Abstract:
The present invention relates to a DNA segment encoding an Onchocerca volvulus antigen: a specific and early marker of onchocerciasis infection. The nvention further relates to recombinant molecules containing such a segment and to methods of utilizing same to produce the Onchocerca volvulus antigen. The invention also relates to the antigen itself. The invention further relates to methods of diagnosing Onchocerciasis infection.

Description:
BACKGROUND OF THE INVENTION 
     Field of the Invention 
     The present invention relates, in general, to a DNA segment and use thereof. In particular, the present invention relates to a DNA segment encoding an Onchocerca volvulus antigen: a specific and early marker of onchocerciasis infection. 
     Background Information 
     The parasitic filarial nematode, Onchocerca volvulus, is the causative agent of onchocerciasis. It infects some 18 million people in Africa and Latin America manifesting itself as a severe disease, of the skin and eyes (&#34;river blindness&#34;) (World Health Organization. Technical Report Series No. 752 (WHO Expert Committee on Onchocerciasis 3rd Report), WHO Geneva (1987)). Although vector control and the advent of ivermectin promise a drastic reduction of the disease, these measures emphasize the crucial need for accurate diagnosis of early and light infections in areas where vector control has been established or where chemotherapeutic control is envisaged (H. R. Taylor et al., Science 250,116 (1990)). Definitive diagnosis currently relies either on detecting microfilariae (mf) in the skin or eyes or on identifying the adult worm in subcutaneous nodules removed surgically, techniques which are invasive and relatively insensitive. Hitherto, serological tests have not been satisfactory, partly because of the broad antigenic cross-reactivity among the filarial and other helminth parasites of humans and partly because they fail to detect prepatent and low-level infections (World Health Organization. Technical Report Series No. 752 (WHO Expert Committee on Onchocerciasis 3rd Report), WHO Geneva (1987)). A species-specific diagnosis has also prime importance since treatment differs for different filarial infections. 
     O. volvulus does not infect convenient laboratory hosts, and the scarcity of parasite material has so far hindered intensive immunological research which is essential for the understanding of the wide spectrum of observed pathological changes. The difficulty in obtaining sufficient amounts of parasite material, which can only be acquired from patients living in remote areas, is circumvented by the present invention which relates to cloning and expressing parasite genes in suitable vectors. 
     Current diagnostic methods lack adequate sensitivity and specificity. The development of immunological tests to discriminate between onchocerciasis and other filarial infections and to detect early prepatent infection in exposed individuals is of primary importance for the field assessment of infection and for control. The present invention provides a method of overexpressing an O. volvulus-specific antigen (OV-16), thereby facilatating isolation of OV-16. The OV-16 antigen produced by the present method can be exploited to identify the presence of O. volvulus parasites in the early &#34;prepatent&#34; period of infection when mf in the skin or in nodules in adults are not detectable. 
     SUMMARY OF THE INVENTION 
     It is a general object of this invention to provide a method of diagnosing onchocerciasis. 
     It is a specific object of this invention to provide a DNA segment coding for a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera. 
     It is a further object of the invention to provide a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera. 
     It is a further object of the invention to provide a recombinant DNA molecule comprising a vector and the above-described DNA segment. 
     It is another object of the invention, to provide a cell that contains the above-described recombinant DNA molecule. 
     It is a further object of the invention to provide a method of producing a polypeptide having an amino acid sequence corresponding to OV-16. 
     It is a further object of the invention to provide a method of diagnosing onchocerciasis. 
     Further objects and advantages of the present invention will be clear from the description that follows. 
     In one embodiment, the present invention relates to a DNA segment coding for a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera. 
     In another embodiment, the present invention relates to a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera and either free from proteins with which it is naturally associated or bound to a solid support. 
     In yet another embodiment, the present invention relates to a recombinant DNA molecule comprising a vector and the DNA segment that codes for a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera. 
     In a further embodiment, the present invention relates to a cell that contains the above described recombinant DNA molecule. 
     In another embodiment, the present invention relates to a method of producing a polypeptide having an amino acid sequence corresponding to OV-16 comprising culturing the above described cell under conditions such that the OV-16 DNA segment is expressed and the polypeptide thereby produced, and isolating the polypeptide. 
     In another embodiment, the present invention relates to a method of diagnosing onchocerciasis in an animal comprising (1) contacting serum from the animal with a low molecular weight antigen uniquely recognized by onchocerciasis patient sera under conditions such that binding of the antigen with an antibody in the serum can be effected, whereby a compound is formed and (2) detecting the compound. 
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS 
     FIG. 1. SDS-PAGE analysis of in vitro translation products and their immunoprecipitation by onchocerciasis and other filarial and non-filarial serum pools, using 12.5% polyacrylamide gel. Lane 1, control lysate in the absence of parasite RNA; lane 2, total translation products from savanna O. volvulus. Immunoprecipitation of in vitro translated polypeptides using: lane 3, normal human serum pool (NHS pool); lane 4, lymphatic filariasis serum pool from India (F-I); lane 5, lymphatic filariasis serum pool from the Philippines (F-P); lane 6, onchocerciasis serum pool from Mali (O.V.-M.); and lane 7, onchocerciasis serum pool from Tanzania (O.V.-T). Lane 8, loiasis serum pool from Congo (F-L); lane 9, M. perstans serum pool (F-M) from West Africa; lane 10, intestinal nematodes serum pool (I-N). Numbers on the right indicate size of molecular weight markers in kDa. See text for details. 
     FIG. 2A-2B. (A) Characterization of the fusion protein encoded by OV-16 cDNA. SDS-PAGE analysis of extracts of E. coli Y1090 cells infected with gtll (lane 1) or clone OV-16 cDNA (lane 2), and Western blot of the same extracts incubated with anti-20-42K antibodies (lanes 3 and 4). Arrow indicates the position of the fusion protein at 134 kDa. (B) Western blots incubated with affinity-purified antibodies from onchocerciasis patients or other filarial and non-filarial serum pools. Extracts of E. coli Y1090 (approximately 80 μg) infected with the recombinant phage OV-16 were fractionated by 7.5% SDS-PAGE and blotted onto nitrocellulose filters. Lane 1 was incubated with affinity-purified antibodies from onchocerciasis patients. Lanes 2 and 3 were incubated with filariasis serum pools from India and the Philippines, respectively; lanes 4, 5, and 6 were incubated with serum pools from patients infected with L. loa, M. perstans, or intestinal nematodes; lane 7  was incubated with normal serum pool. Molecular weight markers are indicated on the left. 
     FIG. 3A-3B. (A) Identification of the native parasite proteins that are antigenic determinants with the OV-16 cDNA fusion protein. SDS-PAGE analysis of O. volvulus proteins (approximately 80 μg) (lane 1) and Western blot probed with antibody selected against the OV-16 cDNA fusion protein (lane 2); lane 3 is a control using HRPO rabbit anti-human IgG (heavy chain); the band running at 50 kDa (asterisk) is the heavy chain of human IgG present in the parasite extract. (B) Identification of the primary translation product of the O. volvulus antigen mRNA. Total parasite proteins synthesized by in vitro translation of parasite RNA were immunoprecipitated with affinity-purified antibody against β-galactosidase (lane 1) or the OV-16 cDNA fusion protein 9 (lane 2). Immunoprecipitation of [ 35  S]methionine-labeled in vitro translated proteins were carried out using 30 μl of antibody selected against the recombinant antigen and 10 μl of rabbit anti-human IgG. Immunoprecipitates were electrophoresed on a 17.5% SDS-poly-acrylamide gel, processed for fluorography, dried, and autoradiographed. 
     FIG. 4A-4B. (A) Nucleotide sequence and predicted amino acid sequence of the OV-16 cDNA. (SEQ ID NO:I and SEQ ID NO:2) Arrowhead, 5&#39; end of the OV-16&#39; cDNA clone. The OV-16&#39; cDNA and OV-16 cDNA EcoRI fragments were subcloned into M13mp18 in both orientations. Internal fragments were obtained by Sau3A restriction enzyme digestion and ligation into the BamHI site of M13mp18. Sequence determination was carried out by the chain termination method (Sanger et al. (1977) Proc. Natl. Acad. Sci. USA 74, 5463-5467). The following subclones from the coding strand were sequenced: EcoRI fragment, nucleotides 1-320; Sau3A fragments, 341-457, 454-686; EcoRI/Sau3A fragment, 1-344; from the non-coding sequence: EcoRI fragment 812-490; Sau3A fragments 686-454, 457-341. The putative signal sequence is underlined. Four potential N-linked glycosylation sites, boxed. The proposed consensus polyadenylation signal AATAAA is doubly underlined. (B) Analysis of the hydropathy of OV-16 cDNA by the procedure of Kyte and Doolittle. Hydropathy values were averaged for a window of 10 amino acid residues. Positive numbers, hydrophobicity; negative numbers, hydrophilicity. 
     FIG. 5. Left-hand panel: parasite sequences hybridizing to the OV-16 cDNA insert 1. Southern blot analysis of genomic DNA from O. volvulus by OV-16 cDNA. EcoRI digest (lane a), HindIII digest (lane b). Markers are HindIII fragments of I 857  (kb). Right-hand panel: Northern blot analysis of total RNA from O. volvulus hybridized to OV-16 cDNA; markers are calf liver 18S and 28S RNA. 
     FIG. 6. Ultrastructural localization by immunoelectron microscopy of parasite antigens that share antigenic determinants with the OV-16 cDNA fusion protein. (1) Hypodermis (h); (2) cortical layer of the cuticle (cl); (3) apical part and surface of the uterine epithelium (ue). First two magnifications x44850; the third, x17940. Immunocytochemistry was carried out on thin sections of O. volvulus worms prepared from electron microscopy using the low-temperature embedding technique in Lowicryl K4M. Thin sections were incubated with antibody selected against the OV-16 cDNA recombinant antigen and subsequently with goat anti-human IgG coupled to 9-nm gold particles for indirect antigen localization. 
     FIG. 7. Construction of pCG808fx OV-16. The recombinant plasmid was obtained by ligating a 682 bp fragment of OV-16 (H. R. Taylor et al., Science 250,116 (1990)) into the EcoRI site of pCG808fx (C. V. Maina et al., Gene 74,365 (1988)). This plasmid contains a portion of the malE gene with its signal sequence fused to the Lac Z coding sequence; fx denotes the recognition site for factor Xa. The ligation mixture was used to transform E. coli 71-18. Transformants expressing the O. volvulus OV-16 antigen were identified by Western blotting using a pool of sera from patients with onchocerciasis. 
     FIG. 8A-8B. Panel A: SDS-PAGE analysis of the expression and isolation of the O. volvulus antigen as a MBP-16 fusion protein and the subsequent separation of the protein domains. Samples subjected to SDS-PAGE (5/15% gradient gels) were 40 μg E. coli lysate before induction (lane 1), 40 μg cell lysate after induction (lane 2), 40 μg flow-through from an amylose column (lane 3), 5 μg purified MBP-16 eluted from the cross-linked amylose column (lane 4), and 5 μg MBP-16 after digestion with factor X a  for 4 days at r.t. (lane 5). Molecular size standards were from Amersham. Panel B: Western blot analysis of the isolated O. volvulus antigen (OV-16). Identical gels (4/20% gradient with 5 μg MBP-16 (lanes 1 and 4), 5 μg fx a  -digested MBP-16 (lanes 2 and 5), and  200 ng of the FPLC-isolated OV-16 (lanes 3 and 6) were blotted onto nitrocellulose. They were probed with rabbit antiserum raised against MBP (1:20,000) (lanes 1, 2, and 3) or with a pool of sera from patients with onchocerciasis (lanes 4, 5, and 6 [1:500]). Bound antibodies were visualized by a second incubation with alkaline phosphatase-conjugated goat antibody to rabbit or human IgG. 
     FIG. 9. Detection of O. volvulus-specific antibodies (total IgG) onchocerciasis patients by means of the recombinant OV-16 antigen in ELISA (11). Sera from clinically well-defined filarial infections including M. ozzardi (N=5), M. perstans (N=2), L. loa (N=14), as well as patients with lymphatic filariasis caused by W. bancrofti (N=25) or B. malayi (N=12). The dotted line represents the cut-off values calculated as the mean of the control sera (N=13) plus three standard deviations. 
     FIG. 10A-10B. Seroreactivity against OV-16 in experimental O. volvulus infection in chimpanzees. Each animal was inoculated with 250±5 infective third-stage (L 3 ) larvae of O. volvulus. Detailed parasitological examinations were carried out monthly from three months before inoculation until 38 months postinoculation (H. R. Taylor et al., Am. J. Trop. Med. Hyg. 39,86 (1988)). ELISA was carried out. Chimpanzees showed a positive titer against OV-16 three months (A) and 12 months (B) prior to the time that mf were first detected in the skin. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     The present invention relates, in part, to a DNA segment coding for a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibodies present in onchocerciasis patient sera. 
     More specifically, the present invention relates to a DNA segment coding for a polypeptide having an amino acid sequence corresponding to OV-16. In one embodiment, the DNA segment has the sequence shown in FIG. 4, or allelic or species variation thereof, or a unique portion of such a sequence (unique portion being defined herein as at least 15-18 bases); complements of such sequences are also within the scope of the present invention. In another embodiment, the DNA segment encodes the amino acid sequence shown in FIG. 4, or allelic or species variation thereof or a unique portion of such a DNA sequence. In another embodiment, the DNA segment encodes amino acids 30 to 152 shown in FIG. 4 (amino acid 30 being immediately preceeded by an arrow), or allelic or species variation thereof or a unique portion of such a DNA sequence. 
     In another embodiment, the present invention relates to a polypeptide having an amino acid sequence corresponding to a low molecular weight antigen uniquely recognized by antibody present in onchocerciasis patient sera and either free of proteins with which it is naturally associated or bound to a solid support. In a specific embodiment, the polypeptide has an amino acid sequence corresponding to OV-16. In one preferred embodiment, the polypeptide has the amino acid sequence as shown in FIG. 4, or allelic or species variation thereof, or a unique portion of such sequences (unique portion being defined herein as at least 5-6 amino acids). In another preferred embodiment, the polypeptide has amino acids 30 to 152 shown in FIG. 4, or allelic or species variation thereof, or a unique portion of such sequences as defined above. 
     In another embodiment, the present invention relates to a recombinant DNA molecule comprising a vector (for example--plasmid or viral vector) and the DNA segment coding for a low molecular weight antigen uniquely recognized by antibody present in onchocerciasis patient sera or the OV-16 polypeptide or amino acids 30 to 152 of the OV-16 polypeptide (amino acid 30 being immediately preceeded by an arrow), as described above. In a preferred embodiment, the encoding segment is present in the vector operably linked to a promoter. In another preferred embodiment, the present invention relates to the recombinant DNA molecule pCG808fx-16. 
     In a further embodiment, the present invention relates to a cell containing the above described recombinant DNA molecule. Suitable host cells include procaryotes (such as bacteria, including E. coli) and both lower eucaryotes (for example yeast) and higher eucaryotes (for example, mammalian cells). Introduction of the recombinant molecule into the host cell can be effected using methods known in the art. 
     In another embodiment, the present invention relates to a method of producing the above described polypeptides, comprising culturing the above described host cells under conditions such that the polypeptide is produced, and isolating the polypeptide. 
     In another embodiment, the present invention relates to a method of diagnosing onchocerciasis in an animal comprising (1) contacting serum from the animal with a low molecular weight antigen uniquely recognized by onchocerciasis patient sera under conditions such that binding of the antigen with an antibody in the serum can be effected, whereby a compound is formed and (2) detecting the compound. In a further embodiment, the present invention relates to a method of diagnosing onchocerciasis in an animal comprising (1) contacting serum from the animal with OV-16 protein under conditions such that binding of the antigen with an antibody in the serum can be effected, whereby a compound is formed and (2) detecting the compound. 
     The use of recombinant antigen OV-16 overcomes many of the problems that previously plagued the diagnosis of onchocerciasis: lack of parasite material, poor specificity and sensitivity of the assays, and insensitivity for detecting prepatent and low level infections. Over most of the large area of the onchocerciasis Control Program in West Africa, O. volvulus transmission has been interrupted by vector control (J. Walsh, Science 232,922 (1986)). However, reinvasion of infective black flies occurs in some border areas and is responsible both for recurrent infections (WHO. Technical Report Series. No. 597. WHO Geneva (1976)) and for infections of children previously unexposed (born after the establishment of effective vector control). The use of OV-16, or of similar specific immunodominant antigens, should allow the early and specific diagnosis of new or reinfections with O. volvulus in such vector reinvasion areas, as well as the detection of light infections in areas where control is being attempted by widespread use of ivermectin (M. A. Aziz, Parasitol. Today 2, 233 (1986)). Such capability will be of paramount importance in monitoring, evaluating and consolidating onchocerciasis control by both the vector control and chemotherapeutic strategies. 
     The present invention is described in further detail in the following non-limiting examples. 
     EXAMPLES 
     The following protocols and experimental details are referenced in the Examples that follow: 
     Parasites. Nodulectomy of onchocerciasis patients was performed in Manambougou (12°45&#39;N, 7°40&#39;W), a small village 30 km north-east of Bamako (Republic of Mali) located on the bank of the Niger River. O. volvulus worms (savanna form) were recovered from these nodules after digesting by collagenase as described by Schulz-Key et al. (Schulz-Key et al. (1977). Tropenmed. Parasitol. 28, 428-430). Isolated worm were maintained in culture in RPMI-1640 medium (gentamicin 50mg ml -1 , penicillin 100,000 U ml -1 ) for 2 days. Only intact and motile filariae were selected and frozen in liquid nitrogen. 
     Isolation of parasite RNA and DNA. The RNA was extracted from 26 frozen filarial worms by grinding to a paste in a mortar according to the hot phenol method (Maniatis et al. (1982) Molecular Cloning. A Laboratory, Manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.), using a 1:1 mixture of phenol and LiDS buffer (20 mM Tris, pH 7.5/200 mM LiCl/2 mM Li-EDTA/1% lithium dodecyl sulfate(LiDS)). 860μg total RNA was obtained from the female worms. O. volvulus genomic DNA was prepared from 3 frozen filarial worms after grinding them to a paste. The frozen powder was thawed and digested in 100 mM Tris, pH 8.5/50 mM Li-EDTA/200 mM LiCl/1% LIDS/200 μg proteinase K per ml at 37° C. for 1 h. The viscous solution was extracted three times with phenol at 5° C. and once with chloroform. The DNA was then prepared according to Maniatis et al. ((1982) Molecular Cloning. A Laboratory, Manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.). A total of 26 μg DNA was obtained from the filarial worms. 
     Isolation of Human DNA. HeLa cells were grown in suspension in Joklik-modified minimal essential medium (Gibco) containing 10% newborn calf serum. HeLa cells (about 5×10 7  cells) were pelleted (200 x g, 10 min, 4° C.) and washed once with cold TBS (Tris-HCl-buffered saline; 10 mM Tris-HCl, pH 7.6, 150 mM NaCl), and DNA extracted as already described (Maniatis et al. (1982) Molecular Cloning. A Laboratory, Manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.). 
     Cell-free synthesis and immunoprecipitation of the in vitro translated polypeptides. Cell-free protein synthesis was carried out in a mRNA-dependent rabbit reticulocyte lysate using a 20 μl incubation mixture prepared as described by Pelham and Jackson (Pelham, H. R. B. and Jackson, R. J. (1976) Eur. J. Biochem. 67,247-256), using 10 μg total filarial RNA, [ 35  S]methionine to 0.29 μCi ∥l -1  (1000 Ci mM -1 ), and 1 h incubation at 30° C. The  35  S-labeled translation products were diluted to 100 μl with immunoprecipitation buffer (Pelham, H. R. B. and Jackson, R. J. (1976) Eur. J. Biochem. 67, 247-256), the clarified labeled products (1.48×10 5  acid-insoluble cpm) were then immunoprecipitated with the appropriate amount of antibody, as already described (E. Lobos and N. Weiss (1986) Parasitology 93, 389-399), and analyzed directly by SDS-polyacrylamide gel electrophoresis and fluorography (Laemmli, U. K. (1970) Nature 227, 680-685; Chamberlain, J. P. (1970) Anal. Biochem. 98, 132-135). 
     Sera. The onchocerciasis serum pool from Mali (O.V.-M), Tanzania (O.V.-T) and the lymphatic filariasis serum pool from India (F-I) have been previously described (E. Lobos and N. Weiss (1986) Parasitology 93,389-399). The serum pool from the Philippines (F-P) consisted of 16 sera from asymptomatic microfilaremic Wucherereia bancrofti patients. No intestinal nematodes were detected. The loiasis serum pool (F-L) was prepared from 6 individuals from Congo with parasitologically proven Loa loa infection. No intestinal nematodes were detected. The Mansonella perstans serum pool (F-M) consisted of 6 sera from people living in different West African countries with parasitologically proven M. perstans infection. Three of them had Trichuris trichiura. The intestinal nematode serum pool (I-N) was prepared from 12 Swiss patients with parasitologically proven Ascaris lumbricoides and/or T. trichiura and who had never been exposed to any human filarial parasite. The normal human serum pool (NHS) was prepared from 6 individuals with no known parasitic infection. 
     Construction of a cDNA library in gtll. cDNA was synthesized with reverse transcriptase (Super RT, Stehelin, Basel, Switzerland) and oligo-dT primers followed by RNase H (Pharmacia, Uppsala, Sweden) and DNA polymerase I (New England BioLabs, Beverly, Mass.) treatment as described (Gubler, V. and Hoffman, B. (1982) Gene 25, 263-269). Treatment of double-stranded cDNA with S1 nuclease was carried out as recommended (Lapeyre, B. and Amalric, F. (1985) Gene 37, 215-220). The cDNA was methylated with EcoRI methylase, then blunt-end ligated to kinased EcoRI linkers and digested with EcoRI restriction endonuclease (all enzymes from New England Bio-Labs). The cDNA was size fractionated in a Bio-Gel A-15M column (Bio-Rad, Richmond, Calif.). Fractions containing cDNA longer than 300 bp were pooled and precipitated with isopropanol. The cDNA was ligated to EcoRI-cut and dephosphorylated gtll vector (Young, R. A. and Davis, R. W. (1983) Proc. Natl. Acad. Sci. USA 80, 1194-1198) in the presence of 15% polyethylene glycol (PEG) (Pheiffer, B. H. and Zimmermann, S. B. (1983) Nucleic Acids Res. 11, 7853-7871). The resulting ligating products were packaged in vitro in phage gtll using extracts and procedures described elsewhere (Maniatis et al. (1982) Molecular Cloning. A Laboratory, Manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.). The resulting library had 4×10 6  recombinant phage, and approximately 95% of the phage contained inserts. 
     Affinity purification of antibodies. SDS-treated protein extract of O. volvulus from Mali (800 μg) was fractionated on a preparative 12.5% SDS-polyacrylamide gel and Western-blotted as described (Towbin et al. (1979) Proc. Natl. Acad. Sci. USA 76, 4350-4354). The region of nitrocellulose between 20-42 kDA was excised and the remaining binding sites blocked with 2.5% bovine serum albumin (BSA), TBS, pH 7.5. The nitrocellulose strips were reacted overnight at 4° C. in 3 ml serum pool of onchocerciasis patients from a hyperendemic savanna region in Mali (O.V.-M) diluted 1:50 in 0.5% BSA, TBS. After 7 washes in TBS, bound antibody was then eluted by a 2-min rinse with 0.15 M glycine-Cl, pH 2.8. The eluate was quickly neutralized with 0.1 M NaOH, and BSA was added to a 0.5% concentration. These affinity-purified antibodies were used for immuno-screening of the O. volvulus cDNA library. Nitrocellulose strips containing 150 μg of the fusion protein transferred from 7.5% SDS-polyacrylamide gel were used to affinity purify antibody as already described (Altmann et al. (1987) Mol. Cell. Biol. 7, 998-1003). These selected antibodies were used to identify the native parasite proteins and the primary translation product, and to establish the subcellular localization of the native parasite antigens. 
     Immunoscreening. Immunoscreening of the gtll cDNA library was as described with Escherichia. coli Y1090 (Altmann et al. (1987) Mol. Cell. Biol. 7, 998-1003). After induction of the lacZ operon, the filters were saturated and incubated overnight with the affinity-purified anti-O. volvulus antibodies. The filters were washed for 1 h in TBS and incubated with [ 125  I]protein A (10 mCi mg -1  protein, 0.3 μCi ml -1 ) in TBS for 30 min. Filters were washed for 1 h with TBS, dried, and exposed to Kodak XAR-5 film using intensifying screens. Good signals were obtained after 3-day exposure at -70° C. 
     DNA analysis of immunoreactive phage. Phage was amplified in E. coli Y1088 on plates and purified by DEAE cellulose chromatography, and their DNA was extracted (Helms et al. (1985) DNA 4, 39-49), To determine the size of the cDNA inserts, total DNA was cut with the restriction enzyme EcoRI. Fragments were separated by agarose gel electrophoresis. 
     DNA Sequencing. The isolated OV-16 cDNA EcoRI fragment was subcloned into M13mp18 in both orientations. Internal fragments were obtained by Sau3A restriction enzyme digestion and ligation into the BamHI site of M13mp18. Sequence determination was carried out by the chain termination method (Sanger et al. (1977) Proc. Natl. Acad. Sci. USA 74, 5463-5467). 
     Production of β-galactosidase-hybrid protein. E. coli strain Y1090 was infected with the recombinant phage on plates to achieve confluent lysis and the synthesis of protein sequences encoded by cDNA inserts was induced as already described (Young, R. A. and Davis, R. W. (1983) Science 222, 778-782). Plates were then washed (Altmann et al. (1987) Mol. Cell. Biol. 7, 998-1003) and proteins in the wash solution were concentrated by ammonium sulphate precipitation (50% saturation) and dissolved in SDS-sample buffer. 
     Immunoblot analysis. Polypeptides were fractionated on 7.5% or 12.5% SDS-polyacrylamide gels and transferred to nitrocellulose (Towbin et al. (1979) Proc. Natl. Acad. Sci. USA 76, 4350-4354). Nitrocellulose sheets were then reacted with the different filarial antisera (diluted 1:50 in 0.5% BSA, TBS) and bound antibody detected with peroxidase-conjugated rabbit anti-human IgG (Dako-Patts, Denmark) or using [ 125  I] protein A as described for the immunoscreening. 
     Hybridization assays. Parasite or human DNA (1 μg) was cut with restriction endonucleases and digestion products electrophoresed on a 1% agarose gel. The DNA was transferred to nitrocellulose (Southern, E. M. (1975) J. Mol. Biol 98, 503-517) and the filter baked in vacuo, hybridized in 6 x standard salt citrate (SSC), 0.5% SDS, 5 x Denhardt&#39;s 100 μg ml -1  salmon sperm DNA. The purified OV-16 cDNA insert was labeled by nick translation and hybridized to the filter, 10 6  cpm ml -1  at 68° C. The filter was washed twice in 2 x SSC, 0.5% SDS at room temperature, and twice in 0.1 x SSC, 0.5% SDS at 65° C., then autoradiographed. For Northern blot analysis, 20 g total RNA from female O. volvulus was denatured with glyoxal (McMaster, G. K. and Gordon, C. G. (1977) Proc. Natl. Acad. Sci. USA 74, 4835-4838), electrophoresed on a 1.5% agarose gel, blotted to nitrocellulose (Thomas, P. S. (1983) Methods Enzymol. 100, 255-266), hybridized with nick-translated OV-16 cDNA insert, 3×10 6  cpm ml -1 , and washed as already described. 
     Immunocytochemistry. Female O. volvulus worms isolated by the collagenase technique (Schulz-Key et al. (1977). Tropenmed. Parasitol. 28, 428-430) were fixed in 0.5% (v/v) glutaraldehyde in 0.1 M phosphate-buffered saline (PBS), pH 7.2, and maintained in 0.1 M PBS. Dehydration with graded ethanol and penetration with Lowicryl K4M were accomplished using a low-temperature embedding technique (Kellenberger et al. (1980) Chemische Werke Lowi GmbH, Wald Kraiburg, F.R.G.). 
     Immunocytochemistry was carried out using antibody selected against the OV-16 cDNA recombinant antigen followed by goat anti-human IgG coupled to 9 nm gold particles (DeMey, J. (1983) Immuno-gold staining of surface cell antigens in cell suspensions. GAMG 30/colloidal gold coated with immunoglobulins. Jansen Life Science Products Division, Belgium) for antigen localization. 
     EXAMPLE 1 
     Immunoprecipatation of Translated O. volvulus Antigens 
     To ensure that the RNA isolated from the female O. volvulus was intact, mRNA in vitro translation was carried out using rabbit reticulocyte lysate, and the [ 35  S]methionine-labeled products were analyzed SDS-PAGE and fluorography (FIG. 1). When 10 μg of total RNA from O. volvulus was added to the system, at least 50 35  S-labeled polypeptides could be detected (FIG. 1, lane 2), ranging from 14-200 kDa, indicating that the RNA isolated from the filariae was sufficiently intact to act as a template in a message-dependent cell-free system. When those  35  S-labeled translation products were immunoprecipitated with the onchocerciasis serum pool from Mali (O.V.-M), 16 different antigens or antigen complexes could be detected (lane 6) ranging from 20 to 104 kDa. The cross-reactivity between the in vitro translated products and the serum pools from patients infected with other filarial parasites (W. bancrofti, L. loa, M. perstans) or with intestinal nematodes (A. lumbricoides, T. trichiura) was minimal (FIG. 1, lanes 4, 5, 8, 9 and 10). 
     Immunoprecipitation of the in vitro-translated polypeptides using onchocerciasis serum pools (FIG. 1, lanes 6 and 7) indicated that there are many O. volvulus polypeptides that do not require further processing and/or post-translational modifications to attain their antigenicity. Although the lymphatic filariasis, loiasis, mansonellosis and intestinal nematode serum pools have been previously shown to cross-react widely with native O. volvulus antigen (E. Lobos and N. Weiss (1986) Parasitology 93, 389-399; Weiss, N. and Karam, M. (1989) Am. J. Trop. Med. Hyg. 40, 261-267), there was relatively little cross-reactivity of these in vitro translated proteins when reacted with these sera. 
     EXAMPLE 2 
     Isolation of OV-16 cDNA Clone 
     To develop a cDNA library, 10 μg of the total RNA from microfilaria-producing female O. volvulus were used to synthesize cDNA as described (Lapeyre, B. and Amalric, F. (1985) Gene 37, 215-20). The resulting library containing approximately 4.1×10 6  recombinants with an average insert size of 1.1 kb. 
     Approximately 300,000 recombinant clones were screened with antibodies affinity-purified from a serum pool from West African onchocerciasis patients (O.V.-M pool). Of the 14 clones identified, the OV-16 cDNA clone was used for further characterization because of the strong antibody response to it. This clone was further characterized by preparing lysates from infected cells that were analyzed by Western blotting to identify the immunoreactive protein with the affinity-purified antisera. The OV-16 cDNA clone was shown to be producing a hybrid protein of 134 kDa, (thus about 18 kDa large than β-galactosidase; FIG. 2A, lane 2). The fusion protein reacted strongly on Western blots, not only with these affinity-purified antibodies (FIG. 2A, lane 4), but also with each of the eight individual sera of which the pool was made up (data not shown). 
     The recombinant antigen also showed striking species specificity (FIG. 2B); it did not react with serum pools obtained from patients infected with lymphatic filariae (W. bancrofti), with other filariae (L. loa, M. perstans), or with intestinal nematodes (A. lumbricoides, T. trichiura). 
     EXAMPLE 3 
     Identification of the Native Parasite Proteins and of the Primary Translation Products 
     To identify the native O. volvulus protein(s) that share antigenic determinants with the OV-16 cDNA fusion protein, the hybrid protein was bound to nitrocellulose and used to affinity purify antibodies from the onchocerciasis serum pool (O.V.-M). Immunoblot analysis with the selected antibodies detected 2 polypeptides strongly (24 and 26 kDa) and 3 weakly (17, 22 and 40 kDa) (FIG. 3A, lane 2). 
     To examine the possibility that the protein encoded by the OV-16 cDNA might be modified in vivo and to identify the primary translation product of the OV-16 cDNA mRNA, [ 35  S]methionine-labeled cell-free translation products were subjected to immunoprecipitation with antibody selected against the parasite epitopes encoded by OV-16 cDNA. As shown in FIG. 3B, lane 2, a polypeptide of 18 kDa was specifically immunoprecipitated. In contrast, the band was not present when antibodies selected against β-galactosidase alone were used as a control (lane 1). 
     EXAMPLE 4 
     Characterization of the OV-16 cDNA Clone and cDNA Sequence 
     The OV-16 cDNA was excised by digestion with EcoRI and subcloned into the sequencing vector M13mp18 in both orientations. The complete sequence of the antigen-producing clone OV-16 cDNA was determined by the dideoxy chain-termination method (Sanger et al. (1977) Proc. Natl. Acad. Sci. USA 74, 5463-5467). The suggested reading frame used to synthesize the native protein is the same reading frame as in the fusion protein. The nucleotide sequence of cDNA for the low-molecular-weight antigen and the predicted amino acid sequence are shown in FIG. 4A. Sequence analysis of the 813-bp insert revealed an open reading frame encoding 152 amino acids; the size for the OV-16 primary translation product deduced from the cDNA sequence is 16.85 kDa. The assignment of the translational initiation codon 50 bp from the 5&#39; end was made since it was the first ATG in the open reading frame and it contained a purine (adenine) in the -3 position, thought to be a prerequisite for an initiation codon (Kozak, M. (1986) Cell 44, 283-292). The initiation codon is followed by a hydrophobic sequence, predicted by hydropathy analysis (FIG. 4B), highly characteristic of a signal peptide. Using the prediction method of von Heijne (Von Heijne, G. (1986) Nucleic Acids Res. 14, 4683-4690), a potential signal peptidase cleavage site could be found, suggesting cleavage after residue 16 (Gly). The polypeptide is terminated by a TAA stop codon followed by a 3&#39; non-coding region of 307 bp. The 3&#39; non-coding region includes the eukaryotic polyadenylation signal AATAAA, which is located 8 nucleotides from the poly(A) tail (FIG. 4A). There are four potential acceptor tripeptides for N-glycosylation (Asn-Xaa-Ser/Thr) in the predicted amino acid sequence, located in the hydrophilic domains of the protein (boxed areas, FIG. 4A). Glycosylation at these sites could adequately account for the difference between the predicted poly-peptide mass of 16.85 kDa and the observed sizes of the native parasite proteins recognized by the affinity-purified antibodies (24, 26 and 40 kDa). 
     By hybridization of the nick-translated OV-16 cDNA with the other antigen producing clones, a cross-hybridizing cloned cDNA was detected with a small insert of 682 bp which encoded a hybrid protein of 129 kDa. This cDNA had the same DNA sequence as OV-16 cDNA, but is 131 bp shorter in its 5&#39; region (data not shown). 
     To determine if there was homology with other proteins, a computer search was conducted (EMBL data bank). There was no homology with other known proteins. 
     EXAMPLE 5 
     DNA and RNA Blot Analysis 
     To identify genomic DNA fragments carrying the gene(s) encoding the parasite antigen OV-16 cDNA, O. volvulus DNA was cut with various restriction enzymes, and the resulting fragments were hybridized to the  32  P-labeled cDNA insert of clone OV-16 cDNA. When DNA was cut with the restriction enzyme EcoRI, two bands of 2.5 and 4.3 kb were detected. HindIII digest revealed two bands of 4.3 and 5.0 kb (FIG. 5, left-hand panel, lanes a and b, respectively). No hybridization signals were detected with human DNA from HeLa cells cut with similar restriction enzymes (data not shown). 
     Northern blot analysis for the parasite RNA revealed the presence of a single OV-16 mRNA transcript of 950 nucleotides in length (FIG. 5, right panel). 
     The data suggest that OV-16 undergoes several post-translational modifications including cleavage of a signal peptide and N-linked glycosylation. A hydropathicity analysis of the polypeptide is reproduced in FIG. 4B. The profile shows a highly hydrophilic polypeptide. 
     EXAMPLE 6 
     Immunolocalization of OV-16 cDNA 
     The ultrastructural localization of parasite antigens that share epitopes with the OV-16 cDNA fusion protein was determined by immunoelectron microscopy on thin sections of O. volvulus female worms using the affinity-purified anti-OV-16 cDNA antibodies and gold-labeled anti-human IgG (DeMey, J. (1983) Immuno-gold staining of surface cell antigens in cell suspensions. GAMG 30/colloidal gold coated with immunoglobulins. Jansen Life Science Products Division, Belgium). The antigens were localized in the hypodermis (the cellular layer from which the cuticle of nematodes is derived; FIG. 6.1), the cortical layer of the cuticle (FIG. 6.2), and the apical part and surface of the uterine epithelium (FIG. 6.3). 
     The subcellular localization and the already-mentioned structural characteristics of the deduced amino acid sequence suggest that OV-16 in its processed form is presented to the host immune system through excretory-secretory mechanisms. 
     EXAMPLE 7 
     Purification of OV-16 Fusion Protein 
     A 682 bp fragment of the OV-16 gene (encoding 123 amino acids) without the leader sequence, was fused to the COOH-terminus of the maltose-binding protein coded for by Male of Escherichia coli (C. V. Maina et al., Gene 74,365 (1988)). The construction of the recombinant plasmid pCG808fx-16 shown in FIG. 7. The signal peptide was not included in the construct, as efficient synthesis of foreign proteins in E. coli often requires deletion of their signal sequences because hydrophobic regions of eukaryotic proteins are toxic to E. coli (J. S. Mort et al., Hoppe Seyler Biol. Chem. 369 suppl.,163 (1988); T. Vernet et al., Gene 77,229 (1989)). The purification of the fusion protein MBP-16 is illustrated in FIG. 8 (panel A). 
     Briefly, E. coli 71-18 ([lac-proAM] thi supE [F&#39; pro A +  B +  lac Iq  ] lac Z M15) bearing the appropriate plasmid construct was grown at 37° C. in 250 ml Luria broth (LB) to 0.8 O.D. (A 600 nm) and induced with (IPTG) for 2 hr. The cells were harvested by centrifugation at 9 K rpm for 15 min, 4° C. The cell pellet was washed 2x in cold sodium phosphate buffer, pH 7.5 (PBS), 5 mM EGTA, and suspended in 25 ml lysis buffer (10 mM Tris-HCl, pH 7.5, 1 mM phenylmethyl-sulfonyl fluoride (PMSF), 10 mM β-mercaptoethanol (β-SH), N-tosyl-L-phenylalanine-chloromethyl-ketone (20 μg/ml), leupeptin (10 μg/ml), 20% sucrose, 30 mM NaCl, 10 mM EDTA, 0.2% Tween 20. Cells were lysed by sonication, and unbroken cells and cell debris were removed by centrifugation for  30 min, 4° C. at 10 K rpm. The supernatant was diluted 1:5 with 10 mM Tris-HCl, pH 7.5, 30 mM NaCl, 0.25% Tween 20, 10 mM EDTA, 1 mM PMSF, 10 mM EGTA, and adsorbed overnight at 4° C. with 25 ml cross-linked amylose resin. The bound fusion protein was eluted with maltose, fractions were collected, pooled and dialysed to remove maltose. The dialysate was concentrated and the protein content estimated (C. V. Maina et al., Gene 74,365 (1988), T. Ferenci and U. Klotz, FEBS Lett. 94,213 (1978)). Approximately 6 mg of fusion protein were obtained from 250 ml culture. MBP-16 fusion protein (1 mg) digested with 10 μg factor X a  for 4 days at r.t. resulted in approximately 60-70% of the fusion protein being cleaved. The cleavage products were separated by FPLC using a Mono S™ column. 
     There is a major protein band with a M r  of 52000 which became prominent after induction with 0.3 mM isopropylthiogalactosidase (IPTG) (FIG. 8, lane 2). After the MBP-16 fusion protein is purified by affinity chromatography on cross-linked amylose, the major band at M r  52000 continues to be present, along with a minor band of M r  40000 which probably represents a premature termination of the fusion protein or its digestion by E. coli proteases (lane 4). As this fusion protein contains the recognition sequence Ile-Glu-Gly-Arg for the protease between the MBP and the OV-16 domains (C. Guan et al., Gene 67,21 (1987); K. Nagai and H. C. Thogersen, Nature 309,810 (1984)), digestion of MBP-16 with activated factor X allowed separation of the two protein domains (panel A, lane 5). Some of the fusion protein remained uncleaved. OV-16 was further purified, from the MBP, the truncated form and the uncut fusion protein, by FPLC using a Mono S™ column. The purification procedure did not affect antigenicity as determined by immunoblot analysis of the fusion protein and the isolated OV-16 (FIG. 8, panel B). 
     EXAMPLE 8 
     Presence of OV-16 in Patients 
     The isolated OV-16 was used in ELISA to analyze the antibody responses of 41 onchocerciasis patients (aged 3-60 years), who had proven infections (mf detected in skin) and were residents of a region highly endemic for O. volvulus in the savanna zone of Mali. Onchocerciasis patients were part of a longitudinal study whose detailed parasitological and serological data have been described elsewhere [M. Karam and N. Weiss, Am. J. Trop. Med. Hyg. 40,261 (1985), N. Weiss and M. Karam, Ciba. Found. Symp. 27,180 (1987)]. `Normal controls` were individuals (Swiss) never exposed to infection with filarial or other nematode parasites of humans. Sera from patients with other filarial infections--Wuchereria bancrofti, Brugia malayi, Mansonella ozzardi, Loa loa, Mansonella perstans--and other helminthic infections (K. Nagai and H. C. Thogersen, Nature 309,810 (1984)) were used to ascertain the diagnostic specificity of OV-16 (FIG. 9). Sera from these patients were from either the WHO or NIH Filariasis Serum Banks. Levels of anti-OV-16 antibody were determined by ELISA. Briefly, Immunolon 4 plates (Dynatech, Alexandria, Va.) were coated with 300 ng OV-16 in coating buffer pH 7.6/ml overnight at 4° C. The plates were blocked with 5% BSA for 1 hr at 37° C. All sera were run in duplicate at a 1:100 dilution and incubated overnight. For assays of total IgG, Fc-specific, alkaline phosphatase-conjugated goat antibody to human IgG (Sigma, St. Louis, Mo.) was added. Thirteen uninfected samples were used to determine the normal range (mean ±3 SD). A high-titered standard reference onchocerciasis serum pool was used to generate calibration curves against which all sera were compared for antibody levels (Flow Cytometric Program 1.5, Munich, Germany). Levels are expressed as arbitrary units/ml. 
     OV-16 allowed for the detection of anti-OV-16 antibodies in 37 of 41 (90%) patients with onchocerciasis (geometric mean 41.4 U/ml [normal&lt;4.6 U/ml]) and was also effective in differentiating onchocerciasis from the other filarial infections, including L. Loa (O/14 positive), W. bancrofti from the Philippines (0/14 positive) and Sri Lanka (0/11), B. malayi from Indonesia (0/12), and M. perstans from west Africa (0/2). For M. ozzardi, the one individual (of 5 studied) from Venezuela who reacted positively in the ELISA, resided in an area where coinfection with O. volvulus was a distinct possibility. Unexposed persons living outside filarial endemic areas (Switzerland) had no antibody to this protein (0/13 positive). Thus, by using this assay, a specificity of 98% (1/57) and a sensitivity of 90% (37/41) for O. volvulus was obtained. 
     No correlation was found between the number of mf per skin snip and the reactivity to OV-16, although there was a decrease in the levels of antibody to OV-16 in microfiladermic patients over 20 years of age (N. Weiss and E. Lobos, unpublished observations), a finding consistent with the modulation of immune responses seen in chronic parasitic infections. While the species-specificity of OV-16 was dramatic (FIG. 9), the antigenicity of OV-16 was also conserved among geographic isolates of O. volvulus with patients from the W. African savanna (described here) as well as those from the W. African rain-forest (Ivory Coast) and from the New World (Guatemala) (E. Lobos and N. Weiss, unpublished observations). 
     EXAMPLE 9 
     Humoral Immune Response 
     Polyclonal antiserum raised to purified OV-16 demonstrated that OV-16 accumulated in parasite-free culture supernatants in its post-translationally modified forms (E. Lobos, unpublished observations), with M r  in the range 2,000-30,000, and was specifically recognized by the monospecific polyclonal antiserum. This finding suggested that OV-16 is a released parasite product and would be available to induce an immune response early in infection. To examine this possibility more directly, the course of the humoral immune response to OV-16 was monitored in parallel with the onset of patency (first detection of mf in the skin) in two chimpanzees experimentally inoculated with infective Ov larvae (H. R. Taylor et al., Am. J. Trop. Med. Hyg. 39,86 (1988)). FIG. 10 shows that antibodies to OV-16 developed 3 months and 12 months prior to the first appearance of skin mf (FIGS. 10A and 10B). 
     EXAMPLE 10 
     Analysis of Parasitologically Negative Children 
     Because infection of children can be an important epidemiologic indicator of ongoing transmission of O. volvulus, the antibody response to OV-16 was analyzed in eight exposed but parasitologically negative children (aged 1-14) who were part of a 4-year longitudinal study carried out in a savanna region of Mali highly endemic for onchocerciasis (Table 1). In three of the children, O. volvulus infection could be detected by the presence of antibodies to OV-16, during the prepatent period, 1-1.5 years before the appearance of mf in the skin. In four other children, there was a sharp increase in the antibody to OV-16 in the same year that mf positivity developed. In the eighth patient, no clinical, parasitological or serological evidence of infection was observed and, therefore, he was assumed to be truly uninfected. 
     
                       TABLE 1*______________________________________Anti-OV-16 Ab**microfilariae       SkinYear                YearPatient  0     1       2   3      0   1     2   3______________________________________1      -     +       +   +      -   -     +   +2      -     +       +   +      -   -     +   +3      +     +       +   +      -   -     +   +4      -     +       +   ND     -   +     +   ND5      -     +       +   ND     -   +     +   ND6      -     -       +   +      -   -     +   +7      -     +       +   +      -   +     +   +8      -     -       -   -      -   -     -   -______________________________________ *Detection of antibodies to OV16 in children (aged 1-14) from a savanna region in Mali hyperendemic for onchocerciasis. The children were followe during a longitudinal study over 4 years (0 yr, 1 yr, 2 yr, 3 yr), and th data reflect the presence of antibodies to OV16 in relation to the appearance of skin mf. Patient number 8 remained parasitologically and serologically negative all through the study. Antibody positivity clearly demonstrates the infection at least 1 year before the parasitological diagnosis (patients 1-3). Patients 4-7 showed a sharp increase in antibod level against OV16 in the same year as the mf appeared. **A positive value is defined as &gt;3 S.D. above the geometric mean of thirteen normal individuals run simultaneously. 
    
     All publications mentioned hereinabove are hereby incorporated in their entirety by reference. 
     While the foregoing invention has been described in some detail for purposes of clarity and understanding, it will be appreciated by one skilled in the art from a reading of this disclosure that various changes in form and detail can be made without departing from the true scope of the invention and appended claims. 
     
         __________________________________________________________________________SEQUENCE LISTING(1) GENERAL INFORMATION:(iii) NUMBER OF SEQUENCES: 2(2) INFORMATION FOR SEQ ID NO:1:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 822 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: double(D) TOPOLOGY: linear(ix) FEATURE:(A) NAME/KEY: CDS (B) LOCATION: 52..507(xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:CAGTTTGAGGATCGGTTGCTTGTTTTTTGCATCAATCGTGTATGCTCGATAATGCAT57MetHis 1TGTTTGCAAGTAGTAATCGCCATAGTATTGTACTCATTTGGAAAAATA105CysLeuGlnValValIleAlaIleValLeuTyrSerPheGlyLysIle510 15TCTGCAGAAAATGCTAATTGCAAAAAGTGCACACCAATGTTAGTAGAT153SerAlaGluAsnAlaAsnCysLysLysCysThrProMetLeuValAsp2025 30TCGGCATTCAAGGAACATGGAATTGTACCGGACGTTGTATCAACAGCT201SerAlaPheLysGluHisGlyIleValProAspValValSerThrAla354045 50CCTACGAAGTTGGTCAATGTTAGTTACAATAATCTCACGGTGAATCTG249ProThrLysLeuValAsnValSerTyrAsnAsnLeuThrValAsnLeu5560 65GGCAATGAACTTACGCCGACGCAGGTAAAGAATCAGCCGACAAAAGTA297GlyAsnGluLeuThrProThrGlnValLysAsnGlnProThrLysVal7075 80TCATGGGATGCGGAACCTGGAGCCTTATATACGCTCGTTATGACTGAT345SerTrpAspAlaGluProGlyAlaLeuTyrThrLeuValMetThrAsp8590 95CCGGACGCACCATCTCGAAAAAACCCCGTATTCAGAGAGTGGCACCAT393ProAspAlaProSerArgLysAsnProValPheArgGluTrpHisHis100105110TGGT TGATAATTAATATTTCTGGACAAAATGTTAGCAGTGGCACAGTG441TrpLeuIleIleAsnIleSerGlyGlnAsnValSerSerGlyThrVal115120125130 TTATCTGATTATTGGATCAGGTCCACGAAAAGGCACAGGACTTCATCG489LeuSerAspTyrTrpIleArgSerThrLysArgHisArgThrSerSer135140145 TTATGTATTCTTGGTTTATAAACAACCTGGAAGTATCACGGATACTCA537LeuCysIleLeuGlyLeu150ACATGGCGGAAATCGCCGAAATTTCAAAGTTATGGATTTTGCAAACAAACATCACTTGGG597AAATCCA GTTGCCGGAAACTTCTTCCAGGCTAAACATGAGGATTAACATGAAGACTGTGA657ATATGAATATGAACTGCTTGAACGACACTAGAGACTCAGCGACTGATACTTATTGATTTG717TTTTTGTAACATTTGAATGAATTTTTCTTTACAGTTATTTGCTAAATTTCGA ATTTAATG777GGAATAAATATTTTTTAAAAAAAAAAAAAAAAAAAAAGGAATTCC822(2) INFORMATION FOR SEQ ID NO:2:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 152 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:MetHisCysLeuGlnValValIleAlaIleValLeuTyrSerPheGly151015LysIleSerAlaGluAsnAlaAsnCysLysLysCysThrProMetLeu 202530ValAspSerAlaPheLysGluHisGlyIleValProAspValValSer354045ThrAlaProThrLysLeuValA snValSerTyrAsnAsnLeuThrVal505560AsnLeuGlyAsnGluLeuThrProThrGlnValLysAsnGlnProThr657075 80LysValSerTrpAspAlaGluProGlyAlaLeuTyrThrLeuValMet859095ThrAspProAspAlaProSerArgLysAsnProValPheArg GluTrp100105110HisHisTrpLeuIleIleAsnIleSerGlyGlnAsnValSerSerGly115120125ThrValLeuSe rAspTyrTrpIleArgSerThrLysArgHisArgThr130135140SerSerLeuCysIleLeuGlyLeu145150