AP80A - Expression of HIV binding proteins. - Google Patents

Expression of HIV binding proteins. Download PDF

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AP80A
AP80A APAP/P/1989/000114A AP8900114A AP80A AP 80 A AP80 A AP 80A AP 8900114 A AP8900114 A AP 8900114A AP 80 A AP80 A AP 80A
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vector
protein
hiv binding
scd
binding protein
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James Arthos
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Smithkline Beecham Corp
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Abstract

Hiv binding proteins derived from the cd-4 receptor protein are expressed in recombinant host cells.

Description

Background of the Invention
The human T-cell glycoprotein, CD-4 (sometimes previously referred to as T4), is one of several non-polymorp'nic T lymphocyte surface receptor proteins that have been implicated in the mediation of efficient T cell-target cell interactions.
The cDNA sequence of the human CD-4 (T-4) receptor is known (Maddon, et al., Cell 42:93(1985)). The complete
CD-4 pre-protein sequence is 458 amino acids in length comprising the putative 23 amino acid secretory leader,
372 amino acid surface (V.-V.), 23 amino acid l 4 transmembrane and 40 amino acid cytoplasmic domains. The surface domain shows four regions of limited homology, 20-30%, to immunoglobulin variable (V) and joining (J)
AP 0 0 0 0 8 0
BAD ORIGINAL &
-'fc regions. Four of the five intron-exon boundaries in the surface domain occur near the junctions of these V-J regions .
The human immunodeficiency virus (HIV), the etiological agent of acquired immune deficiency syndrome (AIDS), shows a marked affinity for CD-4 lymphocytes.
Virus binding to CD-4 is mediated by the gpl20 glycoprotein of the viral envelope. The CD-4 protein can be co-precipitated from lysed HIV infected cells with anti—env antibody and, conversely, gpl20 can be co-precipitated with anti-CD-4 monoclonal antibody, thus demonstrating that virus binding to CD-4 is mediated by the gpl20 glycoprotein of the viral envelope.
Recently, a number of scientific investigators have reported their findings related to the interaction between CD-4 and the AIDS infection using a CD4 derivative expressed in mammalian cell systems.
Deen, et al., Nature 331:82(1988) report the isolation and expression of sCD-4 in several cellular environments. sCD-4 is a soluble derivative of CD-4 which lacks the transmembrane and cytoplasmic domains of CD-4 . Using a dfhr deficient Chinese Hamster Ovary (CHO) cell line they have shown the expressed sCD-4 retains the structural and biological properties of CD-4 on the cell surface, binds to the HIV gp 110 envelope protein and can inhibit the binding of CD-4+ lymphocytes.
Traunecker, et al., Nature 331:84(1988) report use of sCD-4 to inhibit the attachment of virus to the target cell. The data presented shows the inhibition of HIV infection in vitro using a recombinant form of sCD-4.
Fisher, et al., Nature 331:76(1988) report the purification of sCD-4 from (CHO) and its use as a potent inhibitor of both virus replication and virus induced cell fusion.
Hussey, et al., Nature 331:78(1988) report the use of the baculovirus expression system to produce sCD-4 which was found to inhibit virus induced cell fusion (syncytium
BAD ORIGINAL 0 formation) and HIV infaction by binding to gpl20 expressing cells. It was also shown that the sCD-4 protein does not appear to inhibit class II specific T-cell interactions.
Smith, et al,, Science 238:1704(1387) also report use of the CHO mammalian cell system to produce sCD-4. They report the production of a sCD-4 protein in CHO cells which can be shown to bind to HIV gp 120 envelope protein and neutralize the infectivity of HIV-l in vitro. The data indicate that sCD-4 can be used as a basis for therapeutic treatment of AIDS infection.
There is still a need, however, for bacterial and lower eukaryotic systems for expression of s-CD4 proteins.
Summary of the Invention
This invention lies in the discovery that the HIV binding function of the CD-4 protein can be expressed in E, coli and in the discovery that such HIV binding protein can be secreted into the fermentation medium. In particular, therefore, this invention is an Ξ. coli expression vector comprising an HIV binding protein operatively linked to a regulatory element.
This invention also lies in the discovery shat the hiv binding function of the CD-4 protein can be expressed in Streptomyces and in the discovery that such HIV binding protein can be secreted into the fermentation medium. In particular, therefore, this invention is a Streptomyces expression vector comprising an HIV binding prorein operatively linked to a regulatory element.
This invention also lies in the discovery that the
HIV binding function of the CD-4 protein can be expressed in yeast. In. particular, therefore, this invention is a yeast expression vector comprising an HIV binding protein operatively linked to a regulatory element.
AP000080
BAD ORIGINAL
This invention also lies in the discovery that the OMPA leader sequence can be used to export heterologous proteins from E, coli. In particular, therefore, this invention is an E. coll expression vector for expressing exported proteins in E. coli comprising a DNA coding sequence operatively linked to a regulatory element wherein the DNA coding sequence codes for the protein X-Y wherein X is an OMPA leader sequence and Y is a heterologous protein.
Detailed Description of the Invention □Ο
Ο *** ««» β
In accordance with the present invention, HIV binding proteins derived from the CD-4 receptor are expressed in useful quantities for use as therapeutic and/or prophylactic agents to inhibit initial HIV infection and to inhibit cell-to-celi transmission of HIV following host infection; for use in screens for inhibitors of HIV-lymphocyte binding; for use as inhibitors of CD-4+ lymphocyte functions; cr for other uses such as described below. The proteins all have the HIV binding function from CD-4. Preferred examples of such proteins are sCD-4 proteins and derivatives thereof. sCD-4 proteins are derivatives of CD-4 which lack the transmembrane and cytoplasmic domains of CD-4, Examples of sCD-4 proteins are described in separate papers by Deen et al.,
Traunecker et al. , Fisher et al., and Hussey et al., in Nature 331:76-88 (1988) and by Smith et al., Science 238:1704 (1987).
The sCD-4 protein exemplified herein, referred to as SK3sCD-4, is reported by Deen et al., cited above, at 33. It is shewn in the following amine acid and nucleotide sequence. The sequence shows a 5' untranslated region and a leader sequence derived from the CD-4 cDNA reported by Maddon, et al., Cell 42:93(1985). The first amino acid of mature SX3sCD-4 as expressed and secreted by CHO ceils is
BAD ORIGINAL ft the lysine encoded by base pairs 151-153. The transmembrane domain was deleted by restricting CD-4 cDNA with Hpa-II at base pair 1252 and ligating thereto a linker which restored base pairs 1253-1257 and which placed a translation stop codon, TAA, after the C-terminal valine. As reported by Maddon, et al., the first three amino acids of mature CD-4 are glutamine (shown herein as amino acid (-)2) - glycine (shown here as amino acid (-)1) asparagine (shown here as lysine, amino acid (+)1).
Otherwise, the sequence reported below is the same as that reported by Maddon et al.
o 8 0 0 0 o dV
BAD ORIGINAL &
10 30 50
CAACCCCaCAGCCCTCCCaTTTCTGTCCGCTCAGGTCCCTACTCCTCaCCCCCTTCCTCC
90 110
CTCGCCAACGCCACAATGAACCCCGGAGTCCCTTTTACGCACTTGCTrCTGGTGCTGCAA
MetAsnArgGlyValProPheArgHisLeuLeuLeuValLeuGia
130 150 170
CTGGCGCTCCTCCCACCACCCACTCAGGGAAAGAAAGTGGTGCtCGGCAAAAAACCGCAT LeuAlaLeuLeuProAlaAlaThrGlnGlyLysLysValValLeuGlyLysLysGlyAsp
-9 -1 +1
190 210 230 io acagtcgaactcacctctacaccttcccacaacaacaccatacaattccactccaaaaac
ThrValGluLeuTh rCysTh rAlaSe rGlnLysLysSerlleG1nPheHi sTrpLysAsa
250 270 290
TCCAACCACATAAACATTCTCCCAAA'rCACCGCTCCTTCTTAACTAAAGGTCCATCCAAC Se rAsnG 1 η 11 cLy s Γ I eLeuG 1 yAsriG I nG lySe rPheLeuT'n rLy sG I y ProSe rLy s
310 330 350
CTCAATCATCGCCCTCACTCAACAAGAACCCTTTCGCACCAAGCAAACTTCCCCCTCATC LcuAsnAspArgA1aAspSerArgArgSe rLeuTrpAspG1 nG 1yAsnPheProLeulie
370 390, 410
ATCAACAATCTTAACATACAACACTCACAT'ACTTACATCTCTCAACTCGAOCACCACAAC ί1eLysAsnLcuLys Γ1eGluAspSarAspThrTy riIeCysC1uValG1uAspG1aLy s
430 450 470
GAGCAGGTGCAATTGCTAGTGTTCGGaTTCACTCCCAACTCTGACaCCCACCTGCTTCaG
G1uG1uValG1nLcu LeuValPheG1yLeuTh rA1aAsnSe rAssTh rH i sLeuLeuG1 a
104 ~473O 510 530
CCCCaGAGCCTGACCCTGACCTTCOaCAOCCCCCCTCCTACTaCCCCCTCaGTCCAATCT
Cl y G ’ n Se r!, c uThrf, e u Th rf, euG 1 uSerProProG LyScrSerProSerValGIaC vs
550 570 590
AOCaGTOCaaGGCGT\AAAACaTACaCCGCCCCAAGaCCC7C7CCG7G7C7CaCC7C,GAG
ΛrgSe rProA rgC L y Ly sAsn11eG L nG LyGlyLy sTh rLcuSe rVa1Se rG1nLeeC1e
610 630 650 ctccaocatagtgccacctccacatgcactctcttccacaaccacaacaacctccacttc »;»Se rG I y 7h ι-Τ γ pTh rCy sTh r Va 1 LcuG L n/\ s nG 1 π Ly sLy s Va 1 G 1 u Ph e
L e 11G I 11Λ >» j 151
670 690 7 10
AAAaTA0AC7\TCGTGGTGGTAGCT77CCaCAACCCCTCCAGCaTACTCTATAACAAACaC
Lvsi InAspl IeVaIVaI I.euA I al’hcG 1 n LysAI aSe rS·· r I 1 eVa 1 Ty rl.y sLy sG I u
123
BAD ORIGINAL
730 750 770
GGCCAACACGTCCACTTCTCCTVCCCACTCCCCTTTACACTTCAAAACCTCACCCCCaCT G1 yCl uC 1 nVal C1 uPheSe rPhcP roLcuA 1 aPheThrVa.1 C1 uLysLeuTh rG 1 y Se γ
790 810 830
GGCGAGCTGTGGTCGCAGGCGCAGAGGGCTTCCTCCTCCAAGTCTTCCATCACCTTTCAC GlyGluLeuTrpTrpGlnAlaGluArgAlaSerSerSerLysSerTrpIleThrPheAsp
8S0 870 890 ctcaacaacaaggaactgtctgtaaaacggcttacccaccaccctaacctccacatcccc LeuLysAsnLysGluValSerValLysArgValThrGlnAspProLysLeuGlnMecGly
910 930 9S0 aacaagctcccgctccacctcaccctcccccaggccttgcctcactatgctccctctcca
Ly sLy sLeuP roLeuHi sLeuTh rLeuProG1 nA 1aLeuProG1nTy rAlaG1ySe rG1y
970 990 1010
AACCTCACCCTGCCCCTTCAAGCCAAAACACGAAAGTTCCATCACCAACTGAaCCTGCTC Asn LeuTh rLeu A1 aLcuG 1 uA1 aLy sTh rG 1 y \,y sLeu! I i sG 1 nG 1 u Va. 1 asnLe u7a 1
1030 1050 1070
CTCATGAGAGCCACTCAGCTCCACAAAAATTTGACCTCTCAGGTCTCCCGACCCACCTCC Val Me tArgA 1 aTh rG 1 nl.cuC 1 nl.ysAsnl.cuTh rCysG I uValTrpGlyProTh.-Ser
1090 1110 1130 cctaagctgatgctgagcttgaaactggagaacaaggagccaaaggtctcgaaccgcgag
P roLy sLc u.Mc tLeuSe r Lo u Ly sLe uG I uAs π Ly sG 1 nA I aLy sVa 1 Se rLy sA rgC 1 e
AP 0 0 0 0 8 0
1150 1170 1190
AACGCCGTCTGCGTGCTGAACGGTGAGGCGGGGATGTCGCAGTGTCTCCTCAgTGACTGC Ly sA 1 aV alTrpVa1 LeuA.s nP roG 1 nA 1 aG 1 yMe tTrpG1 nCy sLc uLe uSu .··/·. s pSe r
1210 1230 1250
GCACACGTCCTCCTOCAA'rCCAACATCAAGGTTCTGCCCACATCGTCCACCCCCC ’.aa G 1 yG l η Va 1 Le u Le tiG I uSc rAs π I i eLy s Va ! Le υ P roTh rT rp3e r7h r P ro'·'a . Fine ~ 1 > Λ
JO?
351
1270 '-t'.G'-K^ctcLaga
BAD ORIGINAL g>) cs>
&
δ» sCD-4 truncates, and derivatives thereof, which substantially retain the HIV binding affinity of sCD-4 can also be expressed in accordance with this invention. Preferred among such truncates are proteins or polypeptides comprising the HIV binding region of the vi and V2 regions which is comprised approximately within amino acids 1-182. With reference to the sequence shown above, one particular example is the protein herein referred to as V1J4 which has amino acids (-)2-104 (N-glutamine-glycine-lysine- through -alanine-asparagineserine-C) fused to amino acids 351-369 (-glycine-glutamine -valine through -threonine-proline-valine-C). A second example is the protein herein referred to as V1V2J4 which has amino acids (-)2-183 (N-glutamine-glycine-lysinethrough -lysine-alanine-serine-C) fused to amino acids 351-369. A third example is the protein herein referred to as YV1, which comprises amino acids (-)9-151 (N-alanine-leucine-leucine- through -leucine-glutamic acid-leucine-C). A fourth example is the protein herein referred to as SKSYsCD-4 which has amino acids (-)9-369. Each of these HIV binding proteins, based on, e.g., CKT4A binding, has the HIV binding property of sCD-4 proteins, specifically of SKBsCD-4, and, more particularly, has the HIV binding domain of the Vl and V2 regions of sCD-4 proteins, specifically of SKBsCD-4.
In addition to those proteins specifically exemplified herein, one of ordinary skill in the art can readily construct DNA coding sequences for further sCD-4 derivatives. Such derivatives substantially retain the HIV binding function of sCD-4 proteins, i.e., the binding of the protein to the HZV env protein, gpl20, is not significantly adversely affected. For example, one can construct a derivative having only the Vl region, e.g., approximately amino acids 1-94, or a derivative having only a portion of the Vl region of CD-4 . One can also construct derivatives of the proteins specifically
BAD ORIGINAL exemplified herein, such as derivatives differing by one or a few amino acid deletions, additions or substitutions.
Alternatively, a hybrid protein, i.e., a translational fusion, can be constructed between a sCD-4 protein and a protein carrier, another antigen or other sCD-4 molecules to prepare a poly-sCD-4 molecule. In yet another alternative, the sCD-4 deletion mutant can be synthetically conjugated to a carrier molecule.
Affinity of the sCD-4 molecules for HIV can be demonstrated by a competitive binding assay using a sCD-4 molecule having a known affinity or using antibodies which recognize the CD-4 receptor, such as OKT-4 and OKT4A. Useful sCD-4 proteins of the invention are selectively precipitated from conditioned medium by OKT4A as shown in the Examples, below. CD-4, fragments and derivatives can be prepared chemically, after expression, or genetically, prior to expression, by manipulation of the coding sequence for the leader and/or extracellular domain.
A DNA coding sequence for sCD-4 or HIV binding protein derived therefrom can be obtained, for example, by synthesizing the gene using the known DNA sequence, by standard cloning techniques based on the sequence and by reisolation by detection of protein, i.e., transfection of cDNA clones from CD-4 expressing cell lines and identification by antibodies directed against the protein (See Maddon, et al., supra).
cDNA clones carrying the coding sequence of the particular sCD-4 protein can be identified by use of oligonucleotide hybridization probes. The probes can be designed based on the particular sequence of the protein. Having identified a clone carrying the coding sequence of interest, the coding sequence of the protein can be excised by the use of restriction endonucleases and inserted into cloning and/or expression vectors. In an expression vector, the coding sequence of the sCD-4 protein is operatively linked to regulatory functions
8 0 0 0 0 dV
required or desirable for transcription, translation and processing of the coding sequence.
In carrying out the present invention in Ξ. co 1i, a DMA coding sequence which encodes the HIV binding protein, e.g., sCD-4 or derivatives thereof, is operatively linked to a regulatory element within a DNA vector for transformation of E. coli. Numerous gram negative bacterial expression vectors comprising such regulatory elements are available. The regulatory element comprises a promoter which effects RNA polymerase binding and transcription. Regulatable, i.e., inducible or derepressible, promoters are preferred. A variety of useful promoters are available for expression of heterologous polypeptides in 2. coli. These include the trp promoter and the lambda PL promoter. See, e.g,, U.3. Patent 4,578,355; Courtney et al., Nature 313:149 (1985). Most preferably, the regulatory element comprises a leader sequence for transport of the HIV binding protein to or through the cell membrane as it has been discovered in accordance with this invention that the HIV binding protein can be secreted. A leader which has been shown. ft transport a protein to the Ξ. coli outer membrane is that of the 3acillus lichen iformis penicillinase gene. See, Sarvas, et al., J. Sactericl. 155:657(19 83).
Particularly exemplified herein is the leader for the outer membrane polysaccharide A, herein referred to as the CMPA leader or signal. See, Mowa, et al. , J. Moiec.
Biol. 143 :317( 1980) . The CMPA coding sequence comprises a leader sequence which is useful for secreting the HIV binding protein into the fermentation medium. It has now been found that the OMPA leader can be used to cully secrete a variety of low molecular weight proteins or polypeptides into the culture media. For example, the OMPA signal has been used to obtain export of large amounts (e.g., more than 1 to about 10 mg/L) of active
BAD ORIGINAL &
human transforming growth factor-alpha (TGF-alpha), tumor necrosis factor (TNF) and interleukin-l-beta (IL-l-beta), in addition to SKBsCD-4, V1J4 and V1V2J4.
The OMPA signal comprises substantially the following 21 amino acids: N-met-lys-lys-thr-ala-ile-ala-ile-ala-valala-leu-ala-gly-phe-ala-thr-val-ala-gln-ala-C. A DNA coding sequence for such leader can be synthesized, preferably such that one or more restriction sites are placed adjacent the C-terminal amino acid for insertion of a desired DNA coding sequence and such that a terminator is placed downstream of the desired coding sequence. An illustrative synthetic coding sequence is shown in the Examples, below.
In addition to the HIV binding protein minigene, i.e./ coding sequence operatively linked to a regulatory element, the vector used for transformation preferably contains at least one phenotypic transformation marker, i.e., genetic selection marker, such as an antibiotic resistance gene, a chromogenic agent or a gene which complements an auxotrophic mutation. The vector also comprises regions required for autonomous replication.
Illustrative constructions of useful expression vectors for expression of sCD-4 proteins in E. coli are described in detail in the Examples. The proteins were expressed into the medium and were apparently folded properly.
In carrying out the present invention in Streptomyces, a DNA coding sequence which encodes the HIV binding protein, e.g., sCD-4 or derivatives thereof, is operatively linked to a regulatory element within a DNA vector for transformation of Streptomyces. The regulatory element comprises a promoter which effects RNA polymerase binding and transcription. Regulatable, i.e., inducible or derepressible, promoters are preferred. A variety of useful promoters are available for expression of heterologous polypeptides in Streptomyces. Examples
AP 0 0 0 0 8 0
BAD ORIGINAL £
O ?x>
include the galactose-inducible promoter of the
Streptomyces galactose operon (Fornwald, et al. , Proc.
Natl. Acad. Sci. USA 84:2130 (1987)), the constitutive promoter of the S. 1ividans 2-galactosidase gene (Eckhardt, et al. J. Bacteriol. 169:4249 (1987); Brawner, et al, U.S. Patent 4,717,666) and. the S. longisporus trypsin inhibitor gene (European Patent Application No. 87 307 260.7), or a temporally regulated promoter such as that reported in K. echinosporsa (Baum, et al., J. Bacteriol. 170:71 (1983)). Regions for transcription termination in Streptomyces are derived from the 3' end of several Streptomyces genes, for example the termination signal at the end of the Streptomyces galactose operon or that found at the end of the S. fradiae neomycin phosphotransferase gene (Thompson and Gray, Proc. Nat 1. Acad. Sci USA 80:5190 (1983)). Sequences for protein export in Streptomyces include those isolated from the S. lividans β-galactosidase gene, the S. 1ividans LEP-10 gene (European Patent Application No. 87 307 260.7) and the S. longisporus trypsin inhibitor gene.
The sCD-4 gene is incorporated into a larger DNA molecule which comprises a genetic selection marker system. The selection marker system can be any of a number of known marker systems such that the marker gene confers a selectable new phenotype on the transformed cell. Examples include Streptomyces drug resistance genes such as thiostrepton resistance ribosomal methylase (Thompson, et al., Gene 20:51(1982)), neomycin phosphotransferase (Thompson, et al., supra) and erthromycin resistance ribosomal methylase (Thompson, et al., supra). The DNA molecule may also contain a sequence for autonomous replication in Streptomyces, such as the pIJlOl derivatives (Keiser, et al,, Mol. Gen. Genet. 185:223 (1982)) or an SLP1 derived vector (Bibb, et al., Mol. Gen. Genet 184:230 (1981)). The DNA molecule may also contain a marker which permits gene amplification, Such markers
BAD ORIGINAL which serve to amplify gene copy number in Streptomyces include the gene for spectinomycin resistance (Hornemann, et al. J. Bacteriol. 169:2360 (1987)) and arginine axuotrophy (Altenbuchner, et al., Mol. Gen. Genet. 19 5 : 13 4 ( 1984)) .
For the initial expression studies, the CD-4 coding sequence as more fully described in the Examples, below, was fused to the Bgal signal sequence at a position located 8 amino acids downstream of the Qgal signal peptide cleavage site. The Streptomyces replication functions for this expression vector was provided by plasmid pIJ702 (Katz, et al., J. Gen. Microbiol.
129:2703(1983)), which is a derivative of pIJlOl (Keiser, et al., Mol. Gen. Genet. 185:223(1982)). The host strain used was wild-type S. lividans 1326 (Bibb, et aI., Mol. Gen. Genet. 184:230( 1981)) . The Qgal-sCD-4 fusion protein was detected in both the culture supernatant and intact cells. Another series of experiments showed that the LTI promoter could be used to obtain more efficient expression of the sCD-4 proteins.
The LTI expression/secretion vectors are analogous to the Qgal system in that gene expression is directed by the LTI promoter and protein export is facilitated by the LTI signal peptide. Coding sequences for a number of HIV binding proteins have been cloned into the LTI vector including V].V2J4 an<^ Vl^4' Tiie c°din<? sequences for all of these proteins were inserted at a position located 8 amino acids downstream of the LTI signal peptide cleavage site. Like the Qgal fusions, the sCD-4 proteins can be transported into the culture supernatant via the LTI signal peptide. The Streptomyces replication functions were again provided by pIJlOl derivatives: pIJ7Q2 and pIJ351 (Keiser, et al., supra).
SK3sCD-4, V1J4 and V2.V2J4 expression from the LTI expression system was initially examined in S. lividans 1326. Both SKBsCD-4 and V1V2J4 were equally
AP 0 0 0 0 8 0
bad ofug^al
ο ο
ο >
distributed between the culture supernatant and intact cells. Although these proteins are incompletely exported, the intra- and extracellular forms appear to have the same molecular weight as judged by their mobilities on
SCS-polyacrylamide gels. It is unclear if the signal peptide is proteolyticaily removed from the intracellular form. The maximum levels of SKBsCD-4 were estimated to be 30 mg/1 in the culture supernatant and intact cells. The V1V2J4 levels were estimated to be at least 30 mg/1 (culture supernatant and intact cells).
One problem encountered for sCD-4 expression in
S. lividans is its susceptibility to protease activities. This problem can be eliminated or at least significantly diminished by expressing sCD-4 in other Streptomyces species. The sCD-4 proteins can be expressed, for example, in S. coelicolor, S. longisporus and S. albus.
It is expected the stability of 'the molecule will be enhanced using these alternate hosts. Expression of sT4 proteins in S. longisporus may be advantageous since this host secretes comparatively fewer proteins into the culture supernatant which assists in the purification process.
In carrying out the present invention in yeast, a DNA coding sequence which encodes the HIV binding protein,
e.g., sCD-4 or derivatives thereof, is operatively linked to a regulatory element within a DNA vector for transformation of yeast. Any yeast host for which transformation, cloning and expression systems are available can be used. Particular examples include yeasts of the genera Hansenula, Pichia, Kluveromyces,
Schizosaccharcmyces, Candida and Saccharomyces. The preferred yeast host is Saccharomyces cerevisiae.
The regulatory element comprises a promoter which effects RNA polymerase binding and transcription.
Regulatable, i.e., inducible or derepressible, promoters are preferred. A variety of useful promoters are
BAD ORIGINAL ft available for expression'of heterologous polypeptides in yeast. These include the copper inducible metallothionein gene (CUP1) promoter and the constitutive promoter of the glycolytic genes glyceraldehye-3 phosphate dehydrogenase (TDH3) and alcohol dehydrogenase (ADH). Regions for transcriptional termination in yeast are derived from the 3' end of any of several yeast genes, for example the gene for iso-l-cytochrome C (CYC1).
The sCD-4 gene is incorporated into a larger DNA molecule which comprises a genetic selection marker system. The selection marker system can be any of a number of known marker systems, such that the marker gene confers a selectable new phenotype on the transformed cell. Examples include yeast genes for biosynthetic enzymes such as phospho-ribosyl anthranilate isomerase (TRP1) or orotidine-5'-phosphate decarboxylase (URA3) or heterologous drug resistance genes such as G418 resistance or benomyl resistance (BENI). The DNA molecule may also contain a sequence for autonomous replication in yeast, such as the yeast 2-micron-circle ori region or a chromosomal autonomous replication region (ARS), such as ARS1, and a yeast centromere (CEN), such as CEN3 , to allow for autonomous replication of the plasmid.
In the preferred expression system, the HIV binding protein coding sequence is fused to a coding sequence which stabilizes expression, inasmuch as it has been discovered that SKBsCD-4 alone expresses poorly; such poor expression may be due to inefficient transcription and translation or to rapid protein degradation. In any case, 30 it has been demonstrated that the product of a gene fusion, in which the coding sequence of a ubiquitin is fused 5' to the SKBsCD-4 coding sequence is expressed at relatively high levels and is cleaved to yield ubiquitin and the sCD-4 gene product.
A ubiquitin DNA coding sequence can be isolated from yeast or other eukaryotic cell, including mammalian cells,
AP 0 0 0 0 8 0
BAD ORIGINAL by standard gene cloning techniques. Alternatively, it can be synthesized by standard known techniques. The nucleotide sequence of the modular ubiquitin gene used to illustrate the instant invention is that described by Ecker et al., J. Siol. Chem. 262:3524 (1987). The sequence is substantially as follows:
AATTCATTATOCAGATCTTCGTCAAGACGTTAACCGGTAAAACCATAACTCTAGA
AGTTGAATCTTCCGATACCATCGAGAACGTTAAGTCGAAAATTCAAGACAAGGAA
GGCATTCCACCTGATCAACAAAGATTGATCTTTGCCGGTAAGCAGCTCGAGGACG
GTAGAACGCTGTCTGATTACAACATTCAGAAGGAGTCGACCTTACATCTTGTCTT
AAGACTAAGAGGTGGTTGAGGTAC ce
By inserting a DNA sequence for a signal peptide at the 5' end of the HIV binding protein sequence, secretion of protein into the culture medium can be achieved.
Signal sequences useful for this purpose are, for example, those of the yeast mating factor, alpha-factor (Kurjan and Herskowitz, Cell 30:933(1982). In addition, expression may be obtained by integration of the sCD-4 yeast expression module into the yeast chromosome, followed by amplification, using markers such as the yeast DKFR gene to select for increased copy number.
In general, the sCD-4 proteins of the invention can be purified from spent culture media using various protein purification techniques, for example, affinity chromatography; ion exchange chromatography; size exclusion chromatography; hydrophobic chromatography cr reversed phase chromatography.
sCD-4 its fragments and derivatives can be purified by affinity chromatography using general group-specific adsorbents, for example, carbohydrate binding or dye affinity ligands; or using ligands that specifically bind to sCD-4, for example, monoclonal antibody or HIV gpl20 protein or portions thereof.
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Purification comprises, after growing ceils in a selective growth media at about 28 to about 45° C; clarification of the fermentation medium and then separation of the HIV binding protein from other proteins present in the media. In the preferred method, the sCD-4 proteins are purified from culture medium using a series of chromatography steps which are based on the physical properties of the sCD-4 molecule.
An alternative method of purification of sCD-4 proteins involves the use of monoclonal antibodies directed against sCD-4. The protein can be purified in one step by passage of clarified culture media through an affinity gel support to which monoclonal antibody directed against the protein is bound. The protein of interest will bind to the column at the antibody binding site while contaminating proteins wash through the column. The protein is then eluted from the column under conditions that prevent inactivation.
Characterization of the in vitro biological and immunological properties of the sCD-4 proteins indicate the proteins are of value in the prevention and treatment of AIDS. Studies indicate the sCD-4 proteins act as an inhibitor of extracellular and cell to cell spread of the virus. Because sCD-4, fragments and derivatives thereof described in this invention have been shown to block virus binding to CD-4+ target cells in culture, it is believed administration of these proteins to infecred persons would act to inhibit the extracellular spread of the virus. Therefore, sCD-4 proteins are of value both as a prophylactic and therapeutic agent for treatment of AIDS or AIDS-related complex (ARC).
As a prophylactic, sCD-4 proteins are administered to individuals at high-risk for the disease or individuals who show exposure to HIV by the presence of antibodies ro virus. Administration of an effective amounr or the protein at an early stage of the disease or prior to its
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Fusion between HIV infected cells and other CD-4 + lymphocytes also appears to be a route of virus spread. Further, fusion may be responsible, in part, for the impairment of CD-4+ lymphocyte function and ultimately the depletion of CD-4+ lymphocytes in infected individuals. Cell fusion is dependent on both viral envelope gene products and the CD-4 receptor and can be inhibited by the OKT-4A, or similar monoclonal antibodies (Mabs) (Sattentau, et al. , Science 234:1120(1986)). sCD-4 proteins described herein interfere with cell fusion and therefore diminish the cell to cell spread of virus and the loss of CD-4+ lymphocyte function.
The CD-4 receptor is monomorphic and thus sCD-4 proteins are believed to be a universal inhibitor of virus which recognize the surface domain of the CD-4 receptor, including all HIV.
sCD-4 proteins may be used in combination with other agents, for example, in association with agents directed against other HIV proteins, such as reverse transcriptase, protease or tat. An effective therapeutic agent against HIV should prevent virus mediated as well as cell to cell transmission of infection. sCD-4 proteins may also be used in combination with other anti-viral agents, for example, azidothymidine (AZT).
The sCD-4 proteins of this invention also have utility as inhibitors of CD-4+ cell function by binding to extracellular target molecules which normally interact with the surface domain of the CD-4 receptor. Numerous studies suggest a critical role for the CD4 receptor in immune tolerance, particularly in the pathogenesis and progression of autoimmune diseases and in host specific graft rejection.
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As a prophylactic or therapeutic, sCD-4 proteins are administered parenterally, preferably intravenously. The agent can be administered by infusion or by injection, e.g., daily, weekly or monthly. The amount and rare of administration is selected sc as to maintain an effective amount of sCD-4 protein in circulation. An alternative mode of administration would be extracorporeal, employing sCD-4 proteins as dialysis agents.
The sCD-4 protein of this invention can also be used as a reagent to identify natural, synthetic or recombinant molecules which act as therapeutic agents or inhibitors of CD-4 cell interactions.
For example, sCD-4 proteins can be used in screening assays, such as, assays for protein interaction measured by FLISA based methodologies, to provide a biochemically pure, aqueous soluble reagent which may be used in combination with other reagents to assay for competitors of the CD-4 receptor surface domain interactions. For example, since sCD-4 proteins bind to HIV env protein or mixtures containing HIV env proteins, the proteins can be used to screen for inhibitors of virus binding.
3ased on in vitro data showing that sCD-4 proteins bind to cells expressing HIV env proteins, these proteins can also serve as selective targeting molecules for HIV infected cells in vivo. As a target specific carrier protein, sCD-4 proteins can serve, for example, as the carrier protein for delivery of cytotoxic agents to the infected cells.
In addition, based on data showing that the CD-4 receptor specifically associates with Mhc class II antigens on antigen presenting cells as suggested by the class restriction of CD-4+ cells, sCD-4 proteins can be used in combination with class II antigens to test for inhibitors of CD-4 lymphocyte - target cell interactions. In addition to these examples, which are based on direct binding assays between the protein and its target
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A ί» molecules, more complex assays can be designed which rely on the biochemical responses to protein recognition. The deletion mutants can be used in diagnostic assays for the detection of CD-4 proteins or the molecules with which they interact. For example, quantitation of CD-4 and CD-4+ cells and antibodies to CD-4 would be of diagnostic value for AIDS.
In addition, sCD-4 proteins can be used to generate new diagnostic reagents, for example, Mabs or other types of molecules for use in the standard immunologic assays, i.e., ELISA, capture immunoassays, radioimmune assays. Because the sCD-4 display the OKT-4, the OKT-4A and most if not all of the other surface epitopes of the CD-4 receptor, the proteins are especially useful in immunodiagnostic assays for absolute quantitation of CD-4 levels in a system.
The CD-4 receptor resides in three diverse chemical environments: the oxidizing, hydrophylic cell surface;
the hydrophobic membrane; and the reducing, hydrophilic cytoplasm. These diverse environments would most likely preclude the isolation of the receptor in its fully native state. The sCD-4 proteins consist of only select segments of the extracellular domain, are secreted as a soluble proteins into the cell supernatant and their conformation appears to mimic to a significant extent the surface of the receptor surface domain. Thus, the sCD-4 proteins are suitable for detailed structural analysis, in particular «
for x-ray crystallography. Determination of the
3-dimensional structure of the sCD-4 proteins alone or in a compiexed form with other interactive molecules could provide a basis for ohe rational design cf selective antagonists and agonists for sCD-4.
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Examples
The Examples which follow are illustrative, and not limiting of the invention. Enzymes used in the genetic manipulations were obtained from commercial sources and were used substantially in accordance with the vendor's instructions. Except where otherwise indicated, procedures were carried out substantially as described by Maniatis, et al., Molecular Cloning, Cold Spring Harbor Laboratory, 1982.
Example 1: Construction of E. coli expression vectors
Using recombinant DNA manipulations, the coding sequence for the full length SKBsCD-4 and the deletion mutants, V1V2J4 or V1J4, followed by an in frame TAA termination codon (see sequence, above) were placed downstream of the OMPA signal sequence in an E. coli expression vector to create plasmids OMPAST4BBV1, OMPAV1V2 and OMPAV1. The construction of these vectors is as follows:
Construction of plasmid JB.T4 : To create plasmid JRT4, plasmid DSP1 (Pfarr, et al., DNA 4:461(1985)) was cut with Xhol, the SV40 polyA early region was deleted, and the Xhol sites were filled in using Klenow fragment of DNA polymerase. The bovine growth hormone (BGH) polyadenylation region (Pfarr, et al., DNA 5:115(1986)) was cut with PvuII and Kpnl, and the Kpnl site was blunted by treatment with T4 DNA polymerase. This 230 bp fragment was ligated to DSP1 to create DSP1BGH.
DSP1BGH was cut with Smal and Sail and the galK cassette (consisting of the SV40 early promoter, galK coding region and BGH polyA region) was ligated into pUC19 (Yanisch-Perron, et al., Gene 33:103(1985)) at the Sail site by using a synthetic linker consisting of a Sail end, a Bglll site, and a Smal end. This three part ligation resulted in plasmid DSP13Z3GH.JT.
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DSP13ZBGH.JT, which was cut with Stul and 3cII to delete the galK coding region, was ligated to a 1.7 kb EcoRl (filled in)-3amHI fragment, containing the CD-4 cDNA from plasmid pT43 (Maddon, et al., Cell £2:93(1985)) to create plasmid JR.T4 .
Construction of plasmid pUCsT4: To create plasmid pUCsT4, a Haell and Hpall fragment (1125 bp) of the CD-4 cDNA from plasmid pT4b was ligated through the use of synthetic linkers, to vector p(JC13 which had been cut with Kpnl and Xbal. The Haell end of the CD-4 cDNA was ligated to the Kpnl site of pUC18 using a synthetic linker with a Kpnl end and a Haell end. The Hpall end of the CD-4 cDNA was ligated to the Xbal site of pUCIS using a synthetic linker with a Hpall end and an Xbal end. This linker also inserted a TAA stop cocon after nucleotide 1257 cf the CD-4 coding region. The resulting plasmid was pUCsT4. Construction of pST4sal: To create plasmid pST4sal, plasmid JRT4 was cut with Bglll and Sacl and a 959 bp fragment (consisting of the SV40 early promoter and the first 602 nucleotides of the CD-4 cDNA) was isolated. Plasmid pUCsT4 was cut with Sacl and Xbal and a 660 bp fragment (consisting of the CD-4 cDNA from nucleotides 603-1257 followed by the TAA codon from the synthetic linker) was isolated. These two fragments were ligated into DSP1BZ3GH.JT which had been cut with 3glII and Xbal to delete the SV40 early promoter and full length CD-4 coding region. The resulting plasmid was pST4sal. Construction of pST4DKF~x: To create. plasmid pST4DHFR, a 3glII-BamHI fragment containing a β-globin DHFR expression cassette was ligated into the 3amHl site of pST4sal. Che β-glcbin DHFR expression cassette consists of: the mouse β-globin promoter ( 550 bp Hindi fragment from plasmid pPK283 (3erg, et al., Mol. Ceil. Biol. 3:1246(1983)) modified at its 5' end with a synthetic linker tc contain a Bglll site; the mouse DHFR coding region ( 735 bp Hindi 11
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(fill-in) fragment from plasmid pSV2-DHFR (Subramani, et al., Mol. Cell. Biol. 1:854(1981)); Nhel (fill-in)-BamHI (fill-in) SV40 polyA early region from DSP1 (Pfarr, et al., DNA 4:461(1985)); and the mouse DHFR terminator region (907 bp Hindlll (fill-in fragment from plasmid mDH9 (Frayne, et al., Mol. Cell. Biol. 4:2921(1984)), modified at its 3’ end with a synthetic linker to create a BamHI site.
Construction of psT4BBV!DHFR: To create plasmid psT4BBVlDHFR, plasmid pST4DHFR was cut with EcoRI and Xbal and the smaller fragment containing the sCD-4 coding region was deleted. Plasmid sT4sal was cut with Xbal and Bbvl and a 1120 base pair coding fragment containing the sequence for soluble CD-4 minus the leader region was isolated. This fragment was ligated to the EcoRI/Xbal-cut pST4DHFR, using a synthetic linker with an EcoRI end, a Kpnl site, and a Bbvl end. This fragment is compatible with the Bbvl overhang on the sCD-4 fragment isolated above. The resulting plasmid was called pST4BBViDHFR. Construction of OMPAST4: To create'plasmid OMPAST4, plasmid OMPA.GS was digested with Ncol and Sail and the smaller fragment containing the linker region was deleted. OMPA.GS is a derivative of pASl (Rosenberg et al., Meth. Enzymol. 101: 123 (1983); U.S. Patent 4,578,355) having a synthetic sequence inserted into the Ndel site at the 3' end of the ell ribosome binding sequence. The synthetic sequence comprises the OMPA leader followed by a multilinker sequence. The synthecic sequence was substantially as follows:
'-T ATG AAA AAG ACA GCT ATC GCG ATT GCA GTG GCA CTG GCT GGT TTC GCT ACC GTA GCG CAG GCC GGC TCT AGA GTC GAC CTA GTT AAC TAG-3'
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Plasmid pUCsT4 was cut with Ncol and Sail and the 1149 base pair fragment containing sCD-4 sequence (CD-4
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nucleotides 124-1257) was isolated. This fragment was ligated to the Ncol/Sall cut OMPA.GS to create CMPAST4. Construction of 0MPAST43bvI: To create plasmid OMPAST43bvI, plasmid 0MPAST4 was cut with Nael and Xbal. The smaller fragment resulting from this cut, containing the sCD-4 coding region was deleted. Plasmid ST4BBVIDHER was cut with Kpnl and the resulting 3' overhang was blunt ended with T4 DNA polymerase. The blunt ended DNA was then cut with Xbal and the 1124 base pair fragment containing the nucleotides 145-1257 of the CD4 cDNA was isolated. The isolated fragment was ligated to the Nael/Xbal cut 0MPAST4 plasmid to create plasmid 0MPAST4Bbvl.
Construction of puc5T4184: To create plasmid pucST4184, an EcoRI-Nhel fragment from the CD-4 cDNA [a 632 bp fragment encoding amino acids (-25) to (+176)] was ligated to the synthetic linker sk727/725 (Nhel and Aval ends) at the Nhel site. sk727/725 codes for CD-4 amino acids 177-183). The Aval end of sk727/725 was ligated to an Aval-Xba 1 fragment of pucST4 (comprising bp 1193-1257 of the human cDNA and encoding amino acids 351-369 of the CD-4 receptor followed by a TAA termination codon). This sequence, which is flanked by EcoRI and Xbal ends, was inserted into pUC19 at the EcoRI and Xba 1 ends in the pUC19 polylinker (sk727/725). sk727/725 is substantially as follows:
5' ctagctttccagaaggcc 3'
3’ gaaaggtcttccggagcc 5'
Construction of pucST41Q6: To create plasmid pucST4106, an EcoRI-Ava II fragment (comprising bp 1-413, and encoding amino acids (-)25 to 87) of the CD-4 cDNA was joined to the synthetic linker sk791/792 (Ava II-Aval ends) at the Avail site. sk791-792 codes for CD-4 amino acids 88-104. The Aval end of sk791/792 was ligated to an Aval-Xbal fragment of pucST4 (comprising bp 1198-1257 of
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the human cDNA, and encoding amino acids 351-369 of the CD-4 receptor followed by a TAA termination codon), This sequence, which is flanked by EcoRI and Xbal, ends was inserted into pUC19 at the EcoRI and Xbal ends in the p(JC19 polylinker. sk791/792 is substantially as follows:
5' gaccagaaggaggaggtgcaattgctagtgttcggattgactgccaac gtcttcctcctccacgttaacgatcacaagcctaactgacggttgagc 5'
Construction of sT4184.DHFR: To create plasmid
ST4184.DHFR, an EcoRl-Xbal fragment of pucST4184 (encoding amino acids -25 to 183 fused to 351 to 369) was ligated to the EcoRI and Xbal ends of psT4.DHFR in place of the EcoRI-Xbal* fragment encoding SKBsCD-4.
Construction of ST4106.DHFR: To create plasmid sT4106.DHFR an EcoRI-Xbal fragment of pucST4106 (encoding amino acids -25 to 104 fused to 351 to 369) was ligated to the EcoRI and Xbal ends of psT4.DHFR in place of the EcoRI -Xba 1 fragment encoding SKBsCD-4.
Construction of OMPAVl: To create OMPAVl, plasmid OMPAST43bvI was cut with Aflll and Xbal and the smaller fragment containing nucleotides 371-1257 of the CD-4 cDNA coding region was deleted. Plasmid pst4106.DHFR was cut with Aflll and Xbal and a 160 base pair fragment containing nucleotides 371-459, 1198-1257 of the CD-4 cDNA sequence was isolated. The two fragments were ligated to create plasmid OMPAVl.
Construction of QMPAV1V2: To create 0MPAV1V2, plasmid OMPAST4BbvI was cut with Sacl and Xbal and the smaller fragment containing nucleotides 603-1257 of the CD-4 cDNA sequence was deleted. Plasmid ST4184.DHFR was cut with Sacl and Xbal and a 164 base pair fragment containing nucleotides 603-696, 1198-1257 of the CD-4 cDNA sequence was isolated. The two fragments were ligated to create plasmid OMPAV1V2.
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Example 2: Expression of sCD-4 proteins in E.coli
The OMPAVl and 0MPAV1V2 constructions were transformed into defective Ξ.coli lambda lysogens, AR38 (cI857) and AR120 using standard procedures. Heat inductions (Rosenberg, et al., Meth. Enzyraol. 101:123 (1983)) or naladixic acid inductions (Mott, et al., Proc. Natl. Acad. Sci. (JSA 82:88 (1985)) were performed’as described below.
Heat Induction: For cell line AR58, 200 ml of LB (containing 50 ug/ml ampicillin) was seeded with 7 ml from a 10 ml overnight (O.N.) culture of AR58 cells containing the OMPAST4Bbvi, OMPAVl or OMPAV1V2 plasmid, and grown in a shaking incubator at 32° C. At an optical density at 650 nm (O.D.--n) of 0.3 absorbance units, 200 ml of L5, warmed to 55° C, was added to the culture and the flask was transferred to a 42° C shaking incubator. One ml samples of the culture were taken 30, 60 and 90 minutes after the temperature shift, for analysis. At 9C minutes, the cells were chilled for 15 minutes in ice water, and then pelleted at 3500 rpm for 15 minutes at 4” C in a J-6 Beckman centrifuge (Beckman Instruments, Fullerton, California). Cell pellets were stored frozen at -20’ C until processing. Conditioned media was stored frozen at -20° C until processing.
Nalidixic Acid Induction: For cell line AR120, 400 ml of L3 (containing 50 ug/ml ampicillin) was seeded with 13 ml from a 20 mi O.N. culture of AR120 cells containing the 0MPAST43bvl, OMPAVl or OMPAV1V2 plasmid, and grown in a shaking incubator at 37° C. At an O.D.g-θ of 0.4,
400 ul of nalidixic acid (50 mg/ml) were added to the culture. The culture was maintained at 37° C in a shaking incubator and 1 ml samples were taken 1, 3 and 5 hours after addition of the nalidixic acid. At 5 hours, the cells were chilled for 15 minutes in ice water, and then pelleted at 3500 rpm for 15 minutes at 4’ C in a J-6
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Beckman centrifuge. Cell pellets were stored frozen at -20° C until processing. Conditioned media was stored frozen at -20e C until processing.
Following induction, cells were pelleted from the 1 ml samples, and analyzed for expression of the full lengtxh and mutant sT4 proteins (SKBsCD-4, V1J4 and V1V2J4) by western blot, using a rabbit polyclonal antibody to a denatured form of soluble T4 produced in bacteria.
Proteins of the appropriate sizes were detected in cell lysates of both heat and nalidixic induced samples.
Levels detected represented 1-5¾ of total protein. Conditioned Media Processing: Frozen conditioned media was thawed at room temperature and 30 ml aliquots were taken and centrifuged at 4° C for 1 hour at 24,000 rpm in a Beckman SW28 swinging bucket rotor. Following centrifugation, the supernatants were pooled and concentrated 10-20 fold at 4° C by pressure membrane filtration.
Concentrated media was assayed for full length SKBsCD-4, V1J4, or V1V2J4 proteins by western blot analysis (as above), competition ELISA, and immunoprecipitation.
In each sample, protein of the appropriate size was detected in the concentrated conditioned media by western blot, at levels representing 1-5% (0.1-0.5 ng/ml unconcentrated conditioned media) of that detected inside the cell. All 3 proteins bound OKT4A in the competition ELISA assay. The V1J4 and V1V2J4 proteins were further assayed by immunoprecipitation with a panel of monoclonal antibodies to CD-4 (Ortho, Raritan, New Jersey). The protein expressed by OMPAV1, V1J4, was immunoprecipitated by OKT4A, and OKT4D but not by OKT4 , OKT43, OKT4C, ΟΚΤ4Ξ or OKT4F. The protein expressed by OMPAV1V2, V1V2J4, was immunoprecipitated by all of the OKT4 monoclonal antibodies except OKT4 . In addition, the affinity of this protein for OKT4C was lower than for the other monoclcnals.
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Cell Pellet Processing: Cell pellets from the 90 minute time point of the OM?AST43bvl/AR53 heat induction, were thawed on ice, and resuspended in buffer (lOOmM Tris-HCl, pH 3, 0.5 mM EDTA, and 0.5 M sucrose) at 4° C at a pellet to buffer raio of 100 O.D.g50/ml. Lysozyme (10 mg/ml in 0.05 M Tris-HCl, pH 8) was added to a final concentration of 0.2 mg/ml and the suspension incubated on ice for 15 minutes. An equal volume of ice cold water was added and the suspension incubated on ice for 15 minutes. PMSF (50 mM) was added to a final concentration of 1 mM, followed by the addition of MgCl2. (1 M) to a final concentration of 2 mM. The cell suspension was passed through an 18 gauge needle 3 times to reduce viscosity, and then centrifuged at 20,000 x g for 10 minutes, at 4’ C.
Following centrifugation, the pellet was resuspended in 20 mM Tris-HCl, pH 8, 5 mM EDTA, 5 mM 0ΜΕ, in a volume equivalent to that prior to centrifugation. The suspension was sonicated for 60 seconds (10 second bursts with 30 seconds in between for cooling), and then centrifuged at 20,000 x g for 15 minutes at 4° C. Western blot assay of the resulting pellet and supernatant, indicated that 70¾ of the SK3sCD-4 protein was in the supernatant fraction. The supernatant fraction was centrifuged at 100,000 x g for 60 minutes. Western blot analysis of the resulting pellet and supernatant, indicated that ¢5¾ of the SKBsCD-4 protein had remained in solution. The supernatant fraction was diluted with an equal volume of 40 mM MES pH 6.0 and loaded onto a 1 ml S Sepharose (Pharmacia, Piscataway, New Jersey) column equilibrated with 20 mM MES pH 6.0. The column was washed with 10 mis 20 mM MES pH 6.0. The bound SKBsCD-4 was eluted with 20 mM MES pH 6.0, 0.5 M NaCl, collecting 1 ml fractions. Western blot analysis of the flow through, wash, and elution fractions, indicated that <5% of the SK3sCD-4 bound to the column and eluted in fractions 2 and 3 .
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The flow through, wash and elution fractions were assayed for functional SKBsCD-4 by competition ELISA.
Both the flow through and elution fraction 2 contained SK3sCD-4 which bound OKT4A.
Immunoprecipitation: Concentrated media (100 ul) was diluted with an equal volume of precipitation buffer (10 mM sodium phosphate, pH 7.5, lOOmM NaCl, 0.1% NP-40, 0.5% non-fat dry milk) and precleared with 3 ug rabbit IgG for 15 minutes at 4 C. followed by the addition of 30 ul (packed volume) of protein A-Sepharose beads (Pharmacia, Piscataway, New Jersey) for 30 minutes at 4’ C.
Precleared supernatants were incubated with 5 ug of OKT4, 4A, 4B, 4C, 4D, 4E, 4F, OKT8 monoclonal antibodies (Ortho Pharmaceuticals), mouse IgG (Cooper Biomedical, Malvern, Pennsylvania) or rabbit anti-mouse IgG (Cooper Biomedical) for 30 minutes at 4 C. OKT4, 4A, 4C, OKT8, mouse IgG and rabbit anti-mouse IgG were precipitated by incubation with 20 ul (packed volume) of protein A-Sepharose beads for 30 minutes at 4° C. OKT4B, 4D, 4Ξ and 4F were incubated with 10 ug of rabbit anti-mouse IgG for 30 minutes at 4° C prior to addition of the protein A Sepharose beads. Following precipitation, the beads were washed twice with 200 ul of precipitation buffer and once with 200 ul of precipitation buffer without NP-40 and non-fat dry milk. The washed beads were boiled for 5 minutes in 20 ul of sample buffer (125 mM Tris-HCl, pH 6.8, 20% glycerol, 1.4M QMS (beta-mercaptoethanol)). Following boiling, the supernatants were electrophoresed on a 12.5%
SDS-polyacrylamide gel and analyzed by western blot as described above.
Both V1J4 and V1V2J4 proteins were immunoprecipitated by OKT4A. The protein expressed by OMPAVl was immunoprecipitated by OKT4A and OKT4D, but not by OKT4 , OKT4B, OKT4C, 0KT4E or OKT4F. The protein expressed by OMPAV1V2 was immunoprecipitated by all of the OKT4 monoclonal antibodies except OKT4 . In addition, the
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affinity of this protein for 0KT4C was lower than for the other monoclonal antibodies.
Competition ELISA : Microtiter plates (Flow Laboratories, McLean, Virginia) were coated overnight at room temperature with 100 ul/well of 0.1 M NaHCO3/Na2CO3 (pH 9.4) containing 150 ng of purified sCD-4.
Aliquots (2.5-80 ul) of concentrated media or cell extract were incubated with 5 ng of OKT4A in the presence of 1 mg/ml bovine serum albumin (BSA) in a final volume of 100 ul, overnight at room temperature. Samples of less than 100 ul were diluted to 100 ul with phosphate buffered saline (PBS). After incubation, the plates were poured off, rinsed 3 times with PBS and patted dry. To each well was added 380 ul of PBS/0.5% gelatin. The plates were incubated at 37’ C for one hour.
Following incubation at 37° C, the plates were poured off, rinsed 3 times with PBS and patted dry. The 100 ul sample incubations containing the monoclonal antibody were added to the individual wells of the prepared plate and incubated for 5 hours at 37° c.
Following incubation, the plates were poured off, rinsed 5 times with PBS and patted dry. 100 ul of a solution containing biotinylated horse/anti-mouse IgG was added to each well. This antibody preparation was prepared by adding one drop of horse/anti-mouse IgG (Vector Labs, 3urlingame, California) to 10 ml of PBS containing 1% horse serum. The plates were incubated for 30 minutes at 37° C.
Following incubation, the plates were poured off, rinsed 5 times with PBS and patted dry. 100 ul of ABC complex (Vector Labs, Burlingame, California) was added to each well. The plates were then incubated at room temperature for 30 minutes.
The plates were again poured off, rinsed 5 times with PBS and patted dry. 100 ul of p-nitrophenyl phosphate mix
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Example 3: Construction of yeast expression vectors
The plasmids used to construct expression vectors in yeast for the expression of sCD-4 proteins are based on the basic high copy yeast shuttle vector pYSK102 (Rosenberg, et al., Genetic Engineering 8:151(1986). All such plasmids contain an 823 base pair EcoRI-Pstl fragment of the yeast TRP1 gene (Tsumper and Carbon, Gene 10:157 (1980)), which provides a selectable marker; a 2.0 kb EcoRI-Pstl fragment of the yeast 2-micron circle (Hartley and Donaldson, Nature 236:860(1980)), which provides an origin of replication in yeast; a portion of pBR322 (deleted from BamHI to PvuII) (in Cloning Vectors,
Pouwels, Enger, Valk, Eds., 1985), which provides for replication and selection in E. co 1i and a yeast promoter-terminator module inserted between the Hindi11 and 3amHI sites of pBR322. The promoter is either a 431 base pair BamHI-Rsal fragment of CUP1 derived as a BamHI-EcoRI fragment from pYSK12 (Butt, et al., Proc.
Natl. Acad. Sci. USA 81:3332 (1984); Rosenberg et al·., Genetic Engineering 8:151 (1986); Gorman, et al., Gene 48:13 (1986)) or a 1.1 kb TDH3 promoter sequence (Holland, et al., J. Biol, Chem. 255:2596(1980)) derived as a BamHI-EcoRI fragment from plasmid pYSK18 (Rosenberg, et al., supra; Gorman, et al., supra). The terminator is a 361 base pair Kpnl-Hindlll fragment of the CYC1 gene
OBomav bad original (Smith, et al.. Cell 16:753 (1979)). Into the region between the promoter and the CYC1 fragment can be inserted various synthetic sequences as described below.
Construction of pYSK147 and pYSK148: Plasmids pY5K137 (CUPI promoter) and pYSK138 (TDH3 promoter) contain a synthetic oligonucleotide sequence between the EcoRI site at the 3' end of the promoter sequence and a Kpnl site at the 5' end of the terminator sequence. This synthetic sequence contains the unique restriction sites Xhol, Ncol and Sail upstream of translational termination codons in all three reading frames. The synthetic linker has the sequence:
GAATTCTCGAGCCATGGCCAGTCGACGTAGTTAAGTAGGTACC A Ncol-Sall fragment of plasmid pUCsT4, containing bases 124 through 1257 of the sCD-4 sequence was inserted into Ncol-Kpnl cut pYSK137 or pYSK138 to yield pYSKl47 and pYSK148 respectively.
Construction of pYSK154 and pYSK155: Vectors for ubiquitin fusion gene expression contain a casetts adapted synthetic yeast ubiquitin gene (Ecker, et al., J. 3 i ο 1. Chem. 262:3524(1987)) between the promoter and the CYC1 terminator. The ubiquitin sequence is identical to that published by Ecker, et al., except that the terminal AflII-ΚρηΙ fragment was replaced by an oligonucleotide sequence containing an Ncol restriction site at the 3'end. The Ncol-Kpnl fragment of pYSK147, containing the desired sCD-4 sequence was inserted between this Ncol site and the Kpnl site at the 5'end of the CYC1 fragment, to give pYSK154. A derivative of pYSK154, in which the sequence for the first seven amino-terminal amino acids of the sCD-4 sequence in pYSK154 (the leader peptide sequences) were deleted, was constructed by cleavage of pYSK154 with Kpnl, followed by fill-in with the Klenow fragment of
E.coli DNA polymerasel (polIK) and insertion of a KpnI-Xbal sCD-4 sequence (bases 145 through 1257 of sCD-4) from psT4BBViDHFR which had been treated with polIK to
BAD ORIGINAL fill-in the sticky ends. This plasmid is designated pYSK155.
Construction of pYSK159 and pYSK161: The vectors containing a truncated sCD-4 sequence (bases 124-603) were constructed by inserting a synthetic oligonucleotide sequence containing a termination codon at the Sacl site of the sCD-4 sequence (base 602). The synthetic linker (2x stranded) has the sequence:
CTAAGCGGC
TCGAGATTCGCCGGC
This synthetic sequence was inserted into Sacl and Narl cut pYSK143 and pYSK154 to give pYSK159 and pYSK161 respectively. Thus, the CD-4 DNA in pYSK159 has the codons for amino acids -9 (alanine) through 151 (leucine)(YV1).
Example 4: Expression of sT4 in yeast cultures.
Plasmid DNA (2-10 ug/ml) was used to transform yeast (Saccharomyces cerevisiae) using standard techniques (Sherman et al, Methods in Yeast Genetics, Cold Spring Harbor, 1986), selecting for tryptophan prototrophy. The strains employed were strain F762 (Mata, trplil, ura3-52) or PEC1-8B (Mata ,proAb: :URA3,ura3-52, trpl-289, his3). Cultures of selected transformants were grown in Yeast Nitrogen Base (YN3, Difco, Detroit, Michigan) containing supplements (2% glucose, 20 ug/ml uracil, ug/ml histidine). For plasmids utilizing the CUPl promoter, copper sulfate at 100 n\icromolar was included. Cultures were harvested in late log phase by centrifugation and were washed and broken. The cell lysate was analysed for sCD-4 by standard protein immunoblot assay.
In S. cerevisiae containing ~pYSK147 and pYSK148, the sCD-4 protein, SKBYsCD-4, (amino acids -9 to 369) was expressed at low levels (less than about 0.5 ng/1). The activity was found to be associated with the particulate
BAD ORIGINAL fraction, but could be readily solubilized by extraction with non-ionic detergents. The amount of SKBYsCD-4 (amino acids -9 to 369) in cultures of S. cerevisiae containing pYSK154 was between about 2 to about 6 mg/liter (at 2xl08 cells/ml). This was about a five-fold improvement over the amount of the CD-4 protein expressed with pYSK147 and pYSK148, i.e., without the presence of the stabilizing ubiquitin sequence. The estimated size of the sCD-4 protein synthesized was identical in all cases, indicating that the ubiquitin portion of the protein had been cleaved from SKBsCD-4. This was confirmed by immunoblotting procedures, using an antibody to yeast ubiquitin.
The levels of expression of the truncated sCD-4 proteins (YV1) in pYSK159 and pYSK161 were similar to that of the sCD-4 protein expressed as a ubiquitin fusion. The amount of sCD-4 detected was similar in each of the host strains examined.
SKBsYCD—4 from strain F762 containing pYSK154 was partially purified by passage through an S-Sepharose column. A crude extract, prepared in 10 mM Tris buffer, pH 6.0, 1% Tween-20, was centrifuged at 30,000xg. The supernatant was adjusted to pH 4.0 and was applied to an S-Sepharose column equilibrated in 50 mM acetate buffer. The sample was batch eluted with 50 mM MES (2-(N-morpholino)-ethanesulfonic acid], pH 6.0) buffer containing 0.5M NaCl. The presence of SK3YsCD-4 in the eluate was confirmed by immunoblot assay. The material was active as determined by a competition ELISA based assay, utilizing purified SK3sCD-4 from CHO cells and OKT4A antibody, suggesting that the conformation of the yeast derived SKBsYCD-4 mimics that of the mammalian ceil (CHO) derived material.
BAD ORIGINAL
Example 5: Construction of Streptomyces vectors
Using recombinant DNA manipulations, segments of the human CD-4 cDNA sequence were fused to the signal sequence of the S. longisporus trypsin inhibitor (LTI) gene and the S. lividans β-galactosidase (Bgal) gene. The sCD-4 minigenes were joined to Streptomyces plasmids pIJ702 (Katz, et al., supra) and pIJ351 (Kieser, et al., supra) to create plasmids pLTI:sT4/l, pLTI:sT4/7, pLTI:VlV2 and pBgal:sT4/7. The construction of the vectors was as follows.
Construction of pLTI:sT4/l: Plasmid pLTI:sT4/l was constructed from three other plasmids: pUCsT4, pIJ351 and pLTI450. The construction of plasmid pLTI450 is as follows :
Construction of pLTI450: A 0.92 kb Sacl-Kpnl fragment containing the LTI gene was inserted into pUC18 which had been digested with Sacl and Kpnl. This plasmid, pLTI520, was partially digested with Eagl and totally digested with Sail then ligated to a synthetic linker (2x stranded) which had Eagl and Sail ends:
5'-GGCCGCCGCCCCCGCG
CGGCGGGGGCGCAGCT-5’
AP 0 0 0 0 8 0
Plasmids obtained from this ligation were screened for insertion of the synthetic linker into the Eagl site located approximately 0.5 kb from the Sacl site. This Eagl site is located at base pair 86 with respect to the 5' end of the LTI gene. The resulting plasmid contains the LTI promoter and the coding sequence for the signal peptide and signal peptide cleavage site. Both the Eagl and Sail sites can be used to fuse sCD-4 minigenes to the LTI signal sequence.
Construction of pLTI:sT4/l: To create plasmid pLTI:sT4/l, the sCD-4 coding sequence was isolated on an approximately 1.1 kb 3bvl-?stl fragment from pUCsT4. This fragment contains base pairs 149-1257 of the human CD-4 cDNA bad ORIGINAL sequence. Plasmid p(JCsT4 was digested with Bbvi followed by treatment with reverse transcriptase to fill in the 5' protruding ends. The DNA was then digested with Pstl.
This 1.1 ib Bbvi(RT)-Pstl fragment, which encodes SKBsCD-4, was ligated to pLTl450 which had been treated with Sail and reverse transcriptase followed by Pstl digestion. This ligation resulted in plasmid pLTI450sT4/l. The final step in the construction of pLTI:sT4/l required the insertion of Streptomyces replication functions onto pLTI450sT4/l. This was accomplished by digesting pIJ351 (Kieser, et al., supra) with Pstl and ligating it to Pstl digested pLTI450sT4/l. Construction of pLTI:sT4/7: Plasmid pLTI:sT4/7 was constructed from three other plasmids: pUCsT4, pIJ702 and pLTl450. To create plasmid pLTI:sT4/7, the sCD-4 coding sequence was isolated on an approximately 1.1 kb Ncol-Pstl fragment from pUCsT4. This fragment contains base pairs 124-1257 of the human CD-4 cDNA sequence. These base pairs were placed between an ATG initiation codon and a TAA termination codon as previously described in Example 1. The initiation codon makes up part of the Heel recognition sequence. The sCD-4 coding sequence contained on this fragment contains 9 amino acids from the leader sequence of CD-4. pUCsT4 was treated with Ncol and reverse transcriptase followed by digestion with Pstl.
This fragment was then ligated with pLTI450 which had been treated with Hindi and Pstl. This ligation resulted in plasmid pLTl450sT4/7. The Streptomyces replicon was provided by plasmid pIJ702 (Katz, et al,, supra). It was inserted into pLTI450sT4/7 via the unique Pstl sites on both plasmids to create plasmid pLTI:sT4/7.
Construction of plasmid pLTI:V!V2: Plasmid pLTI:VlV2 was constructed from plasmids psT4.184, pLTI450 and pIJ351. A 0.54 kb Xbal-EcoRI fragment was isolated from psT4.184. This fragment was treated with Bbvi and reverse transcriptase. The Bbvi end corresponds to base pair 149
BAD ORIGINAL £ of the human CD-4 cDNA sequence. This blunt-ended fragment was then.ligated to pLTI450 which had been treated with Sail and reverse transcriptase to create plasmid pLTI450ViV2. The Streptomyces replication functions were provided by pIJ351. This plasmid was cloned into pLTI450ViV2 via the unique Pstl site on both pIJ351 and pLTI450VlV2. The resultant plasmid was pLTI:VlV2.
Construction of pGgalsT4/7: Plasmid p6galsT4/7 was constructed from plasmids p(JCsT4, pIJ702 and p3SSXMCP. p3SSXMCP is a pUC9 (Vieira and Messing, Gene 19:259(L982) derivative which contains the β-galactosidase promoter and signal sequence. Twenty-six base pairs downstream of the coding sequence for the signal peptide cleavage site is an XmnI site (Eckhardt, et al., J, Bacteriol.
169:4249(1987)). Inserted into this site was a synthetic linker which contains a BamHI recognition sequence (New England Biolabs, Beverly, Massachusetts) to generate plasmid p3SSX10. This vector was treated with BamHI and reverse transcriptase followed by Xhol digestion. Ligated to this vector was a fragment which had an Ncol end treated with reverse transcriptase to generate a blunt end and a Sail end. Ligation of the filled-in 3amHI site with the filled-in Ncol site recreated both the BamHI and Ncol sites. The resulting plasmid was p3SSXMCP. pUCsT4 was treated with Xbal and reverse transcriptase followed by Ncol digestion. This 1.1 kb Ncol-Xbal(RT) fragment was then inserted into p3SSXMCP which had been treated with Sacl and T4 DNA polymerase I followed by Ncol digestion. The Streptomyces replication functions were provided by pIJ702 which was inserted into p3SSXsT4 via the unique .Bgllt site on both .plasmids . The resulting plasmid was pBgalsT4/7. ...
ad η η ο o 8 0 bad original ( ,
Example 6: Expression of sCD-4 miniqenes in Streptomyces: Plasmids pLTI:sT4/l, pLTI:sT4/7, pLTI:VlV2 and pflgal:sT4/7 were transformed into S. lividans 1326 (Bibb, et al., supra). In addition, pLTI:sT4/l, pLTI:sT4/7, pLTI:VlV2 were introduced into S. coelicolor M124 (Hopwood, et a1., Genetic Manipulation of Streptomyces - A Laboratory Manual, F. Crowe & Sons, Ltd., Norwich, England (1985)), S. albus J1074 (Chater and Wilde, J. Gen. Microbiol. 116:323(1980)) and a white derivative of S. longisporus (ATCC accession number 23931) . All of the plasmids were introduced into the various hosts using the procedure previously described by Thompson, et al., J . Bacteriol. 151:668(1982). Transformants were selected by overlaying the transformation plates with 3ml of 0.4¾ agar containing 100 pg/ml thiostrepton.
The clones which expressed CD-4 minigenes were identified by propagating thiostrepton-resistant transformants in ten milliliters of trypticase soy broth plus 5 pg/ml thiostrepton for 48-72 hours. Culture supernatants and cell lysates were separated on a 12¾ polyacrylamide (30:0.8 acrylamide: bis) - 1¾ sodium dodecylsulfate gel then transferred to nitrocellulose (Towbiη, et al., Proc. Natl. Acad. Sci. USA
26.:4350(1979)). The nitrocellulose filter was probed using the rabbit sCD-4-antiserum as described by Deen, et al., supra.
The pLTI:sT4/l, pLTI:sT4/7 and pGgal:sT4 S. lividans transformants all expressed a protein of approximately 45kD which is the predicted size of the sCD-4 protein ' encoded by these plasmids. Similarly, the pLTI:7172 S. lividans transformants expressed a protein of approximately 20kD which is the predicted size of the 7172 protein. SK3sCD-4 and V1V2J4 expression was also examined in S. coelicolor, S. albus, and S. longisporus. Like S. lividans, proteins of 45 kD (the pLTI:sT4/l and pLTI:sT4/7 transformants) and 20 kD (the pLTI:VlV2 transformants) were expressed by the other Streptomyces species.
• - -a
BAD ORIGINAL
Subsequent quantitation of SKBsCD-4 present in the S. lividans culture supernatants and cell lysates showed levels of 1-5 mg/1. V1V2J4 was present at 2-10 mg/1 in both culture supernatants and cell lysates. Less than 1 mg/1 was expressed by the pflgal:sT4 S. lividans transformants.
Using a pLTI:sT4/7 S. lividans cell line, SKBsCD-4 expression has also been examined in a 12 liter fermentoc. Similar to the small scale expression studies, cells were grown in trypticase soy broth plus 5 pg/mi thiostrepton. Both culture supernatants and cell lysates were analyzed for SKBsCL-4 expression at 7.5, 24, 31.5, 54 and 72 hours after inoculation. The maximum volumetric expression level was 60 mg/1 and occurred at 24 hours after inoculation. The SKBsCD-4 was equally distributed between the culture supernatant and intact cells.
Partially purified supernatants containing V1V2J4 and SKBsCD-4 were shown by competition ELISA to bind OKT4A, indicating that these Streptomyces-derived proteins are HIV binding proteins .
The HIV binding protein, V1J4, was similarly ligated to the LTI promoter and shown by western assay to be expressed in S. lividans
The above Examples demonstrate that HIV binding proteins derived from CD-4, e.g., SKBsCD-4, SK3YsCD-4,
V1J4, V1V2J4 and YVl, which were expressed and secreted by the recombinant organisms of the invention are HIV binding proteins having the HIV binding function of sCD-4. More particularly, they have the HIV binding domain of the Vl region of SKBsCD-4.
The above description, .and Examples fully disclose the invention including preferred embodiments thereof. Modifications and improvements of the embodiments specifically disclosed herein are within the scope of the following claims.
AP 0 0 0 0 8 0

Claims (37)

  1. CLAIMS FOR: AUSTRALIA, CANADA, DENMARK, IRLAND, ISRAEL, JAPAN, MALAYSIA, NEW ZEALAND, OAPI, ESARIPO, PHILIPPINES, SOUTH AFRICA, SOUTH KOREA, TAIWAN AND ZIMBABWE.
    1. An E. coli expression vector comprising a coding sequence for a HIV binding protein operatively linked to a regulatory element.
  2. 2. The vector of claim 1 in which the HIV binding protein is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein.
  3. 3. The vector of claim 1 in which the HIV binding protein is SK3sCD-4 or a derivative thereof having the HIV binding function of SKBsCD-4.
  4. 4. The vector of claim 3 in which the HIV binding protein is selected from the group consisting of SKBsCD-4, V1J4 and V1V2J4.
  5. 5. The vector of claim 1, 2, 3 or 4 in which the regulatory element comprises a promoter and a leader sequence .
  6. 6. The vector of claim 5 in which the leader sequence is a OMPA leader sequence.
  7. 7. An E. coli transformed with the vector of any of claims 1 through 6.
  8. 8. A process for producing a HIV binding protein which comprises culturing E. coli cells which have been transformed with a vector comprising a coding sequence for the HIV binding protein operatively linked to a regulatory element and collecting the HIV binding protein therefrom.
    BAD ORIGINAL ft
  9. 9. A Streptomyces expression vector comprising a coding sequence for a HIV binding protein operatively linked to a regulatory element.
    5
  10. 10. The vector of claim 9 in which the HIV binding protein is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein.
  11. 11. The vector of claim 9 in which the HIV binding protein is SKBsCD-4 or a derivative thereof having the HIV binding function of SKBsCD-4.
  12. 12. The vector of claim 11 in which the HIV binding protein is selected from the group consisting of 15 SKBsCD-4, VIJ4 and V1V2J4.
  13. 13. The vector of claim 9, 10, 11 or 12 in which the regulatory element comprises a promoter and a leader sequence.
  14. 14. The vector of claim 13 in which the regulatory element is the Longisporus Trypsin Inhibitor promoter and leader sequence or the Streptomyces beta-galactosidase promoter and leader sequence.
  15. 15. A Streptomyces transformed with the vector of any of claims 9 through 12.
  16. 16. A Streptomyces transformed with the vector of
    30 , · claim 13.
  17. 17 A Streptomyces transformed with the vector of claim 14.
    35
  18. 18. The Streptomyces of claim 14 which is
    S. lividans.
    0 8 0 0 0 0 dV bad ORIGINAL t r<
    K* 1
  19. 19. The Streptomyces of claim 13 which is S.
    coelicolor, S. longisporus, S. lividans or S. albus.
  20. 20. A process for producing a HIV binding protein which comprises culturing Streptomyces cells which have been transformed with a vector comprising a coding sequence for the HIV binding protein operatively linked to a regulatory element and collecting the HIV binding protein therefrom.
  21. 21. A yeast expression vector comprising a coding sequencer a HIV binding protein operatively linked to a regulatory element.
    15
  22. 22. The vector of claim 21 which is a
    S. cerevisiae vector in which the HIV binding protein is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein.
  23. 23. The vector of claim 21 which is a
    S. cerevisiae vector in which the HIV binding protein is SKBsCD-4 or a derivative thereof having the HIV binding function of SKBsCD-4.
  24. 24. The vector of claim 23 in which the HIV binding protein is selected from the group consisting of SKBsYCD-4 and YV1.
  25. 25. The vector of claim 21, 22, 23 or 24 in which the regulatory element comprises a promoter and a leader sequence.
  26. 26. The vector of claim 21, 22, 23 or 24 in which the HIV binding protein coding sequence is fused at its 5'
    55 end to the 3' end of a coding sequence which stabilizes expression of the HIV binding protein.
    BAD ORIGINAL 1
  27. 27. The vector of claim 26 in which the coding sequence which stabilizes expression is the coding sequence for yeast ubiquitin.
    5
  28. 28. The vector of claim 27 in which the regulatory element is the CUP 1 promoter or the TDH3 promoter.
  29. 29. A yeast transformed with the vector of any of claims 21 through 24.
  30. 30. A yeast transformed with the vector of claim
    26 .
  31. 31. A Saccharomyces cerevisiae transformed with the vector of claim 27.
  32. 32. A Saccharomyces cerevisiae transformed with the vector of claim 28.
  33. 33. A process for producing a HIV binding protein which comprises culturing yeast cells which have been transformed with a vector comprising a coding sequence for the HIV binding protein operatively linked to a regulatory o c element and collecting the HIV binding protein therefrom.
  34. 34. An HIV binding protein which is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein and which is produced in recombinant E. coli.
  35. 35. A HIV binding protein which is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein and which is produced in Ί A J recombinant yeast cells.
    bad original £
  36. 36. A HIV binding protein which is a sCD-4 protein or a derivative thereof having the HIV binding function of a sCD-4 protein and which is produced in recombinant Streptomyces.
  37. 37. An E. coli expression vector for expressing exported proteins in E. coli which comprises a DNA coding sequence operatively linked to a regulatory element wherein the DNA coding sequence codes for the protein X-Y wherein X is an OMPA leader sequence and Y is a heterologous protein.
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