SIV Phylogeny in Western Gorillas
SIV in Western Gorillas
Phylogenetic Analysis of SIV in Western Gorillas
In order to better understand how SIV is transmitted Takehisa et al. (2009) undertook several experiments to determine the phylogenetic relationship between SIVgor and SIVcpz. These experiments depended primarily on sequence homology comparisons, a commonly-used and well-accepted approach for determining phylogenetic relationships.
The specific aims are as follows:
Whole genome sequence homology comparisons will be performed between different strains of SIVgor, SIVcpz, and HIV-1, to establish the relative similarity and thus reveal phylogenetic relationships.
SIVgor sequence will be examined for evidence of recombination. Should a recombination signature be found, it can be used to help search for the most recent common ancestor.
There are multiple strains of SIVcpz infecting chimpanzees from central and eastern Africa, and previous research has shown these strains are geographically-specific. SIVgor sequence comparisons with SIVcpz strains isolated from wild chimpanzee populations will be used to determine whether the SIVgor strains arose through local inter-species transmissions or were derived from a common ancestor.
4. A full-length SIVgor consensus sequence will be assembled and used to produce an infection-competent SiVgor virus. This laboratory virus will then be characterized in terms of its requirements for infecting CD4 T cells.
Materials and Methods
SIVgor RNA was derived from fecal samples collected from wild western gorillas, and then subjected to reverse transcriptase and PCR amplification. The amplified products were sequenced and aligned to generate a full-length consensus sequences representing the four different strains. There was no mention of whether multiple independent reverse transcriptase and PCR amplifications were used to control for mistakes in these laboratory procedures. PCR mistakes are common, depending on which thermostable polymerase is used.
A full-length copy of the SIVgor genome was assembled using multiple overlapping PCR fragments, from multiple PCR amplifications. The sequence of the full length clone was validated using previous SIV and strain-specific primers. This is a standard approach used by laboratories around the world. Direct cloning of isolated RNA molecules could be attempted, but this approach is much more labor intensive and likely to fail. Given the urgency surrounding HIV research efforts, the use of PCR is reasonable.
To produce infectious viruses, the full-length clone was amplified in a bacterial host and then transfected into 293T cells. Infectivity of SIVgor and SIV strains from chimpanzees were assessed using a HeLa cell derivative genetically-modified to express CD4, CCR5, and CXCR4 and containing the luciferase and ?-galactosidase reporter genes under the control of an HIV-1 LTR element. Assays depended on lysing the cells and measuring reporter gene activity. Infectivity of primary chimpanzee and human CD4 T cells isolated from peripheral blood mononuclear cells was also determined. Viral activity was measured by assaying viral reverse transcriptase activity in the cell culture supernatants every three days. Blocking assays involved incubating viral particles with various inhibitors, soluble CD4, and blocking antibodies in the presence of the reporter cell line. This approach seems straight forward and the inclusion of primary CD4 T cells helps to validate the results of in vitro assays relying on genetically-modified cell lines.
Results
Consensus and strain-specific primers were able to amplify three strains derived from the fecal matter recovered from the same region in western Africa. A fourth strain (BQ664), which was derived from gorilla fecal matter located 400 km away, did not amplify as easily. It's possible that the sequence of the fourth strain was too degraded for RT/PCR to be effective, or the PCR primer annealing site had diverged. Aligning the sequences revealed significant differences, including altered amino acid coding sequence, but none of the substitutions introduced a stop or frameshift codon. The authors could have pursued different primer approaches for both the reverse transcriptase reaction and the PCR, such as using random hexamers for primers. The sequence so obtained could be aligned to produce a consensus sequence.
The three SIVgor clones from which full-length sequence was derived varied in length by as much as 109 nt. All three contained nine full-length open reading frames and the predicted conserved cis-regulatory elements. Deduced amino acid sequences for the nine proteins revealed significant divergence, but no obvious SIVgor-specific signatures. Programs designed to predict protein function found strong similarities between the SIVgor-predicted functional sites and those found for SIVcpz and HIV-1 proteins, suggesting function has been conserved despite significant sequence divergence. The homology between SIVgor, and SIVcpz or HIV-1, varied depending on which sequence was used in the comparison.
The phylogeny of the SIVgor strains...
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