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Structure of the yeast Pml1 splicing factor and its integration into the RES complex

机译:酵母Pml1剪接因子的结构及其整合到RES复合物中

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The RES complex was previously identified in yeast as a splicing factor affecting nuclear pre-mRNA retention. This complex was shown to contain three subunits, namely Snu17, Bud13 and Pml1, but its mode of action remains ill-defined. To obtain insights into its function, we have performed a structural investigation of this factor. Production of a short N-terminal truncation of residues that are apparently disordered allowed us to determine the X-ray crystallographic structure of Pml1. This demonstrated that it consists mainly of a FHA domain, a fold which has been shown to mediate interactions with phosphothreonine-containing peptides. Using a new sensitive assay based on alternative splice-site choice, we show, however, that mutation of the putative phosphothreonine-binding pocket of Pml1 does not affect pre-mRNA splicing. We have also investigated how Pml1 integrates into the RES complex. Production of recombinant complexes, combined with serial truncation and mutagenesis of their subunits, indicated that Pml1 binds to Snu17, which itself contacts Bud13. This analysis allowed us to demarcate the binding sites involved in the formation of this assembly. We propose a model of the organization of the RES complex based on these results, and discuss the functional consequences of this architecture.
机译:RES复合物先前已在酵母中鉴定为影响核前mRNA保留的剪接因子。已显示该复合物包含三个亚基,即Snu17,Bud13和Pml1,但其作用方式仍不清楚。为了深入了解其功能,我们对这一因素进行了结构研究。产生明显无序的残基的短N端截短可以使我们确定Pml1的X射线晶体结构。这表明它主要由FHA结构域组成,该结构域已被证明能介导与含磷酸苏氨酸的肽相互作用。然而,使用基于替代剪接位点选择的新的灵敏测定,我们显示了Pml1的磷酸苏氨酸结合口袋的突变不会影响mRNA的剪接。我们还研究了Pml1如何整合到RES复合物中。重组复合物的生产,结合其亚基的连续截短和诱变,表明Pml1与Snu17结合,而Snu17本身与Bud13接触。该分析使我们能够划定参与该装配体形成的结合位点。我们根据这些结果提出了RES复杂系统的组织模型,并讨论了该体系结构的功能后果。

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