinked polyvinylalcohol; e) removing said oil from said spherical 25 Particles of crosslinked polyvinylalcohol; f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinyl_alcohol; g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with physiological aqueou:y buffers; and optionally h) sterilizing said washed spherical particles of crosslinked 30 Polyvinylalcohol. various acidic solutions, aldehydes, amino-containing agents, oils, emulsifiers, agitation speeds, heating conditions and oil removing methods can be used in the process.
various preferred reagents and reaction conditions can be used in the process for producing crosslinked polyvinylalcohol microspheres, as skilled artisans will be aware. For example, in step (a), preferred acidic solutions are 0. 5 M H~SO~-NaCl and 1. M HC1. In step (b) , the preferred aldehyde is selected from the group consisting of formaldehyde, glyoxal, glutaraldehyde and terephalaldehyde.
More preferably, the .aldehyde is glutaraldehyde. In step (c): 1) the preferred oil is selected from the group consisting of vegetal oils (e.g., olive oil, corn oil and sunflower oil), mineral oils (e. g., paraffin oil and silicone oil) and non-polar solvents, and more preferably, the oil is a mineral oil such as paraffin oil; and the preferred emulsifier having HLB less than 5 are preferably used in i5 o°ncentrations from about o.05% to 5%, and can be selected from the group consisting of sorbitan sesquioleate, sorbitan trioleate, sorbitan tristearate, polyethylene sorbitan monostearate, cellulose acetate butyrate and tetradecanol.
The agitation speed used in the process of the present invention will depend upon type of agitation equipment being used and the desired site for the microspheres being produced. In step (d) the heating is preferably conducted at about 80°C for about G hours. In step {e) said oil is removed from said spherical particles of crosslinked polyvinylalcohol using extraction agents such as light non-polar solvents, chlorinated solvents, ethyl-ether, and supercritical carbon dioxide, and preferably by extraction with light non-polar solvent or chlorinated solvent, and more preferably, by extraction with methylene chloride. In step (f) said active aldehyde on said spherical particles of crosslinked polyvinylalcohol is preferably neutralized by an amino-containing agent, such as aminoalcohols, e,g., Tris, 2-aminoethanol, aminosorbitol and glucosamine, and more preferably, by a 0.5 M Tris-HC1 buffer (pH 9).
In still another embodiment, the present invention provides a process f o:r producing crosslinked poly~inylalcohol microspheres further comprising adding a cell adhesion promoter to the acidic polyvinylalcohol solution before adding the aldehyde. In a preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen, DEAF dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, natural biological cell adhesion agents or synthetic biological cell adhesion agents.
In a more preferred embodiment, the cell adhesion promoter is selected from the group consisting of CM dextran, collagen, and DEAE dextran.
In another embodiment, the present invention provides a process for producing crosslinked polyvinylalcohol microspheres further comprising absorbing a marking agent into the crosslinked polyvinylalcohol microspheres.
Preferably, the marking agent is selected from the group Consisting of a dye, an imaging agent and a contrasting.
agent, and more prefs~rably, the marking agent is an imaging agent such as ferrof7.uid.
In still another embodiment, the present invention provides a process for producing crosslinked polyvinylalcohol microspheres furtrier comprising absorbing an anti-angiogenic agent into the crossainked polyvinylalcohol microspheres.
More preferably, the anti-angiogenic agents described in ~
4.1 above can be used.
This inveni:.ion will be more completely described by means of the following examples, which are to be considered illustrative and not limitative.
5. EXAHPLEB
Haterials:
All chemical reagents including polyvinylalcohol are from Aldrich, Europe. All biological reagents such as 3~ dextran derivatives, cell adhesion factor, etc. are from ~ 18 -Sigma, U.S.A. The agitation system and the sieving machine are from Prolabo, France.
Example 1: Preparation of crosslinked microspheres com r'sing 5% polyyinylalcohol Five grams of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring.
The suspension is agitated until a clear solution forms and then 25 ml of formalaldehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraff in oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of formaldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size is managed by the speed of agitation of the emulsion. For' example, in order to obtain microspheres with diameter around 300 um (average dimension), the agitation speed i.s kept at about 250 rpm.
Hydrogel mi,crospheres of polyvinylalcohol are then collected by filtration. Alternatively, hydrogel microspheres of pvlyvinylalcohol may be collected by centrifugation or by simple decanting. Residue oil is extracted by non-polar solvents or chlorinated solvents such as methylene chloride. The resulting oil-free microspheres are then treated with a 0.5 M Tris-HC1 buffer (pH 9) overnight at room temperature to neutralize excess aldehydes.
Finally, the polyvinylalcohol microspheres are washed with physiological aqueous buffers, sieved to desired diameter, sterilized and stored as liquid suspensions. This material can be used for embolization procedure.
Example 2: Prepar,atioa of crosslinked microspheres com~risinQ Zo% aolyvinylalcohol Twenty grams of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring.
The suspension is agitated until a clear solution forms and then 25 ml of formaialdehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation to of formaldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 3: Preparation of crosslinked microspheras comprisinc 10% ~clyvinylalcohol Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M HMSO,-0.1 M NaCl solution under stirring. The Suspension is agitated until a clear solution forms and then ml of a 25% aqueous solution of glutaraldehyde are added to the solution. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension 25 oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of glutaraldehyde on polyvinylaicohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, micrvspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 4: preparation of crosslinked microspheres comcrisina 1o% pol~winvlaiaohol Ten gram o1: polyvinylalcohol are dissolved in 85 ml of a 0.5 M HZSO,-0.1 1K NaCl solution under stirring. The suspension is agitatE:d until a clear solution forms and then 15 ml of a 25% aqueous solution of glyoxal are added to the solution. The resuli;ing mixture is rapidly poured into 500 ml of agitated paraff in oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated a1. about 80°C for at least 6 hours to l0 obtain the condensation of glyoxal on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutrali;aation of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 5: Prepa:catioa of polyvinylalcohol microspheres conta:inina collaaen Ten gram o:E polyvinylalcvhol are dissolved in 75 ml ~ of a 0.5 M H=SO,-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this solution 10 ml of 2% collagen in water are added under stirring and then 15 ml of a 50: aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesguioleat~e. Under these conditions, an emulsion is formed With droplets of polyvinylalcohol in suspension oil. The emulsion i;s heated at about 80°C fvr at least 6 hours to obtain the condensation of glutaraldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle sire control, micrvspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, - zi -sieve and sterilization are conducted as described in Exa~aple 1.
Example 6: Preparation of polyvinyl alcohol microspheres contnining~ DEAF Qextran Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SO,-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this solution 10 ml of 1% DEAF dextran in water are added under stirring and then 15 ml of a 50a aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly l0 poured into 50o ml of agitated paraffin oil containing 2% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of glutaraldehyde on 15 polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutrali2ation of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
20 Example 7: preparation of polyvinylalcohol microspheres conta~.ning~ CM dextran Ten gram of polyvinylalcohol are dissolved in 75 ml of a 0.5 M H,SOq-0.1 M NaCl solution under stirring. The suspension is agitated until a clear solution forms. To this 25 Solution 10 ml of 1% CM dextran in water are added under stirring and then 15 ml of a 50% aqueous solution of glutaraldehyde are added. The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing Z% of sorbitan sesquioleate. Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension 30 oil. The emulsion is heated at about 80°C f or at least 6 hours to obtain the condensation of glutaraldehyde on WO 00/23054 PCT/EP99~07846 polyvinylalcohol chains and thus forming spherical particles of crosslinked polyvinylalcahol.
Particle size control, micraspheres collection, oil extraction, neutralization of aldehydes, micrvspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 8: Preparation of polyvinylalcohol microspheres containing colla en and DEAF Qextran Ten gram of polyvinylalcohol are dissolved in 65 ml of a 0.5 M H2SO,-0.1 M NaCl solution under stirring. The 1o Suspension is agitated until a clear solution forms. To this solution 10 ml of 1% DEAE dextran in water and 10 ml of 2%
collagen in water are. added under vigorous stirring and then ml of a 50% aqueous solution of glutaraldehyde are added.
The resulting mixture is rapidly poured into 500 ml of agitated paraffin oil containing 2% of sorbitan sesquioleate.
15 Under these conditions, an emulsion is formed with droplets of polyvinylalcohol in suspension oil. The emulsion is heated at about 80°C for at least 6 hours to obtain the condensation of gluta.raldehyde on polyvinylalcohol chains and thus forming spherical particles of crosslinked Za polyvinylalcohol.
Particle size control, microspheres collection, oil extraction, neutralization of aldehydes, microspheres wash, sieve and sterilization are conducted as described in Example 1.
Example 9: Preparation of polyvinylalcohol microspberes 2s containing magnetite Fifty ml of polyvinylalcohol microspheres obtained according to Examples 1 to 8 are each packed into a 16 mm diameter chromatographic column and washed with a physiological buffer. The column is then loaded with a 3o colloidal suspension of ferrofluid (very small particles of magnetite) at a flow rate of l0 ml/hour. Particles of wo oonsos4 magnetite are adsorbs:d by the polyvinylalcohol hydrogel network and permanently trapped. Resulting microspheres are used f or regular embolization procedure and can be monitored by MRI.
Example 10: Impregnated polyvinylalcohol mierospheres with ancio5renesie inhibitors Polyvinylal.cohol microspheres obtained according to Examples 1 to 8 are ciehydrated by sequential washing with ethanol to eliminate water. Ethanol is eliminated by washing with acetone and finally the polyvinylalcohol microspheres are dehydrated under dry nitrogen. An aqueous solution of 10 mg/ml of thalidomide is prepared and 1 gram of dry polyvinylalcohol microspheres is mixed with 12 ml of drug solution. The suspension is gently agitated for 2 hours.
Dry microspheres swell while adsorbing the drug in solution.
The resulting microspheres impregnated with the i5 drug are used for a normal embolization procedure.
Example 11: Absorption of drugs by ion exchange on op 1yv_i.nylalcohol micros~heres Polyvinyla7.cohol microspheres obtained according to Examples 6 and 8 containing about 80 ~mol of cationic groups can adsorb anionic molecules by ion exchange. Microspheres are equilibrated with a 10 mM Tris-HCl buffer (pH 7.5) in which the molecule of interest, such as anti-angiogenic or anti-inflammatory agents, are previously dissolved. Under these conditions the molecule of interest is adsorbed by ion ZS exchange effect, and the resulting microspheres can be used for regular embolizat:ion procedures.
The present: invention is not to be limited in scope by the specif is embodliments described herein. Indeed, various modifications. of the invention in addition to those described herein will. become apparent to those skilled in the 3o art from the foregoing description. Such modifications are intended to fall within the scope of the appended claims.
Claims (49)
1. Microspheres useful for embolization wherein said microspheres comprise crosslinked polyvinylalcohol and have a diameter ranging from about 10 µm to about 2,000 µm.
2. The microspheres of claim 1 wherein said microspheres are substantially spherical.
3. The microspheres of claim 1 wherein said microspheres are subtantially uniform in size and shape.
4. The microspheres of claim 1 wherein the diameter of said microspheres is in the range from about 50 µm to about 1, 000 µm.
5. The microspheres of claim 1 wherein said microspheres further comprise a cell adhesion promoter.
6. The microspheres of claim 5 wherein the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen. DEAE dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agent and a synthetic biological cell adhesion agent.
dextran, collagen. DEAE dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agent and a synthetic biological cell adhesion agent.
7. The microspheres of claim 6 wherein the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen and DEAE dextran.
dextran, collagen and DEAE dextran.
8. The microspheres of claim 1 or claim 5 wherein said microspheres further comprise a marking agent.
9. The microspheres of claim 8 wherein the marking agent is selected from the group consisting of a dye, an imaging agent and a contrasting agent.
10. The microspheres of claim 1, claim 5 or claim 8, further comprising an anti-angiogenic agent.
11. An injectable suspension suitable for embolization, which comprises crosslinked polyvinylalcohol microspheres, having a diameter ranging from about 10 µm to about 2,000 µm, and a suitable liquid carrier.
12. The injectable suspension of claim 11 wherein the crosslinked polyvinylalcohol microspheres are substantially spherical.
13. The injectable suspension of claim 11 wherein the crosslinked polyvinylalcohol microspheres are substantially uniform in size and shape.
14. The injectable suspension of claim 11 which injectable suspension is sterile.
15. The injectable suspension of claim 11 Wherein the diameter of the crosslinked polyvinylalcohol microspheres are in the range from about 50 µm to about 1,000 µm.
16. The injectable suspension of claim 11, wherein the crosslinked polyvinylalcohol microspheres in the injectable suspension are comprised of from about 0.5% to about 20% crosslinked polyvinylalcohol by weight in hydrogel form.
17. The injectable suspension of claim 11 wherein said crosslinked polyvinylalcohol microspheres further comprise a cell adhesion promoter.
18. The injectable suspension of claim 17 wherein the cell adhesion promoter is selected from the group consisting of CM dextran, collagen, DEAE dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agent and a synthetic biological cell adhesion agent.
19. The injectable suspension of claim 11 or claim 17 wherein said crosslinked polyvinylalcohol microspheres further comprise a marking agent.
20. The injectable suspension of claim 19 wherein the marking agent is selected from the group consisting of a dye, an imaging agent and a contrasting agent.
21. The injectable suspension of claim 11, further comprising an anti-angiogenic agent.
22. A method for prophylactic or therapeutic embolization in a mammal which comprises administering to said mammal in need of such embolization, an injectable suspension comprising an effective amount of crosslinked polyvinylalcohol microspheres, having a diameter ranging from about 10 µm to about 2,000 µm, and a suitable liquid carrier.
23. The method of claim 22 wherein the mammal is a human.
24. The method of claim 22 wherein said crosslinked polyvinylalcohol microspheres in the injectable suspension are substantially uniform in size and shape.
25. The method of claim 22, wherein the crosslinked polyvinylalcohol microspheres in the injectable suspension are comprised of from about 0.5% to about 20%
crosslinked polyvinylalcohol by weight in hydrogel form.
crosslinked polyvinylalcohol by weight in hydrogel form.
26. The method of claim 22 wherein said crosslinked polyvinylalcohol microspheres further comprise a cell adhesion promoter.
27. The method of claim 26 wherein the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen, DEAE dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agents and a synthetic biological cell adhesion agent.
dextran, collagen, DEAE dextran, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agents and a synthetic biological cell adhesion agent.
28. The method of claim 27 wherein the cell adhesion promoter is selected from the group consisting of CM
dextran, collagen and. DEAF dextran.
dextran, collagen and. DEAF dextran.
29. The method of claim 22 or claim 26 wherein said crosslinked polyvinylalcohol microspheres further comprise a marking agent.
30. The method of claim 29 wherein the marking agent is selected from the group consisting of a dye, an imaging agent and a contrasting agent.
31. The method of claim 22, said crosslinked polyvinylalcohol microspheres further comprise an anti-angiogenic agent.
32. A process for producing crosslinked polyvinylalcohol microspheres, having a diameter ranging from about l0 µm to about 2,000 µm, which comprises:
a) dissolving polyvinylalcohol in an acidic solution;
b) adding an aldehyde to said polyvinylalcohol-containing solution, or vice verse, to form a mixture;
c) adding said mixture, with agitation, to an oil containing from about 0.1% to about l0% of an emulsifier having HLB less than 5, or vice verse, to form an emulsion with droplets of polyvinylalcohol suspended in said oil;
d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming spherical particles of crosslinked polyvinylalcohol;
e) removing said oil from said spherical particles of crosslinked polyvinylalcohol;
f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinylalcohol; and g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with a physiological aqueous buffer.
a) dissolving polyvinylalcohol in an acidic solution;
b) adding an aldehyde to said polyvinylalcohol-containing solution, or vice verse, to form a mixture;
c) adding said mixture, with agitation, to an oil containing from about 0.1% to about l0% of an emulsifier having HLB less than 5, or vice verse, to form an emulsion with droplets of polyvinylalcohol suspended in said oil;
d) heating said emulsion to condense said aldehyde on polyvinylalcohol chains and thereby forming spherical particles of crosslinked polyvinylalcohol;
e) removing said oil from said spherical particles of crosslinked polyvinylalcohol;
f) neutralizing said active aldehyde on said spherical particles of crosslinked polyvinylalcohol; and g) washing said neutralized spherical particles of crosslinked polyvinylalcohol with a physiological aqueous buffer.
33. The process of claim 32 which further comprises the step of sterilizing said washed spherical particles of crosslinked polyvinylalcohol.
34. The process of claim 32, wherein in step (b) the aldehyde is selected from the group consisting of formaldehyde, glyoxal, glutaraldehyde and terephalaldehyde.
35. The process of claim 34, wherein the aldehyde is glutaraidehyde.
36. The process of claim 32, wherein in step (c) the oil is selected from the group consisting of vegetal oil, mineral oil and non-polar solvent.
37. The process of claim 36, wherein the oil is paraffin oil.
38. The process of claim 32, wherein in step (c) the emulsifier having HLB less than 5 is selected from the group consisting of sorbitan sesquioleate, sorbitan trioleate, sorbitan tristearate, polyethylene sorbitan monostearate, cellulose acetate butyrate and tetradecanol.
39. The process of claim 32 or claim 38, wherein in step (c) the emulsifier is present in a concentration from about 0.05% to about 5%.
40. The process of claim 32, wherein in step (d) the heating is conducted at about 80°C for about 6 hours.
41. The process of claim 32, wherein in step (e) said oil is removed from said spherical particles of crosslinked polyvinylalcohol by extraction with a light non-polar solvent or chlorinated solvent.
42. The process of claim 41, wherein the light non-polar solvent or chlorinated solvent is methylene chloride.
43. The process of claim 32, wherein in step (f) said active aldehyde on said spherical particles of crosslinked polyvinylalcohol is neutralized by an aminoalcohol.
44. The process of claim 43, wherein said aminoalcohol is selected from the group consisting of Tris, 2-aminoethanol, aminosorbitol and glucosamine.
45. The process of claim 32, further comprising adding a cell adhesion promoter to the acidic polyvinylalcohol solution before adding the aldehyde.
46. The process of claim 45, wherein the cell adhesion promoter is selected from the group consisting of CM
dextrin, collagen, DEAE dextrin, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agents and a synthetic biological cell adhesion agent.
dextrin, collagen, DEAE dextrin, gelatin, glucosaminoglycans, fibronectin, lectins, polycations, a natural biological cell adhesion agents and a synthetic biological cell adhesion agent.
47. The process of claim 32, further comprising absorbing a marking agent into the crosslinked polyvinylalcohol-containing microspheres.
48. The process of claim 47, wherein the marking agent is selected from the group consisting of a dye, an imaging agent and a contrasting agent.
49. The process of claim 32, further comprising absorbing an anti-angiogenic agent into the crosslinked polyvinylalcohol microspheres.
Applications Claiming Priority (3)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
FR9813019A FR2784580B1 (en) | 1998-10-16 | 1998-10-16 | POLYVINYL-ALCOHOL MICROSPHERES AND METHODS OF MAKING THE SAME |
FR98/13019 | 1998-10-16 | ||
PCT/EP1999/007846 WO2000023054A1 (en) | 1998-10-16 | 1999-10-15 | Polyvinyl alcohol microspheres, and methods for making and therapeutic uses of the same |
Publications (1)
Publication Number | Publication Date |
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CA2345205A1 true CA2345205A1 (en) | 2000-04-27 |
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Application Number | Title | Priority Date | Filing Date |
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CA002345205A Abandoned CA2345205A1 (en) | 1998-10-16 | 1999-10-15 | Polyvinyl alcohol microspheres, and methods for making and therapeutic uses of the same |
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US (4) | US6680046B1 (en) |
EP (1) | EP1128816B1 (en) |
JP (1) | JP4467799B2 (en) |
AT (1) | ATE262319T1 (en) |
AU (1) | AU1039600A (en) |
CA (1) | CA2345205A1 (en) |
DE (1) | DE69915858T2 (en) |
ES (1) | ES2219072T3 (en) |
FR (1) | FR2784580B1 (en) |
WO (1) | WO2000023054A1 (en) |
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-
1998
- 1998-10-16 FR FR9813019A patent/FR2784580B1/en not_active Expired - Fee Related
-
1999
- 1999-10-15 JP JP2000576829A patent/JP4467799B2/en not_active Expired - Lifetime
- 1999-10-15 ES ES99953858T patent/ES2219072T3/en not_active Expired - Lifetime
- 1999-10-15 US US09/419,114 patent/US6680046B1/en not_active Expired - Lifetime
- 1999-10-15 EP EP99953858A patent/EP1128816B1/en not_active Revoked
- 1999-10-15 WO PCT/EP1999/007846 patent/WO2000023054A1/en active IP Right Grant
- 1999-10-15 AT AT99953858T patent/ATE262319T1/en not_active IP Right Cessation
- 1999-10-15 CA CA002345205A patent/CA2345205A1/en not_active Abandoned
- 1999-10-15 DE DE69915858T patent/DE69915858T2/en not_active Expired - Lifetime
- 1999-10-15 AU AU10396/00A patent/AU1039600A/en not_active Abandoned
-
2003
- 2003-10-27 US US10/692,785 patent/US7591993B2/en not_active Expired - Fee Related
-
2009
- 2009-01-05 US US12/348,867 patent/US7670592B2/en not_active Expired - Fee Related
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- 2010-01-12 US US12/686,320 patent/US8673266B2/en not_active Expired - Fee Related
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US7670592B2 (en) | 2010-03-02 |
US8673266B2 (en) | 2014-03-18 |
ATE262319T1 (en) | 2004-04-15 |
JP4467799B2 (en) | 2010-05-26 |
DE69915858D1 (en) | 2004-04-29 |
US20090117196A1 (en) | 2009-05-07 |
WO2000023054A1 (en) | 2000-04-27 |
DE69915858T2 (en) | 2005-03-03 |
ES2219072T3 (en) | 2004-11-16 |
FR2784580A1 (en) | 2000-04-21 |
FR2784580B1 (en) | 2004-06-25 |
AU1039600A (en) | 2000-05-08 |
EP1128816B1 (en) | 2004-03-24 |
US20040091425A1 (en) | 2004-05-13 |
EP1128816A1 (en) | 2001-09-05 |
US20100119572A1 (en) | 2010-05-13 |
US7591993B2 (en) | 2009-09-22 |
US6680046B1 (en) | 2004-01-20 |
JP2002527206A (en) | 2002-08-27 |
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