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Protein composition of human prespliceosomes isolated by a tobramycin affinity-selection method

机译:妥布霉素亲和选择法分离人前剪接体的蛋白质组成

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Detailed knowledge of the composition and structure of the spliceo-some and its assembly intermediates is a prerequisite for understanding the complex process of pre-mRNA splicing. To this end, we have developed a tobramycin affinity-selection method that is generally applicable for the purification of native RNP complexes. By using this method, we have isolated human prespliceosomes that are ideally suited for both biochemical and structural studies. MS identified >70 prespliceosome-associated proteins, including nearly all known U1 and U2 snRNP proteins, and expected non-snRNP splicing factors. In addition, the DEAD-box protein p68, RNA helicase A, and a number of proteins that appear to perform multiple functions in the cell, such as YB-1 and TLS, were detected. Several previously uncharacterized proteins of unknown function were also identified, suggesting that they play a role in splicing and potentially act during prespliceosome assembly. These data provide insight into the complexity of the splicing machinery at an early stage of its assembly.
机译:对剪接体及其组装中间体的组成和结构的详细了解是了解mRNA剪接前复杂过程的前提。为此,我们开发了一种妥布霉素亲和力选择方法,该方法通常可用于纯化天然RNP复合物。通过使用这种方法,我们分离出了非常适合生化和结构研究的人前剪接体。 MS鉴定出> 70个剪接体相关蛋白,包括几乎所有已知的U1和U2 snRNP蛋白,以及预期的非snRNP剪接因子。此外,还检测到DEAD-box蛋白p68,RNA解旋酶A和许多似乎在细胞中执行多种功能的蛋白质,例如YB-1和TLS。还鉴定了几种以前未知功能未知的蛋白,表明它们在剪接体组装过程中发挥了剪接作用并可能发挥作用。这些数据可在组装初期对拼接机械的复杂性提供洞察力。

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