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正常和突变的人β-珠蛋白前体mRNA在体外能够被准确且高效地剪接。

Normal and mutant human beta-globin pre-mRNAs are faithfully and efficiently spliced in vitro.

作者信息

Krainer A R, Maniatis T, Ruskin B, Green M R

出版信息

Cell. 1984 Apr;36(4):993-1005. doi: 10.1016/0092-8674(84)90049-7.

Abstract

Human beta-globin mRNA precursors (pre-mRNAs) synthesized in vitro from a bacteriophage SP6 promoter/beta-globin gene fusion are accurately and efficiently spliced when added to a HeLa cell nuclear extract. Under optimal conditions, the first intervening sequence (IVS 1) is removed by splicing in up to 90% of the input pre-mRNA. Splicing requires ATP and in its absence the pre-mRNA is neither spliced nor cleaved at splice junctions. Splicing does not require that the pre-mRNA contain a correct 5' or 3' end, a 3' poly A tail, or a 5'-terminal cap structure. However, capping of the pre-mRNA significantly affects the specificity of in vitro processing. In the absence of a cap approximately 30%-40% of the pre-mRNA is accurately spliced, and a number of aberrantly cleaved RNAs are also detected. In contrast, capped pre-mRNAs are spliced more efficiently and produce fewer aberrant RNA species. The specificity of splice-site selection in vitro was tested by analyzing pre-mRNAs that contain beta-thalassemia splicing mutations in IVS 1. Remarkably, these mutations cause the same abnormal splicing events in vitro and in vivo. The ability to synthesize mutant pre-mRNAs and study their splicing in a faithful in vitro system provides a powerful approach to determine the mechanisms of RNA splice-site selection.

摘要

从噬菌体SP6启动子/β-珠蛋白基因融合体体外合成的人β-珠蛋白mRNA前体(前体mRNA),添加到HeLa细胞核提取物中时能被准确且高效地剪接。在最佳条件下,高达90%的输入前体mRNA通过剪接去除了第一个内含子序列(IVS 1)。剪接需要ATP,缺乏ATP时,前体mRNA在剪接位点既不被剪接也不被切割。剪接并不要求前体mRNA含有正确的5'或3'末端、3'多聚A尾或5'-末端帽结构。然而,前体mRNA的加帽显著影响体外加工的特异性。在没有帽的情况下,约30%-40%的前体mRNA被准确剪接,同时也检测到一些异常切割的RNA。相比之下,加帽的前体mRNA剪接更高效,产生的异常RNA种类更少。通过分析在IVS 1中含有β-地中海贫血剪接突变的前体mRNA,测试了体外剪接位点选择的特异性。值得注意的是,这些突变在体外和体内导致相同的异常剪接事件。合成突变前体mRNA并在可靠的体外系统中研究其剪接的能力,为确定RNA剪接位点选择机制提供了一种强大的方法。

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