犬胃胰高血糖素原cDNA的克隆

D. Irwin
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引用次数: 6

摘要

在人和大鼠中,相同的胰高血糖素前体的组织特异性蛋白水解处理产生组织特异性胰高血糖素前体衍生肽。相反,在许多非哺乳动物脊椎动物中,不同的mRNA剪接在不同的组织中产生不同的胰高血糖素前体。因此,可选择的mRNA剪接在一定程度上限制了胰高血糖素原衍生肽的选择,这些肽可以通过蛋白水解加工产生。虹鳟和非洲爪蟾胃胰高血糖素原mrna不编码胰高血糖素原衍生肽GLP-2 (glucagon-like peptide 2)。为了确定GLP-2的缺失是否是胃胰高血糖素的普遍特征,我们从狗的胃和胰腺中分离并表征了胰高血糖素前基因,狗是一种在胃中表达胰高血糖素前基因的哺乳动物。在胃和胰腺中分别鉴定出约1100个碱基的胰高血糖素原转录物和约800个碱基的次级转录物。胃胰高血糖素原转录本和胰胰高血糖素原转录本的编码序列相同。因此,组织特异性蛋白水解加工,而不是替代mRNA剪接,必须调节狗胃中组织特异性胰高血糖素原衍生肽的产生。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
cDNA Cloning of Proglucagon from the Stomach and Pancreas of the Dog
In human and rat, tissue-specific proteolytic processing of identical proglucagon precursors yield tissue-specific proglucagon-derived peptides. In contrast, in many non-mammalian vertebrates alternative mRNA splicing yields different proglucagon precursors in different tissues. Thus alternative mRNA splicing, in part, limits the choices of proglucagon-derived peptides that can be produced by proteolytic processing. Stomach proglucagon mRNAs from the rainbow trout and Xenopus laevis were found not to encode the proglucagon-derived peptide glucagon-like peptide 2 (GLP-2). To determine if the absence of GLP-2 was a general feature of stomach proglucagons we isolated and characterized proglucagon cDNAs from the stomach and the pancreas of the dog, a mammal that expresses the proglucagon gene in the stomach. A major proglucagon transcript of about 1100 bases and a minor transcript of about 800 bases were identified in both stomach and pancreas. The coding sequences of both the stomach and pancreatic proglucagon transcripts were identical. Therefore, tissue-specific proteolytic processing, and not alternative mRNA splicing, must regulate the production of tissue-specific proglucagon-derived peptides from the stomach of the dog.
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