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首页> 外文期刊>Bioscience Reports >GPKOW is essential for pre-mRNA splicing in?vitro and suppresses splicing defect caused by dominant-negative DHX16 mutation in?vivo
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GPKOW is essential for pre-mRNA splicing in?vitro and suppresses splicing defect caused by dominant-negative DHX16 mutation in?vivo

机译:GPKOW对于在体外进行mRNA前剪接至关重要,并且可以抑制体内显性负DHX16突变引起的剪接缺陷

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摘要

Human GPKOW [G-patch (glycine-rich) domain and KOW (Kyrpides, Ouzounis and Woese) domain] protein contains a G-patch domain and two KOW domains, and is a homologue of Arabidopsis MOS2 and Saccharomyces Spp2 protein. GPKOW is found in the human spliceosome, but its role in pre-mRNA splicing remains to be elucidated. In this report, we showed that GPKOW interacted directly with the DHX16/hPRP2 and with RNA. Immuno-depletion of GPKOW from HeLa nuclear extracts resulted in an inactive spliceosome that still bound DHX16. Adding back recombinant GPKOW restored splicing to the depleted extract. In?vivo, overexpression of GPKOW partially suppressed the splicing defect observed in dominant-negative DHX16 mutant expressing cells. Mutations at the G-patch domain greatly diminished the GPKOW–DHX16 interaction; however, the mutant was active in splicing and was able to suppress splicing defect. Mutations at the KOW1 domain slightly altered the GPKOW–RNA interaction, but the mutant was less functional in?vitro and in?vivo. Our results indicated that GPKOW can functionally impact DHX16 but that interaction between the proteins is not required for this activity.
机译:人GPKOW [G-patch(富含甘氨酸)结构域和KOW(Kyrpides,Ouzounis和Woese)结构域)蛋白包含G-patch结构域和两个KOW结构域,是拟南芥MOS2和酿酒酵母Spp2蛋白的同源物。在人的剪接体中发现了GPKOW,但其在mRNA前剪接中的作用仍有待阐明。在此报告中,我们表明GPKOW与DHX16 / hPRP2和RNA直接相互作用。 HeLa核提取物对GPKOW的免疫耗竭导致仍然结合DHX16的非活性剪接体。加回重组GPKOW,将恢复的剪接结合到耗尽的提取物中。在体内,GPKOW的过表达部分抑制了在显性阴性DHX16突变体表达细胞中观察到的剪接缺陷。 G-patch域的突变大大减少了GPKOW-DHX16的相互作用。但是,该突变体具有剪接活性,并且能够抑制剪接缺陷。 KOW1结构域的突变稍微改变了GPKOW-RNA的相互作用,但该突变体在体内和体内的功能较弱。我们的结果表明,GPKOW可以在功能上影响DHX16,但该活性不需要蛋白质之间的相互作用。

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