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大鼠肝脏中葡萄糖激酶信使核糖核酸的可变剪接

Alternative splicing of glucokinase mRNA in rat liver.

作者信息

Hayzer D J, Iynedjian P B

机构信息

Department of Medical Biochemistry, University of Geneva School of Medicine, Switzerland.

出版信息

Biochem J. 1990 Aug 15;270(1):261-3. doi: 10.1042/bj2700261.

Abstract

The sequences of two near full-length cDNAs encoding rat liver glucokinase are reported. One of the cDNAs is essentially identical to the cDNA cloned by Andreone, Printz, Pilkis, Magnuson & Granner. [(1989) J. Biol. Chem. 264, 363-369]. The other cDNA contains a 151 bp insertion and a downstream 52 bp deletion. The inserted block of bases has been shown to originate from an optional cassette exon, termed 2A, between the previously described exons 1 and 2. The conceptual translation product from the variant mRNA is identical to the original glucokinase protein for the first 15 amino acids. Next there is a novel polypeptide sequence of 87 residues, comprising 50 residues encoded by the cassette exon and 37 residues specified by an altered reading frame in exon 2. Due to the 52 bp deletion, 17 amino acids of the reference sequence are then missing, after which the sequence reverts to the original. Northern blot analysis with oligonucleotide probes has shown that alternatively spliced mRNA represents about 5% of total glucokinase mRNA. Alternative splicing of glucokinase mRNA in liver may explain earlier findings of minor isoforms of hepatic glucokinase.

摘要

报道了两个编码大鼠肝脏葡萄糖激酶的近全长cDNA序列。其中一个cDNA与Andreone、Printz、Pilkis、Magnuson和Granner克隆的cDNA基本相同。[(1989年)《生物化学杂志》264卷,363 - 369页]。另一个cDNA包含一个151 bp的插入片段和一个下游52 bp的缺失。已证明插入的碱基块源自一个可选的盒式外显子,称为2A,位于先前描述的外显子1和2之间。来自变体mRNA的概念翻译产物在前15个氨基酸上与原始葡萄糖激酶蛋白相同。接下来是一个由87个残基组成的新多肽序列,包括由盒式外显子编码的50个残基和由外显子2中改变的阅读框指定的37个残基。由于52 bp的缺失,参考序列中的17个氨基酸随后缺失,之后序列恢复为原始序列。用寡核苷酸探针进行的Northern印迹分析表明,可变剪接的mRNA约占总葡萄糖激酶mRNA的5%。肝脏中葡萄糖激酶mRNA的可变剪接可能解释了早期关于肝脏葡萄糖激酶小异构体的发现。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cd19/1131708/dae9fec771d2/biochemj00177-0255-a.jpg

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