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秀丽隐杆线虫中特定let-7微小RNA结合复合物的鉴定。

Identification of specific let-7 microRNA binding complexes in Caenorhabditis elegans.

作者信息

Chan Shih-Peng, Ramaswamy Gopalakrishna, Choi Eun-Young, Slack Frank J

机构信息

Department of Molecular, Cellular and Developmental Biology, Yale University, New Haven, Connecticut 06520, USA.

出版信息

RNA. 2008 Oct;14(10):2104-14. doi: 10.1261/rna.551208. Epub 2008 Aug 21.

Abstract

Little is known about the protein complexes required for microRNA formation and function. Here we used native gel electrophoresis to identify miRNA ribonucleoprotein complexes (miRNPs) in Caenorhabditis elegans. Our data reveal multiple distinct miRNPs that assemble on the let-7 miRNA in vitro. The formation of these complexes is affected but not abolished by alg-1 or alg-2 null mutations. The largest complex (M*) with an estimated molecular mass of >669 kDa cofractionates with the known RISC factors ALG-1, VIG-1, and TSN-1. The M* complex and two complexes, M3 and M4, with similar molecular weights of approximately 500 kDa, also assemble on all other miRNAs used in our experiments. Two smaller complexes, M1 (approximately 160 kDa) and M2 (approximately 250 kDa), assemble on the members of the let-7 miRNAs family but not lin-4 or mir-234, and their formation is highly dependent on specific sequences in the 5' seed region of let-7. Moreover, an unidentified protein, p40, which only appears in the M1 and M2 complexes, was detected by UV triggered cross-linking to let-7 but not to lin-4. The cross-linking of p40 to let-7 is also dependent on the let-7 sequence. Another unidentified protein, p13, is detected in all let-7 binding complexes and lin-4 cross-linked products. Our data suggest that besides being present in certain large miRNPs with sizes similar to reported RISC, the let-7 miRNA also assembles with specific binding proteins and forms distinct small complexes.

摘要

关于微小RNA形成和功能所需的蛋白质复合物,我们了解得还很少。在这里,我们使用非变性凝胶电泳来鉴定秀丽隐杆线虫中的微小RNA核糖核蛋白复合物(miRNP)。我们的数据揭示了在体外组装在let-7微小RNA上的多种不同的miRNP。这些复合物的形成受到alg-1或alg-2基因敲除突变的影响,但并未被消除。估计分子量>669 kDa的最大复合物(M*)与已知的RNA诱导沉默复合体(RISC)因子ALG-1、VIG-1和TSN-1共分离。M*复合物以及另外两个分子量相似、约为500 kDa的复合物M3和M4,也在我们实验中使用的所有其他微小RNA上组装。两个较小的复合物M1(约160 kDa)和M2(约250 kDa)在let-7微小RNA家族成员上组装,但不在lin-4或mir-234上组装,并且它们的形成高度依赖于let-7 5'种子区域中的特定序列。此外,通过紫外线触发交联到let-7而非lin-4检测到一种未鉴定的蛋白质p40,它仅出现在M1和M2复合物中。p40与let-7的交联也依赖于let-7序列。在所有let-7结合复合物和lin-4交联产物中检测到另一种未鉴定的蛋白质p13。我们的数据表明,除了存在于某些大小与报道的RISC相似的大型miRNP中,let-7微小RNA还与特定的结合蛋白组装并形成不同的小复合物。

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