| Literature DB >> 24684932 |
Carolyn M Phillips1, Brooke E Montgomery2, Peter C Breen1, Elke F Roovers3, Young-Soo Rim1, Toshiro K Ohsumi1, Martin A Newman1, Josien C van Wolfswinkel4, Rene F Ketting5, Gary Ruvkun6, Taiowa A Montgomery7.
Abstract
More than 2,000 C. elegans genes are targeted for RNA silencing by the mutator complex, a specialized small interfering RNA (siRNA) amplification module which is nucleated by the Q/N-rich protein MUT-16. The mutator complex localizes to Mutator foci adjacent to P granules at the nuclear periphery in germ cells. Here, we show that the DEAD box RNA helicase smut-1 functions redundantly in the mutator pathway with its paralog mut-14 during RNAi. Mutations in both smut-1 and mut-14 also cause widespread loss of endogenous siRNAs. The targets of mut-14 and smut-1 largely overlap with the targets of other mutator class genes; however, the mut-14 smut-1 double mutant and the mut-16 mutant display the most dramatic depletion of siRNAs, suggesting that they act at a similarly early step in siRNA formation. mut-14 and smut-1 are predominantly expressed in the germline and, unlike other mutator class genes, are specifically required for RNAi targeting germline genes. A catalytically inactive, dominant-negative missense mutant of MUT-14 is RNAi defective in vivo; however, mutator complexes containing the mutant protein retain the ability to synthesize siRNAs in vitro. The results point to a role for mut-14 and smut-1 in initiating siRNA amplification in germ cell Mutator foci, possibly through the recruitment or retention of target mRNAs.Entities:
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Year: 2014 PMID: 24684932 PMCID: PMC4010136 DOI: 10.1016/j.cub.2014.02.060
Source DB: PubMed Journal: Curr Biol ISSN: 0960-9822 Impact factor: 10.834