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载脂蛋白B信使核糖核酸的核糖核酸编辑。体外偶联转录编辑确定的序列特异性。

RNA editing of apolipoprotein B mRNA. Sequence specificity determined by in vitro coupled transcription editing.

作者信息

Chen S H, Li X X, Liao W S, Wu J H, Chan L

机构信息

Department of Cell Biology, Baylor College of Medicine, Houston, Texas 77030.

出版信息

J Biol Chem. 1990 Apr 25;265(12):6811-6.

PMID:2324099
Abstract

Apolipoprotein (apo) B-48 mRNA is produced by in vivo RNA editing which involves a C----U conversion of the first base of the codon CAA for Gln-2153, changing it to UAA, an in-frame stop codon. We have reproduced the editing reaction in vitro using nuclear extracts. Efficient RNA editing was demonstrated by using apoB mRNA segments as substrate or in a coupled transcription-editing reaction using apoB minigenes as template. ApoB minigenes were constructed by ligating the adenovirus major late promoter to a fragment of apoB-100 DNA containing the editing site and used for the transcription-editing reaction. We defined the sequence specificity of the editing reaction using site-specific single and multiple base mutants constructed by the polymerase chain reaction. Among 22 different mutant apoB-100 minigene constructs containing mutations in the bases immediately flanking the edited C-6666, 20 were edited in the coupled transcription-editing reaction. The results suggest a relatively lax sequence specificity for apoB mRNA editing. Our observation may have important implications for apoB-48 biogenesis as well as for the editing process as a general biologic regulatory mechanism.

摘要

载脂蛋白(apo)B - 48信使核糖核酸(mRNA)是通过体内RNA编辑产生的,该编辑涉及密码子CAA(对应谷氨酰胺-2153)的第一个碱基由C向U的转换,将其变为UAA,这是一个框内终止密码子。我们利用核提取物在体外重现了编辑反应。通过使用apoB mRNA片段作为底物或在以apoB小基因作为模板的转录-编辑偶联反应中,证明了高效的RNA编辑。通过将腺病毒主要晚期启动子连接到包含编辑位点的apoB - 100 DNA片段上构建apoB小基因,并将其用于转录-编辑反应。我们使用通过聚合酶链反应构建的位点特异性单碱基和多碱基突变体来确定编辑反应的序列特异性。在22种不同的突变apoB - 100小基因构建体中,这些构建体在紧邻编辑的C - 6666的碱基处含有突变,其中20种在转录-编辑偶联反应中被编辑。结果表明apoB mRNA编辑的序列特异性相对宽松。我们的观察结果可能对apoB - 48的生物合成以及作为一种普遍生物学调节机制的编辑过程具有重要意义。

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