IE904083A1 - Diagnostic proteins to test for more than one antibody - Google Patents

Abstract

This invention is directed to the discovery that certain envelope peptide fragments of the Human Immunodeficiency Virus 2 (HIV-2) are particularly immunoreactive against HIV-2 antibodies. These fragments can therefore be applied to immunodiagnostic tests for the detection of antibodies to HIV-2. This invention is also directed to certain chimeric proteins that are made from immunogenic portions of the envelope gene of HIV-2, HIV-1, or HTLV-I that can be used to test for antibodies to HIV-2, HIV-1, and HTLV-I and HTLV-II.

Description

Human Immunodeficiency Viruses (HIVs) are retroviruses which carry their genetic code on RNA. In humans, Acquired Immune Deficiency Syndrome (AIDS) may be caused by either of two types of HIV: HIV-1 or HIV-2.

HIV-1 (originally HTLV-III) was Isolated and Identified by Gallo and Montagler et_al.. U.S. 4,520,113. Ratner et al., Nature 111:277-284 (1985); Mueslng el al.. Nature 211:450-458 (1985); Sanchez-Pescador et al.. Science £2Z:484-492 (1985); and Hain-Hobson et al.. Cell lfl:9-17 (1985) disclose the complete DNA sequence of the HTLV-III virus. -2HIV-2 (originally LAV-2) was first Isolated fro» West Africans with AIDS-like Illness (Clavel, F. et al.. Science 222:343-346 (1986); Clavel, F. at al.. Nature 324:691-695 (1986)).

HIV-1 and HIV-2 are related to the human T-cell leukemialymphoma (HTLV) virus family of T4 tropic retroviruses. HTLV1 1s the etiological agent of T-cell leukemia and lymphoma. HTLV-II, originally Isolated from a patient with hairy-cell leukemia, is associated with the development of malignant leukemia of mature T-lymphocytes. The complete nucleotide sequence of the provirus genome of HTLV-I 1s given 1n Se1k1 si 41.» Proc.Nat'l Acad, Scl, (USA) 80:3618-3622 (1983).

When a retrovirus Infects a host cell, a DNA copy of Its genome 1s Integrated into the chromosome of Its host. With some retroviruses, the DNA 1s Integrated Into the host cell's chromosomes 1n the form of a sequence known as a provirus. The DNA copy of the retrovirus' genetic code 1s synthesized by a viral enzyme called RNA dependent DNA polymerase, or reverse transcriptase. The host cells transcribe the DNA of the viral gene and synthesize the proteins encoded by the virus, which are then assembled Into new viruses.

The HIV viruses and HTLV viruses contain at least (1) a gag gene that encodes the Internal structural (neurocapsid or core) proteins, (11) a pol gene that encodes the reverse transcriptase, and (111) an env gene that encodes the envelope glycoproteins of the virus.

In early studies with HIV-1, Gallo (Gallo, R.C. et aK. Science 221:300:503 (1984); Sarnagadharen, N.G. et al.. Science 224:506-508 (1965)) and Nontagnler (Barre-S1nouss1, F. et al.. Science 220:068-871 (1983)), using Western blots, demonstrated that most AIDS patients had antibodies to HIV-1 antigens. From this work, and because 1t was not widely appreciated that blots could have nonspecific reactions at p!7, p24, and other HIV-1 antigens, It was commonly believed -3that gag antigens were the appropriate antigens to be used for screening for HIV-1 antibodies. However, not all AIDS sera 1s reactive 1n Western blots against gag antigens. The first and most reliable markers of Infections are the presence of antibodies to the envelope protein.

Viral lysates of HIV-1 are currently widely used for the detection of antibodies to HIV-l In human sera. The viral lysate comes from HIV-1 that has been grown 1n tissue culture and partially purified as the antigen source. The tests are quite sensitive, but suffer from a relatively high rate of false positives. Hany scientists have attributed these false positives to cellular proteins contaminating the virus preparations (Honter, J.B. et al.. Lancet 1:1222-1223 (1985); Sayers, H.H., Transfusion ££:113-115 (1986)) and the presence of cross-reactive antibodies (Thlry, L. et al.. Science £2Z:1484 (1985,j Volsky, D.J., New Engl, J, Med, 115:457-458 (1986)).

The HTLV-I and HTLV-Π virus can be readily transferred from the peripheral blood leukocytes of anti body-positive people to leukocytes of antibody-negative people when the two are cultivated together. Popovlc et al.. Science £l£;856-859 (1983). Consequently, there Is a risk of Infection Involved 1n whole blood transfusions when the transfused blood contains Infected cells.

Moreover, Individuals Infected with one retrovirus nay also be harboring a second retrovirus infection. Biological specimens from people with an HIV-1 Infection often also give a positive test for antibodies to HTLV-I or HTLV-II. Assays were conducted 1n the following studies for HTLV-I and HIV-1 antibodies 1n patient sera: Rossi et al.. Eur. J, Cancer CUn. Oncol ££:411-418 (1986); Aok1 et al,. Lancet. October , 1984, pages 936-937; Tedder et al.. Lancet. July 21, 1984, pages 125-128; and Robert-Guroff et al.. Lancet. July 21, 1984, pages 128-130. In these studies, the HTLV-I was -4detected by viral lysate (Rossi et al. and Aokl et al. 1 and with core antigen (Tedder et al. and Robert-Guroff et al J.

The Pasteur ELAVIA mixed assay has been reported to preferentially detect HIV«2 antibodies over HIV-1 antibodies. (Lelie, However, this assay 1s based on the use of a HIV-2 viral lysate assay and thus requires the use of whole virus.

In the United States, human blood must be screened for antibodies to HIV-1 and to HTLV-I and for hepatitis. It 1s expected that soon human blood sera will also need to be screened for antibodies to HIV-2. Thus, 1t would be desirable to have a reliable screening assay to test for the presence of antibodies to HIV-2 1n human biological samples. It would also be desirable to have a single test that would be able to detect more than one antibody 1n human biological samples.

SUMMARY QE THE INVENTION The Invention comprises the amino acid sequences of Immunoreactive env HIV-2 peptides that can be used for detecting antibodies to HIV-2. The Invention also comprises the amino add sequences of Immunodlagnostlc chimeric env peptides which are able to detect more than one antibody. Specifically, these chimeric env peptides are able to detect antibodies to HIV-2, HIV-1, and HTLV-I and HTLV-II. Thus, this Invention comprises chimeric env peptides comprising Immunodlagnostlc env peptide fragments of HIV-2-HZV-lt HIV2-HIV-l-HTLV-I; HIV-2-HTLV-I; and HIV-l-HTLV-I.

BRIEF DESCRIPTION OF THE DRAWINGS Figure 1 shows the construction of plasmid pKl from plasmids K3D, containing the HIV-1 clone K30, and pCBCl. -5Figure 2 1s an electrophoretic gel showing an Induced 34 kd protein, called Kl.

Figure 3 1s a Western blot showing the reaction of the induced protein, Kl, with human sera from HIV-2 infected Individuals.

Figure 4 gives the complete DNA sequence of the coding region of the Kl and the derived amino acid sequence.

Figure 5 shows the construction of plasmid pK3 and a 1038 base pair fragment from position 7101 to position 8139 and the ligation of K3D Into the expression vector pCBC2.

Figure 6 Is an electrophoretic gel showing an Induced 40 kd protein, called K3.

Figure 7 1s a Western blot showing the reaction of the induced protein, K3, with human sera from HIV-2 Infected Individuals.

Figure 8 gives the complete DNA sequence of the coding region of the K3 and the derived amino add sequence.

Figure 9 shows the construction of the plasmid pKlDG71 from plasmids pLCBC0DG71A and pKl.

Figure 10 1s en electrophoretic gel showing an induced 55 kd chimeric protein, called K1DG71.

Figure 11A 1s a Western blot showing the reaction of the Induced protein, K1DG71, with human sera from HIV-1 Infected individuals.

Figure 11B 1s a Western blot showing the reaction of the Induced protein, K1DG71, with human sera from HIV-2 Infected Individuals.

Figure 12 gives the complete DNA sequence of the coding region of the pKlDG71 and the derived amino add sequence.

Figure 13 shows the construction of the plasmid pDG71353.

Figure 14 shows the construction of the plasmid pKlDG71353.

Figure 15 gives the complete DNA sequence of the coding region of the pKlDG71353 and the derived amino add sequence. -βFigure 16 1s an electrophoretic gel showing an Induced 68 kd chimeric protein, K10G71353.

Figure 17 1$ a Western blot showing the reaction of the induced protein, K1DG713S3, with human sera from HIV-l positive individuals.

Figure 18 Is a Western blot showing the reaction of the Induced protein, K1DG71353, with human sera from HIV-2 positive Individuals.

Figure 19 1s a Western blot showing the reaction of the induced protein, K1DG71353, with human sera from HTLV-I positive Individuals.

Figure 20 shows that no specific reactivity was seen with negative sera 1n a Western blot of the induced protein K1DG71353.

Figure 21 gives the complete DNA sequence of the coding region of the K1DG71353 protein and the derived amino acid sequence. -7DEFINITIONS In the description that follows, a number of terms used in recombinant ONA technology and Immunology are extensively utilized. In order to provide a clearer and consistent understanding of the specification and claims, Including the scope to be given such terms, the following definitions are provided.

Promoter. A DNA sequence located proximal to the start codon at the 5' end of the transcribed sequence. At the promoter region, transcription of an adjacent operably linked gene(s) 1$ Initiated.

Gene. A DNA sequence that contains Information for transcription of a mRNA which codes for a polypeptide or protein. Typically, the nucleotide of the first transcribed codon 1s numbered +1, and the nucleotides are numbered consecutively with positive Integers through the transcribed regions of the gene. Nucleotide +1 may or may not also code for the first translated amino acid. A gene may have regions at the 5' end and 3' end which are transcribed but which are not translated. Similarly, the gene may or may not contain Intron Information which must be spliced out prior to translation of the mRNA. The mRNA may or may not have regions at the 5' end and/or the 3' end which are not translated.

The numbering of nucleotides In the promoter and transcriptional regulatory region 5' to the transcribed region proceeds consecutively with negative Integers with the 5' nucleotide next to the first transcribed codon being numbered -1.

A complementary DNA or cDNA gene Includes recombinant genes synthesized by reverse transcription of mRNA and from which Intervening sequences (Introns) have been removed. -8· Ooerablv linked. As used herein, operably linked means that two elements are physically arranged such that factors which influence one element also Influence the other. For example, factors which Induce a specific promoter to function also Induce the transcription of a gene operably linked to that promoter.

Expression. Expression 1s the process by which the information encoded within a gene 1s revealed. If the gene encodes a protein, expression Involves both transcription of the DNA Into mRNA and translation of the mRNA Into protein.

Cloning vehicle. A plasmid or phage DNA or other DNA sequence which Is able to replicate autonomously 1n a host cell, and which 1s characterized by one or a small number of endonuclease recognition sites at which such DNA sequences may be cut in a determinable fashion without loss of an essential biological function of the vehicle, and into which DNA may be spliced 1n order to bring about Its replication and cloning. The cloning vehicle may further contain a marker suitable for use in the identification of cells transformed with the cloning vehicle. Markers, for example, are tetracycline resistance or amp1c1ll1n resistance. The word vector 1s sometimes used for cloning vehicle.

Expression vehicle. A vehicle or vector similar to a cloning vehicle but which 1s capable of expressing a gene which has been cloned Into it, after transformation into a host. The cloned gene 1s usually placed under the control of (1,e., operably linked to) certain control sequences such as promoter sequences. Expression control sequences will vary depending on whether the vector 1s designed to express the operably linked gene 1n a prokaryotic or eukaryotic host and may additionally contain transcriptional elements such as enhancer elements, termination sequences, tlssue-speclfldty elements, and/or translational Initiation and termination sites. -9Host. Any organism that 1s the recipient of a replicable expression vehicle.

Pentlde fragment. The term peptide fragment Is meant to Include any amino acid sequence which represents a segment of HIV-2, HIV-l, and/or HTLV-I, which 1s capable of 1mmunolog1cal1y reacting with the respective antibody and Includes naturally-occurring peptide sequences; synthetic, chemically-synthesized peptide sequences; and expressed, genetically engineered peptide sequences.

DESCRIPTION OF THEPREFERRED EMBODIMENTS The Invention comprises the amino acid sequences of Immunoreactlve env HIV-2 peptides that can be used for detecting antibodies to HIV-2. The Invention also comprises genetic sequences coding for the Immunoreactlve env peptides, expression vehicles containing the genetic sequences, and hosts transformed therewith.

The Invention also comprises the amino acid sequences of Immunoreactlve chimeric env peptides which are able to detect more than one antibody. Specifically, these chimeric env peptides are able to detect antibodies to HIV-2, HIV-l, and HTLV-I and HTLV-II. Thus, this Invention comprises chimeric env peptides comprising Inmunodlagnostic env peptide fragments of HIV-2-HIV-1; HIV-2-HIV1-IITLV-I; HIV-2-HTLV-1; and HIV-1HTLV-I. By a chimeric env peptide Is meant a peptide wherein said peptide contains an amino add sequence which encodes domains of different viral peptides. Two peptides are said to be different peptides If they are not covalently joined 1n their mature form In the native virus. The Inventors have discovered that by combining domains of peptides from different retroviruses there Is created a chimeric peptide that 1$ able to detect antibodies to HIV-2, HIV-l, and HTLV-I •ίοand HTLV-II, depending on the particular construction of the chimeric peptide.

The chimeric env peptides may contain domains from any HIV-2, HIV-1, and HTLV-I env peptide as long as those domains are capable of being Immunoreactive against their respective antibodies or of being combined with another domain In such a way as to maintain, enhance or induce antibody recognition.

A complete HIV-2 nucleotide sequence from HIV-2$l/isy 1s described 1n (Franch1n1 et aL. Proc. Natl, Acad, Sc1, USA 21:2433-2437 (1989)). The preferred peptide fragments are those described In Examples 1, below, and shown 1n Figure 4, which gives the complete DNA sequence of the coding region of the K1 peptide fragment and the derived amino acid sequence and 1n Example 2, below, and shown 1n Figure 8, which gives the complete DNA sequence of the coding region of the K3 peptide fragment and the derived amino add sequence.

The preferred env peptides of HIV-1 are those described 1n Beltz et al.. U.S. 4,753,873, particularly the clone G peptide fragment and those peptide fragments derived therefrom. The most preferred env peptide fragment 1s CBre3, derived fro· the gpl2Q and gp41 regions of the HIV-1 env gene. CBre3, also Identified as delta G71A, 1s described 1n Thorn it il·, An enzyme Immunoassay using a novel recombinant polypeptide to detect human Immunodeficiency virus, J, Clin. Microbiol, 12:1207-1212 (1987) and In Beltz fit_il., U.S. 4,753,873. A cell line expressing the recombinant antigen 1s also on deposit at the American Type Culture Collection (ATCC), accession number 53455. Other recombinant HIV-1 antigens may be used 1n this Invention, provided that the antigens exhibit 1mmunoreact1v1ty to HIV-1 antibodies. Examples of such recombinant HIV-1 antigens are described 1n Chang, et al.. Bio/Technoloav. 2:905-909 (1985)5 Cabradllla it -11ll.. Blo/Technoloav. 1:128-133 (1985); and U.S. 4,629,783, all Incorporated herein by reference.

Essex ii_al·, PCT/US84/00561, publication no. WO 84/04327, describes the env glycoproteins of HTLV-I. Any 1mmunoreact1ve peptide fragment encoded by the env gene of HTLV-I may be used in this Invention. The preferred peptide fragment 1$ the HTLV-I envelope gene from base pairs 6101-6118 and 6170-6499 based on the published sequence of Se1k1 et al. (Rroc, Natl, Acad, Sci, USA fifl:3618 (1983)) Incorporated herein by reference. Other preferred peptide fragments are those described in Samuel et al.. Science 126:1094-1097 (1984), Incorporated herein by reference, which gives a restriction map of the env gene of HTLV-I. HTLV-II antibodies can also be detected with use of HTLV-I antigens.

As will be understood by one of skill 1n the art, there may be variations In the first one or two amino acids of the peptide fragments due to proper alignment of the cloned nucleotide sequence 1n the expression vehicle.

Also as will be understood by one of skill 1n the art, there may also be some variation 1n the peptide fragments, provided however, that these peptides retain immunoreactlvlty to antibodies to HIV-2, HIV-1, or HTLV-I, respectively. Thus the ranges 1n the length of the peptide fragments need not be precisely fixed. Amino acids of the peptide fragments may be deleted or added without loss of Immunoreactlvlty. Additionally, amino adds could be exchanged, e.g. a neutral amino adds such as a valine could be exchanged with another neutral amino add such as leudna. The changes 1n amino adds may be either conservative or non-conservative. There 1s also genomic variation 1n amino add sequence and nucleotide sequence between viral Isolates (see, for example, Wong-Staal, F. at al.. Science 229:759-762 (1985)). It 1s to be understood that such variations are Included 1n the peptide fragments of this Invention, provided that the peptide -12fragment 1s able to detect the appropriate antibody. By conservative substitutions 1s Intended combinations such as gly, ala; val, 11e, leu; asp, glu; asn, gin; ser, thr; lys, arg; and phe, tyr.

In the description of the methods that follow, the HIV-2 env peptide fragments are used for Illustration. The HIV-l and HTLV-I env peptides used 1n the chimeric env diagnostic peptides may also be used 1n these described methods.

The native peptide fragments of the HIV-2 virus may be used as a source of the peptide domains and may be obtained directly from the Infected host cell. The peptide fragment would then be obtained by fragmenting the naturally-occurring virus using suitable enzymes or chemical methods.

It 1s also possible to obtain the peptide fragments by chemical synthesis, for example, by well known solid phase peptide synthesis methods (Merrifield, J. Am, them, Soc, ££:2149 (1962); Bodanszky, M., Peotlde Chemistry:, A Practical Textbook. 19B6, Springer-Verlag, New York).

A preferred method of obtaining the peptide fragment 1s by cloning a polynucleotide fragment which codes for the desired peptide, using genetic engineering techniques. The advantages of using genetic engineering and recombinant clones are twofold: the first advantage 1s that 1t 1s difficult and time-consuming to obtain large amounts of the viral peptides either by direct Isolation from the virus or by chemical synthesis; the second advantage 1s that recombinant peptides are devoid of human antigens that may reduce the reliability of a diagnostic test.

The genetic constructs and the methods for using them can be utilized for expression of the peptide fragments 1n hosts, Including prokaryotic and eukaryotic hosts.

In a preferred embodiment, the Introduced sequence Is Incorporated Into a plasmid or viral vector capable of autonomous replication 1n a prokaryotic host. Any of a wide -13variety of vectors may be employed for this purpose, as outlined below.

Factors of Importance 1n selecting a particular plasmid or viral vector Include: the ease with which recipient cells that contain the vector may be recognized and selected from those recipient cells which do not contain the vector; the number of copies of the vector which are desired 1n a particular host; and whether 1t 1s desirable to be able to shuttle the vector between host cells of different species. The procaryotic hosts may Include bacteria such as E. coll. JL tYPhlffUrLyni, Serratla_marcescftPS or Bacillus subtllls.

Preferably, the peptides of the invention are expressed 1n prokaryotes and especially 1n E, coli.

The preferred bacterial host for expression 1s an E, coll strain that contains a temperature sensitive bacteriophage lambda CI857 gene, such as MZ1, described in Lautenberger ii al.. Gene,Anal, Tech, 1:63-66 (1984). Suitable vector systems for expression in E, col 1 are pCBCl, described by Beltz, U.S. 4,753,873, and pJL6 Lautenberger, gt,_j]L, Gene Anal. Tech. 1:83-66 (1984) wherein the bacteriophage lambda pL promoter, synthetic ribosome binding site and the first 13 amino acids from the bacteriophage lambda Cjj gene are provided on the vector together with a BamHI site for cloning purposes and synthetically derived DNA containing translation termination codons In all three reading frames.

Eukaryotic hosts may also be used and Include yeast, filamentous fungi, Insect cells and mammalian cells (Smith ii aF. Mol, Cell B1o1, 2:2156-2165 (1983)) and especially mammalian cells which have been Immortalized and may be maintained 1n cell culture.

Preferred eukaryotic plasmids Include those derived from the bovine papilloma virus, vaccinia virus, SV40, and, 1n yeast, plasmids containing the 2-micron circle, etc., or their derivatives. Such plasmids are well known 1n the art (BotIE 904083 -14Stein, D., et ik, Miami Mntr. Svmo. 12:268-274 (1982); Broach, J.R., In: The Molecular Biology of the Yeast Saccharomvces: Life Cycle and Inheritance. Cold Spring Harbor Laboratory, Cold Spring Harbor, NY, p. 445-470 (1981); Broach, J.R., CflU 22:203-204 (1982); Bollon, D.P., et al.. J, Clin. Hematol. Oncol. 12:39-48 (1980); Manlatls, T., In: £ftll Biology; A Comprehensive Treatise. Vol.. 3. Gene Expression.

Academic Press, NY, pp. 563-608 (1980)), and are commercially available. For example, mammalian expression vector systems which utilize the MSV-LTR promoter to drive expression of the cloned gene, and 1n which 1t is possible to cotransfect with a helper virus to amplify plasmid copy number, and, Integrate the plasmid Into the chromosomes of host cells have been described (Perkins, A.S. at al.. Mol, Cell B1o1. $:1123 (1983); Clontech, Palo Alto, California).

The DNA sequence of the peptide fragments can also be Inserted Into the genome of viruses which 1s used to Infect e cell; for example, vaccinia virus and bacculovlrus may be used. (Mackett, M. et al.. Proc, Natl, Acad. 5c1. USA 22:7415 (1982); Panical 1, D. pt al·.. Proc. Natl. Acad. Sci. USA 22:5364 (1983); and Smith, G.L. at al,. Nature 302:490 (1983)) The recombinant vaccinia virus replicates 1n any mammalian cell and the fragment of Interest appears on the envelope or 1n Internal viral proteins.

The DNA sequence nay be chemically constructed 1f 1t 1s not desired to utilize the HIV-2 genome as the source of the genetic Information. Methods of chemically synthesizing DNA are well known 1n the art (Oligonucleotide Synthesis. A Practical Approach. M. J. Galt, ed., IRS Press, Washington, D.C., 1984; Synthesis and Applications of DNA and, RNA. S.A. Narang, ed., Academic Press, San Diego, CA, 1987). Because the genetic code 1s degenerate, more than one codon may be used to construct the DNA sequence encoding e particular amino -15ac1d (Watson, J.D., In: Molecular Btoloov of the Sena. 3rd Ed., W.A. Benjamin, Inc., Menlo Park, CA (1977), pp. 356-357).

To express the recombinant HIV-2 peptides of the Invention, transcriptional and translational signals recognizable by an appropriate host are necessary. The cloned HIV-2 peptide encoding sequences, obtained through the methods described above, and preferably 1n a double-stranded form, may be operably linked to sequences controlling transcriptional expression In an expression vector, and Introduced Into a host cell, either prokaryote or eukaryote, to produce the recombinant HIV-2 peptides of the Invention or functional derivatives thereof.

Expression of the HIV-2 peptides 1n different hosts may result 1n different post-tran$lat1onal modifications which may alter the properties of the peptides. It 1s necessary to express the peptides 1n a host wherein the ability of the peptides to be Immunologlcally recognized by HIV-2 antibodies Is not hindered.

In general, expression vectors containing transcriptional regulatory sequences, such as promoter sequences, which facilitate the efficient transcription of the Inserted gene fragment, and which are derived from spades compatible with the host cells, are used 1n connection with these hosts. The expression vector typically contains discrete elements such as, for example, a) either an origin of replication which allows for autonomous replication of the vector or elements which promote Insertion of the vector Into the host's chromosome, b) a suitable transcriptional promoter to which the sequence of Interest can be operably linked, c) a transcriptional terminator sequence 1f necessary, and d) specific genes which are capable of providing phenotypic selection In transformed cells. The precise nature of the regulatory regions needed for gene expression will vary between species or cell types and there are many appropriate -16expression vector systems that are commercially available (For example, through Pharmacia, Boehrlnger Mannheim or Clontech).

A nucleic acid molecule, such as DNA, 1s said to be capable of expressing a polypeptide 1f 1t contains expression control sequences which contain transcriptional regulatory Information and such sequences are operably linked to the nucleotide sequence which encodes the polypeptide.

An operable linkage 1s a linkage 1n which a sequence Is connected to a regulatory sequence (or sequences) 1n such a way as to place expression of the sequence under the Influence or control of the regulatory sequence. Two DNA sequences (such as HIV-2 peptide encoding sequence and a promoter region sequence linked to the 5' end of the encoding sequence) are said to be operably linked 1f Induction of promoter function results In the transcription of the peptide encoding mRNA and 1f the nature of the linkage between the two DNA sequences does not (1) result 1n the introduction of e frame-shift mutation, (2) Interfere with the ability of the expression regulatory sequences to direct the expression of the HIV-2 peptide, or (3) Interfere with the ability of the HIV-2 peptide template to be transcribed by the RNA polymerase. Thus, a promoter region would be operably linked to a DNA sequence If the promoter were capable of effecting transcription of that DNA sequence.

Expression of the HIV-2 peptides 1n eukaryotic hosts requires the use of regulatory regions functional In such hosts, and preferably eukaryotic regulatory systems. A wide variety of transcriptional and translational regulatory sequences can be employed, depending upon the nature of the eukaryotic host. The transcriptional and translational regulatory signals can also be derived from the genomic sequences of viruses which Infect eukaryotic cells, such as HIV, SIV, adenovirus, bovine papilloma virus, Simian virus, -17herpes virus, or the like. Preferably, these regulatory signals are associated with a particular gene which 1s capable of a high level of expression 1n the host cell. If desired, a fusion product of the HIV-2 peptides may be constructed. For example, the sequence coding for the HIV-2 peptides may be linked to a signal sequence which will allow secretion of the protein from, or the compartmentallzatlon of the protein In, a particular host. Such signal sequences may be designed with or without specific protease sites such that the signal peptide sequence 1s amenable to subsequent removal.

Transcriptional Initiation regulatory signals can be selected which allow for repression or activation, so that expression of the operably linked genes can be modulated. Of Interest are regulatory signals which are temperaturesensitive so that by varying the temperature, expression can be repressed or Initiated, or are subject to chemical regulation, e.g., metabolite.

Where the native expression control sequence signals do not function satisfactorily 1n the host cell, then sequences functional 1n the host cell may be substituted.

The vectors of the Invention may further comprise other operably linked regulatory elements such as enhancer sequences, or DNA elements which confer species, tissue or cell-type specific expression on an operably linked gene.

Once the vector or DNA sequence containing the construct(s) 1s prepared for expression, the DNA construct(s) 1s Introduced Into an appropriate host cell by any of a variety of suitable means, for example by transformation of bacterial cells. After the Introduction of the vector, recipient cells are grown 1n a selective medium, which selects for the growth of vector-containing cells. Expression of the cloned gene sequence(s) results 1n the production of the HIV-2 peptide or 1n the production of a fragment of this peptide. This -18expression can take place 1n a continuous manner 1n the transformed cells, or 1n a controlled manner.

If the HIV-2 peptide DNA encoding sequence and an operably linked promoter 1s introduced Into a recipient host cell as a non-replIcatlng DNA (or RNA) molecule, which may either be a linear molecule or, more preferably, a closed covalent circular molecule which 1s Incapable of autonomous replication, the expression of the HIV-2 peptide may occur through the transient expression of the Introduced sequence.

Genetically stable transformants may be constructed with vector systems, or transformation systems, whereby the HIV-2 peptide DNA Is Integrated Into the host chromosome. Such Integration may occur de novo within the cell or be assisted by transformation with a vector which functionally Inserts Itself Into the host chromosome, for example, with retroviral vectors, transposons or other DNA elements which promote Integration of DNA sequences 1n chromosomes. A vector 1s employed which Is capable of Integrating the desired gene sequences Into a mammalian host cell chromosome.

Cells which have been transformed with the HIV-2 peptidecontaining DNA vectors of the Invention are selected by also Introducing one or more markers which allow for selection of host cells which contain the vector, for example, the marker may provide biocide resistance, e.g., resistance to antibiotics, or heavy metals, such as copper, or the like.

The transformed host cell can ba fermented (if prokaryotic) or cultured (1f eukaryotic) according to means known 1n the art to achieve optimal cell growth, and also to achieve optimal expression of the cloned HIV peptide sequence fragments. As described herelnbelow, high level of HIV-2 peptide expression for the cloned sequences coding for peptide fragments can be achieved according to a preferred procedure of this Invention. -19After expression of the cloned HIV-2 peptide fragments, the fragments will typically be recovered and purified according to means known 1n the art. When bacteria are used as the host, high-level expression of the clones usually results 1n the formation of Insoluble inclusion bodies or aggregates. To purify the expressed proteins, the Insoluble Inclusion bodies must be made soluble. In the preferred embodiment of this Invention, the expressed peptide fragments are purified 1n a process using N-acylat1on of amino groups, for example, by citraconylatlon (Marclanl, D.J. et al.. Protein .Purification: Micro to Macro. Alan. R. L1ss, Inc., 1987 pp. 443-458.

An alternative to recombinant genetic engineering techniques for producing peptide fragment antigen Includes enzyme polymerase directed 1n vitro transcription and translation systems. An amplification system for producing peptide fragments 1s described, for example, 1n U.S. 4,683,202.

The purified Immunogenic and diagnostic peptide fragments according to this invention are specifically recognized by antibodies produced 1n response to the HIV-2 virus. The HIV-2 antibodies 1n blood or tissue samples can be detected using the peptide fragments 1n Immunoassays wherein the peptides can be utilized 1n liquid phase or bound to a solid phase carrier. In addition, the peptide fragments can be detectably labeled 1n various ways for use In Immunoassay* for virus. The preferred Immunoassays for detecting HIV-2 antibodies using the peptide fragments of this Invention Include radioimmunoassays, enzyme-1 Inked Immunosorbent assays (ELISA), or other assays known In the art, such as Immunofluorescent assays, chemiluminescent assays, or blolumlnescent assays. -20Radloactlve Isotopes which ire particularly useful 1n assays are 3H, 125I, ^31I, 32P, 33S, ^C, 31Cr, 3®C1, 57ς0> 58Co, 5*Fe, 75Se, and 152Eu.

While radiolabeling represents one embodiment, alternatively, the peptide sequence or antibodies thereto may also be labeled using fluorescent labels, enzyme labels, free radical labels, av1d1n-b1ot1n labels, or bacteriophage labels, using techniques known to the art (Chard, Laboratory Techniques In Biology. An Introduction to Radioimmunoassay and Related Techniques,” North Holland Publishing Company (1978).

Typical fluorescent labels Include fluorescein Isothiocyanate, rhodamlne, phycoerythrln, phycocyanln, allophycocyanln, o-phthaldehyde, and fluorescamine.

Typical chemiluminescent compounds Include luminol, 1solum1nol, aromatic acr1d1n1um esters, Imidazoles, acrldlnlum salts, and the oxalate esters. Typical blolunlnescent compounds Include 1uc1fer1n, luclferase, and aequorln.

Typical enzymes Include alkaline phosphatase, pg«1«ctos1dase, glucose-6·phosphate dehydrogenase, maleate dehydrogenase, glucose oxidase, and peroxidase.

Two principal types of enzyme assays are enzyme-1 inked immunosorbent assay (ELISA) and the homogeneous enzyme Immunoassay, also known as enzyme-multiplied Immunoassay (EMIT) (Syva Corp.). The EMIT system depends on deactivation of the enzyme 1n the tracer-anti body complex; the activity can thus be measured without the need for a separation step.

The Immunoassays within the scope of the present invention Include latex agglutination assays, 1mmunometr1c assays and competitive assays.

Latex agglutination assays have been described In Beltz, G.A. et al.. 1n Molecular Probes: Techniques and Medical Applications. A. Albert1n1 et aL·. eds., Raven Press, New York, 1989, Incorporated herein by reference. In the latex -21agglutination assay, a antigen-coated latex particles and serum to be tested are mixed and the results then read. With samples lacking HIV-2 antibodies, the latex particles remain 1n suspension and retain a smooth, milky appearance. However, 1f antibodies reactive with the recombinant antigen are present, the latex particles clump into visibly detectable aggregates. There are several ways to read the results of the latex agglutination assay, Including visually with slides, see for example, R1gg1n at el.. EPO Published Patent Application No. 289,339, Incorporated herein by reference, and with specially made slides which are read either visually or with a spectrophotometer, for example those devices described 1n U.S. 4,596,895 and 4,775,515, Incorporated herein by reference. The latex agglutination assay 1s especially suitable for small volume users, emergency situations, and areas lacking the sophisticated laboratory equipment and supplies needed for 1mmunometr1c assays.

An agglutination assay can also be used to detect HIV-2 antibodies wherein the desired peptide fragment Is Immobilized on a suitable particle other than latex beads, for example, on gelatin, red blood cells, nylon, liposomes, gold particles, etc. The presence of antibodies 1n the same causes agglutination, similar .to that of a precipitation reaction, which can then be detected by such techniques as nephelometry, turbidity, Infrared spectrometry, visual Inspection, colorimetry, and the like.

Immunometrlc assays Include forward sandwich, reverse sandwich Immunoassays and simultaneous assay. Each of these terms 1s well understood by those skilled In the art. The Immunometrlc assays will be described for the detection of antibodies to HIV-2. In these essays, the peptide fragment Is bound to the solid-phase carrier and ant1-IgG antibodies are detectably labeled. -22In a forward sandwich Immunoassay, a sample suspected of containing antibodies against HIV-2 1$ first incubated with a sol Id-phase Immunoabsorbent containing the peptide fragment. Incubation 1s continued for a period of time sufficient to allow the antibodies In the sample to bind to the Immobilized peptide fragment. After the first Incubation, the solid-phase Immunoabsorbent 1s separated from the Incubation mixture and washed to remove Interfering substances which also may be present 1n the sample. Solid-phase Immunoabsorbentcontalnlng antibodies bound to the Immobilized peptide fragments are subsequently Incubated for a second time with soluble labeled antibody cross-reactive with a different domain on the antibody to be detected. After the second Incubation, another wash 1s performed to remove unbound labeled antibody from the solid-phase Immunoabsorbent and to remove non-spedflcally bound labeled antibody. Labeled antibody bound to the solid-phase Immunoabsorbent Is then detected and the amount of labeled antibody detected serves as a direct measure of the amount of antibodies present 1n the original sample. Alternatively, labeled antibody which 1s not associated with the Immunoabsorbent complex can also be detected, 1n which case the measure 1s 1n Inverse proportion to the amount of antigen present 1n the sample. Forward sandwich assays are described, for example, 1n United States Patents 3,867,517; 4,012,294; end 4,376,110.

In a reverse sandwich assay, the sample suspected of containing test antibodies against HIV-2 Is Initially incubated with labeled anti-antibody, after which the solidphase Immunoabsorbent containing immobilized peptide fragment cross-reactive with a different domain on the test antibody 1s added thereto, and a second Incubation Is carried out. The initial washing step required by a forward sandwich assay 1s not required, although a wash 1s performed after the second -23incubatlon. Reverse sandwich assays have been described, for example, 1n U.S. Patent No. 4,098,876 and 4,376,110.

In a simultaneous sandwich assay, the sample, the Immunoabsorbent having Immobilized peptide fragment thereon and labeled soluble antibody specific to a different domain of the test antibody are Incubated simultaneously In one Incubation step. The simultaneous assay requires only a single Incubation and does not require washing steps. The use of a simultaneous assay Is a very helpful technique, providing ease of handling, homogeneity, reproducibility, linearity of the assays, and high precision. A simultaneous sandwich assay is described, for example, 1n U.S. Patent No. 4,376,110.

So-called delayed 1mmunometr1c assays can also be utilized, as are, for example, described 1n Chu, U.S. Patent No. 4,289,747, and Wolters, U.S. Patent No. 4,343,896.

Another Inmunometrlc assay Involves capturing the Fc capture technique . In the Fc capture Immunoassay, total serum antibodies are captured through anti-human Fc antibodies, typically bound to a solid support. Thus, bound, the Fc region of the antibody to be detected does not participate 1n other protein-protein Interactions. The antibodies to be detected can then be screened with the HIV-2 peptide fragment(s) or with the appropriate chimeric peptide fragment(s) of this Invention. A preferred Fc capture Immunoassay Is described 1n U.S. Serial No. 07/203,730, filed June 8, 1988, Incorporated herein by reference.

In each of the above assays, the sample-containing antibody, sol Id-phase Immunoabsorbent with Immobilized peptide fragment and labeled soluble antibody are Incubated under conditions and for a period of time sufficient to allow the test antibodies to bind to the Immobilized peptide fragments and to the soluble antibodies. In general, It 1s desirable to provide Incubation conditions sufficient to bind as much -24antlbody as possible, since this maximizes the binding of labeled antibody to the solid phase, thereby increasing the signal. Of course, the specific concentrations of labeled antibodies and Immobilized fragments, the temperature and time of Incubation, as well as other such assay conditions, can be varied, depending upon various factors Including the concentration of antibody 1n the sample, the nature of the sample, and the like. Those skilled 1n the art will be able to determine operative end optimal assay conditions for each determination by employing routine experimentation.

There are many solid-phase Immunoabsorbents which have been employed and which can be used In the present invention. Well-known Immunoabsorbents Include beads formed from glass» polystyrene, paper, polypropylene, dextran, nylon, and other material; tubes formed from or coated with such materials, and the like. The Immobilized peptide fragments may be covalently or physically bound to the solid-phase immunoabsorbent, by techniques such as covalent bonding via an amide or ester linkage or by adsorption. Those skilled In the art will know many other suitable carriers for binding peptide fragments, or will be able to ascertain such, using routine experimentation.

General. competitive binding assay techniques useful for the detection of minute amounts of organic molecules such as hormones, proteins, antibodies, and the like are well-known 1n the art. See Chard, supra. Any of these competitive binding essay techniques can be used for the purposes of detecting HIV-2 antibodies. In order to carry out a competitive binding assay, typically a radioimmunoassay (RIA), It 1s necessary to provide a binding molecule which has affinity for the labelcontaining antibody raised 1n response to e peptide fragment, and for the HIV-2 antibody to be tested as well. A smell amount of the fluid or tissue sample containing an unknown quantity of HIV-2 antibody 1s Incubated in the presence of the -25ralsed labeled antibody and also a known amount of antibodyspecific peptide fragment.

The raised antibody 1s preferably generated with antigenic peptide fragments of the Invention. Once the Incubation of the test sample with the fragment and tracercontaining antibody 1s complete, 1t 1$ necessary to determine the distribution of the tracer-containing molecule between the free and bound (Immunocomplexed) form. Usually, but not always» t^1s requires that the bound fraction be physically separated from the free fraction. For example, the specific peptide fragment can be bound to a plate. A variety of other techniques may be used for that purpose, each exploiting physical-chemical differences between the tracer-containing molecule 1n Its free and bound form. The generally available methodologies have been described by Yalow, 1n Pharmacol. Rev, ££:151 (1973). These techniques Include adsorption, precipitation, salting out techniques, organic solvents, electrophoretic separation, and the like. See Chard, uiph, pp. 405-422.

As 1n the 1mmunometr1c assays described above, the soluble antibody may be labeled with any detectable label, such as a radiolabel, a fluorescent label, an enzyme label, a free radical label, or a bacteriophage label. Most commonly, the label 1s a radiolabel or an enzyme label.

The HIV-2 Immunogenic peptide fragments according to this Invention may be used to stimulate the production of antibodies. In order to stimulate the production of antibody, the peptide fragment may be coupled to a carrier protein such as bovine serum albumin or keyhole limpet hemocyanln (KLH), utilizing techniques well-known and commonly used In the art. Preferably, the carrier protein Is KLH, linked to the peptide fragment through a cysteine residue.

Additionally, the HIV-2 peptide fragments can be admixed with an Immunologically Inert or active carrier. Carriers -26· which promote or Induce Immune responses, such as Freund's complete adjuvant, can be utilized.

The preparation of antisera In animals 1s a well-known technique (see, for example, Chard, supra, pp. 385-396; and Antibodies, A Practical Handbook. Vols. I and II, D. Catty, ed., IRL Press, Washington, D.C. (1988)). The choice of animal 1s usually determined by a balance between the facilities available and the likely requirements 1n terms of volume of the resultant antiserum. A large species such a goat, donkey and horse may be preferred, because of the larger volumes of serum readily obtained. However, It Is also possible to use smaller species such as rabbit or guinea pig which often yield higher titer antisera. Usually, subcutaneous Injection of the antigenic material (the peptide fragment hapten-carrier protein conjugate) are Introduced Into the Immune system of the animal In which antibodies are to be raised. The detection of appropriate antibodies may be carried out by testing the antisera with appropriately labeled tracer-containing molecules. Fractions that bind tracercontaining molecules are then Isolated and further purified 1f necessary.

Antibodies thus obtained may then be utilized 1n various Immunoassays to Identify and quantitate the HIV-2 virus or fragments thereof. 8oth polyclonal antibodies and monoclonal antibodies, produced by well-known techniques as described 1n Catty, ϋΐΛΕΙ» raised 1n response to the peptide fragments of this Invention can be utilized In Immunoassays.

When one uses 1mmunometr1c assays to detect the HIV-2 virus or portions thereof, two separate and distinct antibodies are required. One of these antibodies 1s bound to the solid-phase support while the other 1s detectably labeled. In essence, the two different antibodies, although specific for HIV-2 virus, are cross-reactive with different domains on viral protein. In one embodiment, the two different -27ant1bodies may be prepared by using two different peptide fragments according to this invention. The use of antibodies to different peptide fragments, one bound to a carrier and the other detectably labeled, 1s useful In various sandwich assays.

Alternatively, 1t 1s also possible to prepare antibodies which are specific to HIV-2 virus, but cross-reactive with different domains by producing the antisera 1n two different species, for example, 1n rabbit and 1n mouse, utilizing the same peptide fragment.

In addition, the materials for use in the assays of the Invention are Ideally suited for preparation of a kit. Such a kit may comprise a carrier means being compartmentalized to receive In close confinement one or more container means such as vials, test tubes, and the like. Each of said container means comprises one of the separate elements to be used 1n the method.

For example, one of said container means may comprise an 1mmunoab$orbent-bound peptide fragment. Such fragment may be bound to a separate solid-phase Immunoabsorbent or directly to the Inner walls of a container. A second container may comprise detectably labeled ant1-ant1body In lyophilized form or 1n solution.

The carrier may also contain, 1n addition, a plurality of containers each of which comprises different, predetermined and known amounts of antibody. These latter containers can then be used to prepare a standard curve from which can be Interpolated the results obtained from the sample containing the unknown amount of antibody.

In the practice of this Invention, the presence of the HIV-2 antibody or the virus Itself or portions thereof may be detected 1n biological fluids and tissues. Any sample containing the unknown amount of HIV-2 antibodies or HIV-2 can be used. Normally, a sample is a liquid such as, for example, -28urlne, saliva, tear drops, cerebrospinal fluid, blood, serum and the like, or a solid or semi-solid such as, for example, tissues, feces, end the like. As 1s known 1n the art, the HIV-2 virus and antibodies to the virus are associated with the T-cell disorder, Acquired Immune Deficiency Syndrome (AIDS) and pre-AIDS conditions, such as AIDS-related complex (ARC). In addition, 1t Is also known 1n the art that antibodies to HIV-2 may be present in a human's or animal's biological fluids or tissue, without such human or animal suffering from AIDS or ARC.

The peptide fragments according to this Invention may also be used as a vaccine against the HIV-2 virus. The peptide fragment may be prepared and administered to an animal, as 1s generally known 1n the art, to stimulate the production of antibodies. Preferably, the vaccinia virus can be used according to known means for the preparation of HIV-2 vaccines.

The following examples further describe the materials and methods used 1n carrying out the Invention. The examples are not Intended to limit the Invention In any manner.

EXAMPLES Example 1: Construction of HIV-2 envelope expressing clone MZ-1/pKl The K3D clone Is a subgenomlc fragment of a complete H1V2 clone HIV-2S|yISY (FrancMnl et -Al m Proc. Natl. Acad, Sci, USA 22:2433-2437 (1989)), prepared by Insertion of a KPNI fragment of HIV-2sbl/isy from position 5295 to position 9012 Into a Bluescrlpt vector (Stratagem, Inc.). The HIV-2 clone K3D was provided by Genoveffe Franehinl. -29The strategy for construction of pKl, a plasmid for expression of a peptide fragment of the env region of HIV-2 1n E, coll. Is Illustrated In Figure 1.

K3D DNA was digested with restriction enzyme EcoRI with cuts at position 7297. The EcoRI end was made blunt with Klenow polymerase and Bglll linkers were added. The DNA was then digested with Bglll and Sau3AI. A fragment of approximately 848 base pairs extending from the EcoRI site (converted to Bglll) at position 7297 to the Sau3AI site at position 8139 was purified and cloned Into Bam Hl restricted v the expression vector pCBCl to generate the clone pKl.

Plasmid pCBCl 1$ an E. coll expression vector that makes use of the bacteriophage lambda pL promoter. pCBCl 1s similar to pJL6 (Lautenberger Gene Anal. Tqch. 1:53 (1984)) whose construction 1s described completely 1n Beltz et al.. U.S. Patent No. 4,753,873, incorporated herein by reference.

Using E, coll strain MZ-1, a strain lysogenic for bacteriophage lambda, ¢1357, as a host strain for pKl, recombinant protein synthesis was Induced by temperature shift from 32’C to 42'C (Naghl et al.. Nature 202:810 (1984)). As shown 1n Figure 2, the temperature shift resulted in the synthesis of a 34 kd protein. Following Western blot transfer of the separated proteins, the induced protein, called Kl, reacted specifically with human sera from HIV-2 Infected individuals (Figure 3). The complete ONA sequence of the coding region of Kl and the derived amino acid sequence 1s presented In Figure 4.

Example-2: Construction of HIV-2 envelope expressing clone MZ-l/pK3 K3D (described 1n Example 1) was digested with Sau3AI. This cutting resulted 1n a 1038 base pair fragment from position 7101 to position 8139 (figure S). After purifying -30the fragment, It was ligated Into the expression vector pCBCZ. pCBC2 differs from pCBCl by a single base pair Just 5' to the BamHI cloning site. pCBC2 was used 1n this case rather than pCBCl to allow for proper reading frame alignment. pCBC2 Is also described 1n Beltz U.S. Patent No. 4,753,873, Incorporated herein by reference. The resulting plasmid, pK3, was transferred Into the E, coll host NZ-1. Upon temperature shift of MZ-l/pK3 culture from 32*C to 42*C, synthesis of a recombinant protein of 40 kd was Induced (Figure 6). Western blot analysis has shown that this protein, called K3, reacted specifically with sera from HIV-2 Infected Individuals (Figure 7). The complete DNA sequence of the coding region of pK3 and the derived amino acid sequence 1s presented 1n Figure 6.

Example 3: Construction of an HIV-2-HIV-1 chimeric envelope expressing clone M2-l/pKlDG71 The strategy for the construction of the plasmid to express a chimeric envelope clone Is Illustrated 1n Figure 9. The plasmid clone pLCBC0DG71A has been described 1n Beltz ii al.. U.S. 4,753,873, Incorporated herein by reference. This plasmid 1s used for expression of HIV-1 envelope polypeptide. pLCBC0DG71A was digested with BglII and BamHI. Bglll cleaves at position 407 and BamHI cleaves at position 944. A 537 BP fragment was Isolated. pKl plasmid DNA, described 1n Example 1, was digested with BamHI which cleaves at position 890. The 537 BP BglIIBamHl fragment of pLCBC0DG71A was ligated to BamHI digested pKl. The resulting plasmid, pK10G71, was transferred to E, coll host MZ-1. Upon temperature shift of MZ-l/pKlDG71 culture from 32*C to 42*C, synthesis of a recombinant protein of approximately 55 kd was Induced (Figure 10). Western blot analysis was done with sera from HIV-I Infected Individuals, -31HIV-2 Infected Individuals and negative controls. The Western blots (Figure 11) showed that the chimeric HIV-2-HIV-1 protein, K1DG71, reacts with sera from HIV-l Infected Individuals (Figure 11A) and sera from HIV-2 Infected individuals (Figure 11B). No reactivity was seen with negative sera (Figure 11C).

The complete DNA sequence of the coding region of PK1DG71 and the derived amino acid sequence Is presented 1n Figure 12.

Example 4: Construction of an HIV-2-HIV-l-HTLV-I-Ch1mer1c Envelope Expressing Clone The strategy for construction of an HIV-2-HIV-1 -HTLV-1 chimeric envelope expressing clone 1s Illustrated 1n Figure 13 and Figure 14. pCB1353 1s en expression plasmid containing regions of the HTLV-I envelope gene from base pairs 6101-6118 and 6170-6499 based on the published sequence of Selkl et al, (Proc. Natk Acad, Sd. USA 84:3618 (1983)) cloned Into expression plasmid pCBCl. The plasmid pCBC1353 was digested with BamHI and Sail to generate a 370 base pair fragment. The 370 BP fragment was inserted Into the plasmid pCB2DG71 which had been digested with BamHI and Sail. pCBC2DG71 Is an expression plasmid coding for a polypeptide of the HIV-l envelope protein. This plasmid has been described by Beltz il llx, U.S. 4,753,873, Incorporated herein by reference. The resulting plasmid, pDG71353, codes for a chimeric polypeptide of HIV-l-HTLV-I. The sequence of the coding region of pDG71353 1s shown 1n Figure 15.

Figure 14 shows the remaining steps for the HIV-2-HIV-1HTLV-1 construction. pDG71353 was digested with Hlndlll and Sail. The Insert which contains sequences coding for the HIV1-HTLV-I polypeptide was ligated Into the vector pKlDG71 which had been digested with Hlndlll and Sail. pKlDG71 1s described -321n Example 3. The resulting plasmid 1s called pKlDG71353. pKlDG71353 was transferred Into the bacterial strain MZ-1.

When MZ-1 pKlDG71353 was induced by a temperature shift from 32*C to 42*C, a protein of 68 kd was produced (Figure 16). Following Western blot transfer of the separated protein, the induced protein reacted specifically with sera from HIV-1 positive Individuals, Figure 17> with sera from HIV-2 positive Individuals, Figure 18; and with sera from HTLV-I positive Individuals, Figure 19. No specific reactivity was seen with negative sera (Figure 20). The complete sequence of the coding region of pKlDG71353 1s shown In Figure 21.

Example 5: Purification of HIV-2 env (K-l) and HIV-2-HIV-1 Chimeric Antigens The following purification procedure has been used to purify both HIV-2 env (K-l) and HIV-2-HIV-1 chimeric antigens.

E. coll cells were lysed by enzymatic digestion with lysozyme (1 mg/gram of cells) for 10 minutes 1n 50 mM TrisHCl, pH 7.5 (3 ml/gram of cells) containing 2 mM PMSF, aprotlnln (0.1 mg/gram of cells) and DNase 1 (0.1 mg/gram of cells). The solution was brought up to 1% triton X-100 and stirred for 30 minutes at room temperature. Insoluble material was collected by centrifugation at 12,000 xg for 30 minutes and redigested as above with the exception that RNase I (0.05 mg/gram of cells) and 2.5 mM MgClj were added. After digestion, the pellet was collected by centrifugation as above.

The Insoluble material was then sequentially washed with the following buffers (0.2 gram of cells/ml): 1) 50 mM TrisHCl, pH 9.0 containing 10 mM EDTA and 0.5X Zwittergent 3-14, 2) 50 mM TrisHCl, pH 9.0/1M NaCl, -333) 6M urea In 50 nN TrlsHCl, pH 7.5, 4) 8M urea 1n 50 mM TrlsHCl, pH 9 with 1% &mercaptoethanol.

In each case, the recombinant antigens remained In the Insoluble pellet. The pellet from the 8M urea wash was then solubilized with 7M guanid1ne-HC1 pH 11.0/0.5% fimercaptoethanol. Both HIV-2 env antigen and HIV-2-HIV-1 chimeric protein are very hydrophobic and tend to form aggregates upon removal of guan1d1ne-HC1. To prevent this aggregation, the solubilized antigens were subjected to the following chemical modifications designed to Increase the solubility of the antigens 1n aqueous buffers.

The solubilized protein 1n 6M guan1d1ne-HCl was first alkylated with 1.2 fold excess of 1odoacet1c add over βmercaptoethanol at pH 8.5. Any unreacted 1odoacet1c acid was quenched with l-mercaptoethanol. The alkylated sample was dialyzed 3 times against 200 fold 50 mN borate, pH 9.0. The protein became Insoluble upon dialysis. The Insoluble material was collected by centrifugation and redissolved 1n 8M Urea, 50 mM borate, pH 9.0 for acylation.

To acylate the alkylated antigen, a 50-fold excess of dtraconlc anhydride over amino groups on the antigen was added and the pH of the solution was maintained between 8.5 to 9.0 with NaOH. After the reaction was complete, the dtraconylated sample was dialyzed against 50 mM borate, pH 9.0 at 4*C. After dialysis, the dtraconylated protein was soluble in aqueous buffer and amenable to standard chromatographic technique.

The modified protein sample was then applied to a DEAETSK column, equilibrated 1n 50 mM borate, pH 9.0. The column was developed with a linear gradient of 0.3-1M NaCl to elute the recombinant antigen. Fractions containing HIV-2 env, K-l, antigen or HIV-2-HIV-1 chimeric protein, K1DG71, were pooled. -34The 1mmunoreact1v1ty of purified Kl and the chimeric K1DG71 antigens were tested using an Indirect immunoassay (EIA). Recombinant antigen was coated onto microtiter wells at concentrations of 0.5 ug and 1.0 ug for K-2 and the chimeric antigen respectively. After washing and blocking non-specific binding sites on the wells, human sera diluted 1:20 was added and any antibodies present allowed to bind to the recombinant antigen for 1 hour at 37‘C. Wells were washed to remove unbound antibodies and the presence of bound antibody was detected with horse radish peroxidase labelled goat anti human antibody and a substrate of TmB (3,3', 5,5'tetramethy/benzldine). Reactions were terminated with H2SO4 and 00490 determined. Distribution of signals obtained with each antigen for various sera are presented in Table 1. 355 0 ·*» ·« I > ( ο 0> •f Saapte* in each 0*499 -36Now having fully described this Invention, 1t will be understood by those with skill in the art that the scope may be performed within a wide and equivalent range of condition, parameters, and the like, without affecting the spirit or scope of the Invention or of any embodiment thereof.

Claims (19)

WHAT IS CLAIMEDIS:

1, A peptide fragment encoded by nucleotides of about 848 base pairs of the envelope region of the HIV-2 virus wherein said peptide fragment 1s encoded by the HIV-2 provirus nucleotides at position 7297 to position 8139 as shown 1n Figure 4.

2. A peptide fragment encoded by nucleotides of about 1038 base pairs of the envelope region of the HIV-2 virus wherein said peptide fragment 1s encoded by the HIV-2 provirus nucleotides at position 7101 to position 8139 as shown 1n Figure 8.

3. A chimeric HIV-2-HIV-1 peptide fragment comprising an Immunodlagnostic peptide fragment the envelope region of the HIV-2 virus and an Immunodlagnostic peptide fragment of the envelope region of the HtV-1 virus.

4. A chimeric HIV-2-HIV-1 peptide fragment comprising said Immunodlagnostic peptide fragment of the envelope region of the HIV-2 virus of claim 1 or 2 and an Immunodlagnostic peptide fragment of the envelope region of the HIV-l virus.

5. The chimeric HIV-2-HIV-1 peptide fragment of claim 4 wherein said 1mmunod1agnost1c peptide fragment of the envelope region of the HIV-l virus 1s selected from the group consisting of clone G or peptide fragments derived therefrom.

6. 8. The chimeric HIV-2-HIV-1 peptide fragment of claim 4 wherein said Immunodlagnostic peptide fragment of the envelope region of the HIV-l virus Is CBre3. -387. A chimeric HIV-2-HIV-1-HTLV-I peptide fragment comprising an Immunodlagnostlc peptide fragment the envelope region of the HIV-2 virus, an Immunodlagnostlc peptide fragment of the envelope region of the HIV-1 virus, and an Immunodlagnostlc peptide fragment of the envelope region of the HTLV-I virus. 8. The chimeric HIV-2-HIV-1-HTLV-I peptide fragment of claim 7 wherein said Immunodlagnostlc peptide fragment of the envelope region of the HIV-2 virus 1s encoded by the HIV-2 provirus nucleotides at position 7297 to position 8139 as shown 1n Figure 4 or 1s encoded by the HIV-2 provirus nucleotides at position 7101 to position 8139 as shown 1n Figure 8.

7. 9. The chimeric HIV-2-HIV-1-HTLV-I peptide fragment of claim 7 wherein said Immunodlagnostlc peptide fragment of the envelope region of the HIV-1 virus comprises the HIV-1 coding sequence of K1DG71353 as shown 1n Figure 21.

8. 10. A chimeric HIV-2-HTLV-I peptide fragment comprising an Immunodlagnostlc peptide fragment the envelope region of the HIV-2 virus and an Immunodlagnostlc peptide fragment of the envelope region of the HTLV-I virus.

9. 11. The chimeric HIV-2-HTLV-I peptide fragment of claim 10 wherein said Immunodlagnostlc peptide fragment of the envelope region of the HIV-2 virus 1s encoded by the HIV-2 provirus nucleotides at position 7297 to position 8139 as shown 1n Figure 4 or 1s encoded by the HIV-2 provirus nucleotides at position 7101 to position 8139 as shown 1n Figure 8. •3912. The chimeric HIV-2-HTLV-I peptide fragment of claim 10 wherein said immunodiagnostic peptide fragment of the envelope region of the HTLV-I virus 1s encoded by the HTLV-I provirus nucleotides at position 6101-5118 and 6170-6499.

10. 13. A chimeric HIV-l-HTLV-I peptide fragment comprising an Immunodiagnostic peptide fragment the envelope region of the HIV-1 virus and an Immunodiagnostic peptide fragment of the envelope region of the HTLV-I virus.

11. 14. The chimeric HIV-l-HTLV-I peptide fragment of claim 13 wherein said Immunodiagnostic peptide fragment of the envelope region of the HIV-1 virus is selected from the group consisting of clone G or peptide fragments derived therefrom.

12. 15. The chimeric HIV-l-HTLV-I peptide fragment of claim 13 wherein said immunodiagnostic peptide fragment of the envelope region of the HIV-1 virus Is CBre3.

13. 16. The chimeric HIV-l-HTLV-I peptide fragment of claim 13 wherein said Immunodiagnostic peptide fragment of the envelope region of the HTLV-1 virus 1s encoded by the HTLV-I provirus nucleotides at position 6101-6118 and 5170-5499.

14. 17. A recombinant vector for transforming a host cell comprising a DNA encoding any of the peptide fragments of claims 1 to 16. -401β. A method for detecting HIV-2 antibodies comprising the steps of: (a) contacting a sample suspected of containing antibodies to HIV-2 with a peptide fragment of any of claims 1, 2, 3, 6, or 10 and (b) detecting the presence of said antibodies.

15. 19. A method for detecting HIV-l antibodies comprising the steps of: (a) contacting a sample suspected of containing antibodies to HIV-2 with a peptide fragment of any of claims 3, 6, 13 and (b) detecting the presence of said antibodies.

16. 20. A method for detecting HTLV-I and/or HTLV-II antibodies comprising the steps of: (a) contacting a sample suspected of containing antibodies to HIV-2 with a peptide fragment of any of claims 6, 10, or 13 and (b) detecting the presence of said antibodies.

17. 21. A kit for detecting either HIV-2, HIV-l or HTLV-I and HTLV-Π antibodies, or e combination of antibodies thereof, 1n a sample comprising a carrier being compartmentalized to receive one or more containers In close confinement therein and further comprising 1. a first container means comprising a peptide fragment of any of claims 1 to 15; and 2. a detection system for determining the presence of HIV-2, HIV-l, or HTLV-I and HTLV-II antibodies, or a combination thereof. - 41 18. A peptide fragment according to claim 1 or 2, substantially as hereinbefore described and exemplified. 19. A chimeric HIV-2-HIV-1 peptide fragment, substantially as hereinbefore described and exemplified. 20. A chimeric HIV-2-HIV-1-HTLV-I peptide fragment according to claim 7 or 8, substantially as hereinbefore described and exemplified. 21. A chimeric HIV-2-HTLV-I peptide fragment according to claim 10, substantially as hereinbefore described.

18. 22. A chimeric HIV-1-HTLV-I peptide fragment according to claim 13, substantially as hereinbefore described and exemplified .

19. 23. A recombinant vector according to claim 17, substantially as hereinbefore described and exemplified.