Sugiyama Takato, Nobuta Risa, Ando Koji, Matsuki Yasuko, Inada Toshifumi
Graduate School of Pharmaceutical Science, Tohoku University, Aoba-ku, Sendai 980-8578, Japan.
Graduate School of Pharmaceutical Science, Tohoku University, Aoba-ku, Sendai 980-8578, Japan.
Biochem Biophys Res Commun. 2017 Jun 17;488(1):122-128. doi: 10.1016/j.bbrc.2017.05.020. Epub 2017 May 5.
Up-frameshift (Upf) complex facilitates the degradation of aberrant mRNAs containing a premature termination codon (PTC) and its products in yeast. Here we report that Sse1, a member of the Hsp110 family, and Hsp70 play a crucial role in Upf-dependent degradation of the truncated FLAG-Pgk1-300 protein derived from PGK1 mRNA harboring a PTC at codon position 300. Sse1 was required for Upf-dependent rapid degradation of the FLAG-Pgk1-300. FLAG-Pgk1-300 was significantly destabilized in ATP hydrolysis defective sse1-1 mutant cells than in wild type cells. Consistently, Sse1 and Hsp70 reduced the level of an insoluble form of FLAG-Pgk1-300. We propose that the Sse1/Hsp70 complex maintains the solubility of FLAG-Pgk1-300, thereby stimulating its Upf-dependent degradation by the proteasomes.
在酵母中,上移码(Upf)复合体促进含有提前终止密码子(PTC)的异常mRNA及其产物的降解。在此,我们报道热休克蛋白110(Hsp110)家族成员Sse1和热休克蛋白70(Hsp70)在Upf依赖的、源自PGK1 mRNA(其在密码子位置300处含有PTC)的截短型FLAG-Pgk1-300蛋白的降解中发挥关键作用。Sse1是Upf依赖的FLAG-Pgk1-300快速降解所必需的。与野生型细胞相比,在ATP水解缺陷型sse1-1突变细胞中,FLAG-Pgk1-300明显不稳定。一致地,Sse1和Hsp70降低了FLAG-Pgk1-300不溶性形式的水平。我们提出,Sse1/Hsp70复合体维持了FLAG-Pgk1-300的溶解性,从而通过蛋白酶体刺激其Upf依赖的降解。
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