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Assembly of Snu114 into U5 snRNP requires Prp8 and a functional GTPase domain

机译:将Snu114组装到U5 snRNP中需要Prp8和功能性GTPase结构域

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摘要

Snu114 is a U5 snRNP protein essential for pre-mRNA splicing. Based on its homology with the ribosomal translocase EF-G, it is thought that GTP hydrolysis by Snu114 induces conformational rearrangements in the spliceosome. We recently identified allele-specific genetic interactions between SNU114 and genes encoding three other U5 snRNP components, Prp8 and two RNA-dependent ATPases, Prp28 and Brr2, required for destabilization of U1 and U4 snRNPs prior to catalysis. To shed more light onto the function of Snu114, we have now directly analyzed snRNP and spliceosome assembly in SNU114 mutant extracts. The Snu114–60 C-terminal truncation mutant, which is synthetically lethal with the ATPase mutants prp28–1 and brr2–1, assembles spliceosomes but subsequently blocks U4 snRNP release. Conversely, mutants in the GTPase domain fail to assemble U5 snRNPs. These mutations prevent the interaction of Snu114 with Prp8 as well as with U5 snRNA. Since Prp8 is thought to regulate the activity of the DEAD-box ATPases, this strategy of snRNP assembly could ensure that Prp8 activity is itself regulated by a GTP-dependent mechanism.
机译:Snu114是U5 snRNP蛋白,对mRNA的预剪接至关重要。基于其与核糖体转座酶EF-G的同源性,认为Snu114的GTP水解在剪接体中诱导构象重排。最近,我们确定了SNU114与编码其他三个U5 snRNP组件Prp8和两个RNA依赖性ATPases Prp28和Brr2的基因之间的等位基因特异性遗传相互作用,这些催化作用需要在催化之前使U1和U4 snRNP不稳定。为了更加了解Snu114的功能,我们现在直接分析了SNU114突变体提取物中的snRNP和剪接体组装。 Snu114–60 C端截短突变体与ATPase突变体prp28–1和brr2–1合成致命,它组装了剪接体,但随后阻止了U4 snRNP的释放。相反,GTPase域中的突变体无法组装U5 snRNP。这些突变阻止了Snu114与Prp8以及与U5 snRNA的相互作用。由于认为Prp8可以调节DEAD-box ATPase的活性,因此snRNP组装的这种策略可以确保Prp8的活性本身受GTP依赖性机制的调节。

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