A1 Refereed original research article in a scientific journal

Elimination of phosphorylation sites of Semliki Forest virus replicase protein nsP3.




AuthorsVihinen H, Ahola T, Tuittila M, Merits A, Kääriäinen L

Publication year2001

JournalJournal of Biological Chemistry

Journal name in sourceThe Journal of biological chemistry

Journal acronymJ Biol Chem

Volume276

Issue8

First page 5745

Last page52

Number of pages8

ISSN0021-9258

DOIhttps://doi.org/10.1074/jbc.M006077200


Abstract
nsP3 is one of the four RNA replicase subunits encoded by alphaviruses. The specific essential functions of nsP3 remain unknown, but it is known to be phosphorylated on serine and threonine residues. Here we have completed mapping of the individual phosphorylation sites on Semliki Forest virus nsP3 (482 amino acids) by point mutational analysis of threonine residues. This showed that threonines 344 and 345 represented the major threonine phosphorylation sites in nsP3. Experiments with deletion variants suggested that nsP3 itself had no kinase activity; instead, it was likely to be phosphorylated by multiple cellular kinases. Phosphorylation was not necessary for the peripheral membrane association of nsP3, which was mediated by the N-terminal region preceding the phosphorylation sites. Two deletion variants of nsP3 with either reduced or undetectable phosphorylation were studied in the context of virus infection. Cells infected with mutant viruses produced close to wild type levels of infectious virions; however, the rate of viral RNA synthesis was significantly reduced in the mutants. A virus totally defective in nsP3 phosphorylation and exhibiting a decreased rate of RNA synthesis also exhibited greatly reduced pathogenicity in mice.



Last updated on 2024-26-11 at 22:05