env Sequences of Simian Immunodeficiency Viruses from Chimpanzees in Cameroon Are Strongly Related to Those of Human Immunodeficiency Virus Group N from the Same Geographic Area

doi:10.1128/JVI.74.1.529-534.2000

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Journal of Virology, January 2000, p. 529-534, Vol. 74, No. 1
0022-538X/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

env Sequences of Simian Immunodeficiency Viruses from Chimpanzees in Cameroon Are Strongly Related to Those of Human Immunodeficiency Virus Group N from the Same Geographic Area

Sylvie Corbet,¹^, Michaela C. Müller-Trutwin,¹ Pierre Versmisse,¹ Severine Delarue,¹ Ahidjo Ayouba,² John Lewis,³ Soren Brunak,⁴ Paul Martin,² Françoise Brun-Vezinet,⁵ François Simon,⁵^,⁶ Françoise Barre-Sinoussi,¹^,^* and Philippe Mauclere²

Unité de Biologie des Rétrovirus, Institut Pasteur,¹ and Laboratoire de Virologie, Hôpital Bichat,⁵ Paris, France; Centre Pasteur du Cameroon, Yaoundé, Cameroon²; International Zoo Veterinary Group, Keighley, West Yorkshire, United Kingdom³; Center for Biological Sequence Analysis, Technical University of Denmark, Copenhagen, Denmark⁴; and CIRMF, Franceville, Gabon⁶

Received 24 May 1999/Accepted 22 September 1999

	ABSTRACT

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Human immunodeficiency virus type 1 (HIV-1) group N from Cameroon is phylogenetically close, in env, to the simian immunodeficiencyvirus (SIV) cpz-gab from Gabon and SIVcpz-US of unknown geographicorigin. We screened 29 wild-born Cameroonian chimpanzees and foundthat three (Cam3, Cam4, and Cam5) were positive for HIV-1 by Westernblotting. Mitochondrial DNA sequence analysis demonstrated thatCam3 and Cam5 belonged to Pan troglodytes troglodytes and thatCam4 belonged to P. t. vellerosus. Genetic analyses of the virusestogether with serological data demonstrated that at least oneof the two P. t. troglodytes chimpanzees (Cam5) was infected inthe wild, and revealed a horizontal transmission between Cam3and Cam4. These data confirm that P. t. troglodytes is a naturalhost for HIV-1-related viruses. Furthermore, they show that SIVcpzcan be transmitted in captivity, from one chimpanzee subspeciesto another. All three SIVcpz-cam viruses clustered with HIV-1N in env. The full Cam3 SIVcpz genome sequence showed a very closephylogenetic relationship with SIVcpz-US, a virus identified ina P. t. troglodytes chimpanzee captured nearly 40 years earlier.Like SIVcpz-US, SIVcpz-cam3 was closely related to HIV-1 N inenv, but not in pol, supporting the hypothesis that HIV-1 N resultsfrom a recombination event. SIVcpz from chimpanzees born in thewild in Cameroon are thus strongly related in env to HIV-1 N fromCameroon, demonstrating the geographic coincidence of these humanand simian viruses and providing a further strong argument infavor of the origin of HIV-1 being inchimpanzees.

	TEXT

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Human immunodeficiency virus type 1 (HIV-1) groups M, N, and O are considered to result from at least three independent introductionsof simian immunodeficiency virus (SIV) cpz from chimpanzees intothe human population (23). Four subspecies of chimpanzees arecurrently recognized: Pan troglodytes verus and P. t. vellerosusin West Africa, P. t. troglodytes in Central Africa, and P. t.schweinfurthii in East Africa (6, 17). The three SIVcpz virusesso far fully characterized originate either from P. t. troglodytes(SIVcpz-gab1 and SIVcpz-US) or from P. t. schweinfurthii (SIVcpz-ant)(4). SIVcpz-ant was isolated in former Zaire (19) and doesnot cluster within HIV-1 group M, N, or O (4). The closestrelatives of HIV-1 have been found in P. t. troglodytes, and ithas been suggested that this subspecies is the primary reservoirof HIV-1 (4). SIVcpz-gab1 was thus isolated from a wild P.t. troglodytes chimpanzee caught in Gabon (20), and is particularlyrelated to HIV-1 N in env (23). The more recently characterizedSIVcpz-US, from a P. t. troglodytes born in 1959 in an unknownCentral African country, is even more closely related to HIV-1N in env (4). It has been suggested that HIV-1 N arose throughancient recombination events between SIVcpz-US-related virusesand other SIVcpz strains in P. t. troglodytes, and subsequenttransmission to humans (4). If this is so, SIVcpz viruses phylogeneticallystrongly related to HIV-1 group N might circulate in the samegeographic area as group N viruses. All HIV-1 N viruses so farisolated originate from Cameroon (23). However, it is not knownwhether chimpanzees from Cameroon harbor SIVcpz viruses or whetherthese viruses are related to HIV-1. In addition, Cameroon is amajor epidemiological center of group O viruses, but SIV clusteringwith group O (or group M) has not been identified yet. This promptedus to screen wild-born chimpanzees from Cameroon in order to lookfor HIV-1-related viruses in theseapes.

The serological survey involved 29 wild-born chimpanzees that were rescued throughout Cameroon. All animals were screenedwith HIV-1 New Lav Blot kits (Sanofi-Pasteur, Paris, France).Three animals, Cam3, Cam4, and Cam5, were HIV-1-seropositive byWestern blotting (data not shown). These chimpanzees were recoveredin three distinct regions of Cameroon. Cam3 was found in 1992in a village near the southern border with Gabon. Cam4 was rescuedin 1992 in the southwestern province, near the border with Nigeria.Cam3 and Cam4 had estimated ages of 1 year and 2.5 years, respectively,at the time of rescue. They were housed together, first as petsand then, after November 1993, in the same enclosure at the WildlifeRescue Center in the southwestern province. Cam3 died suddenlyin 1998 with subacute pneumonia. Cam4 remained healthy, apartfrom episodes of fever and diarrhea. Cam5 was recovered in 1998in the central province of Cameroon at an age of less than 1 year,and was housed at Yaoundé Zoo. The mother was killed by hunters.Cam5 rapidly died with diarrhea after arriving at the zoo, andall the samples were obtained postmortem. None of the clinicalsigns observed in the animals could be associated with an acquiredimmunodeficiencysyndrome.

The sera of Cam3, Cam4, and Cam5 were further tested with a peptide-based enzyme immunoassay (EIA) (15). All three showedstrong cross-reactivity with SIVcpz-gab and HIV-1 N peptides (Table1), a pattern resembling that observed for sera from HIV-1 N-infectedpatients (23). The Cam5 serum was also strongly reactive withan HIV-1 group M Env peptide, possibly on account of the youngage at sampling (26).

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TABLE 1. Reactivity of the sera from three SIVcpz-infected chimpanzees of Cameroon with distinct V3 and gp41 reference peptides^a

Virus isolation was attempted by means of coculture with phytohemagglutinin-stimulated human peripheral blood mononuclearcells (PBMC) from HIV-negative blood donors (23). Virus productionwas detected after 9 days of culture in each case, confirmingthat all three chimpanzees wereinfected.

For Cam5 it was clear that the infection occurred in the wild since the sampling was performed immediately after its arrivalat the zoo. Cam3 and Cam4 were, however, housed in the same enclosurefor 5 years before being tested. We therefore sequenced both ahighly conserved fragment (178 bp of the integrase region in pol)and a variable genomic region (1,332 bp in env) of SIVcpz-cam3and SIVcpz-cam4, in order to determine their nucleotide diversity.SIVcpz-cam3 DNA was amplified from genomic DNA of 9-day PBMC cultures.Two long, overlapping fragments were separately amplified. Theprimers LSiGi-forward (positions 534 to 562 in SIVcpz-gab [23])and ZRT6-reverse (5'-ACCTGCCATCTGTTTTCCATAATC-3'; positions 5099to 5121) were used to amplify the 5' half, and ZRT4 (5'-AAAAGAAAAGGGGGGATTGGGGGGTACA-3';positions 4846 to 4873) and LSiGi-reverse (23) were used toamplify the 3' half. Five microliters of the primary PCR productwas submitted to a secondary PCR amplification with the followingprimer sets: LSiGi-forward and YRT1 (5'-GTATTITTATGGATTTTCIGGICCTATT-3'),LPBS (23) and ZRT6, ZRT4 and SK68 (5'-CCATAGTGCTTCCTGCTGC-3'),and ENV (5'-ATTCCIATACAITATTGTGCICCAGC-3') and ZU3' (5'-ACAGGCAGAAAGCAGCTGCTTATATGCA-3').Cycling conditions using a long PCR procedure (Elongase; Gibco-BRL)comprised a hot start (5 min at 94°C), then 35 cycles of denaturation(94°C for 30 s), annealing (55°C for 40 s), and elongation (68°Cfor 8 min), followed by a final elongation step (68°C for 2 to7 min). PCR products were purified and directly sequenced by usingthe ABI PRISM Big Dye Terminator Cycle Sequencing Ready Reactionkit with AmpliTaq FS DNA polymerase (Perkin-Elmer, Norwalk, Conn.)and an automated DNA sequencer (ABI-377A; Applied Biosystems).Serial SIVcpz-cam primers were synthesized to walk along the genomicfragments. For SIVcpz-cam4, genomic DNA from noncultured PBMCwas used for PCR. The pol fragment was amplified with the Hpolprimer set (3), and the env fragment was amplified by usingZRT6 sense and ZU3' as the outer primers and V3SJ (5'-GCCAATTCCAATACATTACTGTGC-3')and ENVas (5'-TATGTCAAACCAATTCCA-3') as the innerprimers.

We found very strong nucleotide identity between SIVcpz-cam3 and SIVcpz-cam4 (96.6 and 95.8% in pol and env, respectively),indicating that one of the animals had been infected by the otherin captivity. The serum of Cam3 showed strong reactivity againstall viral proteins in the Western blot assay, whereas the serumof Cam4 showed only weak reactivity, especially against the Poland Env proteins (data not shown), a situation typically encounteredin recent seroconvertors (10). These data suggested that itwas Cam3 that was infected in the wild and that infected Cam4in captivity. They demonstrate that captive chimpanzees can beinfected by SIVcpz, and that they can transmit SIV to other animalsin thecolony.

As the chimpanzees' sera showed strong serological cross-reactivity with HIV-1 peptides, in particular group N but also groupM peptides, we also compared the SIVcpz env sequences with thoseof HIV-1 M, N, and O. Previously described SIVcpz env sequences(4, 8, 27) were included in the comparative analysis.We used the same 1,332-bp env sequence used to study the relationshipbetween SIVcpz-cam3 and SIVcpz-cam4, because it spans the regionscoding for the V3 and gp41 peptides used in the EIA test. In addition,we determined the corresponding env sequence of the third chimpanzee(SIVcpz-cam5). The env fragment of SIVcpz-cam5 was amplified fromgenomic DNA of 9-day PBMC cultures with the same conditions asthose used for SIVcpz-cam4. Amino acid sequences were alignedwith the CLUSTAL W program to find the largest common overlap,and were then multiply aligned by the hidden Markov model in theSAM software package (9, 14). The shortest amino acid alignmentswith the fewest gaps were preferred and were corrected manually.The alignments were then backtranslated into codons by using theoriginal nucleotide sequences. Phylogenetic analyses were basedon both codon-based nucleotide and amino acid alignments. Treeswere constructed by the neighbor-joining method (21) as implementedby the CLUSTAL W program (25). Multiple substitutions were correctedby the Kimura method (13). Tree topologies were also inferredby using the Fitch-Margoliash, maximum parsimony, and maximumlikelihood methods with the FITCH, DNAPARS, and DNAML modulesof the PHYLIP software package, respectively (2). Trees werealso inferred by the maximum likelihood method implemented inPAUP4 (24). The empirical nucleotide frequencies were used,and transition-to-transversion ratios were set to 1.49, 1.5, and2.2 for env, gag, and pol, respectively. Substitution rates wereassumed to follow a gamma distribution with shape parameters estimatedby maximum likelihood. The gamma distribution shape parameterswere estimated to be 0.81, 0.55, and 0.46 for env, gag and pol,respectively. We used the Hasegawa-Kishino-Yano evolutionary modelwith rate heterogeneity (7). Estimating separate substitutionrates for each position in the codon yielded significantly decreasedlikelihoodvalues.

All three Cameroonian SIVcpz sequences clustered with SIVcpz-US and the HIV-1 N prototype strain YBF30 (Fig. 1a). The phylogeneticrelationship with HIV-1 N was supported by a remarkably high bootstrapvalue (99%). None of the three Cameroonian sequences was clearlyrelated to HIV-1 M or HIV-1 O. Interestingly, SIVcpz-cam3 andSIVcpz-cam5 were only slightly more closely related to each otherthan to SIVcpz-US, even though the latter had infected its hostnearly 40 years earlier (4).

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FIG. 1. Phylogenetic relationship of SIVcpz-cam with other members of the HIV-1 and SIVcpz lineage. Nucleotide sequences for all viruses but SIVcpz from Cameroon were obtained from the HIV data bank (http://hiv-web.lanl.gov/). HIV-1 N is represented by the YBF30 strain (23). Sites with gaps or unidentified nucleotides were stripped from the alignment. The trees were rooted with HIV-2 Rod. Trees based on the codon-based nucleotide alignments and constructed by the neighbor-joining method are shown. The percentages of concordant branching during bootstrapping in 10,000 resamplings are displayed at the branch nodes. The branch lengths are drawn to scale. The bar indicates a genetic distance of 0.1 (10% of nucleotide divergence). The neighbor-joining trees were consistent with those inferred by the Fitch-Margoliash, the maximum parsimony, and the maximum likelihood methods. Only minor variations in branch lengths were seen for the maximum likelihood trees. No significant differences in the trees based on the amino acids of Pol and Env were observed. (a) Phylogenetic relationship of SIVcpz-cam3, SIVcpz-cam4, and SIVcpz-cam5 with other members of the HIV-1 and SIVcpz lineage in a partial (1,332-bp) env fragment (from C2 to the ectodomain of gp41); (b) SIVcpz-cam3 phylogenetic relationships with other HIV-1 and SIVcpz viruses in the whole env gene (2,164 nucleotides included); (c) SIVcpz-cam3 phylogenetic relationships with other HIV-1 and SIVcpz viruses in the pol gene.

We then analyzed the full-length genome (9,155 bp) of one Cameroonian SIVcpz virus (SIVcpz-cam3) by using the sequence approachdescribed above. The SIVcpz-cam3 genome displayed the genomicorganization typical of SIVcpz and HIV-1. Analysis of deducedamino acid sequences indicated that all the genes studied potentiallyencoded functional proteins. The highest nucleotide identity wasalways observed with SIVcpz-US (83% in pol and 76% in env). Phylogeneticanalysis based on the entire gag, pol, and env genes confirmedthe clustering of SIVcpz-cam3 and SIVcpz-US throughout their genomes(Fig. 1 and data not shown). These data demonstrate that virusesclosely related to SIVcpz-US are currently circulating in wild-livingchimpanzees inCameroon.

The nucleotide identities of SIVcpz-cam3 with HIV-1 N and SIVcpz-gab were also high (respectively, 79 and 80% in pol and 73and 69% in env). We therefore scanned the HIV-1 N genome withthe recombinant identification program (Fig. 2 and data not shown).Significant similarity, as indicated by sites with statisticalconfidence above 90%, was observed between HIV-1 N YBF30 and SIVcpz-cam3in two short stretches in gag (99 sites in total), a 300-bp regionin vif, a short region in 5' env (V2, 130 bp), and a long fragmentin 3' env (1,210 bp). A long stretch of significant homology wastherefore found only in env. The regions of higher identity arevisualized in the similarity plot (Fig. 2). Phylogenetic analysisbased on the entire env gene confirmed the clear clustering ofSIVcpz-cam3 with HIV-1 N YBF30, with a highly significant bootstrapvalue (100%) (Fig. 1b). SIVcpz-cam3 and HIV-1 N YBF30 branchedtogether with the same high bootstrap value (100%) in the treesbased on the amino acid sequences of env (data not shown). Thebootstrap value for gag was lower (82% with the codon-based nucleotidealignment and <50% with the amino acid alignment [data not shown]).No such clustering was observed for pol (Fig. 1c); indeed, HIV-1N YBF30 rather formed an independent branch closely related toHIV-1 M, as previously reported (23). The clustering of HIV-1N with group M viruses in pol is supported by highly significantbootstrap values in the trees based on both nucleotide alignment(99%, Fig. 1c) and amino acid sequence alignment (98% [data notshown]). The different branching orders of HIV-1 N observed accordingto the gene analyzed could be explained by ancestral recombinationevents as previously suggested (4, 12).

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FIG. 2. Similarity plot comparing the sequence relationships of HIV-1 N YBF30 with SIVcpz-cam3 and HIV-1 and SIVcpz reference sequences. The similarity plot was obtained by using the Recombinant Identification Program (http://hiv-web.lanl.gov) (22). The search was made in windows of 400 bp, with a threshold of 90% for statistical confidence; gaps were stripped. Similarity plots were obtained using a codon-based alignment of concatenated full-length gag, pol, and env nucleotide sequences. The background alignment included SIVcpz-cam3 (black), SIVcpz-US (red), SIVcpz-gab (green), HIV-1 group M subtype B HXB2 (purple), and HIV-1 group O ANT70 (blue). The x axis shows the nucleotide position along the alignment. The y axis indicates the similarity index between the viral nucleotide sequences (0.1 = 10% similarity).

Since two distinct chimpanzee subspecies are present in Cameroon (6, 17), we determined the subspecies of Cam3, Cam4,and Cam5 by mitochondrial DNA (mtDNA) sequence analysis. DNA ofthe mitochondrial control region (D loop) was amplified from unculturedPBMC of Cam3 and Cam4. Previously described primers (1) wereused for PCR amplification and sequence determination of the PCRproduct. For Cam5, only genomic DNA from a 9-day coculture ofchimpanzee PBMC with human PBMC was available. We therefore designedprimers that specifically amplify either human or chimpanzee mtDNA.For amplification of chimpanzee mtDNA we designed the primersmtcpzs (5'-CCTAAGTATTGGCTTATTCATT-3') and mtcpzas (3'-CTATCTGAGGGGGGGCATCCG-3').Human mtDNA was amplified as a control with the primers mthums(5'-CCCAAGTATTGACTCACCCATC-3') and mthumas (5'-CTATCTGAGGGGGGTCATCCA-3').

Phylogenetic analysis of mtDNA from the three source chimpanzees in our study showed that two animals (Cam3 and Cam5) belongedto P. t. troglodytes (Fig. 3). The third seropositive chimpanzee(Cam4) did not cluster with P. t. troglodytes but with the P.t. vellerosus lineage (Fig. 3). This classification of Cam4 basedon the mtDNA sequence fits with the geographic origin of the chimpanzee(Southwest Cameroon). This is the first time that a West Africanchimpanzee has been shown to be infected by SIVcpz. Serologicaland genetic analysis suggest that Cam4 was infected by Cam3 incaptivity, although we cannot totally exclude that the virus crossedfrom Cam4 to Cam3. It is the first documented case of cross-subspeciestransmission of SIVcpz in captivity. As both apes were males,transmission might have occurred through biting, a common routeof lentivirus transmission in animals (18), and not by sexualcontact. These data also confirm that P. t. troglodytes is a naturalhost of HIV-1-related viruses, since Cam5, and maybe also Cam3,was infected in the wild (4). Both animals were captured ata very young age, as were all four other SIVcpz-infected chimpanzeesreported in the literature (4, 19, 20). As two of the 29infants tested here were apparently infected in the wild, theseroprevalence of SIVcpz in free-living adult chimpanzees mayindeed be higher than previously assumed (4).

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FIG. 3. Phylogenetic tree of mtDNA (D loop) sequences. The trees constructed by the Fitch-Margoliash method are shown. The transition/transversion ratio was set to 10. For clarity, only bootstrap values over 50% are shown. Previously described chimpanzee mtDNA sequences were included (4, 6, 17). The three chimpanzees of this study together with the four other chimpanzees reported to carry SIVcpz (4, 11, 19, 20) are boxed. Brackets on the right indicate chimpanzee subspecies as previously proposed (6, 17).

An important implication of this study is that the area of HIV-1 N endemicity coincides with the natural habitat of chimpanzeescarrying HIV-1 N-related SIVcpz, providing the most persuasiveevidence that SIVcpz is the evolutionary ancestor of HIV-1.

The similarity between SIVcpz from P. t. troglodytes and HIV-1 N was, however, only seen in env. HIV-1 N therefore most likelyresulted from an ancestral recombination event between virusesrelated to SIVcpz-cam/US and HIV-1 M (4). The recombinationprobably occurred in a chimpanzee (4), although one cannotentirely exclude the possibility that it occurred in a human.Only the discovery of such a recombinant virus in chimpanzeesor of an HIV-1 N virus related to SIVcpz-cam/US throughout itsgenome can settle the matter. Additional HIV-1 N and SIVcpz sequencesare needed to determine in which species and where exactly inthe genome recombination tookplace.

HIV-1 groups M, N, and O are all circulating in Cameroon (16). It is therefore surprising that all Cameroonian SIVcpz sequencesso far identified show a particular relationship with HIV-1 N,but not with HIV-1 M, as the latter has a considerably higherprevalence than N and O in Cameroon (16). It is also surprisingthat none is related to HIV-1 group O, as Cameroon is currentlythe epidemiological center of this group (16). The possibilitythat HIV-1 derives from species other than chimpanzees is unlikely,but it cannot be totally ruled out. Another explanation mightbe that group M- and group O-related viruses no longer exist inchimpanzees. Studies of wild-born chimpanzees are too limitedto exclude, however, the presence of HIV-1 M- or O-related virusesin animals of other geographic regions or in subspecies distinctfrom P. t. troglodytes. The existence of divergent viruses (SIVcpz-gaband SIVcpz-cam/US) within chimpanzees of the same subspecies (P.t. troglodytes) but from distinct geographic origins, as wellas the presence of the highly divergent SIVcpz-ant in anothersubspecies of East Africa (P. t. schweinfurthii), indicates indeedthat chimpanzees in Eastern and Central Africa may harbor a broadspectrum of SIVcpz-type viruses. West African chimpanzees mightharbor SIVcpz as well. Indeed, we report here on a case of cross-subspeciestransmission between a Central and a West African chimpanzee incaptivity. As both subspecies occur in Cameroon, it is easilyconceivable that such transmissions occurred in the past betweenwildanimals.

Although HIV-1 group M- and O-related viruses have not been identified yet in chimpanzees (or in any other nonhuman primatespecies), these African apes are clearly the best candidates forexplaining the origin of HIV-1. HIV-2, as is generally agreed,originates from SIVsm present in a West African nonhuman primate,the sooty mangabey (5). The ancestors of SIVcpz and SIVsm,in contrast, are still totally unknown. The reservoir of SIVcpzand SIVsm (if it still exists) would be a further key to understandingthe origin of these primatelentiviruses.

In conclusion, we demonstrate that SIVcpz and closely related HIV-1 viruses currently cocirculate in both wild chimpanzeesand humans from the same geographic area, providing a furtherstep towards the missing link between HIV-1 and related virusesin nonhumanprimates.

Nucleotide sequence accession numbers. SIVcpz-cam sequences have been deposited at the GenBank database under accession no. AF115393 to AF115395 and AF135498.Mitochondrial sequences of Cam3, Cam4, and Cam5 have been depositedat the GenBank database under accession no. AF13495 to AF135497.

	ACKNOWLEDGMENTS

We are grateful to P. Jenkins, L. Gadsby, A. Randall, and P. Gleason (Pandrillus association) for their collaboration at theLimbe Wildlife Rescue Center, to C. Mitchell at the Yaoundé Zoo,and to E. Nerrienet at the Centre Pasteur in Yaoundé, Cameroon.We thank J. Mfoupouendoun, E. Tina Abada, and S. Souquières forexpert technical assistance, and C. Rapacki and H. H. Staerfeldt(Center for Biological Sequence Analysis, Technical Universityof Denmark) for their precious support. We are indebted to D.L. Swofford for providing the latest update of PAUP (version 4.062).We thank J. Felsenstein, E. Holmes, and D. L. Swofford for helpfuldiscussions. We thank D. Young for checking theEnglish.

This work was supported by the French National Agency for AIDS research (ANRS) and the Danish National Research Foundation.M.C.M.-T. was the recipient of a SIDAction fellowship, and A.A.had a fellowship from the French Ministry ofCooperation.

	FOOTNOTES

^* Corresponding author. Mailing address: Unité de Biologie des Rétrovirus, Département de Virologie, 25, rue du Dr Roux,75724 Paris Cédex 15, France. Phone: 33 1 45 68 87 30. Fax: 331 45 68 89 57. E-mail: fbarre{at}pasteur.fr.

Present address: Statens Serum Institut, 2300 Copenhagen S,Denmark.

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18. Nérrienet, E., X. Amouretti, M. C. Müller-Trutwin, V. Poaty-Mavoungou, I. Bedjebaga, H. Thi Nguyen, G. Dubreuil, S. Corbet, E. J. Wickings, F. Barré-Sinoussi, A. J. Georges, and M.-C. Georges-Courbot. 1998. Phylogenetic analysis of SIV and STLV type I in mandrills (mandrillus sphinx): indications that intracolony transmissions are predominantly the result of male-to-male aggressive contacts. AIDS Res. Hum. Retrovir. 14:785-796[Medline].

19. Peeters, M., K. Fransen, E. Delaporte, M. van den Haesevelde, G. Gershy-Damet, L. Kestens, G. van der Groen, and P. Piot. 1992. Isolation and characterization of a new chimpanzee lentivirus (simian immunodeficiency virus isolate cpz-ant) from a wild captured chimpanzee. AIDS 6:447-451[Medline].

20. Peeters, M., C. Honore, T. Huet, L. Bedjabaga, S. Ossari, P. Bussi, R. W. Cooper, and E. Delaporte. 1989. Isolation and partial characterization of an HIV-related virus occurring naturally in chimpanzees in Gabon. AIDS 3:625-630[Medline].

21. Saitou, N., and M. Nei. 1987. The neighbor-joining method: a new method for reconstructing phylogenetic trees. Mol. Biol. Evol. 4:406-425[Abstract].

22. Siepel, A. C., and B. Korber. 1995. Scanning the database for recombinant HIV-1 genomes. Los Alamos National Laboratory, Los Alamos, N.Mex

23. Simon, F., P. Mauclère, P. Roques, I. Loussert-Ajaka, M. C. Müller-Trutwin, S. Saragosti, M.-C. Georges-Courbot, F. Barré-Sinoussi, and F. Brun-Vézinet. 1998. Identification of a new human immunodeficiency virus type 1 distinct from group M and group O. Nat. Med. 4:1032-1037[CrossRef][Medline].

24. Swofford, D. L. 1984. Phylogenetic analysis using parsimony (PAUP). Illinois Natural History Survey, Champaign

25. Thompson, J. D., D. G. Higgins, and T. J. Gibson. 1994. CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Res. 22:4673-4680[Abstract/Free Full Text].

26. Turbica, I., F. Simon, J. M. Besnier, B. LeJeune, P. Choutet, A. Goudeau, and F. Barin. 1997. Temporal development and prognostic value of antibody response to the major neutralizing epitopes of gp120 during HIV-1 infection. J. Med. Virol. 52:309-315[CrossRef][Medline].

27. Vanden Haesevelde, M. M., M. Peeters, G. Jannes, W. Janssens, G. van der Groen, P. M. Sharp, and E. Saman. 1996. Sequence analysis of a highly divergent HIV-1-related lentivirus isolated from a wild captured chimpanzee. Virology 221:346-350[CrossRef][Medline].

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19.	Peeters, M., K. Fransen, E. Delaporte, M. van den Haesevelde, G. Gershy-Damet, L. Kestens, G. van der Groen, and P. Piot. 1992. Isolation and characterization of a new chimpanzee lentivirus (simian immunodeficiency virus isolate cpz-ant) from a wild captured chimpanzee. AIDS 6:447-451[Medline].
20.	Peeters, M., C. Honore, T. Huet, L. Bedjabaga, S. Ossari, P. Bussi, R. W. Cooper, and E. Delaporte. 1989. Isolation and partial characterization of an HIV-related virus occurring naturally in chimpanzees in Gabon. AIDS 3:625-630[Medline].
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23.	Simon, F., P. Mauclère, P. Roques, I. Loussert-Ajaka, M. C. Müller-Trutwin, S. Saragosti, M.-C. Georges-Courbot, F. Barré-Sinoussi, and F. Brun-Vézinet. 1998. Identification of a new human immunodeficiency virus type 1 distinct from group M and group O. Nat. Med. 4:1032-1037[CrossRef][Medline].
24.	Swofford, D. L. 1984. Phylogenetic analysis using parsimony (PAUP). Illinois Natural History Survey, Champaign
25.	Thompson, J. D., D. G. Higgins, and T. J. Gibson. 1994. CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Res. 22:4673-4680[Abstract/Free Full Text].
26.	Turbica, I., F. Simon, J. M. Besnier, B. LeJeune, P. Choutet, A. Goudeau, and F. Barin. 1997. Temporal development and prognostic value of antibody response to the major neutralizing epitopes of gp120 during HIV-1 infection. J. Med. Virol. 52:309-315[CrossRef][Medline].
27.	Vanden Haesevelde, M. M., M. Peeters, G. Jannes, W. Janssens, G. van der Groen, P. M. Sharp, and E. Saman. 1996. Sequence analysis of a highly divergent HIV-1-related lentivirus isolated from a wild captured chimpanzee. Virology 221:346-350[CrossRef][Medline].