Abstract
TRIM5α is an interferon inducible restriction factor which contributes to intrinsic defense against HIV infection by targeting the HIV capsid protein CA. Although human TRIM5α (huTRIM5α) does not potently inhibit HIV-1 infection, the ability of huTRIM5α to exhibit some control of HIV-1 infection is evidenced by a single nucleotide polymorphism in huTRIM5α which substitutes aspartic acid to glycine at position 249 (G249D) in the L2 region and is associated with higher susceptibility to HIV-1 infection. To understand the mechanistic basis for the reduced antiviral activity, we employed biophysical and cell biological methods coupled with molecular dynamics simulations to compare WT and the G249D polymorphism of huTRIM5α. We investigated the differences in conformational dynamics of rhesus and huTRIM5α Coiled Coil–Linker 2 (CC-L2) dimers utilizing circular dichroism and single molecule-Fluorescence Energy Transfer (sm-FRET). These methods revealed that the G249D dimer exhibits secondary structure and conformational dynamics similar to WT huTRIM5α. Homology modelling revealed that G249 was present on the hairpin of the antiparallel dimer, in a position which may act to stabilize the adjacent BBox2 domain which mediates the inter-dimeric contacts required for the formation of TRIM5 assemblies. We therefore asked if the G249D mutant forms assemblies in cells with the same efficiency as WT protein by expressing these proteins as YFP fusions and quantifying the number of assemblies in cells. In cells expressing comparable amounts of protein, the G249D mutant formed fewer assemblies than WT protein, in agreement with our homology modeling predictions and molecular dynamics simulations of dimers and higher oligomers of TRIM5α, providing a mechanistic explanation of the reduced antiviral activity of the G249D polymorphism.
Highlights
TRIM5α is a potent restriction factor against retroviruses that mediates a post-entry block to infection by faciltating abortive disassembly of capsid core [1,2,3]
The ability of huTRIM5α to inhibit HIV-1 infection in humans has been supported by studies of huTRIM5α single nucleotide polymorphisms (SNPs), which reveal some polymorphisms are associated with increased susceptibility to HIV-1 infection and disease progression [34,35,36,37,38]
We quantified the change in infectivity of wild type (WT) or G249D huTRIM5α expressing cell lines by normalizing percent green fluorescent protein (GFP) positive cells to the untransduced cell line infected with the same viral titer
Summary
TRIM5α is a potent restriction factor against retroviruses that mediates a post-entry block to infection by faciltating abortive disassembly of capsid core [1,2,3]. The ability of huTRIM5α to inhibit HIV-1 infection in humans has been supported by studies of huTRIM5α single nucleotide polymorphisms (SNPs), which reveal some polymorphisms are associated with increased susceptibility to HIV-1 infection and disease progression [34,35,36,37,38]. One of these SNPs is located in L2 region which substitute aspartic acid to glycine at position 249 (G249D) and is associated with higher susceptibility to HIV-1 infection and higher viral titers in HIV infected patients [39,40,41]
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