WO1993018146A2

WO1993018146A2 - Proteins forming complexes with chaperones and ligands thereof, fragments thereof, preparation thereof and biological uses thereof

Info

Publication number: WO1993018146A2
Application number: PCT/FR1993/000219
Authority: WO
Inventors: Marie-Claire Lebeau; Nelly Massol; Michel Renoir; Christine Radanyi; Jean-Paul Mornon; Isabelle Callebaut; Etienne-Emile Baulieu; Béatrice CHAMBRAUD
Original assignee: Institut National De La Sante Et De La Recherche Medicale (I.N.S.E.R.M.)
Priority date: 1992-03-04
Filing date: 1993-03-04
Publication date: 1993-09-16
Also published as: FR2688227A1; WO1993018146A3

Abstract

Nucleotide sequences capable of hybridizing with the nucleotide sequence shown in figure 1, and the corresponding coded amino acid sequences, are disclosed. Said nucleotide sequences are particularly suitable for detecting complementary sequences in biological samples.

Description

PROTEINS FORMING COMPLEXES WITH CHAPERONES AND THEIR LIGANDS, THEIR FRAGMENTS, THEIR PRODUCTION AND THEIR BIOLOGICAL APPLICATIONS.

The invention relates to immunophilin proteins, p59 and related proteins, forming complexes with chaperones and their ligands.

It relates more particularly to the sequences of nucieotides encoding proteins related to those of these complexes, or to fragments of these proteins, as well as to the corresponding proteins and fragments.

The invention also relates to the biological applications of these nucieotide and protein sequences, in particular for research and study of new pharmacological ligands for immunophilin as well as for clinical diagnosis.

The term chaperone protein denotes proteins associated with other biologically active proteins with which they interact and modify their functioning. The invention relates in particular to proteins forming complexes with the hsp90 chaperone which is a heat shock protein capable of binding with numerous ligands such as the receptors for steroid hormones, vitamin D, and dioxin and such as tyrosine inases of viral oncogenes (for example ppδOsrc), actin, tubulin and other proteins whose structural change and intracellular traffic are important for the physiology and pathology of the cell. In the context of work on steroid hormone receptors, some of the co-inventors of the present application have described the binding of hsp90 to steroid hormone receptors and its role in preventing the interaction of these receptors with DNA (see Joab et al., 1984, Nature, 308, 840, 853 and Catelli et al., 1989, EMBO J.4, 3131-3135).

A protein of molecular weight 59kDa has also been characterized in rabbits during the purification of these receptors. In the absence of a ligand, the receptors for all steroid hormones are found associated in the cell with other proteins which do not bind the hormone, constituting the non-activated form of these receptors. The separation of proteins will release the receptor itself which will then be able to interact with DNA (Baulieu et al., 1971, Rec. Progr. Horm. Res. 27, 351-419 and Sherman et al., 1984, Ann. Rev Physiol. 46, 83-125).

The structures and sequences of these p59 type proteins have not been elucidated to date, their function in the cell could not be precisely defined.

By screening a rabbit liver c-DNA library, the inventors succeeded in isolating and sequencing clones containing a sequence of nucieotides capable of coding for a protein homologous to the rabbit p59 protein as it has was defined by its immunoreaction with the monoclonal antibody KN382 / EC1. (Nakao et al., 1985, Can. J. Biochem. Cell. Biol. 63, 33-40).

The object of the invention is therefore to provide such nucieotide sequences as well as the amino acid sequences expressed or deduced from the nucieotide sequences.

It also aims to obtain these different sequences.

The invention also aims to provide polyclonal and monoclonal antibodies directed against these proteins or protein fragments obtained.

According to another aspect, the invention relates to the use of the sequences of nucieotides or proteins, or antibodies, in biological applications, in particular for diagnostic purposes.

The nucieotide sequences of the invention are characterized in that they include or are formed by a sequence of nucieotides capable of hybridize under stringent conditions with one or more sequences of a gene whose cDNA has a sequence corresponding to the sequence (I) of nucieotides. The sequences of the nucieotide and protein sequences to which reference is made in the description and the claims are given at the end of the description.

The expression "stringent conditions" as used in this text means that a hybridization is obtained by operating according to the conditions described by Sambrook, Fritsch Maniatis in "Molecular Cloning", 1989.

According to a provision of the invention, the nucieotide sequences are characterized in that they contain the genetic information to code for all or part of the protein responding to sequence II.

Sequences of this type are characterized in that they are formed, or that they comprise, at least part of the sequence I.

The invention relates in particular to sequences of nucieotides constituted by a part or the whole of the open reading frame going in the sequence (I) from position 4 to position 1380.

This sequence, without the leader sequence, has 2067 base pairs. Such sequences are further characterized in that they are capable of coding for a potential protein of 458 amino acids responding to sequence II.

Sequences of great interest include the genetic information to code for one or more amino acid sequences of sequence II corresponding to a region of this sequence capable of binding with an immunosuppressant of the FK 506 type having the structural characteristics for a rotamase activity.

Other preferred sequences include genetic information to code for one or more sequence II amino acid sequences corresponding to a region capable of binding to ATP (adenosine triphosphate) / GTP (guanosine triphosphate).

Still other preferred sequences include

Genetic information to code for one or more sequence II amino acid sequences corresponding to a region capable of binding to calmodulin

According to another aspect, the invention relates to a recombinant sequence comprising one of the sequences defined above, optionally associated with a promoter capable of controlling the transcription of the sequence and a DNA sequence coding for the termination signals of the transcription.

Such sequences advantageously contain sequences coding for chaperones.

Preferred sequences of this type contain coding sequences for hsp90, in particular for the hydrophilic region A, of this negatively charged protein (Binart et al., J. Steroid. Biochem. 1989, vol. 34, no. 1) , 369-374).

The purine and pyrimidine bases of the nucieotide sequences under consideration may have a different order than that found in the cloned cDNA and / or if appropriate, may be substituted. It is understood that such sequences fall within the scope of the invention, when a fragment of these sequences used as a probe gives rise to hybridization with a gene coding for proteins as defined above.

The invention also relates to the RNAs and the complementary sequences of the various defined nucleotide sequences as well as the corresponding coded proteins.

The invention also relates to recombinant cloning and expression vectors capable of transforming an appropriate host cell, comprising at least part of a nucieotide sequence as defined above, under the control of regulatory elements allowing his expression. The strains of transformed or transfected microorganisms also fall within the scope of the invention.

These strains comprise one of the nucieotide sequences defined above or else a recombinant vector as defined above.

The invention also relates to the amino acid sequences deduced, according to the universal genetic code, from the nucieotide sequences defined above, and the proteins expressed by the genes comprising these sequences. Sequences according to the invention, which are of great interest with regard to the applications envisaged in diagnosis, are characterized in that they correspond to sequences capable of binding to heat shock proteins or that they have the properties of such proteins .

According to another advantageous arrangement of the invention, these are sequences capable of binding to hsp90, even when hsp90 is involved in hetero-oligomeric complexes with other proteins as indicated above. These may be complexes involved in the formation of steroid receptors or in other complexes, for example with oncogenes and proteins of the cytoskeleton.

The complexes of these protein sequences with hsp90 or with other heat shock proteins involved in these hetero-oligomers, or with regions of these different proteins, are also part of the invention.

According to another arrangement of the invention, if necessary taken in combination with at least one of the above, the amino acid sequences are characterized in that they have one or more domains of the type of FKBP, identical or different from each other. The corresponding proteins will hereinafter be called HBI proteins, that is to say proteins of the immunophilin type binding heat shock proteins. FKBP is an immunophilin that binds at least two immunosuppressive drugs, namely FK506 and rapamycin.

Such amino acid sequences are more particularly characterized in that they have the structural characteristics for binding with an immunosuppressant of the FK506 type and for peptidyl-prolyl isomerase cis-trans activity.

The amino acid sequences of the invention, according to another provision of the invention, taken if appropriate in combination with at least one of the above, include an ATP binding site.

According to another aspect, the amino acid sequences of the invention are characterized in that they comprise a consensus sequence of binding to calmodulin.

According to yet another aspect, the amino acid sequences are characterized in that they correspond to the hinge regions between two domains. They are more specifically hydrophilic regions, accessible to proteolytic enzymes.

In an alternative embodiment of the invention, amino acid sequences of the FKBP type comprise or are formed by only one of the FKBP type domains. In another variant, they comprise or are formed by two of these areas, identical or different, connected by a hinge.

In yet another variant, the amino acid sequences comprise or are formed by a plurality of identical or different sequences corresponding to one of the domains of the FKBP type.

In these different variants, these are domains having a very strong three-dimensional (3D) structure homology with FKPB of the order of 80 to 100%, or domains having a lower homology, in particular of the order of 35 to 80% or even 25 to 35% approximately.

The amino acid sequences of the invention are also characterized in that they are such that obtained by transformation of host cells using a recombinant vector as defined above, culturing, in an appropriate medium, transformed or transfected host cells and recovery of the protein from these cells or directly from culture medium.

The proteins or sequences of the invention can therefore possibly be in the form of fusion proteins. The production of these proteins by such a process also forms part of the invention.

The proteins of the invention and their fragments, which can also be obtained by chemical synthesis, advantageously have a high degree of purity and are used to form, according to conventional techniques, polyclonal antibodies and monoclonal antibodies.

Such polyclonal antibodies, as well as monoclonal antibodies capable of specifically recognizing an epitope of the above amino acid sequences, or of a fragment of these sequences by giving rise to an antigen-antibody type reaction, are also targeted by the invention.

Antibodies of great interest are directed against one of the domains of the HBI proteins and are therefore useful for detecting the receptors of immunosuppressants and can serve to inhibit the function exerted by this domain.

The invention further relates to the biological applications of the nucieotide sequences, of the corresponding proteins and of the monoclonal or polyclonal antibodies.

These applications include the development, from purified intragenic fragments, or from corresponding RNA, of molecular probes to search for the possible presence in various cell types of sequences of nucieotides related to the gene capable of coding for proteins associated with hsp90 in hetero-oligomeric complexes as indicated above. The development of these probes includes, in particular the denaturation of the double-stranded sequences to obtain a single-stranded sequence.

The tests carried out to detect the presence of complementary sequences in various tumors and tissues in humans or animals have demonstrated the great specificity of these intragenic fragments.

The use of these probes has thus made it possible to show that the gene containing the nucleotide sequences defined above is expressed in mammals.

The invention therefore relates to detection probes characterized in that they comprise at least part of a sequence of nucieotides defined above.

Substitutions or alterations of nucieotides can be made in these sequences, provided that the corresponding probe is capable of hybridizing with the gene for the HBI protein as defined above.

The construction of the probe is advantageously carried out according to conventional techniques, in particular a sufficient number of nucieotides is used to obtain the required specificity and the formation of a stable hybrid.

It is possible to use fragments reaching several kb, results of high specificity being however also obtained with shorter fragments of approximately 20 to 40 nucieotides.

These probes are advantageously marked with a group allowing their recognition in a hybrid state with the preparation containing the nucieotides to be studied.

According to conventional techniques, these probes are brought into contact with the biological sample to be tested or their nucleic acids, under conditions allowing hybridization between the nucieotide sequence of the probe and a complementary sequence, when it is contained in the product studied. One can, for example, have recourse to the method of hybridization on spots or to the method of hybridization on replica, according to the technique of Southern. In the first method, according to the conventional technique, a aliquot of denatured DNA on nitrocellulose membranes. The second method comprises the electrophoretic separation in agarose gel of the DNA fragments generated after treatment of the DNA with restriction enzymes, the transfer after alkaline denaturation on appropriate membranes and their hybridization with the probe under the usual conditions.

These probes constitute markers by allowing the early detection of the expression of the gene containing HBI, that is to say capable of expressing the protein of sequence II, which normally is little or not expressed in the tissues corresponding normal. The invention thus provides means for assessing tumor development and / or differentiation. The invention also relates to a method for detecting in vitro the presence in a biological sample of sequences complementary to those defined above.

This method is characterized in that it comprises the steps of: - bringing the sample to be studied into contact with a nucleotide probe as defined above, under conditions allowing hybridization between the probe and the desired nucieotide sequence , and

- detection of the hybridization complex. This method allows rapid and highly specific detection of DNAs and different species of transcription mRNA.

It allows in particular the screening of a bank of diseased tissues, the study of the development of tumor differentiation and the early detection of the expression of the gene for the HBI protein.

The method defined above for in vitro detection, based on the use of nucleotide probes, is advantageously implemented using kits comprising: - a determined quantity of a nucleotide probe according to the invention, - a medium suitable for hybridization between the probe used and the sequence to be detected, and advantageously, reagents allowing the detection of the hybridization complexes formed.

The invention also relates to the immunological applications of the amino acid sequences defined above, more especially for the development of specific antisera as well as polyclonal and monoclonal antibodies.

The polyclonal antibodies are as induced according to conventional techniques by injection of the amino acid sequences into animals, followed by the recovery of the antisera then, from the latter, if desired antibodies, for example by chromatography of 'affinity.

Monoclonal antibodies are produced in the usual way by fusing myeloma cells with spleen cells from animals previously immunized with the proteins of the invention. In this respect, one operates advantageously according to the technique described by Kôhler and Milstein in Nature, vol 256, p 495, 1975.

The antibodies of the invention make it possible to detect in vitro the products of expression of the nucleotide sequences defined above or those of the genes coding for a heat shock protein related to those of the heterooligomeric complexes defined above, in particular steroid receptors.

The in-vitro screening method in a biological sample for the possible presence of these expression products is characterized in that it comprises:

bringing the sample to be studied into contact with an antibody according to the invention, under conditions allowing the formation of an immunological complex between all or part of the proteins expressed by the nucleotide sequences and this antibody, and

- detection of the immunological complex. For this in vitro screening method _r advantageously use kits, comprising: - a determined quantity of a polyclonal or monoclonal antibody according to the invention, - a medium suitable for carrying out an immunological reaction between at least one part of the products expressed and the antibody and, advantageously, of the reagents allowing the detection of the immunological complexes formed. The amino acid sequences defined above also constitute tools of great interest for the study and / or regulation of the functions of proteins associated with said complexes.

The invention thus provides very effective means for studying and preventing or treating pathologies linked to the dysfunction of proteins associated with the hetero-oligomeric complexes mentioned above.

Mention will be made, for example, of diseases of the immune or autoimmune system, cancers, deficiencies in vitamin D responsible for rickets, or in retinoic acid or even intoxication by dioxin or related products.

These means, whether polynucleotides, amino acid sequences or antibodies also allow the localization of proteins associated with the hetero-oligomeric complexes described above.

It was thus possible to note that the natural protein associated with hsp90 in these complexes is localized in the nucleus of normal tissue cells whereas in tumor cells, it appears abundantly in the cytoplasm. The use of the means of the invention therefore makes it possible to make significant localization differences in pathologies. According to another aspect of great interest, they also make it possible to find natural ligands capable of occupying the binding sites recognized by the immunosuppressants. The HBI proteins are useful for the search for new reagents and drugs which bind to this protein, and which can influence the functioning of the heat shock protein and the proteins associated with it on receptors for steroid hormones and other ligands for receptors for the same family, on the activity of oncogenes having protein kinase activity, on the structure and functioning of cytoskeleton proteins and any protein associated with hsp90. This results in applications of great interest in the endocrine, cancer and immunological fields.

In the examples which follow, other characteristics and advantages of the invention are reported.

In these examples, reference is made to FIGS. 1 to 7 which respectively represent:

FIG. 1, the rabbit liver cDNA sequence coding for an HBI protein and the corresponding amino acid sequence,

FIG. 2, the representations established by the method of analysis of hydrophobic clusters (ACH) of the domains of an HBI protein compared to the FKBP and to domains of the FKBP type identified in various proteins,

FIGS. 3 and 4, the ACH representations of human FKBP and of the HBI protein and the alignments of the corresponding amino acid sequences,

FIG. 5, a representation of the structure of the domains of pHBI using the main chain of FKBP as a matrix,

FIG. 6, a schematic representation of the main characteristics of pHBI, FIG. 7, a diagram representing the construction of a cassette for the production of fragments of pHBI, and

- Figure 8, the results of a Western blot performed with an anti-HBI polyclonal antibody

The invention. Example 1: Cloning and sequencing of the cDNA coding for an HBI protein.

For the purpose of cloning a rabbit liver cDNA library, probes are constructed from oligonucleotides whose sequence has been deduced from that of a fragment of 19 amino acids corresponding to the sequence:

ALA GLU GLU MET LYS ALA THR GLU SER GLY ALA GLN X ALA PRO LEU PRO MET GLU

It is the fragment of the N-terminal part of a protein identified in complexes of unprocessed steroid receptors described by Sanchez et al. in Biochemistry 1990, 29, 5145-5152. The construction of the probe is carried out by operating according to the aforementioned work of Maniatis Volume 2, chapter 11 "Synthetic oligonucleotidic probes".

The screening of the cDNA library is carried out according to the method described in chapter 8 of the abovementioned book "Construction and analysis of cDNA libraries".

The longest positive clone cDNA is isolated and subcloned into pGEM 7Zf (Promega Biotec), transcribed and translated into a rabbit reticulocyte lysate system. Transcription and translation are carried out as described by the manufacturer of the plasmid in the presence of 35s methionine.

The cDNA subcloned into the vector pGEM 7Zf is digested with exonuclease III to generate deletion subclones which are then sequenced using the T7 RNA polymerase promoter as a primer. The cDNA can also be subcloned into the vectors M13 MP 18/19 and sequenced according to the conventional technique as described for example in the aforementioned work by Maniatis.

The nucieotide sequence and the amino acid sequence derived from the entire open reading frame are reported in Figure 1. The underlined sequence corresponds to that used to generate the polyclonal antibody discussed below in Example 3 . The dotted line indicates the region corresponding to the site of interaction with calmodulin.

Ex mpl 2: Study of the HBI protein, hereinafter called pHBI, by the method of analysis of hydrophobic clusters (abbreviated ACH)

MATERIAL AND METHODS

Hydrophobic cluster analysis strategies

2D (ACH) and their applications were first proposed by Gaboriaud et al., 1987, FEBS Lett. 224, 149, 155 and are described in detail by Lemesle-Varloot et al., 1990, Biochemistry, 72, 555-574. ACH is a method using the general principles of protein folding. It is based on the search for successive correspondences of hydrophobic clusters which are relevant to the secondary structure and the 3D folding of the protein domains. In related proteins, it is possible to deduce precise alignment of sequences from ACH representations by proceeding from the hydrophobic nucleus of similar clusters to regions linking clusters (loops) where insertions / deletions are allowed.

For these HCA alignments, a numerical value (HCA score) can be calculated between the clusters to determine the alignments.

The 3D studies were carried out with the MANOSK program (Cherfils et al. 1988, J. Mol. Graph. 6, 155-160) on Evans & Sutherland PS390.

The analysis of the pHBI shows that it comprises, starting from the N-terminal end, three successive domains. , Identification of immunophilin domains: pHBI I and pHBI II domains.

Figure 2 gives aligned, ACH representations of human FKBP (FKBPh) and domains I and II of pHBI. This figure also mentions the FKBP type domains already identified in other proteins. It is the RBP1 protein binding rapamycin from Saccharomyces cerevisiae (Koltin et al. 1991, Mol. Cell Biol. 11, 1718-1723), the FKBP from Neurospora crassa (Tropschug et al. 1990, Nature, 346, 674 -677, a cryptic sequence of Neisseria meningiditis (Perry et al. 1988, J. Bact. 170, 1691-1697), a 25.3 kDa protein from Pseudomonas aeruginosa (n ° JQ 0140), the cell surface protein mip from Legionella pneumophila (Engleberg et al. 1989 Inf. Immunity 57, 1263-1270), the L2 protein of Chlamydia trachomatis (Lundemose et al. 1991, Mol. Microbiology 5, 109-115).

Hatched hydrophobic clusters highlight anchor points for sequence alignments.

The secondary structure of the FKB h is indicated above its sequence in accordance with the description of the 3D structure. The β sheets are indicated by the symbols O ^ ^and ^are helices α by UH-X.

The black columns indicate the conserved residues, the gray columns and with dotted lines the hydrophobic and hydrophilic homologous residues and those open those particularly rich in P, G, S, T and / or A. Amino acids (main and / or side chains ) which are essential for the binding of FK506 to FKBP and are fully conserved for p59 I are indicated by arrows. Parentheses have been mentioned when alignment between amino acids is not possible. Analysis of this figure shows that the pHBI comprises two successive domains of approximately 100 residues (pHBI I and pHBI II) having a strong homology with the FKBP.

The first domain has a sequence identity of 49% with FKBP without the introduction of deletion or insertion.

The second domain has a 28% sequence identity with FKBP and comprises 4 insertion or deletion zones totaling 9 amino acids. These domains are assigned, in view of their structural homology with FKBP, a topology for folding anti-parallel β sheets, accompanied by an α helix and an additional β sheet. Reference is made to this β sheet as being of type A (chains A1 to A5).

In FIG. 3, the graphical representations according to ACH of the human FKBP and of the segmented pHBI are reported so as to show its internal symmetry. Above the representation of the FKBP, we indicate as in Figure 2, its secondary structure.

The protein sequences are drawn on a conventional α helix flattened on a cylinder, cut parallel to its axis and unrolled to provide a two-dimensional representation.

The representation is doubled vertically to restore a complete two-dimensional environment for each amino acid.

A group of hydrophilic amino acids (VILFWMY) are surrounded in clusters. The classic letter code is used for all amino acids, except for P

(designated by a star) which is a cluster switch, G (designated by a diamond-shaped symbol) which shows great conformational flexibility and T and S (open and dotted squares respectively) which are frequently encountered in loops, but can also be found in hydrophobic environments where

The hydrophilicity of their hydroxyl groups is neutralized by hydrogen bonds with the main chains. The box reproducing the N-terminal part of the pHBI also indicates how the sequence is read linearly (see slightly oblique arrow).

The vertical lines delimit the segmentation of the structures (SI to S6) inside the domains.

Hatched hydrophobic clusters highlight anchor points for sequence alignments. The examination of FIG. 3 shows that the classic segmentation of the globular domains into regular secondary structures (β sheets and α helices), statistically centered on the hydrophobic clusters of the representations according to ACH and in the loops linking these structures is clearly preserved for FKBP, pHBI I and pHBI II.

There is an overall similarity centered on the S4 segment, between pHBI I, pHBI II and an extension of sequence according to pHBI II.

This extension is attributed to a third globular domain of pHBI (pHBI III).

Using the S4, S5 and S6 graphical representations according to ACH of the pHBI I and pHBI II domains as anchor points, amino acid by amino acid alignment was carried out.

These alignments are shown in Figure 4.

The pressed lines represent the nuclei limits of the sequences of the third domain of pHBI (pHBI III) used to establish the alignments statistically.

Their dimensions are 8, 7, 2, 23, 6, 12 amino acids for the pHBI III / pHBI II comparisons and 6,8,3,27,7,11 amino acids for the pHBI III / pHBI I comparisons, at namely 58 and 62 amino acids respectively.

Above and below, the circle identities and the conservative mutations for pHBI III / pHBI II and pHBI III / pHBI I have been indicated by solid circles and bars. A sequence identity of approximately 13% is observed between the pHBI III and pHBI II domains.

The pHBI III domain has a 10% sequence identity with the pHBI I domain.

A comparison between pHBI III and the two other domains of pHBI makes it possible to establish a relationship between them, based on the following observations: - the positions of the insertions and deletions present between the pHBI I and pHBI II domains are all preserved,

the pHBI III also shares 13% of sequence identity with the L2 protein of the FKBP type of Chlamydia trachomatis, the sequence of which is reported in FIG. 2. In this sequence, an extension of 21 amino acids (273-293 of pHBI III and 135-152 of L2) has 45% identity with pHBI III.

Main characteristics of the pHBI domains.

Reference will be made in the following to FIGS. 2 and 3 already considered and to FIG. 5 which gives a representation of the complete structure of pHBI I using as matrix the main chain of FKBP in the form of a ribbon (it will be noted that there are no insertions or deletions between the domains of these two proteins). The numbering of pHBI I residues is indicated five by five.

The FK506 ligand linked to FKBP was kept as reference (balls).

The side chains of amino acids that can be critical for a hypothetical binding of a ligand similar to FK506 are fully represented (see Fig. 2). The specificities of the pHBI II domain are underlined:

1 / shortening (4 amino acids) of the 38-45 loop (FKBP numbering), 2 / lengthening (3 amino acids) of the 55- loop

56 (ATP binding site,

3 / insertion (an amino acid) into the 87-90 loop (ATP phosphate stabilization),

4 / deletion (an amino acid) in the loop 31-35. PHBI I: No deletions or insertions are observed in pHBI I with respect to FKBP. All the main or secondary chains involved in the binding of FK506 by FKBP are conserved in the domain of pHBI I.

Indeed, it can be noted that the replacement of FKBP Q53 by a glycine in HBI I does not modify the interaction of the corresponding main chain CO with the ligand, if it exists.

Similarly, the replacement of H87 with a serine seems to have only a weak influence since it interacts by a Van der Waals contact at a rather long distance (3,8-4A).

A similar mutation (alanine) occurs in the same place for the human protein FKBP13. Consequently, all the structural requirements related to the catalytic site of FKBP appear preserved in pHBI I. pHBI II: Although the domain of p59 II is clearly related to the matrix of FKBP, it has specific characteristics as shown in the figures 2, 3 and 5. 1/8 of the 12 essential amino acids for the binding of FK506 to FKBP are not conserved.

2 / The v55 _ τ.56 loop (β / α type loop - FKBP numbering) of FKBP is extended by 3 amino acids making it impossible to maintain the binding of a ligand similar to FK506, since these residues are in contact with the very important pipecolinyl cycle of FK506 (deepest part of the active site).

3 / The loop 87-90 (loop A2-A3) is largely modified with elongation of an amino acid and introduction of basic residues, (see symbol in snowflakes in figure 5).

4 / The well exposed omega loop from 38 to 45 (loop

A5-β) is shortened by 4 amino acids (large star), leading to a direct link between positions 39 and 45 via a continuous β chain connecting A5 and β

(see figures 2 and 5).

5 / Loop 31-35 (loop A4-A5) is slightly modified by a deletion (G33; small star) pHBI III: this domain shares with pHBI II the same distribution of insertions and deletions with respect to the first domain and has a sequence significantly related to this first domain. However, it lacks many of the characteristics of FKBP that appear in the first two areas. All essential amino acids for binding to FK506 have been mutated and the sequence identity with FKBP is only 5.7%. Hinge regions - N and C terminal regions.

The hinge regions linking the above globular domains are indicated in FIGS. 2, 3 and 6.

Figure 6 gives a schematic representation of the main structural characteristics of pHBI with indication of the sequence identities of pHBI II (26%) and pHBI I (13%) compared to pHBI I (100%).

As shown in the figures above, the hinge 1 connects pHBI I and pHBI II via 10 strongly hydrophilic and acidic amino acids. Hinge 2 links pHBI II and pHBI III via 13 mainly acidic residues.

The pHBI has a short N-terminal part before pHBI I and is after pHBI III a longer C-terminal part.

F ^χ epp, ^ 3: Obtaining fragments of pHBI:

Given the domain structure of the pHBI protein, its cDNA was cut into 4 fragments corresponding to the different domains. These fragments were subcloned into vectors allowing their expression either in E.Coli, or in mammalian cells, or in a lysate of reticulocytes. The division strategy allows each domain to be recombined with all the others.

The expressed proteins, corresponding to one, two or three domains, make it possible to determine the functions of each domain independently, as well as the influence of one domain on the other. The peptidyl-prolyl isomerase activity of these truncated proteins, expressed in the form of a fusion protein with glutathione-S-transferase, has been studied as well as their binding to immunosuppressants. The site of association of the pHBI with the heat shock protein hsp90 was sought by expressing these mutated proteins in a reticulocyte lysate or in mammalian cells. It was also possible to determine in which domain the epitope of the monoclonal antibody KN382 EC-1 which is mentioned in the beginning of the description is found. These proteins corresponding to the isolated domains have similar or different properties to FKBP12. The latter mainly resembles the HBI-1 domain, which contains an active binding site for immunosuppressants. The domains of pHBI could explain certain side effects observed in vivo during the administration, for immunosuppressive purposes, of FK 506 and rapamycin. We will measure the great interest, both pharmacological and therapeutic, of isolated domains as reagents to study these effects. The antibodies generated against the isolated domains make it possible, for example, to inhibit a function corresponding to one or the other domain.

MATERIAL AND METHODS

In the cDNA coding for the pHBI protein, cloned into the vector pGEM 72f at the Eco RI site, 5 restriction sites were introduced by site-directed mutagenesis at the N and C ends of the different domains of the protein.

These restriction sites were chosen so that they do not exist in the cDNA or in the vector, that they are compatible with each other, and that they do not change the reading phase of the protein.

The Eco RV site was introduced into the N-terminal part of the protein, just after the initiator codon Met; the Bail site was introduced into the terminal C part of the protein, just after amino acid 458 and before the STOP codon. The Hpal, NruI, and Eco47III sites were introduced respectively between amino acids 148 and 149, between 267 and 268 and between 374 and 375 as indicated in FIG. 7.

From this molecule constructed in cassette, the different independent domains were obtained by the classic subcloning technique (see the work "Molecular Cloning" by Sambrook, Fritsch and Maniatis mentioned above). After hydrolysis of this cassette molecule by Hpal and Bail, the fragment of 4100 base pairs corresponding to the vector pGEM 72f, plus the first domain was ligated and transformed in E.Coli to obtain the first domain. The second domain was obtained by ligating the 350 base pair Hpa I-Nru I fragment with the Eco RV-Bal I fragment of the cassette molecule. This process was applied to obtaining the other domains.

Domains I, II, III, IV were thus constructed independently, as well as domains I + II, III + IV, I + II + III, II + III and II + III + IV (see Figure 7). The sequences of these constructions have been verified (Sanger technique). When expressed in the rabbit reticulocyte lysate, the size of the proteins obtained corresponded to this expected. Some of these constructions have been subcloned at the Eco RI site, either in the vector pGEX 1 \ T (Pharmacia) in order to be able to express them in large quantities in E.Coli as a fusion protein with glutathione-S-transferase, or in the vector pSG5 (Stratagene) which allows transient expression in Cos cells (established line of monkey kidney cells transformed by SV40).

Ex-am l. =. 4: Preparation of anti-HBI antibodies

The amino acid sequence of the terminal carboxy part of the sequence II going from position 441 to 458 is used. This peptide fragment is coupled to KLH and injected into rabbits according to the usual techniques.

The IgG fractions recovered are purified by precipitation with ammonium sulphate and ion exchange chromatography with each bleeding.

Polyclonal antibody preparations are used either for immunoblot analysis or for density gradient analysis to study their ability to recognize pHBI in different tissues and species, as well as in the heterooligomeric structure of progesterone .

The Western blot results are reported in FIG. 8, with different samples, namely rabbit uterus cytosol (lane 1, 10 μl), rat hepatoma cells (lane 2) and human cell cytosols HeLa (lane 3) subjected to electrophoresis after ion exchange chromatography.

The position of the markers is indicated on the left of the figure. HC designates the heavy chains of rabbit immunoglobulins detected by a second anti-rabbit antibody.

With the anti-HBI antibody used, a single band at 59 kDa is observed at the same position as that recognized by EC1 (see reference by Nakao et al. Above). This antibody also reacts with human protein and recognizes a protein of the same size in rats, which is not detected by EC-1.

Sequences

1: sequence of nucieotides sequence I

10 20 30 40 50 60

GCCATGACCG CCGAGGAGAT GAAGGCGGCC GAGAGCGGGG CGCAGTCGGC GCCGCTGCCC

70 80 90 100 110 120

CTCGAGGGCG TGGACATCAG CCCCAAGCAA GACGAAGGCG TGCTGAAGGT CATCAAGCGA

130 140 150 160 170 180 GAGGGCACAG GCACCGAGAC ACCCATGATC GGGGACCGAG TCTTTGTCCA CTACACTGGC

190 200 210 220 230 240 TGGCTCTTGG ATGGCACGAA GTTTGACTCC AGTCTGGACC GCAAGGACAA ATTCTCCTTT

250 260 270 280 290 300 GACCTGGGAA AAGGGGAGGT CATCAAGGCT TGGGACATTG CTGTTGCAAC CATGAAGGTG

310 320 330 340 350 360 GGGGAATTGT GCCGCATCAC CTGCAAACCC GAATATGCCT ACGGTTCGGC AGGCAGCCCT

370 380 390 400 410 420 CCAAAGATCC CCCCCAACGC CACACTTGTG TTCGAGGTGG AATTGTTTGA GTTCAAGGGA

430 440 450 460 470 480 GAGGATCTGA CAGACGACGA AGACGGCGGA ATCATCCGCA GAATACGGAC TCGGGGTGAA

490 500 510 520 530 540 GGCTATGCTA GGCCCAACGA TGGTGCTATT GTGGAGGTCG CACTGGAAGG GTACTACAAG

550 560 570 580 590 600 GACCGGCTCT TTGACCAGCG GGAACTCCGC TTTGAGGTCG GCGAGGGGGA GAGTCTGGAT

610 620 630 640 650 660 CTGCCTTGTG GGCTAGAGAA GGCCATTCAG CGCATGGAGA AAGGCGAACA TTCCATCTTG

670 .680 690 700 710 720 TACCTCAAGC CCAGTTACGC GTTTGGCAAT GCTGGGAAGG AAAAGTTTCA GATCCCGCCA

730 740 750 760 770 780 TATGCTGAGC TGAAATATGA AGTCCACCTC AAGAGTTTTG AGAAGGCCAA GGAGTCCTGG

790 800 810 820 830 840 GAGATGAGCT CGGAGGAGAA GCTGGAGCAG AGCGCCATCG TGAAAGAGCG AGGCACCGTG

850 860 870 880 890 900 TACTTCAAGG AAGGCAAGTA CAAGCAGGCT CTGCTACAGT ACAAGAAGAT TGTGTCTTGG

910 920 930 940 950 960 CTGGAATACG AGTCAAGTTT TTCCAGTGAG GAAGTGCAAA AGGCACAGGC CCTGCGCCTG

970 980 990 1000 1010 1020

GCCTCCCACC TCAACCTGGC TATGTGTCAC CTGAAGCTAC AGGCCTTCTC GGCAGCCGTG

1030 1040 1050 1060 1070 1080

GAAAGCTGTA ACAAGGCCCT GGAACTGGAC AGCAACAACG AGAAGGGCCT CTTCCGCCGG

1090 1100 1110 1120 1130 1140

GGAGAGGCCC ACCTGGCTGT GAACGACTTT GACCTGGCAC GGGCTGACTT CCAGAAGGTC

1150 1160 1170 1180 1190 1200

CTGCAGCTCT ACCCCAGCAA CAAAGCGGCT AAGGCCCAGC TGGCTGTGTG CCAGCAGCGG

1210 1220 1230 1240 1250 1260

ATCCGCAAGC AGATTGCCCG GGAGAAGAAG CTCTACGCCA ACATGTTTGA GAGGCTGGCA

1270 1280 1290 1300 1310 1320

GAGGAGGAGA ACAAGGCGAA GGCAGAAGTG GCCGCAGGCG ACCATCCCAT GGACACAGAG

1330 1340 1350 1360 1370 1380

ATGAAGGATG AGCGGAACGA CGTGGCTGGA AGCCAGTCTC AGGTGGAGAC AGAAGCATAG

1390 1400 1410 1420 1430 1440

CCTCTCTGGC CTGACTCCTG CGACTGCCCG CCTCCTGCTC CCCTGCCCTA CTCCACCCTG

1450 1460 1470 1480 1490 1500

TTAGTTTTGT AAAAACTGAA GAATTTTGAG TGACTTAGAC CTTTATTTTT CTATCTGGTT Chain I continued

1510 1520 1530 1540 1550 1560

GGATGGTGGC TTTGCGAGGA GGGGGGAAAG ACTAGGCTGG GAACGCTGAG GTAGGGCTGA

1570 1580 1590 1600 1610 1620

TTCTAGGGAG TGTCACCCGC CCCCCTTCCC CCATCACACG TGAATGTACA TCCATCCACA

1630 1640 1650 1660 1670 1680

CACACGCAAC TGAATGTTCG TGCATTTTGC TCCCTCTGTT AGGTCTACTC TGCAAATGGT

1690 1700 1710 1720 1730 1740 AGAAGGGGGC AAGTGGTGGG GATGGGGTCT GATGTGAAAC CAGGGTGGAG AGGGAGACCG

1750 1760 1770 1780 1790 1800 ACTCCTGGGC AGCTGCTTTC CTGATCCTTG TCCTCTCCCA GTCCCTTTCA AACTGTGGCC

1810 1820 1830 1840 1850 1860 TCCAGGTGGG GGGTGCTGGG GGTGGGGAAA CCATTGCTGT GCCTGTTACC TCTCAGTCCC

1870 1880 1890 1900 1910 1920 TTCCTCACCC CAGATGGTGT GGCTGACTGT GTCTGGTGTC CAAGACCACC CCCGTCCCCC

1930 1940 1950 1960. 1970 1970 ATTCTGGTAT TGGCCTTCCT AGCAGTTTCC CTTCTCAGCC AGGTTGTATC CCCACCCTCC

1990 2000 2010 2020 2030 2040 CACCCTGTCA GCCTCTTCTC TGCACGTTGC TGAAAGTCCA GGCTCGCCTC AAGTTCTGTG

2050 2060 2070 CTTGAGCAAT AAAGTGGAAA CAATAAAAAA

2. Amino acid sequences: sequence II

10 20 30

MTAEEMKAAE SGAQSAPLPL EGVDISPKQD

40 50 60

EGVLKVIKRE GTGTETPMIG DRVFVHYTGW

70 80 90

LLDGTKFDSS LDRKDKFSFD LGKGEVIKAW

100 110 120 DIAVATMKVG ELCRITCKPE YAYGSAGSPP

130 140 150 KIPPNATLVF EVELFEFKGE DLTDDEDGGI

160 170 180 IRRIRTRGEG YARPNDGAIV EVALEGYYKD

190 200 210 RLFDQRELRF EVGEGESLDL PCGLEKAIQR

220 230 240 MEKGEHSILY LKPSYAFGNA GKEKFQIPPY

250 260 270 AELKYEVHLK SFEKAKES E MSSEEKLEQS

280 290 300 AIVKERGTVY FKEGKYKQAL LQYKKIVSWL

310 320 330 EYESSFSSEE VQKAQALRLA SHLNLAMCHL

340 350 360 KLQAFSAAVE SCNKALELDS NNEKGLFRRG

370 380 390 EAHLAVNDFD LARADFQKVL QLYPSNKAAK

400 410 420 AQLAVCQQRI JSKQIAREKKL YANMFERLAE

430 ^"" 44 ^" 0 ~ 450 EENKAKAEVA AGDHPHDTEM KDERNDVAGS

458 QSQVETEA Example 5: Applications of the pHBI protein and its constituents.

The functioning of certain steroid hormone receptors can be affected by the binding of immunosuppressants to pHBI. (Renoir et al, C.R. Acad. Sci. Paris, t.135, Série III, p 421-428, 1992).

The pHBI protein and its constituents can therefore be used to search for immunosuppressants which do not interact with HBI. We will measure the interest of such results which make it possible to avoid the endocrine effect of immunosuppressants, such as the hyperandrogyny with hirsutism which has been observed during immunosuppressive treatments. . The mechanism of brain complications due to immunosuppressants is poorly understood. However, by using pHBI or its constituents, one can detect interactions other than those of FKBP12 with certain proteins involved in the mechanism of action of neurotransmitters.

The use of antibodies directed against the pHBI protein or its constituents makes it possible to detect the presence of membrane receptors of the immunosuppressants and to locate them (N.A. Cacalano et al, PNAS, 1992, £ 2., P 4353-4357).

rc ^ mp ¹ "- fi: Detection of m-RNA of the protein pHBI in various conditions.

DNA encoding the pHBI protein has been used to detect the presence of its mRNA in various tissues. Northern techniques followed by hybridization were used following the protocol described in the aforementioned work by Maniatis. The presence of pHBI mRNA has been demonstrated in rats in the placenta, heart, thymus, spleen, brain and uterus. On the other hand, under the conditions of the experiment, no detection could be carried out in the liver of chicken or xenopus. Using a Southern blot marketed by Clontech containing genomic DNA, pHBI DNA was detected in human placenta, monkey, mouse, rat liver, dog kidney, bovine liver and rabbit. Under the conditions of the experiment, the detection was negative in S-cerevisiae.

Claims

1 / Sequences of nucieotides, characterized in that they comprise or that they are formed by a sequence of nucieotides capable of hybridizing, under stringent conditions, with one or more sequences of a gene whose cDNA has a sequence corresponding to the sequence (I) of nucieotides.

2 / Sequences of nucieotides, characterized in that they contain the genetic information to code for all or part of the protein responding to sequence II. 3 / Sequences of nucieotides, characterized in that they are formed, or that they comprise, at least part of the sequence I.

4 / Sequences of nucieotides according to claim 3, constituted by part or all of the open reading frame going in the sequence (I) from position 4 to position 1380.

5 / Sequences of nucieotides according to claim 3, capable of coding for a potential protein of 458 amino acids responding to sequence II. 6 / Sequences of nucieotides according to one of the preceding claims, characterized in that they include the genetic information to code for one or more amino acid sequences of sequence II corresponding to a region capable of binding with a immunosuppressant type FK 506 and having the structural characteristics for rotamase activity.

7 / Sequences of nucieotides according to one of claims 1 to 6, characterized in that they include the genetic information to code for one or more amino acid sequences of sequence II, corresponding to a region capable of bind to ATP / GTP.

8 / Sequences of nucieotides according to one of claims 1 to 7, characterized in that they contain genetic information to code for one or more sequence II amino acid sequences corresponding to a region capable of binding to calmodulin. 9 / Recombinant sequence comprising one of the nucieotide sequences defined in any one of claims 1 to 8, if appropriate associated with a promoter capable of controlling the transcription of the sequence and a DNA sequence coding for the signals of termination of transcription.

10 / Sequences of nucieotides according to one of claims 1 to 9, characterized in that they contain coding sequences for chaperone proteins, in particular coding sequences for hsp90, in particular for the hydrophilic region A of this protein.

11 / The RNAs and the complementary sequences of the various nucleotide sequences defined in one of claims 1 to 10, as well as the corresponding coded proteins.

12 / Recombinant cloning and expression vectors capable of transforming an appropriate host cell, comprising at least part of a nucieotide sequence according to any one of claims 1 to 11, under the control of regulatory elements allowing its expression.

13 / Strains of transformed or transfected microorganisms, characterized in that they comprise at least one of the nucieotide sequences defined in one of claims 1 to 11, or also a recombinant vector as defined in claim 12.

14 / Amino acid sequences deduced, according to the universal genetic code, nucieotide sequences according to one of claims 1 to 11 and the proteins expressed by the genes comprising these sequences.

15 / Amino acid sequences according to claim 14, characterized in that they correspond to sequences capable of binding to heat shock proteins or that they have the properties of these proteins, and that in particular they are coding sequences for chaperone proteins, in particular coding sequences for hsp90, in particular for the hydrophilic A region of this protein.

16 / Amino acid sequences according to one of claims 14 or 15, characterized in that they have one or more domains of the type of FKBP, identical or different, in particular that they have the structural characteristics for a bond with an immunosuppressant of the FK506 type and for a rotamase activity, and / or that they comprise an ATP binding site, and / or a consensus binding sequence to calmodulin, and / or that they correspond to the hinge regions between two areas.

17 / Amino acid sequences according to one of claims 10 to 16, characterized in that they are such as obtained by transformation of host cells using a recombinant vector according to claim 12, cultured in an appropriate medium, transformed or transfected host cells and recovery of the protein from these cells, or directly from the culture medium.

18 / The complexes of the proteins of the amino acid sequences according to one of claims 1, 4 to 17 with hsp90 or with other heat shock proteins involved in these hetero-oligomers, or with regions of these different proteins .

19 / Polyclonal and monoclonal antibodies capable of specifically recognizing the amino acid sequences and the complexes according to one of claims 14 to 18.

20 / Application of the nucieotide sequences according to one of claims 1 to 11 for the development of probes for detecting genes coding for proteins forming complexes with chaperones and their ligands.

21 / Method for in vitro detection of the presence in a biological sample of nucieotide sequences complementary to those defined in one of claims 1 to 11, comprising the steps of

bringing the sample to be studied into contact with a nucleotide probe produced using a sequence according to one of claims 1 to 11, under conditions allowing hybridization between the probe and the desired nucieotide sequence, and

- detection of the hybridization complex.

22 / Kits for the In Vitro Detection of the Presence in a Biological Sample of Nucieotide Sequences Complementary to Those Defined in One of Claims 1 to 11, characterized in that they comprise

a determined quantity of a nucleotide probe produced from a sequence of nucieotides according to one of claims 1 to 11,

- a medium suitable for hybridization between the probe used and the sequence to be detected, and advantageously, - reagents for the detection of the hybridization complexes formed.

23 / Method for in vitro screening in a biological sample of the possible presence of the expression products of the nucieotide sequences according to one of claims 1 to 11 or those of the genes coding for a heat shock protein, characterized in that she understands

contacting the sample to be studied with an antibody according to claim 19, under conditions allowing the formation of an immunological complex between all or part of the proteins expressed by the nucleotide sequences and this antibody, and

- detection of the immunological complex.

24 / Kits for the in vitro detection in a biological sample of the possible presence of the expression products of the nucieotide sequences according to one of claims 1 to 11 or those of the genes encoding for a heat shock protein, characterized in that they comprise: a determined quantity of a polyclonal or monoclonal antibody according to claim 19, - a medium suitable for carrying out an immunological reaction between at least part of the products expressed and the antibody and, advantageously, reagents allowing the detection of the immunological complexes formed.