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A homolog of lariat-debranching enzyme modulates turnover of branched RNA

机译:套索解脱酶的同源物调节分支RNA的周转

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Turnover of the branched RNA intermediates and products of pre-mRNA splicing is mediated by the lariat-debranching enzyme Dbr1. We characterized a homolog of Dbr1 from Saccharomyces cerevisiae, Drn1/Ygr093w, that has a pseudo-metallophosphodiesterase domain with primary sequence homology to Dbr1 but lacks essential active site residues found in Dbr1. Whereas loss of Dbr1 results in lariat-introns failing broadly to turnover, loss of Drn1 causes low levels of lariat-intron accumulation. Conserved residues in the Drn1 C-terminal CwfJ domains, which are not present in Dbr1, are required for efficient intron turnover. Drn1 interacts with Dbr1, components of the Nineteen Complex, U2 snRNA, branched intermediates, and products of splicing. Drn1 enhances debranching catalyzed by Dbr1 in vitro, but does so without significantly improving the affinity of Dbr1 for branched RNA. Splicing carried out in in vitro extracts in the absence of Drn1 results in an accumulation of branched splicing intermediates and products released from the spliceosome, likely due to less active debranching, as well as the promiscuous release of cleaved 5′-exon. Drn1 enhances Dbr1-mediated turnover of lariat-intermediates and lariat-intron products, indicating that branched RNA turnover is regulated at multiple steps during splicing.
机译:套索状脱支酶Dbr1介导分支RNA中间体和mRNA前体剪接产物的周转。我们表征了来自酿酒酵母Drn1 / Ygr093w的Dbr1的同源物,它具有与Dbr1具有基本序列同源性的伪金属磷酸二酯酶结构域,但缺少在Dbr1中发现的基本活性位点残基。 Dbr1的丢失会导致套索内含子广泛丧失营业额,而Drn1的丢失会导致套索内含子-内含子积累水平低下。有效的内含子周转需要Drn1 C末端CwfJ域中的保守残基,而Dbr1中不存在这些残基。 Drn1与Dbr1,十九复合体的成分,U2 snRNA,分支中间体和剪接产物相互作用。 Drn1增强了Dbr1在体外催化的去分支作用,但并没有显着提高Dbr1对分支RNA的亲和力。在没有Drn1的情况下在体外提取物中进行的剪接导致积累的分支剪接中间体和产物从剪接体中释放出来,这可能是由于活性低的分支作用以及裂解的5'-外显子的混杂释放所致。 Drn1增强了Dbr1介导的套索中间体和套索内含子产物的转运,表明分支的RNA转运在剪接过程中的多个步骤受到调节。

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