A Specific Region of 37 Amino Acid Residues in the
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病菌学杂志 2005年第14期
Department of Viral Infections, Research Institute for Microbial Diseases, Osaka University, Osaka
BioResource Center, RIKEN Tsukuba Institute, Tsukuba
Toyama Institute of Health, Toyama, Japan
ABSTRACT
Human immunodeficiency virus type 1 (HIV-1) efficiently enters cells of Old World monkeys but encounters a block before reverse transcription. This restriction is mediated by a dominant repressive factor. Recently, a member of the tripartite motif (TRIM) family proteins, TRIM5, was identified as a blocking factor in a rhesus macaque cDNA library. Among Old World monkey cell lines, the African green monkey kidney cell line CV1 is highly resistant to not only HIV-1 but also simian immunodeficiency virus SIVmac infection. We analyzed TRIM5 of CV1 cells and HSC-F cells, a T-cell line from a cynomolgus monkey, and found that both CV1- and HSC-F-TRIM5s could inhibit CD4-dependent HIV-1 infection, as well as vesicular stomatitis virus glycoprotein-mediated infection. CV1-TRIM5 could also inhibit SIVmac infection, whereas HSC-F-TRIM5 could not. In the SPRY (B30.2) domain of CV1-TRIM5, there was a 20-amino-acid duplication that was not present in HSC-F-TRIM5. A chimeric TRIM5 containing 37 amino acid residues from CV1-TRIM5, which spanned the 20-amino-acid duplication, in the background of HSC-F-TRIM5 fully gained the ability to inhibit SIVmac infection. Conversely, the mutant CV1-TRIM5 lacking the 20-amino-acid duplication completely lost the ability to restrict SIVmac infection. These findings clearly indicated that a specific region of 37 amino acid residues in the SPRY domain of CV1-TRIM5 contained a determinant of species-specific restriction of SIVmac.
INTRODUCTION
Human immunodeficiency virus type 1 (HIV-1) is thought to have been introduced into the human population from chimpanzees (9) and shows a very narrow host range limited only to humans and chimpanzees. HIV-1 does not experimentally infect Old World monkeys, such as rhesus and cynomolgus monkeys, and fails to replicate in activated CD4-positive T lymphocytes obtained from these monkeys (13, 31). In contrast, simian immunodeficiency virus (SIV) isolated from a macaque monkey (SIVmac) can replicate well in rhesus (13, 31) and cynomolgus monkeys (2, 3). The restricted host range of HIV-1 has greatly hampered its use in animal experiments and, hence, caused difficulty in developing prophylactic vaccines against HIV-1 infection.
Several studies have suggested that the block of HIV-1 replication in Old World monkey cells occurred at a postentry step (7, 13, 31) and appeared to result from a failure to initiate reverse transcription (13). The block was still observed when CD4-negative monkey cells were infected with HIV-1 pseudotyped with vesicular stomatitis virus glycoprotein (VSV-G) and was overridden by a high multiplicity of infection (MOI) with VSV-G-pseudotyped virus or virus-like particles lacking genomic RNA (5, 10, 16, 19). Importantly, resistance against HIV-1 infection was shown to be dominant in heterokaryons between human and Old World monkey cells, suggesting the presence of inhibitory factor(s) against HIV-1 infection in Old World monkey cells (19). Studies on chimera of HIV-1 and SIVmac have suggested that restriction determinants lie within the HIV-1 P24 capsid protein (CA) (11, 23, 24, 29).
Recently, the screening of a rhesus monkey cDNA library identified tripartite motif 5 (TRIM5), a component of cytoplasmic bodies, as a factor that confers resistance to HIV-1 infection (33). Shortly after, TRIM5 of African green monkey, another Old World monkey, was also shown to restrict HIV-1 infection, whereas human TRIM5 was reported to restrict N-tropic murine leukemia virus (12, 14, 25, 36).
An African green monkey kidney cell line, CV1, was shown to be highly resistant to SIVmac infection, as well as to HIV-1 infection. We analyzed TRIM5 of CV1 cells and HSC-F cells, a T-cell line from a cynomolgus monkey, and report here that the ability of CV1-TRIM5 to suppress SIVmac infection was determined by a small region composed of 37 amino acid residues in the SPRY (B30.2) domain of CV1-TRIM5.
MATERIALS AND METHODS
Cloning and expression of TRIM5. TRIM5 cDNA was amplified by reverse transcription-PCR from the human T-cell line MT4, cynomolgus monkey T-cell line HSC-F (2, 3), and African green monkey cell lines CV1 and Vero by using 5'-GCGGCCGCTACTATGGCTTCTGG-3' as a forward primer and 5'-GAATTCTCAAGAGCTTGGTGA-3' as a reverse primer. Amplified products were then cloned into the vector pCR-2.1TOPO (Invitrogen), and the nucleotide sequence of 10 clones for each TRIM5 was determined.
The entire coding regions of selected clones were transferred to pcDNA3.1 (Invitrogen) by using NotI and EcoRI sites, which were introduced by primers used in the PCR step. Hamster TK-ts13 cells (4) were transfected with pcDNA3.1 carrying TRIM5 cDNA and cultured in the presence of 0.75 mg of G418 (Gibco)/ml for 14 days. The colonies obtained were examined for the expression of TRIM5 by using the TaqMan PCR method according to the manufacturer's instructions (Applied Biosystems). Sequences of the probe and primers used to specifically detect each TRIM5 were as follows: MT4-TRIM5, forward primer (5'-AACCTGGAGAAGGAGGAGGAAGAC-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TCAGTTTCAGAGTTCG-TAMRA-3'); HSC-F-TRIM5, forward primer (5'-AACCTGGAGAAGGAGAAAGAAGAC-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TTCGTTTCAGACTTTG-TAMRA-3'); and CV1-TRIM5, forward primer (5'-AACCTGGAGAAGGAGGAAGAAGA-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TCCGTTTCAGACTTCG-TAMRA-3'). These primers amplify the coiled-coil region of TRIM5 genes. Plasmid DNA used for transfection served as a standard to determine the number of copies of TRIM5 transcripts. The parental TK-ts13 cells were totally negative for the primate TRIM5 expression. Clones expressing each TRIM5 at comparable levels (ca. 4 to 6 x 107 copies/μg of total RNA) were used for subsequent experiments.
To generate CV1-TRIM5 and HSC-F-TRIM5 cDNAs carrying a hemagglutinin (HA) tag (YPYDVPDYAA) at their C termini, cloned CV1-TRIM5 and HSC-F-TRIM5 cDNAs in pcDNA3.1 were used as templates for PCR amplification with a primer containing a nucleotide sequence corresponding to the HA tag fused with the C-terminal portion of TRIM5. The C-terminal portion of TRIM5 fused with the HA tag (BamHI to NotI) and the N-terminal portion of TRIM5 (NotI to BamHI) were assembled on a pCEP4 vector (Invitrogen). To generate chimeric TRIM5 HSC-F+60tag, the 182-bp SphI-BamHI fragment of HSC-F-TRIM5-tag was replaced with the corresponding 242-bp SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. Conversely, the 242-bp SphI-BamHI fragment of CV1-TRIM5 was replaced with the 182-bp SphI-BamHI fragment of HSC-F-TRIM5-tag in the background of CV1-TRIM5-tag to generate CV1-60tag. PCR-based mutagenesis of HSC-F-TRIM5-tag was performed to generate HSC-delete-tag, which possessed the 5'-proximal 84 bp of the SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag, and HSC-insert-tag, which possessed 3'-proximal 158 bp of the SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. Similarly, CV1-delete-tag, which possessed the 3'-proximal 98 bp of the SphI-BamHI fragment of HSC-F-TRIM5 in the background of CV1-TRIM5-tag, was generated by a PCR-based mutagenesis of CV1-TRIM5-tag. The entire coding sequences of these TRIM5-tags were then transferred to the NotI site of pSeV18+b(+). Recombinant Sendai viruses (SeVs) carrying various TRIM5-tags were recovered according to a previously described method (32). The viruses passaged a second time in embryonated chicken eggs were used as stock for all experiments. The wild-type Z strain of SeV served as a control in all of the experiments.
To establish human cell lines which constitutively express primate TRIM5s or their chimeras, human osteosarcoma C143 cells were transfected with pCEP4 containing cDNA of CV1-TRIM5-tag, HSC-F-TRIM5-tag, CV1-60tag, or HSC-F+60tag, and cells were cultured in the presence of 0.3 mg of hygromycin B (Gibco)/ml for 14 days.
Immunoprecipitation and Western blot analysis. When we performed Western blot analysis of cells expressing HA-tagged TRIM5 proteins, we consistently observed nonspecific binding of anti-HA antibody to a protein that comigrated with HSC-F-TRIM5. Therefore, we analyzed the expression of each HA-tagged TRIM5 protein in the hygromycin B-resistant C143 cells or MT4 cells infected with recombinant SeVs by immunoprecipitation, followed by Western blot analysis as described previously (20) to reduce nonspecific background. Briefly, cell lysate was first adsorbed with protein A-agarose before the addition of anti-HA antibody to avoid nonspecific protein binding to protein A-agarose. TRIM5 proteins in the cell lysate were then precipitated with anti-HA high-affinity rat monoclonal antibody (Roche) by using a protein A-immunoprecipitation kit (Roche). Precipitated materials were subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis on a 4 to 12% NuPAGE Bis-Tris gel (Invitrogen). Proteins in the gel were then electronically transferred to a polyvinylidene difluoride membrane (Immobilon; Millipore). Blots were blocked and probed with anti-HA antibody overnight at 4°C and then incubated with peroxidase-conjugated anti-rat immunoglobulin G (American Qualex) and developed by using the Immun-Star HRP chemiluminescence kit (Bio-Rad). Visualized image was recorded by LAS1000 (Fuji) and quantified by ImageGauge (Fuji). At least three independent experiments were performed, and the means and standard deviations (SD) for the data were calculated.
Viruses and HIV-1 lentivirus vector. VSV-G-pseudo typed HIV-1-NL43, SIVmac239, or HIV-2-GH123 was prepared by transfection of 293T cells with a combination of pMD.G (17, 18) and pNL432 (1), pBRmac239 (15), or pGH123 (30), respectively. HIV-1 vector expressing green fluorescence protein (GFP) was prepared as described previously (17, 18). Two days after transfection, culture supernatants of 293T cells were collected and assayed for reverse transcriptase activity using a reverse transcriptase colorimetric assay (Roche).
Viral infection. Assays for the HIV-1 vector expressing GFP were performed in 24-well plates containing 4 x 104 Tk-ts13-derived target cells. Serially diluted VSV-pseudotyped HIV-1 vectors encoding GFP were inoculated, and infected cells were enumerated by using a flow cytometer (FACScan; Becton Dickinson) 40 h after infection. For VSV-pseudotyped HIV-1, SIVmac239, and HIV-2 infection assays, we inoculated viruses containing 1 ng of reverse transcriptase into 4 x 104 C143 cells. For CD4-dependent infection assays, 2.5 x 105 MT4 cells were infected with SeV expressing CV1-TRIM5-tag, HSC-F-TRIM5-tag, or the parental Z strain of SeV at a MOI of 10 PFU per cell, followed by incubation at 37°C for 9 h. Cells were then superinfected with 30 ng of p24 of an X4 HIV-1 strain, NL43, or 30 ng of p27 of SIVmac239. The culture supernatants were collected periodically, and the level of p24 or p27 was measured by using a RETROtek antigen ELISA kit (ZeptoMetrix).
Data deposition. The sequences described here have been deposited in the GenBank database under accession numbers AB210050 to AB210052.
RESULTS
Variation in TRIM5. We cloned TRIM5 cDNA from the human T-cell line MT4, cynomolgus monkey T-cell line HSC-F, and African green monkey kidney cell lines CV1 and Vero. The predicted amino acid sequences of TRIM5s are compared in Fig. 1A and B.
Human TRIM5 from MT4 cells differed at an amino acid position 249 (G249D) from the previously published sequence (33) and was designated MT4-TRIM5. The cynomolgus monkey TRIM5 from HSC-F (HSC-F-TRIM5) was two amino acids shorter than the rhesus monkey TRIM5 (33) and two amino acids longer than the human TRIM5. All 10 clones derived from Vero cells had the same sequence as the previously published one (36). On the other hand, we found at least two distinct TRIM5 sequences in CV1 cells. The two major TRIM5 sequences obtained from CV1 were designated CV1-TRIM5-type1 and CV1-TRIM5-type2, and five amino acids were found to differ between the two sequences (I259V, L337S, R351L, G359R, and G438S). Among 10 cDNA clones obtained from CV1, there were four type 1 clones and four type 2 clones. The remaining two clones were most likely chimeric artifacts. Two recently published sequences of TRIM5 from CV1 cells (AY593973 and AY625002) showed differences at three positions—L7V, I259V, and G438S—and have S, L, and R at positions 337, 351, and 359, respectively (14, 36), whereas both the type 1 and 2 clones had leucines at the seventh position. All sequences obtained from Vero and CV1 contained a 20-amino-acid duplication within the SPRY domain, which was not observed in human MT4 and cynomolgus monkey HSC-F (Fig. 1B).
The phylogenetic tree of various TRIM5 sequences showed that cynomolgus and rhesus monkey TRIM5s are similar to each other, a finding consistent with the fact that these two monkeys belong to the genus Macaca (Fig. 1C).
African green monkey and cynomolgus monkey TRIM5 inhibit HIV-1 infection in nonprimate cells. We first sought to determine whether or not each TRIM5 can inhibit HIV-1 infection in the context of nonprimate cells because human and primate cells express endogenous TRIM5 that could complicate a functional analysis of TRIM5-mediated restriction. The hamster cell line TK-ts13 was used, because it is very susceptible to a VSV-G-pseudotyped, HIV-1-based GFP-expressing lentivirus vector, HIV-1-GFP. Cell clones stably expressing MT4-, CV1-, and HSC-F-TRIM5 were selected according to the method described in Materials and Methods. The levels of expression of TRIM5 were determined by using a real-time PCR, and cells expressing comparable amounts of TRIM5 (4 x 106 to 6 x 106 copies/μg of total RNA) were used for subsequent study. Restriction can be quantified by comparing the percentage of GFP-positive cells with or without TRIM5.
As can be seen in Fig. 2A, MT4-TRIM5 had a very weak anti-HIV-1 effect (1.2-fold), a finding consistent with a previous study (33). In contrast, restriction of HIV-1 was clearly evident over a wide range of initial MOIs in cells expressing HSC-F-TRIM5, CV1-TRIM5-type1, and CV1-TRIM5-type2 (ca. 5- to 10-fold). There was no significant difference between CV1-TRIM5-type1 and type2; therefore, we chose CV1-TRIM5-type1 to be representative of CV1-TRIM5 in the subsequent experiments. We obtained the same results as described above when we used an HA-tagged version of TRIM5 (data not shown).
African green monkey and cynomolgus monkey TRIM5 inhibit CD4-dependent HIV-1 infection in human cells. To test the restriction properties of TRIM5 in CD4-dependent HIV-1 infection, we constructed a recombinant SeV expressing TRIM5 fused with the HA tag in the C-terminal of HSC-F-TRIM5 or CV1-TRIM5 (HSC-F-TRIM5-tag SeV or CV1-TRIM5-tag SeV). Human T-cell line MT4 cells were first infected with the SeV expressing TRIM5-tag (Fig. 2B), incubated at 37°C for 9 h, and then infected with an X4-tropic HIV-1 strain NL43. As can be seen in Fig. 2C, both HSC-F-TRIM5-tag and CV1-TRIM5-tag completely inhibited HIV-1 replication, whereas MT4 cells infected with SeV empty vector fully supported HIV-1 replication.
Distinct patterns of restriction for SIVmac among nonhuman primate TRIM5. In African green monkey CV1 cells, both HIV-1 and SIVmac239 were restricted, whereas only HIV-1 was restricted in cynomolgus monkey HSC-F cells (Fig. 3A). Therefore, we examined whether or not CV1-TRIM5 also could inhibit the replication of SIVmac. In MT4 cells infected with recombinant SeV expressing HSC-F-TRIM5-tag, the replication of SIVmac239 was not suppressed at all (Fig. 3B), indicating that the HSC-F-TRIM5 showed a similar specificity to rhesus monkey TRIM5 (33). In MT4 cells infected with recombinant SeV expressing CV1-TRIM5-tag, in contrast, the replication of SIVmac239 was completely suppressed. These results suggested that the distinct sensitivity of African green monkey and cynomolgus monkey cells to HIV-1 and SIVmac infection was, at least partly, determined by TRIM5.
A small region of 37 amino acid residues in the SPRY domain of CV1-TRIM5 determines SIVmac restriction. A comparison of the human and nonhuman primate TRIM5 sequences showed the presence of a highly variable region in the N-terminal portion of the SPRY domain (Fig. 1A and B). In this region, CV1 and Vero TRIM5 had a 20-amino-acid repetition that was totally absent in HSC-F-TRIM5. These findings prompted us to test whether this highly variable region of TRIM5 determined the species-specific inhibition of SIVmac infection. We constructed chimeric TRIM5s from HSC-F-TRIM5-tag and CV1-TRIM5-tag by using SphI and BamHI restriction enzyme digestion (Fig. 4A). HSC-F+60tag contained the 242-bp fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. The reciprocal chimera, CV1-60tag, contained a 182-bp fragment of HSC-F-TRIM5 in the background of the CV1-TRIM5-tag. In this fragment, the differences between CV1 and HSC-F TRIM5, including the 20-amino-acid repetition, were located in a small region of 37 amino acid residues (Fig. 1B). Human osteosarcoma C143 cells stably expressing various TRIM5s (Fig. 4B) were infected with VSV-G-pseudotyped HIV-1 NL43, and levels of P24 in the culture supernatants were assayed periodically. As expected, both chimeric TRIM5s and parental TRIM5s clearly inhibited the replication of HIV-1 NL43 (Fig. 4C). When these cells were infected with VSV-G-pseudotyped SIVmac239, the parental CV1-TRIM5-tag could also inhibit the replication of SIVmac239, whereas CV1-60tag, which contained the 182-bp fragment of HSC-F-TRIM5 in the background of CV1-TRIM5-tag, could not. Conversely, the parental HSC-F-TRIM5-tag did not inhibit the replication of SIVmac239 at all, whereas HSC-F+60tag, which contained the 242-bp fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag, clearly inhibited SIVmac239 (Fig. 4C). We obtained the same results as described above when we used SeVs to express parental TRIM5-tag or chimeras (Fig. 4D). These results indicated that the determinant of the species-specific inhibition of SIVmac239 replication is located in 37 amino acid residues in the SPRY domain of CV1-TRIM5.
To narrow the SIVmac restriction determinant more precisely, we generated two more chimeric TRIM5s (Fig. 4A). HSC-delete-tag contained a CV1-derived 17-amino-acid fragment without the 20-amino-acid duplication in the background of the HSC-TRIM5-tag. HSC-insert-tag contained the HSC-F-derived 17-amino-acid fragment with the CV-1 derived 20-amino-acid duplication in the background of HSC-TRIM5-tag. Recombinant SeVs expressing these chimeric TRIM5s were generated and used in the subsequent experiments. Although the expression levels of mRNA of each chimericTRIM5 was virtually identical to each other (data not shown), we observed considerable variations in the levels of TRIM5 protein expression among chimeras (Fig. 4E). The HSC-delete-tag showed slightly higher levels of protein expression than those of HSC-F+60tag. However, HSC-delete-tag failed to inhibit SIVmac replication, whereas it restricted HIV-1 replication as completely as HSC-F+60tag did (Fig. 4F). These results clearly indicated that the CV1-derived 17-amino-acid region alone was not sufficient for SIVmac restriction. On the other hand, HSC-insert-tag partially restricted both HIV-1 and SIVmac, although this chimera showed lower levels of protein expression than other chimeras did (Fig. 4E and F). These results indicated that the CV1-specific 20-amino-acid duplication was important in SIVmac restriction.
To determine whether the CV1-specific 20-amino-acid duplication was indispensable for SIVmac restriction, we generated CV1-delete-tag, which lacked the 20-amino-acid duplication in the CV1-TRIM5-tag (Fig. 4A). The protein expression level of CV1-delete-tag was comparable to that of CV1-60tag (Fig. 4E), and CV1-delete-tag inhibited HIV-1 replication as completely as CV1-60tag did. However, CV1-delete-tag was shown to lose the ability to inhibit SIVmac infection (Fig. 4F). Taken together, our data clearly indicated that the 20-amino-acid duplication of CV1-TRIM5 was necessary for SIVmac restriction and suggested that the adjacent 17-amino-acid region of CV1-TRIM5 was also necessary to fully restrict SIVmac infection.
HIV-2 GH123 is sensitive to cynomolgus monkey TRIM5, as well as African green monkey TRIM5. HIV-2 is closely related to SIVmac (9). We tested whether or not the sensitivity of HIV-2 to various TRIM5s was similar to that of SIVmac239. C143 cells expressing CV1, HSC-F, and their chimeric TRIM5s were infected with the VSV-G-pseudotyped HIV-2 strain GH123. Surprisingly, HSC-F-TRIM5-tag inhibited HIV-2 replication as CV1-TRIM5-tag had done (Fig. 5). Both chimeric TRIM5s, CV1-60tag and HSC-F+60tag, also inhibited HIV-2 replication to a similar extent (Fig. 5). These results indicated that HIV-2 strain GH123 was sensitive to cynomolgus monkey TRIM5 despite its high level of sequence homology to SIVmac239.
DISCUSSION
In the present study, we showed that both cynomolgus and African green monkey TRIM5s could inhibit HIV-1 infection. African green monkey TRIM5 could also inhibit SIVmac infection, whereas cynomolgus monkey TRIM5 could not. Experiments on chimeras of the cynomolgus and African green monkey TRIM5s unequivocally demonstrated that a small region composed of 37 amino acid residues in the SPRY domain of African green monkey TRIM5 was responsible for restricting the SIVmac infection.
A previous study showed that rhesus monkey TRIM5, a splicing variant lacking the SPRY domain, did not suppress HIV-1 infection (33). In the case of TRIM7, the SPRY domain alone was sufficient for binding to its ligand glycogenin (38). Deletion of the entire SPRY domain from TRIM11 also abolished its ability to bind Humanin (21). Therefore, it is reasonable to assume that the variable N-terminal region of the SPRY domain of TRIM5 binds to HIV-1 or SIVmac CA protein. This assumption is consistent with the recent findings that in owl monkey cells, HIV-1 infection was restricted by a TRIM5-cyclophilin A fusion protein in which the SPRY domain was replaced with cyclophilin A, since cyclophilin A is a well-known ligand of HIV-1 CA protein (22, 28).
In the attempt to further narrow the SIVmac restriction determinant more precisely, we were able to demonstrate that the African green monkey-specific 20-amino-acid duplication was indispensable for SIVmac restriction and that the adjacent 17-amino-acid region of African green monkey alone was not sufficient. However, HSC-insert-tag carrying the cynomolgus monkey-derived 17-amino acid region with African green monkey-specific 20-amino-acid duplication showed low levels of protein expression and only partial suppression of HIV-1 and SIVmac replication. It is possible that an artificial combination of African green monkey-specific 20-amino-acid duplication with the cynomolgus monkey-derived 17-amino-acid region made TRIM5 molecules unstable. Further studies, including mutational analysis of the African green monkey-specific 17-amino-acid region, are necessary to determine the precise role of this region in SIVmac restriction.
Despite its close similarity to SIVmac, HIV-2 strain GH123 was restricted by cynomolgus monkey TRIM5, as well as by African green monkey TRIM5. Although both HIV-2 and SIVmac were considered to come from SIVsm (9), it is possible that HIV-2 has been replicating in the human population in the absence of TRIM5 restriction for a certain period and has lost its ability to escape from cynomolgus monkey TRIM5. However, it has also been reported that there was a considerable degree of variation in the ability to grow in monkey cells among HIV-2 strains (6, 8, 26). Therefore, it is necessary to examine various HIV-2 strains for their sensitivity to human and monkey TRIM5s before we can draw a definite conclusion. It would also be interesting to identify specific amino acid changes determining the sensitivity to cynomolgus monkey TRIM5 in viral CA proteins, since nearly 90% of the amino acid residues in SIVmac239 CA protein are conserved in HIV-2GH123.
In CV1 cells, the level of TRIM5 gene expression was ca. 3 x 106 copies/μg of total RNA, a level similar to that observed in other human cell lines examined (data not shown). Although HIV-1 infection was suppressed in hamster TK-ts13 or human C143 cells expressing CV1-TRIM5, relatively high levels of TRIM5 (nearly 5 x 107 copies/μg of total RNA) appeared to be required for a level of suppression similar to that observed in CV1 cells. One possible explanation for this discrepancy is that certain molecules cooperating with TRIM5 also showed species specificity, and CV1-TRIM5 was not fully supported in hamster and human cells. Because TRIM5 gene products are suspected to be an E3 ubiquitin ligase (35), it is important to identify the E2 ubiquitin-conjugating enzyme interacting with TRIM5. Alternatively, restriction factors other than TRIM5 may exist in CV1 cells, or certain molecules required for efficient lentivirus infection may be absent in CV1 cells.
After we submitted these findings for publication, small amino acid differences in the SPRY domain between human and rhesus monkey TRIM5s were reported to determine HIV-1 restriction (27, 34, 37). Our findings are in good agreement with the results of these studies.
ACKNOWLEDGMENTS
We thank Setsuko Bando for skillful technical assistance. HSC-F cells were kindly supplied by Hirofumi Akari. pGH123 was a gift from Akio Adachi.
This study was supported by grants from the Human Science Foundation; the Ministry of Education, Culture, Sports, Science, and Technology; and the Ministry of Health, Labour, and Welfare of Japan.
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BioResource Center, RIKEN Tsukuba Institute, Tsukuba
Toyama Institute of Health, Toyama, Japan
ABSTRACT
Human immunodeficiency virus type 1 (HIV-1) efficiently enters cells of Old World monkeys but encounters a block before reverse transcription. This restriction is mediated by a dominant repressive factor. Recently, a member of the tripartite motif (TRIM) family proteins, TRIM5, was identified as a blocking factor in a rhesus macaque cDNA library. Among Old World monkey cell lines, the African green monkey kidney cell line CV1 is highly resistant to not only HIV-1 but also simian immunodeficiency virus SIVmac infection. We analyzed TRIM5 of CV1 cells and HSC-F cells, a T-cell line from a cynomolgus monkey, and found that both CV1- and HSC-F-TRIM5s could inhibit CD4-dependent HIV-1 infection, as well as vesicular stomatitis virus glycoprotein-mediated infection. CV1-TRIM5 could also inhibit SIVmac infection, whereas HSC-F-TRIM5 could not. In the SPRY (B30.2) domain of CV1-TRIM5, there was a 20-amino-acid duplication that was not present in HSC-F-TRIM5. A chimeric TRIM5 containing 37 amino acid residues from CV1-TRIM5, which spanned the 20-amino-acid duplication, in the background of HSC-F-TRIM5 fully gained the ability to inhibit SIVmac infection. Conversely, the mutant CV1-TRIM5 lacking the 20-amino-acid duplication completely lost the ability to restrict SIVmac infection. These findings clearly indicated that a specific region of 37 amino acid residues in the SPRY domain of CV1-TRIM5 contained a determinant of species-specific restriction of SIVmac.
INTRODUCTION
Human immunodeficiency virus type 1 (HIV-1) is thought to have been introduced into the human population from chimpanzees (9) and shows a very narrow host range limited only to humans and chimpanzees. HIV-1 does not experimentally infect Old World monkeys, such as rhesus and cynomolgus monkeys, and fails to replicate in activated CD4-positive T lymphocytes obtained from these monkeys (13, 31). In contrast, simian immunodeficiency virus (SIV) isolated from a macaque monkey (SIVmac) can replicate well in rhesus (13, 31) and cynomolgus monkeys (2, 3). The restricted host range of HIV-1 has greatly hampered its use in animal experiments and, hence, caused difficulty in developing prophylactic vaccines against HIV-1 infection.
Several studies have suggested that the block of HIV-1 replication in Old World monkey cells occurred at a postentry step (7, 13, 31) and appeared to result from a failure to initiate reverse transcription (13). The block was still observed when CD4-negative monkey cells were infected with HIV-1 pseudotyped with vesicular stomatitis virus glycoprotein (VSV-G) and was overridden by a high multiplicity of infection (MOI) with VSV-G-pseudotyped virus or virus-like particles lacking genomic RNA (5, 10, 16, 19). Importantly, resistance against HIV-1 infection was shown to be dominant in heterokaryons between human and Old World monkey cells, suggesting the presence of inhibitory factor(s) against HIV-1 infection in Old World monkey cells (19). Studies on chimera of HIV-1 and SIVmac have suggested that restriction determinants lie within the HIV-1 P24 capsid protein (CA) (11, 23, 24, 29).
Recently, the screening of a rhesus monkey cDNA library identified tripartite motif 5 (TRIM5), a component of cytoplasmic bodies, as a factor that confers resistance to HIV-1 infection (33). Shortly after, TRIM5 of African green monkey, another Old World monkey, was also shown to restrict HIV-1 infection, whereas human TRIM5 was reported to restrict N-tropic murine leukemia virus (12, 14, 25, 36).
An African green monkey kidney cell line, CV1, was shown to be highly resistant to SIVmac infection, as well as to HIV-1 infection. We analyzed TRIM5 of CV1 cells and HSC-F cells, a T-cell line from a cynomolgus monkey, and report here that the ability of CV1-TRIM5 to suppress SIVmac infection was determined by a small region composed of 37 amino acid residues in the SPRY (B30.2) domain of CV1-TRIM5.
MATERIALS AND METHODS
Cloning and expression of TRIM5. TRIM5 cDNA was amplified by reverse transcription-PCR from the human T-cell line MT4, cynomolgus monkey T-cell line HSC-F (2, 3), and African green monkey cell lines CV1 and Vero by using 5'-GCGGCCGCTACTATGGCTTCTGG-3' as a forward primer and 5'-GAATTCTCAAGAGCTTGGTGA-3' as a reverse primer. Amplified products were then cloned into the vector pCR-2.1TOPO (Invitrogen), and the nucleotide sequence of 10 clones for each TRIM5 was determined.
The entire coding regions of selected clones were transferred to pcDNA3.1 (Invitrogen) by using NotI and EcoRI sites, which were introduced by primers used in the PCR step. Hamster TK-ts13 cells (4) were transfected with pcDNA3.1 carrying TRIM5 cDNA and cultured in the presence of 0.75 mg of G418 (Gibco)/ml for 14 days. The colonies obtained were examined for the expression of TRIM5 by using the TaqMan PCR method according to the manufacturer's instructions (Applied Biosystems). Sequences of the probe and primers used to specifically detect each TRIM5 were as follows: MT4-TRIM5, forward primer (5'-AACCTGGAGAAGGAGGAGGAAGAC-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TCAGTTTCAGAGTTCG-TAMRA-3'); HSC-F-TRIM5, forward primer (5'-AACCTGGAGAAGGAGAAAGAAGAC-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TTCGTTTCAGACTTTG-TAMRA-3'); and CV1-TRIM5, forward primer (5'-AACCTGGAGAAGGAGGAAGAAGA-3'), reverse primer (5'-CTGGGTCTGCTGCACCAT-3'), and probe (5'-FAM-TCCGTTTCAGACTTCG-TAMRA-3'). These primers amplify the coiled-coil region of TRIM5 genes. Plasmid DNA used for transfection served as a standard to determine the number of copies of TRIM5 transcripts. The parental TK-ts13 cells were totally negative for the primate TRIM5 expression. Clones expressing each TRIM5 at comparable levels (ca. 4 to 6 x 107 copies/μg of total RNA) were used for subsequent experiments.
To generate CV1-TRIM5 and HSC-F-TRIM5 cDNAs carrying a hemagglutinin (HA) tag (YPYDVPDYAA) at their C termini, cloned CV1-TRIM5 and HSC-F-TRIM5 cDNAs in pcDNA3.1 were used as templates for PCR amplification with a primer containing a nucleotide sequence corresponding to the HA tag fused with the C-terminal portion of TRIM5. The C-terminal portion of TRIM5 fused with the HA tag (BamHI to NotI) and the N-terminal portion of TRIM5 (NotI to BamHI) were assembled on a pCEP4 vector (Invitrogen). To generate chimeric TRIM5 HSC-F+60tag, the 182-bp SphI-BamHI fragment of HSC-F-TRIM5-tag was replaced with the corresponding 242-bp SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. Conversely, the 242-bp SphI-BamHI fragment of CV1-TRIM5 was replaced with the 182-bp SphI-BamHI fragment of HSC-F-TRIM5-tag in the background of CV1-TRIM5-tag to generate CV1-60tag. PCR-based mutagenesis of HSC-F-TRIM5-tag was performed to generate HSC-delete-tag, which possessed the 5'-proximal 84 bp of the SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag, and HSC-insert-tag, which possessed 3'-proximal 158 bp of the SphI-BamHI fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. Similarly, CV1-delete-tag, which possessed the 3'-proximal 98 bp of the SphI-BamHI fragment of HSC-F-TRIM5 in the background of CV1-TRIM5-tag, was generated by a PCR-based mutagenesis of CV1-TRIM5-tag. The entire coding sequences of these TRIM5-tags were then transferred to the NotI site of pSeV18+b(+). Recombinant Sendai viruses (SeVs) carrying various TRIM5-tags were recovered according to a previously described method (32). The viruses passaged a second time in embryonated chicken eggs were used as stock for all experiments. The wild-type Z strain of SeV served as a control in all of the experiments.
To establish human cell lines which constitutively express primate TRIM5s or their chimeras, human osteosarcoma C143 cells were transfected with pCEP4 containing cDNA of CV1-TRIM5-tag, HSC-F-TRIM5-tag, CV1-60tag, or HSC-F+60tag, and cells were cultured in the presence of 0.3 mg of hygromycin B (Gibco)/ml for 14 days.
Immunoprecipitation and Western blot analysis. When we performed Western blot analysis of cells expressing HA-tagged TRIM5 proteins, we consistently observed nonspecific binding of anti-HA antibody to a protein that comigrated with HSC-F-TRIM5. Therefore, we analyzed the expression of each HA-tagged TRIM5 protein in the hygromycin B-resistant C143 cells or MT4 cells infected with recombinant SeVs by immunoprecipitation, followed by Western blot analysis as described previously (20) to reduce nonspecific background. Briefly, cell lysate was first adsorbed with protein A-agarose before the addition of anti-HA antibody to avoid nonspecific protein binding to protein A-agarose. TRIM5 proteins in the cell lysate were then precipitated with anti-HA high-affinity rat monoclonal antibody (Roche) by using a protein A-immunoprecipitation kit (Roche). Precipitated materials were subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis on a 4 to 12% NuPAGE Bis-Tris gel (Invitrogen). Proteins in the gel were then electronically transferred to a polyvinylidene difluoride membrane (Immobilon; Millipore). Blots were blocked and probed with anti-HA antibody overnight at 4°C and then incubated with peroxidase-conjugated anti-rat immunoglobulin G (American Qualex) and developed by using the Immun-Star HRP chemiluminescence kit (Bio-Rad). Visualized image was recorded by LAS1000 (Fuji) and quantified by ImageGauge (Fuji). At least three independent experiments were performed, and the means and standard deviations (SD) for the data were calculated.
Viruses and HIV-1 lentivirus vector. VSV-G-pseudo typed HIV-1-NL43, SIVmac239, or HIV-2-GH123 was prepared by transfection of 293T cells with a combination of pMD.G (17, 18) and pNL432 (1), pBRmac239 (15), or pGH123 (30), respectively. HIV-1 vector expressing green fluorescence protein (GFP) was prepared as described previously (17, 18). Two days after transfection, culture supernatants of 293T cells were collected and assayed for reverse transcriptase activity using a reverse transcriptase colorimetric assay (Roche).
Viral infection. Assays for the HIV-1 vector expressing GFP were performed in 24-well plates containing 4 x 104 Tk-ts13-derived target cells. Serially diluted VSV-pseudotyped HIV-1 vectors encoding GFP were inoculated, and infected cells were enumerated by using a flow cytometer (FACScan; Becton Dickinson) 40 h after infection. For VSV-pseudotyped HIV-1, SIVmac239, and HIV-2 infection assays, we inoculated viruses containing 1 ng of reverse transcriptase into 4 x 104 C143 cells. For CD4-dependent infection assays, 2.5 x 105 MT4 cells were infected with SeV expressing CV1-TRIM5-tag, HSC-F-TRIM5-tag, or the parental Z strain of SeV at a MOI of 10 PFU per cell, followed by incubation at 37°C for 9 h. Cells were then superinfected with 30 ng of p24 of an X4 HIV-1 strain, NL43, or 30 ng of p27 of SIVmac239. The culture supernatants were collected periodically, and the level of p24 or p27 was measured by using a RETROtek antigen ELISA kit (ZeptoMetrix).
Data deposition. The sequences described here have been deposited in the GenBank database under accession numbers AB210050 to AB210052.
RESULTS
Variation in TRIM5. We cloned TRIM5 cDNA from the human T-cell line MT4, cynomolgus monkey T-cell line HSC-F, and African green monkey kidney cell lines CV1 and Vero. The predicted amino acid sequences of TRIM5s are compared in Fig. 1A and B.
Human TRIM5 from MT4 cells differed at an amino acid position 249 (G249D) from the previously published sequence (33) and was designated MT4-TRIM5. The cynomolgus monkey TRIM5 from HSC-F (HSC-F-TRIM5) was two amino acids shorter than the rhesus monkey TRIM5 (33) and two amino acids longer than the human TRIM5. All 10 clones derived from Vero cells had the same sequence as the previously published one (36). On the other hand, we found at least two distinct TRIM5 sequences in CV1 cells. The two major TRIM5 sequences obtained from CV1 were designated CV1-TRIM5-type1 and CV1-TRIM5-type2, and five amino acids were found to differ between the two sequences (I259V, L337S, R351L, G359R, and G438S). Among 10 cDNA clones obtained from CV1, there were four type 1 clones and four type 2 clones. The remaining two clones were most likely chimeric artifacts. Two recently published sequences of TRIM5 from CV1 cells (AY593973 and AY625002) showed differences at three positions—L7V, I259V, and G438S—and have S, L, and R at positions 337, 351, and 359, respectively (14, 36), whereas both the type 1 and 2 clones had leucines at the seventh position. All sequences obtained from Vero and CV1 contained a 20-amino-acid duplication within the SPRY domain, which was not observed in human MT4 and cynomolgus monkey HSC-F (Fig. 1B).
The phylogenetic tree of various TRIM5 sequences showed that cynomolgus and rhesus monkey TRIM5s are similar to each other, a finding consistent with the fact that these two monkeys belong to the genus Macaca (Fig. 1C).
African green monkey and cynomolgus monkey TRIM5 inhibit HIV-1 infection in nonprimate cells. We first sought to determine whether or not each TRIM5 can inhibit HIV-1 infection in the context of nonprimate cells because human and primate cells express endogenous TRIM5 that could complicate a functional analysis of TRIM5-mediated restriction. The hamster cell line TK-ts13 was used, because it is very susceptible to a VSV-G-pseudotyped, HIV-1-based GFP-expressing lentivirus vector, HIV-1-GFP. Cell clones stably expressing MT4-, CV1-, and HSC-F-TRIM5 were selected according to the method described in Materials and Methods. The levels of expression of TRIM5 were determined by using a real-time PCR, and cells expressing comparable amounts of TRIM5 (4 x 106 to 6 x 106 copies/μg of total RNA) were used for subsequent study. Restriction can be quantified by comparing the percentage of GFP-positive cells with or without TRIM5.
As can be seen in Fig. 2A, MT4-TRIM5 had a very weak anti-HIV-1 effect (1.2-fold), a finding consistent with a previous study (33). In contrast, restriction of HIV-1 was clearly evident over a wide range of initial MOIs in cells expressing HSC-F-TRIM5, CV1-TRIM5-type1, and CV1-TRIM5-type2 (ca. 5- to 10-fold). There was no significant difference between CV1-TRIM5-type1 and type2; therefore, we chose CV1-TRIM5-type1 to be representative of CV1-TRIM5 in the subsequent experiments. We obtained the same results as described above when we used an HA-tagged version of TRIM5 (data not shown).
African green monkey and cynomolgus monkey TRIM5 inhibit CD4-dependent HIV-1 infection in human cells. To test the restriction properties of TRIM5 in CD4-dependent HIV-1 infection, we constructed a recombinant SeV expressing TRIM5 fused with the HA tag in the C-terminal of HSC-F-TRIM5 or CV1-TRIM5 (HSC-F-TRIM5-tag SeV or CV1-TRIM5-tag SeV). Human T-cell line MT4 cells were first infected with the SeV expressing TRIM5-tag (Fig. 2B), incubated at 37°C for 9 h, and then infected with an X4-tropic HIV-1 strain NL43. As can be seen in Fig. 2C, both HSC-F-TRIM5-tag and CV1-TRIM5-tag completely inhibited HIV-1 replication, whereas MT4 cells infected with SeV empty vector fully supported HIV-1 replication.
Distinct patterns of restriction for SIVmac among nonhuman primate TRIM5. In African green monkey CV1 cells, both HIV-1 and SIVmac239 were restricted, whereas only HIV-1 was restricted in cynomolgus monkey HSC-F cells (Fig. 3A). Therefore, we examined whether or not CV1-TRIM5 also could inhibit the replication of SIVmac. In MT4 cells infected with recombinant SeV expressing HSC-F-TRIM5-tag, the replication of SIVmac239 was not suppressed at all (Fig. 3B), indicating that the HSC-F-TRIM5 showed a similar specificity to rhesus monkey TRIM5 (33). In MT4 cells infected with recombinant SeV expressing CV1-TRIM5-tag, in contrast, the replication of SIVmac239 was completely suppressed. These results suggested that the distinct sensitivity of African green monkey and cynomolgus monkey cells to HIV-1 and SIVmac infection was, at least partly, determined by TRIM5.
A small region of 37 amino acid residues in the SPRY domain of CV1-TRIM5 determines SIVmac restriction. A comparison of the human and nonhuman primate TRIM5 sequences showed the presence of a highly variable region in the N-terminal portion of the SPRY domain (Fig. 1A and B). In this region, CV1 and Vero TRIM5 had a 20-amino-acid repetition that was totally absent in HSC-F-TRIM5. These findings prompted us to test whether this highly variable region of TRIM5 determined the species-specific inhibition of SIVmac infection. We constructed chimeric TRIM5s from HSC-F-TRIM5-tag and CV1-TRIM5-tag by using SphI and BamHI restriction enzyme digestion (Fig. 4A). HSC-F+60tag contained the 242-bp fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag. The reciprocal chimera, CV1-60tag, contained a 182-bp fragment of HSC-F-TRIM5 in the background of the CV1-TRIM5-tag. In this fragment, the differences between CV1 and HSC-F TRIM5, including the 20-amino-acid repetition, were located in a small region of 37 amino acid residues (Fig. 1B). Human osteosarcoma C143 cells stably expressing various TRIM5s (Fig. 4B) were infected with VSV-G-pseudotyped HIV-1 NL43, and levels of P24 in the culture supernatants were assayed periodically. As expected, both chimeric TRIM5s and parental TRIM5s clearly inhibited the replication of HIV-1 NL43 (Fig. 4C). When these cells were infected with VSV-G-pseudotyped SIVmac239, the parental CV1-TRIM5-tag could also inhibit the replication of SIVmac239, whereas CV1-60tag, which contained the 182-bp fragment of HSC-F-TRIM5 in the background of CV1-TRIM5-tag, could not. Conversely, the parental HSC-F-TRIM5-tag did not inhibit the replication of SIVmac239 at all, whereas HSC-F+60tag, which contained the 242-bp fragment of CV1-TRIM5 in the background of HSC-F-TRIM5-tag, clearly inhibited SIVmac239 (Fig. 4C). We obtained the same results as described above when we used SeVs to express parental TRIM5-tag or chimeras (Fig. 4D). These results indicated that the determinant of the species-specific inhibition of SIVmac239 replication is located in 37 amino acid residues in the SPRY domain of CV1-TRIM5.
To narrow the SIVmac restriction determinant more precisely, we generated two more chimeric TRIM5s (Fig. 4A). HSC-delete-tag contained a CV1-derived 17-amino-acid fragment without the 20-amino-acid duplication in the background of the HSC-TRIM5-tag. HSC-insert-tag contained the HSC-F-derived 17-amino-acid fragment with the CV-1 derived 20-amino-acid duplication in the background of HSC-TRIM5-tag. Recombinant SeVs expressing these chimeric TRIM5s were generated and used in the subsequent experiments. Although the expression levels of mRNA of each chimericTRIM5 was virtually identical to each other (data not shown), we observed considerable variations in the levels of TRIM5 protein expression among chimeras (Fig. 4E). The HSC-delete-tag showed slightly higher levels of protein expression than those of HSC-F+60tag. However, HSC-delete-tag failed to inhibit SIVmac replication, whereas it restricted HIV-1 replication as completely as HSC-F+60tag did (Fig. 4F). These results clearly indicated that the CV1-derived 17-amino-acid region alone was not sufficient for SIVmac restriction. On the other hand, HSC-insert-tag partially restricted both HIV-1 and SIVmac, although this chimera showed lower levels of protein expression than other chimeras did (Fig. 4E and F). These results indicated that the CV1-specific 20-amino-acid duplication was important in SIVmac restriction.
To determine whether the CV1-specific 20-amino-acid duplication was indispensable for SIVmac restriction, we generated CV1-delete-tag, which lacked the 20-amino-acid duplication in the CV1-TRIM5-tag (Fig. 4A). The protein expression level of CV1-delete-tag was comparable to that of CV1-60tag (Fig. 4E), and CV1-delete-tag inhibited HIV-1 replication as completely as CV1-60tag did. However, CV1-delete-tag was shown to lose the ability to inhibit SIVmac infection (Fig. 4F). Taken together, our data clearly indicated that the 20-amino-acid duplication of CV1-TRIM5 was necessary for SIVmac restriction and suggested that the adjacent 17-amino-acid region of CV1-TRIM5 was also necessary to fully restrict SIVmac infection.
HIV-2 GH123 is sensitive to cynomolgus monkey TRIM5, as well as African green monkey TRIM5. HIV-2 is closely related to SIVmac (9). We tested whether or not the sensitivity of HIV-2 to various TRIM5s was similar to that of SIVmac239. C143 cells expressing CV1, HSC-F, and their chimeric TRIM5s were infected with the VSV-G-pseudotyped HIV-2 strain GH123. Surprisingly, HSC-F-TRIM5-tag inhibited HIV-2 replication as CV1-TRIM5-tag had done (Fig. 5). Both chimeric TRIM5s, CV1-60tag and HSC-F+60tag, also inhibited HIV-2 replication to a similar extent (Fig. 5). These results indicated that HIV-2 strain GH123 was sensitive to cynomolgus monkey TRIM5 despite its high level of sequence homology to SIVmac239.
DISCUSSION
In the present study, we showed that both cynomolgus and African green monkey TRIM5s could inhibit HIV-1 infection. African green monkey TRIM5 could also inhibit SIVmac infection, whereas cynomolgus monkey TRIM5 could not. Experiments on chimeras of the cynomolgus and African green monkey TRIM5s unequivocally demonstrated that a small region composed of 37 amino acid residues in the SPRY domain of African green monkey TRIM5 was responsible for restricting the SIVmac infection.
A previous study showed that rhesus monkey TRIM5, a splicing variant lacking the SPRY domain, did not suppress HIV-1 infection (33). In the case of TRIM7, the SPRY domain alone was sufficient for binding to its ligand glycogenin (38). Deletion of the entire SPRY domain from TRIM11 also abolished its ability to bind Humanin (21). Therefore, it is reasonable to assume that the variable N-terminal region of the SPRY domain of TRIM5 binds to HIV-1 or SIVmac CA protein. This assumption is consistent with the recent findings that in owl monkey cells, HIV-1 infection was restricted by a TRIM5-cyclophilin A fusion protein in which the SPRY domain was replaced with cyclophilin A, since cyclophilin A is a well-known ligand of HIV-1 CA protein (22, 28).
In the attempt to further narrow the SIVmac restriction determinant more precisely, we were able to demonstrate that the African green monkey-specific 20-amino-acid duplication was indispensable for SIVmac restriction and that the adjacent 17-amino-acid region of African green monkey alone was not sufficient. However, HSC-insert-tag carrying the cynomolgus monkey-derived 17-amino acid region with African green monkey-specific 20-amino-acid duplication showed low levels of protein expression and only partial suppression of HIV-1 and SIVmac replication. It is possible that an artificial combination of African green monkey-specific 20-amino-acid duplication with the cynomolgus monkey-derived 17-amino-acid region made TRIM5 molecules unstable. Further studies, including mutational analysis of the African green monkey-specific 17-amino-acid region, are necessary to determine the precise role of this region in SIVmac restriction.
Despite its close similarity to SIVmac, HIV-2 strain GH123 was restricted by cynomolgus monkey TRIM5, as well as by African green monkey TRIM5. Although both HIV-2 and SIVmac were considered to come from SIVsm (9), it is possible that HIV-2 has been replicating in the human population in the absence of TRIM5 restriction for a certain period and has lost its ability to escape from cynomolgus monkey TRIM5. However, it has also been reported that there was a considerable degree of variation in the ability to grow in monkey cells among HIV-2 strains (6, 8, 26). Therefore, it is necessary to examine various HIV-2 strains for their sensitivity to human and monkey TRIM5s before we can draw a definite conclusion. It would also be interesting to identify specific amino acid changes determining the sensitivity to cynomolgus monkey TRIM5 in viral CA proteins, since nearly 90% of the amino acid residues in SIVmac239 CA protein are conserved in HIV-2GH123.
In CV1 cells, the level of TRIM5 gene expression was ca. 3 x 106 copies/μg of total RNA, a level similar to that observed in other human cell lines examined (data not shown). Although HIV-1 infection was suppressed in hamster TK-ts13 or human C143 cells expressing CV1-TRIM5, relatively high levels of TRIM5 (nearly 5 x 107 copies/μg of total RNA) appeared to be required for a level of suppression similar to that observed in CV1 cells. One possible explanation for this discrepancy is that certain molecules cooperating with TRIM5 also showed species specificity, and CV1-TRIM5 was not fully supported in hamster and human cells. Because TRIM5 gene products are suspected to be an E3 ubiquitin ligase (35), it is important to identify the E2 ubiquitin-conjugating enzyme interacting with TRIM5. Alternatively, restriction factors other than TRIM5 may exist in CV1 cells, or certain molecules required for efficient lentivirus infection may be absent in CV1 cells.
After we submitted these findings for publication, small amino acid differences in the SPRY domain between human and rhesus monkey TRIM5s were reported to determine HIV-1 restriction (27, 34, 37). Our findings are in good agreement with the results of these studies.
ACKNOWLEDGMENTS
We thank Setsuko Bando for skillful technical assistance. HSC-F cells were kindly supplied by Hirofumi Akari. pGH123 was a gift from Akio Adachi.
This study was supported by grants from the Human Science Foundation; the Ministry of Education, Culture, Sports, Science, and Technology; and the Ministry of Health, Labour, and Welfare of Japan.
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