4.7 Article

Interaction of Hsp40 with influenza virus M2 protein: implications for PKR signaling pathway

Journal

PROTEIN & CELL
Volume 1, Issue 10, Pages 944-955

Publisher

SPRINGEROPEN
DOI: 10.1007/s13238-010-0115-x

Keywords

M2 protein of influenza virus; Hsp40; P58(IPK); protein interaction; PKR signal pathway

Categories

Funding

  1. National Natural Sciences Foundation of China (NSFC) [30670091, 30599434]
  2. National Basic Research Program (Project 973) of China Ministry of Science and Technology [2011CB504703]
  3. National Key Technologies RD Program [2006BAD06A01]
  4. NSFC Innovative Research Group [81021003]

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Influenza virus contains three integral membrane proteins: haemagglutinin, neuraminidase, and matrix protein (M1 and M2). Among them, M2 protein functions as an ion channel, important for virus uncoating in endosomes of virus-infected cells and essential for virus replication. In an effort to explore potential new functions of M2 in the virus life cycle, we used yeast two-hybrid system to search for M2-associated cellular proteins. One of the positive clones was identified as human Hsp40/Hdj1, a DnaJ/Hsp40 family protein. Here, we report that both BM2 (M2 of influenza B virus) and A/M2 (M2 of influenza A virus) interacted with Hsp40 in vitro and in vivo. The region of M2-Hsp40 interaction has been mapped to the CTD1 domain of Hsp40. Hsp40 has been reported to be a regulator of PKR signaling pathway by interacting with p58(IPK) that is a cellular inhibitor of PKR. PKR is a crucial component of the host defense response against virus infection. We therefore attempted to understand the relationship among M2, Hsp40 and p58(IPK) by further experimentation. The results demonstrated that both A/M2 and BM2 are able to bind to p58(IPK) in vitro and in vivo and enhance PKR autophosphorylation probably via forming a stable complex with Hsp40 and P58(IPK), and consequently induce cell death. These results suggest that influenza virus M2 protein is involved in p58(IPK)-mediated PKR regulation during influenza virus infection, therefore affecting infected-cell life cycle and virus replication.

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