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  • Impact of H216 on the DNA binding and catalytic activities of the HIV restriction factor APOBEC3G.

Impact of H216 on the DNA binding and catalytic activities of the HIV restriction factor APOBEC3G.

Journal of virology (2013-04-19)
Stefan Harjes, William C Solomon, Ming Li, Kuan-Ming Chen, Elena Harjes, Reuben S Harris, Hiroshi Matsuo
ZUSAMMENFASSUNG

APOBEC3G has an important role in human defense against retroviral pathogens, including HIV-1. Its single-stranded DNA cytosine deaminase activity, located in its C-terminal domain (A3Gctd), can mutate viral cDNA and restrict infectivity. We used time-resolved nuclear magnetic resonance (NMR) spectroscopy to determine kinetic parameters of A3Gctd's deamination reactions within a 5'-CCC hot spot sequence. A3Gctd exhibited a 45-fold preference for 5'-CCC substrate over 5'-CCU substrate, which explains why A3G displays almost no processivity within a 5'-CCC motif. In addition, A3Gctd's shortest substrate sequence was found to be a pentanucleotide containing 5'-CCC flanked on both sides by a single nucleotide. A3Gctd as well as full-length A3G showed peak deamination velocities at pH 5.5. We found that H216 is responsible for this pH dependence, suggesting that protonation of H216 could play a key role in substrate binding. Protonation of H216 appeared important for HIV-1 restriction activity as well, since substitutions of H216 resulted in lower restriction in vivo.

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L-Histidin, suitable for cell culture, meets EP, USP testing specifications, from non-animal source
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L-Histidin, ReagentPlus®, ≥99% (TLC)
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L-Histidin, Pharmaceutical Secondary Standard; Certified Reference Material
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L-Histidin, certified reference material, TraceCERT®, Manufactured by: Sigma-Aldrich Production GmbH, Switzerland