H11/HSPB8 Restricts HIV-2 Vpx to Restore the Anti-Viral Activity of SAMHD1

Ayumi Kudoh; Kei Miyakawa; Satoko Matsunaga; Yuki Matsushima; Isao Kosugi; Hirokazu Kimura; Satoshi Hayakawa; Tatsuya Sawasaki; Akihide Ryo

doi:10.3389/fmicb.2016.00883

H11/HSPB8 Restricts HIV-2 Vpx to Restore the Anti-Viral Activity of SAMHD1

Front Microbiol. 2016 Jun 13:7:883. doi: 10.3389/fmicb.2016.00883. eCollection 2016.

Authors

Ayumi Kudoh¹, Kei Miyakawa¹, Satoko Matsunaga¹, Yuki Matsushima², Isao Kosugi³, Hirokazu Kimura⁴, Satoshi Hayakawa⁵, Tatsuya Sawasaki⁶, Akihide Ryo¹

Affiliations

¹ Department of Microbiology, School of Medicine, Yokohama City University Yokohama, Japan.
² Kawasaki City Health and Safety Research Center Kanagawa, Japan.
³ Department of Regenerative and Infectious Pathology, Hamamatsu University School of Medicine Hamamatsu, Japan.
⁴ Infectious Disease Surveillance Center, National Institute of Infectious Diseases Tokyo, Japan.
⁵ Division of Microbiology, Department of Pathology and Microbiology, Nihon University School of Medicine Tokyo, Japan.
⁶ Proteo-Science Center, Ehime University Matsuyama, Japan.

Abstract

Virus-host interactions play vital roles in viral replication and virus-induced pathogenesis. Viruses rely entirely upon host cells to reproduce progeny viruses; however, host factors positively or negatively regulate virus replication by interacting with viral proteins. The elucidation of virus-host protein interaction not only provides a better understanding of the molecular mechanisms by which host cells combat viral infections, but also facilitates the development of new anti-viral therapeutics. Identification of relevant host factors requires techniques that enable comprehensive characterization of virus-host protein interactions. In this study, we developed a proteomic approach to systematically identify human protein kinases that interact potently with viral proteins. For this purpose, we synthesized 412 full-length human protein kinases using the wheat germ cell-free protein synthesis system, and screened them for their association with a virus protein using the amplified luminescent proximity homogenous assay (AlphaScreen). Using this system, we attempted to discover a robust anti-viral host restriction mechanism targeting virus protein X (Vpx) of HIV-2. The screen identified H11/HSPB8 as a Vpx-binding protein that negatively regulates the stability and function of Vpx. Indeed, overexpression of H11/HSPB8 promoted the degradation of Vpx via the ubiquitin-proteasome pathway and inhibited its interaction with SAMHD1, a host restriction factor responsible for blocking replication of HIV. Conversely, targeted knockdown of H11/HSPB8 in human trophoblast cells, which ordinarily express high levels of this protein, restored the expression and function of Vpx, making the cells highly susceptible to viral replication. These results demonstrate that our proteomic approach represents a powerful tool for revealing virus-host interaction not yet identified by conventional methods. Furthermore, we showed that H11/HSPB8 could be a potential host regulatory factor that may prevent placental infection of HIV-2 during pregnancy.

Keywords: AlphaScreen; H11; HIV-2; Vpx; virus–host interaction; wheat germ cell-free protein synthesis.