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标记核酶反应位点以追踪哺乳动物细胞中的反式剪接。

Tagging ribozyme reaction sites to follow trans-splicing in mammalian cells.

作者信息

Jones J T, Lee S W, Sullenger B A

机构信息

Department of Experimental Surgery, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Nat Med. 1996 Jun;2(6):643-8. doi: 10.1038/nm0696-643.

Abstract

In mammalian cells, genetic instructions are usually revised by RNA splicing before they are translated to proteins. Here we demonstrate that a trans-splicing group I ribozyme can be employed to intentionally modify the sequence of targeted transcripts in tissue culture cells. By analyzing the ribozyme reaction products, we demonstrate that targeted trans-splicing can proceed in murine fibroblasts with high fidelity, providing direct evidence that ribozymes function as anticipated in a therapeutically relevant setting. Trans-splicing is not very specific however, and the ribozyme reacted with and tagged a variety of cellular transcripts with its 3' exon sequence. RNA tagging provides a unique approach to study RNA catalysis in mammalian cells. Such analysis should facilitate the logical development of safe, therapeutic ribozymes that can repair mutant RNAs associated with a variety of inherited diseases.

摘要

在哺乳动物细胞中,遗传指令通常在被翻译成蛋白质之前通过RNA剪接进行修正。在此我们证明,一种反式剪接I组核酶可用于在组织培养细胞中有意修饰靶向转录本的序列。通过分析核酶反应产物,我们证明靶向反式剪接能够在小鼠成纤维细胞中高保真地进行,提供了直接证据表明核酶在治疗相关环境中按预期发挥作用。然而,反式剪接的特异性不强,该核酶会与其3'外显子序列反应并标记多种细胞转录本。RNA标记为研究哺乳动物细胞中的RNA催化提供了一种独特的方法。这样的分析应该有助于合理开发能够修复与多种遗传性疾病相关的突变RNA的安全治疗性核酶。

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