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Systematical identification of splicing regulatory cis-elements and cognate trans-factors

机译:剪接调控顺式元件和同源反式因子的系统鉴定

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摘要

The majority of human genes undergo alternative splicing to generate multiple isoforms with distinct functions. This process is generally controlled by cis-acting splicing regulatory elements (SREs) that recruit trans-acting factors to promote or inhibit the use of nearby splice sites. The growing interest in understanding the regulatory rules of splicing necessitates the systematic identification of these SREs and their cognate protein factors using experimental and computational approaches. Here we describe a strategy to identify and analyze both cis-acting SREs and trans-acting splicing factors. This strategy involves a cell-based screen to identify SREs from a random sequences library and a modified RNA affinity purification approach to unbiasedly identify the splicing factors. These methods can be adopted to identify splicing enhancers or silencers in both exons and introns, and can be extended to different cultured cells. The resulting SREs and splicing factors can be further analyzed with a series of computational and experimental approaches. This approach will help us to collect a molecular part-list for splicing regulation, providing a rich data source that enables a better understanding of the "splicing code".
机译:大多数人类基因经过选择性剪接,以产生具有不同功能的多种同工型。此过程通常由顺式剪接调节元件(SRE)控制,该元件募集反式作用因子以促进或抑制附近剪接位点的使用。对理解剪接调控规则的兴趣日益浓厚,因此有必要使用实验和计算方法对这些SRE及其同源蛋白因子进行系统鉴定。在这里,我们描述了一种识别和分析顺式SRE和反式剪接因子的策略。该策略涉及从随机序列文库中鉴定SRE的基于细胞的筛选,以及无偏见地鉴定剪接因子的改良RNA亲和纯化方法。这些方法可用于鉴定外显子和内含子中的剪接增强子或沉默子,并可扩展到不同的培养细胞。可以使用一系列计算和实验方法进一步分析所得的SRE和剪接因子。这种方法将帮助我们收集用于拼接调控的分子零件清单,从而提供了丰富的数据源,可以更好地理解“拼接代码”。

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