Department of Experimental Neurosciences, Fondazione Santa Lucia, Rome, Italy.
Nucleic Acids Res. 2011 Jan;39(2):635-47. doi: 10.1093/nar/gkq797. Epub 2010 Sep 17.
The complex of the yeast Lsm1p-7p proteins with Pat1p is an important mRNA decay factor that is involved in translational shutdown of deadenylated mRNAs and thus prepares these mRNAs for degradation. While the Lsm proteins are highly conserved, there is no unique mammalian homolog of Pat1p. To identify proteins that interact with human LSm1, we developed a novel immunoprecipitation technique that yields virtually pure immunocomplexes. Mass-spec analysis therefore identifies mostly true positives, avoiding tedious functional screening. The method unambiguously identified the Pat1p homolog in HeLa cells, Pat1b. When targeted to a reporter mRNA, Pat1b represses gene expression by inducing deadenylation of the mRNAs. This demonstrates that Pat1b, unlike yPat1p, acts as an mRNA-specific deadenylation factor, highlighting the emerging importance of deadenylation in the mRNA regulation of higher eukaryotes.
酵母 Lsm1p-7p 蛋白与 Pat1p 的复合物是一种重要的 mRNA 降解因子,它参与去腺苷酸化 mRNA 的翻译关闭,从而为这些 mRNA 的降解做准备。虽然 Lsm 蛋白高度保守,但没有独特的哺乳动物 Pat1p 同源物。为了鉴定与人类 LSm1 相互作用的蛋白质,我们开发了一种新的免疫沉淀技术,几乎可以获得纯免疫复合物。因此,质谱分析主要识别真正的阳性结果,避免了繁琐的功能筛选。该方法明确鉴定出 HeLa 细胞中的 Pat1p 同源物 Pat1b。当靶向报告 mRNA 时,Pat1b 通过诱导 mRNA 的去腺苷酸化来抑制基因表达。这表明,Pat1b 不像 yPat1p 那样作为一种 mRNA 特异性去腺苷酸化因子发挥作用,突出了去腺苷酸化在高等真核生物 mRNA 调控中的重要性。
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