Structural insights into RNA bridging between HIV-1 Vif and antiviral factor APOBEC3G

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作者
Takahide Kouno
Satoshi Shibata
Megumi Shigematsu
Jaekyung Hyun
Tae Gyun Kim
Hiroshi Matsuo
Matthias Wolf
机构
[1] Okinawa Institute of Science and Technology Graduate University,Molecular Cryo
[2] Thomas Jefferson University,Electron Microscopy Unit
[3] Frederick National Laboratory for Cancer Research,Computational Medicine Center, Sidney Kimmel Medical College
[4] Academia Sinica,Cancer Innovation Laboratory
[5] Tottori University,Institute of Biological Chemistry
[6] Sungkyunkwan University,Division of Bacteriology, Department of Microbiology and Immunology, Faculty of Medicine
[7] Gyeongbuk Institute for Bio Industry,School of Pharmacy
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Great effort has been devoted to discovering the basis of A3G-Vif interaction, the key event of HIV’s counteraction mechanism to evade antiviral innate immune response. Here we show reconstitution of the A3G-Vif complex and subsequent A3G ubiquitination in vitro and report the cryo-EM structure of the A3G-Vif complex at 2.8 Å resolution using solubility-enhanced variants of A3G and Vif. We present an atomic model of the A3G-Vif interface, which assembles via known amino acid determinants. This assembly is not achieved by protein-protein interaction alone, but also involves RNA. The cryo-EM structure and in vitro ubiquitination assays identify an adenine/guanine base preference for the interaction and a unique Vif-ribose contact. This establishes the biological significance of an RNA ligand. Further assessment of interactions between A3G, Vif, and RNA ligands show that the A3G-Vif assembly and subsequent ubiquitination can be controlled by amino acid mutations at the interface or by polynucleotide modification, suggesting that a specific chemical moiety would be a promising pharmacophore to inhibit the A3G-Vif interaction.
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