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大豆和菜豆的糖基化种子贮藏蛋白。基因与蛋白质的结构同源性。

The glycosylated seed storage proteins of Glycine max and Phaseolus vulgaris. Structural homologies of genes and proteins.

作者信息

Doyle J J, Schuler M A, Godette W D, Zenger V, Beachy R N, Slightom J L

出版信息

J Biol Chem. 1986 Jul 15;261(20):9228-38.

PMID:3013879
Abstract

Considerable information is now available concerning the 7 S seed storage proteins of legumes and the genes that encode them. Our study compares the gene encoding a beta-type subunit of phaseolin (Pvu beta), the 7 S protein of common bean (Phaseolus vulgaris), with the gene encoding an alpha'-subunit of beta-conglycinin (Gma alpha'), the 7 S protein of soybean (Glycine max). The comparison involves 2880 base pairs of Pvu beta and 3636 base pairs of Gma alpha' and includes approximately 1 kilobase pair of 5'-flanking sequences, and 5' and 3' untranslated sequences, as well as the six exons and five introns that are found to occur in similar positions in both genes. Conserved sequences in the 5'-flanking regions of these genes are discussed in light of their potential regulatory role. Published sequences for 7 S genes of pea (Pisum sativum) permit the inference of the nature and direction of evolutionary change and, in particular, show that the major size difference between the large Gma alpha' polypeptide and the smaller polypeptides of pea and common bean is due to a large insertion in the first exon of Gma alpha'. Comparisons of protein primary structure, potential glycosylation sites, and predicted protein hydropathy show that strongly conserved features of 7 S proteins cut across exon boundaries and that nonconserved regions exist that may have potential for protein modification.

摘要

目前已有大量关于豆科植物7S种子贮藏蛋白及其编码基因的信息。我们的研究将菜豆(Phaseolus vulgaris)的7S蛋白——菜豆球蛋白β型亚基(Pvuβ)的编码基因,与大豆(Glycine max)的7S蛋白——β-伴大豆球蛋白α'-亚基(Gmaα')的编码基因进行了比较。该比较涉及Pvuβ的2880个碱基对和Gmaα'的3636个碱基对,包括约1千碱基对的5'侧翼序列、5'和3'非翻译序列,以及在两个基因相似位置发现的6个外显子和5个内含子。根据这些基因5'侧翼区域的潜在调控作用,对其中的保守序列进行了讨论。豌豆(Pisum sativum)7S基因的已发表序列有助于推断进化变化的性质和方向,特别是表明Gmaα'大多肽与豌豆和菜豆较小多肽之间的主要大小差异是由于Gmaα'第一个外显子中的一个大插入。蛋白质一级结构、潜在糖基化位点和预测的蛋白质亲水性比较表明,7S蛋白的强保守特征跨越外显子边界,并且存在可能具有蛋白质修饰潜力的非保守区域。

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