GB2273099A

GB2273099A - Glycoprotein encoded by a human endogenous retrovirus K envelope gene

Info

Publication number: GB2273099A
Application number: GB9223542A
Authority: GB
Inventors: Manfred P Dierich; Werner Vogetseder
Original assignee: Asta Medica GmbH
Current assignee: Asta Medica GmbH
Priority date: 1992-11-10
Filing date: 1992-11-10
Publication date: 1994-06-08
Also published as: WO1994011514A1; GB9223542D0

Abstract

By means of a polymerase chain reaction a 1053 bp DNA segment from the putative outer membrane part of the human endogenous retrovirus (HERV)-K-envelope gene was amplified. A 959bp part of the amplified DNA was inserted into the pAX-bacterial-expression-vector. A recombinant fusion protein of a HERV-K-envelope-portion with * small Greek beta *-galactosidase was obtained. A monoclonal antibody was generated which recognizes the envelope portion of the fusion protein (FP). This mAb is capable of immunoprecipitating a 67kD glycoprotein from the human breast carcinoma cell line T47D, the amount of which is strongly enhanced after stimulation with estradiol/progesterone. The same band could be precipitated from other carcinoma cell lines (Hep2, MCr7 and HELA), but not from the human B-lymphoblastoid cell line Raji and the mouse myeloma cell line Ag8.653. The data suggests that the antigen recognized by the anti-HERV1 mAb is the translational product of an active HERV-K-env gene or whole HERV-K provirus.

Description

UTILISATION OF A 67 KD GLYCOPROTEIN FROM HUMAN TUMOR CELL LINES, AND A MONOCLONAL ANTIBODY ESTABLISHED AGAINST A RECOMBINANT HUMAN ENDOGENOUS RETROVIRUS-K ENVELOPE-GENE ENCODED PROTEIN FOR DIAGNOSTIC AND THERAPEUTIC PURPOSES In the early forties the murk we mammary tumor virus (MMTV) was found to be involved in murine mammary carcinogenesis (Vlscher, M. B., Green, R. G. & BR< Bitter, J. D. (1942) Pro.Soc.Exp.Blol.Med. 49, 94-96). By means of hybridization techniques the existence of genomic integrated proviruses could be detected in all strains of mice, in both those with high or low risk of mammary tumor development (Varmus, H.E., Bishop, J.M. Nowinski, R.C. & Sarkar, N.H.

(1972) Nature 238, 189-190). This fact suggested that, besides the presence of MMTV-proviruses, other factors also must participate in mammary carcinogenesis, such as, perhaps, the expression of neighbouring genes driven by the MMTV promotor. Even retroviruses lacking viral oncogenes may be involved in tumorgenesis by integration into sites where they can activate transcription of cellular oncogenes (Varmus, H.E.

(1982) Cancer Surv. 2, 301). Meanwhile, the protooncogenes c-myc, Into1 and c-neu were described to be possible targets of an insertion of MMTV-provirus resulting in the development of mammary tumors (Sinn, E., Muller, W., Pattengale, P.,Tepler, I., Wallace R & Leder, P. (1987) Cell 49, 465-475), (Tsukamoto, A.S., Grosschedl, R., Guzman, R.C., Parslow, T & Varmus, H.E. (1988) Cell 55, 619-625), (Muller, W.J., Slnn, E., Pattengale, P.K., Wallace, R.

& Leder, P. (1988) Cell 54, 105-115).

Recently MMTV has been drawn to the attention of immunologists, because it has been found that endogenous MMTV may have a major impact on the formation of the T-cell repertoire. MMTVs are shown to encode for superantigens, which by binding to MHc class II antigens and to the VR-domaln of the T-cell receptors (Acha-Orbea, H. & Palmer, E. (1991) Immunol.

Today 12, 356-361).

The existence of a human mammary tumor virus has been considered for a long time, but not conclusively proven. In the early seventies the presence of reverse transcriptase activity and "retrovRruslRke partlcles" (RLVP) in the human milk samples was described (Schlom, J., Spiegelman, S. & Moore, D. (1971) Nature 231, 97-100). But, until now, there has been no evidence for the infectivity of these particles. RVLP with reverse transcriptase activity were also found in the human breast carcinoma cell line T47D after stimulation with estradlol and progesterone.These particles were shown to contain a glycoprotein gp69 that is recognized by antisera raised against MMTV-gp52 (Ohno, T., Mesa-Tejada, R., Keydar, I., Ramanarayanan, M., Bausch, J. & Spiegelman, S. (1979) Proc.Natl.Acad.Sci.USA 76, 2460-2464), (Segev, N., Hizi,A., Kirenberg, F. & Keydar, I.(1985) Proc.Natl.Acad.Sci.USA 82, 1531-1535).

These publications describe for the first time the detection of a possible retrovirus encoded protein in the human tumor cellline T47d.

Another approach to identify a MMTV-analog in humans was attempted by cloning and characterization of human endogenous retroviral sequences which hybridize with MMTV-probes under low stringency conditions (May, F.B., Westley, B.R. & Rocheford, H. (1983) Nucl .Acids.Res.11, 4127-4139), (Westley, B. & May, F.E.B. (1984) Gene 28, 221-227), (Deen, K.C. & Sweet, R.W. (1986) J.Virol. 57,422-432).

These publications describe the MMTV-analoge in the human genome.

One group of human endogenous retroviral genomes, designated HERV-K genomes (K represents the existance of a primer binding site for a putative tRNA-Lysin primer for reverse transcription), was detected by hybridization with a Syrian hamster A-type particle pol probe. Typical HERV-K-genomes were 9.1 or 9.4 kilobases in length, having long terminal repeats of ca. 970 bp and genes for gag, pol, and env as well as a gene likely to encode for a protease (prt). The env gene is divided into parts putatively encoding for a signal peptide, an outer membrane protein, and a transmembrane protein. The outer membrane part contains 7, the transmembrane part 4 possible glycosilation sites. Sequence comparison of the HERV-K10+ genome revealed distinct homologies between HERV-K and MMTV, especially in the putative envelope-gene-region.In contrast to other human endogenous retroviral genomes, this HERV-K-genome contains large open reading frames in the putative gag, prt, pol and env., reglon. The HERV-K10+ sequence contains a stop codon at pos. 7210 that is not present in the three other characterized HERV-K-genomes (Ono, M., Yasunaga,T., Miyata, T. & Ushikubo, H. (1986) J.

Virol. 60, 589-598).

Thus, it seems possible that a HERV-K-provirus exists which may encode for a complete env protein. It has been calculated by filter hybridizations that around 50 HERV-K-proviruses exist per haploid genome, although it is not known if they are all complete.

Furthermore, an 8.8 kb HERV-K-mRNA transcript was detected in estradiol/progesterone treated T47D cells and in other carcinoma cell lines by hybridization with probes from the gag-, pol- and env-gene region of HERV-K10 (Ono. M., Kawakami, M. & Ushikubo, H. (1987) J. Virol. 61, 2059-2062). He describes the DNA-Sequence of the HERV-K retrovirus.

The products of the HERV-K-genes have not yet been characterized, but it has been speculated that a relationship between RVLP and the HERV-K-genomes could perhaps be found (Ono, M., Yasunaga,T., Miyata, T. & BR< Ushikubo, H. (1986) J. Virol. 60, 589-598).

In the present application we describe for the first time the identification of a 67 kD glycoprotein which is detectable in lysates from T47D cells as well as in other human carcinoma cell lines by means of a mAb raised against a recombinant HERV-K-envel ope protein representing a large segment of the putative outer membrane protein.

Materials Restriction enzymes and T4DNA-l igase were purchased from Pharmacia (Uppsala, Sweden), IPTG, DNAseI, lysozyme and BSA from Sigma (St. Louis, USA). FXa and Endoglycosidase F were obtained from Boehringer (Mannheim, Germany). 125Iodine was purchased from Amersham (Buckinghamshire, UK). The pAX-vector was obtained from Medac (Braunschweig, Germany) and the pINIII-ompA vector was a friendly gift from Dr. W.

Schwäble, Mainz, Germany.

CELL LINES The T47D, MCF7 (both human breast adenocarcinoma), HELA (human squamous cell carcinoma), Hep2 (human laryngeal squamous cell carcinoma), Raji (human B-lymphoblastoid) as well as Ag8.653 (mouse myeloma) cell lines were maintained in RPMI containing 10% FCS.

Stimulation of the T47 D cell line with estradiol/ progesterone (Sigma, St.Louis, USA) was done as previously described (Ono. M., Kawakami, M. & BR< Ushikubo, H. (1987) J. Virol. 61, 2059-2062).

ANTIBODIES BALBc-mice were immunized intraperitoneally three times in intervals of 2 weeks with 10 p9 rHERV-env-OM-FP emulgated in complete Freund's adj uvants and finally immunized intraspleenically once with rHERV-env-OM-FP lacking adjuvants . A monoclonal antibody, anti-HERV1, recognizing a recombinant HERV-K-envelope protein was prepared by standard techniques (Fazekas de St. Groth, S. & Scheidegger, D.

(1980) J. Immunol.Methods 35, 1-12). This revlew describes the production of monoclonal antibodies.

Hybridomas were screened by ELISA and confirmed by Western blot using rHERV-env-OM-FP and control proteins.

Example PCR AND CLONING PROCEDURE A standard 100Rl amplification reaction vessel containing 5pg T47D genomic DNA, 100pM each primer (5'CAGTCACATGGATGGATAAT, nt.6791-6810, according to (Ono, M.,Yasunaga, T., Miyata, T. & Ushikubo, H.

(1986) J. Vlrol. 60, 589-598) and 5'TCTTTTGGATCTATTTAAAACACC antisense to nt.7842-7819, same reference as above, 200us dNTPs, 10pl 10x amplification buffer and 2U Taq polymerase (both Promega, Madison, USA) was amplified in a Bio-med 60 Thermocycler for 25 cycles (920C 90 sec, 560C 2 min, 720C 3 min). The resulting 1053bp DNA fragment was purified by agarose electrophoresis and consecutive electroelution and then ligated into the blunt-ended HindIII site of pINIII-ompAl (Ghrayeb, J., Kimura, H., Takahara, M., Hsiung, H., Masui, Y. & Inouye, M.

(1984) EMBO J. 3, 2437-2442). This publication descrlbes a expression-vector for E. Coli, which is utilized in this invention.

The DNA fragment was then digested with BamHI and partially with EcoRI and after agarose gel purification of the resulting 959 bp fragment ligated into a EcoRI/ BamHI cut pAX-vector (provided by Medac, Braunschweig FRG). Positive recombinants were screened by hybridization with the PCR fragment. The identity of the insert was checked by sequencing of 200bp from the 3'terminus and found to be 99% homologous to the HERF-K-10+sequence. All cloning, hybridization, and sequencing procedures were done according to standard protocols (Sambrook, J., Fritsch, E.F. & Maniatis, T.

(1989) Molecular cloning Second Edition (Cold Spring Habour Laboratory Press, New York).

EXPRESSION OF rHERV-env-OM-FP The pAX-Pi asmi d containing a HERV-K-envelope insert, designated pHERVKENV-pAX4, was transfected into the E.coli TG2 strain and the expression of rHERV-env-OM-FP was inducted by IPTG as described by Sambrook, J., Fritsch, E.F. & Maniatis, T. (1989) Molecular Cloning, Second Edition (Cold Spring Habour Laboratory Press, New York).

The fusion protein was extracted from the inclusion bodies by the following procedure: The bacteria from a IPTG induced 500 ml culture were harvested by centrifugation at 7000g, 40C and 10 mien. The cells were suspended in 5 ml PBS containing 1 mg/ml Lysozym, 1% Triton-X-100, 10pg/ml DNAseI and 15 mM MgCl2 and incubated 60 minutes on ice. The lysate was then centrifuged at 7000g 15mien 40C. The pellet was suspended in 10 ml 10mM Sodiumtetraborate pH 9.0 containing 0.5 CHAPS and incubated 30 minutes at room temperature; The lysate was again centrifuged at 7000 g 15 min 40C and the pellet suspended in 10 ml 50 mM Tris/HCl pH 8.0 containing 8 M Urea, 1 mM EDTA and 0,15 M NaCl and incubated for 30 minutes at room temperatur.After centrifugation at 7000g 15 min 40C the supernatant containing rHERV-env-OM-FP was dialysed against 50 mM TRIS/Hcl pH 8.0 containing 1M UREA, 1 mM EDTA and 0,1M NaCl and then loaded onto a 20ml DEAE-Trisacryl chromatography column. Washing of the column was done with 500ml of 50mM TRIS/HCl pH 8.0 contaning 1M Urea, lmM EDTA and 100 mM NaCl and rHERV-env-OM-FP was eluted with 50mM TRIS/HCl pH 8.0 containing 1 M UREA, 1 mM EDTA and 0,25M NaCl.

DIGESTION OF rHERV-env-OM-FP WITH ENDOPROTEINASE Xa (FACTOR Xa) 200pg protein from the 8M Urea fraction were loaded onto a SDS-PAGE according to Laemmli (Laemmli1 U.K: (1970) Nature 227,680-685). After separation, the band containing rHERV-env-OM-FP was cut from the gel and quenched 16h in 1,5 ml PBS at 40C. After centrifugation at 1500g for 10mien the supernatant was removed and dialysed against FXa cleavage buffer (0,5M Urea, 0,1M NaCl,lmM CaCl2, 50mM TRIS pH 8.0) and then transferred to microfuge tubes and incubated with or without lug FXa 16h at 180C (200pl/reaction). The reactlon was stopped by addition of SDS-PAGE sample buffer containing 5% 13-mercaptoethanol and boiling for 2 min.The samples were analysed by Western blot with mAb anti-HERV1 and a negative control antibody from the same Ig-subclass.

IMMUNOPRECIPITATION BSA, anti-HERV1 and an anti-tubulin mAb as a negative control were coupled to CNBr-activated Sepharose according to the manufacturers instructions (Pharmacia, Uppsala, Sweden).

Adherent cells (5 x 107cells) were washed four times with PBS and harvested with 5mM EDTA in PBS with the aid of a rubber policeman. Cells grown in suspension were washed four times with PBS. The cells were centrifuged at 1200g for 10mien at 40C and the cell pellet solubilized 15 min on ice with lysis buffer (0,5% Nonidet P40, 0,5% Triton X-100, 0,5% Deoxycholate, 5mM EDTA, 2mM PMSF in PBS). The lysate was then centrifuged at 15000g for 10mien and the supernatant labeled with iodine-125 by the iodogen/iodobead method according to the manufacturers instructions (Piece, Oud-Beijerland, Netherland) . Labeled proteins were recovered from free iodine 125 by chromatography on a small Sephadex G 50 column.The lysates were then precleared by incubation with 200 > 1 BSA-sepharose (lh, RT) and then divided into two aliquots and incubated elther with 25 111 anti-HERV1-sepharose or with antl-tubulln-sepharose (lah, RT). The sepharoses were washed six times with lysin buffer containing 0,5M NaCl and then SDS-sample buffer containing 5g(V/V)ss-mercaptoethanol (50pal) was added and incubated 2 min at 960C. The supernatant was loaded onto a SDS-PAGE according to Laemmli (Laemmli, U.K: (1970) Nature 227,680-685).

After electrophoresis, the gel was stained with Coomassie-brill lant-blue, dried and exposed to Cronex4 film (Dupont, Bad Homburg, Germany) for 24-48 hrs.

In one experiment iodine-labeled Hep2-lysate was incubated with BSA-sepharose and anti-HERV1-sepharose as above. After 4 times washing with the above lysis buffer with 0,5M NaCl, the sepharose was washed once with PBS containing 0,38 Triton-X100 and 0,1M sodium acetate. The sepharose was divided into two al iquots in 100 111 of PBS with 0,38 Triton-X100 and 0,1M sodium acetate and incubated with or without 0,5U Endoglycosidase F 16h at RT. Washing was again done twice with lysis buffer with 0,5M NaCl. The samples were then analysed by SDS-PAGE and autoradiography as above.

Results PCR AND CLONING OF A HERV-K ENVELOPE GENE FRAGMENT A 1053 bp DNA fragment (nt.6791-7842,ref.14) corresponding to the majority of the putative outer membrane env fragment (nt.6733-7842, ref. (Ono, M.,Yasunaga, T., Miyata, T. & Ushikubo, H. (1986) J.

Virol . 60, 589-598) of HERV-K10+ was amplified by PCR using T47D genomic DNA as a template and an oligonucleotide -primer-pair synthesized according to the published HERV-K10+ sequence. This fragment was ligated into the pINIII-ompAl vector and subsequently digested with BamHI and partially with EcoRI. A 959bp fragment (pos.6791-7749, ref. Ono, M.,Yasunaga, T., Miyata, T. & Ushikubo, H. (1986) J. Virol. 60, 589-598 containing the EcoRI-site from the pINIII-ompAl-vector on its 5'terminus was isolated and then ligated into an EcoRI/BgIII cut pAX-expression vector.This vector allows the production of a beta-galactosidase FP which should contain a recombinant HERV-env-OM (fig.1). The identity of the insert as a HERV-K-envelope gene was checked by partial sequence analysis. 200bp were sequenced on the 3'terminus and found to be identical with the sequence of HERV-K10+ except for two A to T substitutions at nt. 7657 and 7691 (Ono, M., Yasunaga, T., Miyata, T. & Ushikubo, H. (1986) J. Virol. 60, 589-598), which results in a substitution of Ser instead of Thr and Val instead of Asp, respectively.

However, as found by restriction enzyme digestion, our cloned insert contains two EcorRI restriction sites which are not present in the published HERV-K10+ sequence and which are not located inside the 200 bp at the 3'terminus.

Figure 1 shows the cloning procedure schematically.

GENERATION OF rHERV-enf-OM-FP After induction of FP synthesis with IPTG, the inclusion bodies were prepared from the bacteria and then fractionally solubilized. The rHERV-env-OM-FP was found to be extractible in the presence of 8 M UREA.

As determined by SDS-PAGE, rHERV-env-OM-FP has a m.w.

of 155 kD which is composed of a 118kD ss-galactosidase portion and a 37kD HERV-K-envelope-outer-membrane-protein portion which is the expected size for complete translation of the 959bp insert.

PRODUCTION OF A MONOCLONAL ANTIBODY REACTING WITH THE ENVELOPE PROTEIN PORTION OF rHERV-env-OM-FP One monoclonal antibody (anti-HERV1) recognizing the HERV-K-envelope-protein portion of rHERV-env-OM-FP was obtained after immunization of BALBc mice with rHERV-env-OM-FP and generation of hybridomas. This mAb exhibited reactivity with rHERV-env-OM-FP but lacked reactivity with (3-galactosidase. Other bacterial proteins extracted from IPTG-induced E.coli transfected with the plasmid pAX without insert were also not recognized.

Furthermore, anti-HERV1 recognized the 37kD envelope protein after cleavage of rHERV-env-OM-FP with endoproteinase Xa.

By means of an ELISA this mAb has been identified as a mouse IgM mAb.

IMMUNOPRECIPITATION OF A 67KD GLYCOPROTEIN FROM HUMAN CARCINOMA CELL LINES The human breast carcinoma cell line T47D, either untreated or after stimulation with estradiol/pro- gesterone, as well as the Hep2 (human laryngeal carcinoma), HELA (human squamous cell carcinoma), MCF7 (human breast carcinoma), Rayi (human B-lymphoblastoid) and the Ag8.653 (mouse myeloma) cell lines were lysed and the immunoprecipitated with the anti-HERV1 mAb. From all these cell lines, with exception of Raji and Ag8.653 cells, a 67kD protein could be precipitated with the anti-HERV1 mAb, but not with a control mAb from the same Ig-subolass (IgM).

Stimulation of T47D with estradiol/progesterone strongly enhanced the expression of the 67kD protein Treatment of the 67 kD-protein with endoproteinase F reduced the m. w. to 58-60kD, indicating the presence of N-linked carbohydrate moieties of at least 7-9kD In the present report, we describe the detection of a 67kD antigen in the estradiol/progesterone treated human breast carcinoma cell line T47D and in the carcinoma cell lines HELA, Hep2 and MCF-7 by a mAb raised against a recombinant protein encoded by the outer membrane part of a HERV-K-env gene.

For the generation of a recombinant HERV-K-envouter-membrane protein (rHERV-env-OM-FP) we used the pAX-expression-vector system, because it allows high level expression of a B-galactosidase-FP in which the D-galactosidase part and the foreign-protein protion are separated by a collagen "spacer" that facilitates independent folding of the foreign protein during its syntheses. A further advantgage is that the FP could be cleaved by FXa into a R-galactosidase-collagen- spacer protein and the foreign protein. Our insert is slightly different from the published HERV-K10+ sequence, as it contains 2 EcoRI sites which are not present in HERV-K10+ and at least in the 200th base-position form the 3'-terminus.

(Ono, M., Yasunaga, T., Miyata, T. & Ushikubo, H.

(1986) J. Virol. 60, 589-598).

The env part of rHERV-env-OM-FP has a m. w. of 37kD, indicating that the 959bp insert was fully translated without internal termination. This protein represents -the translational product of nt. 6791 to 7749, thus, 86,5% of the whole outer membrane portion (nr.6733-7842, ref. (Ono, M.,Yasunaga, T., Miyata, T.

& Ushikubo, H. (1986) J. Virol. 60, 589-598) of the HERV-K10-env gene. It seems likely that that a complete outer membrane protein has a peptid core of approximately 43KD and carbohydrate moieties of 25 kd since the outer membrane env gene of HERV-K10+ contains 7 possible glycosilation sites. By treatment with Endoglycosidase F we could reduce the molecular weight of the 67kd protein to about 59kd.

However, it seems possible that the gp67 is not completely deglycosilated, since the Endoglycosidase F treatment was performed on an immobilized antibody/antigen complex.

T47D cells, established from pleural effusion from a human breast cancerpatient, have receptors for estrogen, progesterone and androgen (Keydar, I., Chen, L. Karby, S., Weiss, F.D., Delarea, J., Radu, M.

Chaitchek,S. & Brenner, H.J. (1979) Eur. J. Cancer 15, 659-670).

In these cells HERV-K-mRNA transcripts had already been detected, but only at a basal level when the cells were kept in normal tissue culture medium supplemented with 10tFCS. This expression could be increased when the cells were treated with 1OnM estradiol on day 1 and 100nM progesterone on day 2.

mRNA-transcripts for HERV-K have also been described in Hep 2 and HELA cells, whereas the MCF-7-cell line has not been examined (Ono. M., Kawakami, M. & BR< Ushikubo, H. (1987) J. Virol. 61, 2059-2062).

This is in line with our description of the distrl- bution of the 67kD antigen, characterized by our anti-HERV1.mAb. The expression of our 67kD antigen in T47D was also up regulated by the combination of estradiol and progesterone.

Particles containing "reverse transcriptase activity" as well as other structural features of retroviruses and therefore termed RVLP are released from T 47D cells depending upon stimulation with estradiol followed by progesterone. One antigen associated with PVLP, gp68, has been identified to be recognized by a polyclonal antibody raised agains the MMTV-env-gp5Z (Segev, N., Hizi, A., Kirenberg, F. & Keydar, I., (1985) Proc.Natl.Acad.Sci.USA 82, 1531-1535).

A mAb (H23) has been raised against T47D-RVLP which was found to recognize a 68kD glycoprotein associated with T47D-RVLP. In the same study (Keydar, I., Chou, C.S., Hareuveni, M., Tsarfaty, I., Sahar, E. Selzer, G., Chaitchik, S. & Hizi, A. (1989) Proc.Natl.Acad.Sci.USA 86, 1362-1366) it was speculated that the gp68 recognized by the antl-MMTV-gp52-antiserum and the gp68 detected by H23 are very similar and possibly identical. In this publication, the cell-line T47D are described in detail. In contrast to those findings, a later study revealed that the H23 mAb recognized two high molecular mass proteins ( > 200kD) from T47D cell extracts and culture supernatants.Furthermore, it was found that H23 did not recognize a MMTV protein which is explained by an only restricted similarity of a few epitopes between MMTV and T47D-RVLP. Sequences derived from cDNA clones isolated by immunoscreening with the H23 mAb revealed that H23 recognizes a mucin-like epithelial tumor antigen. However, the H23 mAb demonstrated a high specifity for breast carcinoma tissue, but it has also been detected on the surface of T47D cells as well as in culture supernatants and in pleural effusion fluids from breast cancer patients.

We assume that our gp67, which is characterized by the antl-HERV1-mAb, is located mainly intracellular, since we could not precipitate labeled antigen from surface-labeled cells. Furthermore, the antigen was not detected by immunoprecipitation with our mAb in a pleural effusion fluid of a patient with breast cancer. The detection of this protein by indirect immunofluorescence and lmmunohistochemistry has also been unsuccessful. One possible explanation could be that the epitope of anti-HERV1 is blocked by an associated, retrovirally or chromosomally encoded protein and only lysis, as done by the immunopre capitation experiments, liberated the site recognized by our mAb.Some immunofluorescence or immunohistochemistry fixation procedures also result in a high unspecific background when an IgM mAb is used.

Several facts support the hypothesis of Ono, M. et al, that RVLP or at least the RVLPgp68, recognized by anti-MMTV-gp52, may be encoded by an active HERV-K-provirus: (a) HERV-K-genomes have (especially in the env-region) significant relationship to MMTV with respect to thelr deduced amino acids and structure, (b) antibodies to MMTV have been shown to crossreact with T47D-RVLP (c) transcription HERV-K-genomes as well as the production of RVLP are induced on T47D cells by treatment with estradiol and progesterone and (d) our descriptlon of a 67kD antigen that possibly is related or identical to the gp68 recognized by anti-MMTV-gp52 and that is recognized by a mAb established against a recombinant HERV-K-env-outer-membrane-proteln.

Durlng biosynthesis the precursor protein may be split into an outer membrane glycoproteln and a transmembrane glycoprotein by a virus-encoded protease, as it has been demonstrated for many retroviruses including MMTV and HIV.

The H23 epitope seems to be restricted to breast carcinoma tissue, whereas gp67 is also found in carcinoma cells of other than breast origin. The presence of H23-antigen in these cell lines has not yet been described in the literature. The breast carcinoma specifity of the H23 mAb may be due to an epitope variability of the broader distributed epithelial tumor antigen.

Finally, it seems likely that different HERV-K-proviruses encode for env-glycoproteins which may differ from each other in respect to cellular location, distribution, and reactivity with distinct mAbs.

ABBREVIATIONS BSA bovine serum albumine ELISA enzyme linked sorbent assay FP fusion protein FXa endoproteinase Xa (blood coagulatlon factor Xa) HERV human endogenous retrovirus IPTG Isopropyl-ss-D-thlogalactopyranosid mAb monoclonal antibody MMTV murine mammary tumor virus nt. nucleotide position PAGE polyacrylamid-gelelectrophoresis PBS phosphate buffered saline PCR polymerase chain reaction RVLP retrovirus-like-particles RNA ribonucleic acid tRNA transfer ribonucleic acid Ig Immunglobulln

Claims

Claims 1. Monoclonal antibody, characterized in that it is specific versus a glycoprotein of human tumor cells.
2. Glycoproteln or protein, characterized in that it is encoded by a human endogenous retrovirus K-envelope-gene.
3. Process for the production of a protein or a glycoprotein according to claim 2, characterized in that a pax-vector is expressed and hybridized according to per se known methods, the resulting plasmid is transfected to E.coli TG2-strain and the protein is expressed by the bacterium and isolated.
4. Use of the monoclonal antibody, according to claim 1, for the diagnosis and treatment of cancer.
5. Medicament for the treatment of Cancer, containing a monoclonal anti body according to claim 1 and the usual fillers and auxiliaries.
6. Process for producing a medicament according to claim 5, characterized in that the monoclonal antibody is processed in the usual way with conventional fillers and auxiliaries.
7. A monoclonal antibody as claimed in claim 1 substantially as hereinbefore described with reference to the examples.
8. A glycoprotein or protein as claimed in claim 2 substantially as hereinbefore described with reference to the examples.
9. A process as claimed in claim 3 substantially as hereinbefore described with reference to the examples.