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经修饰的U7小核RNA对前体mRNA剪接模式的稳定改变。

Stable alteration of pre-mRNA splicing patterns by modified U7 small nuclear RNAs.

作者信息

Gorman L, Suter D, Emerick V, Schümperli D, Kole R

机构信息

Lineberger Comprehensive Cancer Center and Department of Pharmacology, University of North Carolina, Chapel Hill, NC 27599, USA.

出版信息

Proc Natl Acad Sci U S A. 1998 Apr 28;95(9):4929-34. doi: 10.1073/pnas.95.9.4929.

Abstract

In several forms of beta-thalassemia, mutations in the second intron of the beta-globin gene create aberrant 5' splice sites and activate a common cryptic 3' splice site upstream. As a result, the thalassemic beta-globin pre-mRNAs are spliced almost exclusively via the aberrant splice sites leading to a deficiency of correctly spliced beta-globin mRNA and, consequently, beta-globin. We have designed a series of vectors that express modified U7 snRNAs containing sequences antisense to either the aberrant 5' or 3' splice sites in the IVS2-705 thalassemic pre-mRNA. Transient expression of modified U7 snRNAs in a HeLa cell line stably expressing the IVS2-705 beta-globin gene restored up to 65% of correct splicing in a sequence-specific and dose-dependent manner. Cell lines that stably coexpressed IVS2-705 pre-mRNA and appropriately modified U7 snRNA exhibited up to 55% of permanent restoration of correct splicing and expression of full-length beta-globin protein. This novel approach provides a potential alternative to gene replacement therapies.

摘要

在几种β地中海贫血形式中,β珠蛋白基因第二个内含子中的突变会产生异常的5'剪接位点,并激活上游一个常见的隐蔽3'剪接位点。结果,地中海贫血β珠蛋白前体mRNA几乎完全通过异常剪接位点进行剪接,导致正确剪接的β珠蛋白mRNA缺乏,进而导致β珠蛋白缺乏。我们设计了一系列载体,这些载体表达修饰的U7小核仁RNA,其包含与IVS2 - 705地中海贫血前体mRNA中异常的5'或3'剪接位点反义的序列。在稳定表达IVS2 - 705β珠蛋白基因的HeLa细胞系中瞬时表达修饰的U7小核仁RNA,以序列特异性和剂量依赖性方式恢复了高达65%的正确剪接。稳定共表达IVS2 - 705前体mRNA和适当修饰的U7小核仁RNA的细胞系显示,正确剪接和全长β珠蛋白蛋白表达的永久恢复率高达55%。这种新方法为基因替代疗法提供了一种潜在的替代方案。

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