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牛肾上腺髓质多巴胺-β-羟化酶的分子克隆、结构与表达

Molecular cloning, structure, and expression of dopamine-beta-hydroxylase from bovine adrenal medulla.

作者信息

Wu H J, Parmer R J, Koop A H, Rozansky D J, O'Connor D T

机构信息

Department of Medicine, University of California, San Diego.

出版信息

J Neurochem. 1990 Jul;55(1):97-105. doi: 10.1111/j.1471-4159.1990.tb08826.x.

DOI:10.1111/j.1471-4159.1990.tb08826.x
PMID:1693949
Abstract

Dopamine-beta-hydroxylase (DBH), the enzyme that catalyzes the conversion of dopamine to norepinephrine, remains the topic of many unanswered questions. We isolated DBH cDNA clones from a bovine adrenal medulla cDNA library in the vector lambda gt10. The longest cDNA had an open reading frame encoding an entire mature DBH 578 amino acid (64,808 dalton) polypeptide chain, though lacking a portion of the signal peptide. Additional 5' clones, obtained by the polymerase chain reaction, established the sequence of a 19 amino acid signal peptide. The mature protein sequence was 84% homologous to that of human pheochromocytoma DBH, including preservation of four potential copper ligand sites (HH or HXH) and substrate binding domains. There were no hydrophobic (putative membrane spanning) domains, other than the signal peptide. All available DBH peptide and protein sequence data can be accounted for by the cDNA-deduced 578 amino acid mature protein primary structure. Prokaryotic DBH expression yielded a 65-kilodalton DBH-immunoreactive peptide that differed from eukaryotic adrenal DBH only in N-linked, endoglycosidase F-sensitive glycosylation in the latter. Southern analysis suggested one DBH gene, whereas Northern analysis suggested a single 2.6 kbp tissue-specific DBH transcript. Comparison of the DBH primary structure with other reported sequences [Protein Identification Resource (PIR), New Atlas (NEWAT)] did not indicate that DBH is a member of any known gene family. The results suggest that a single DBH gene encodes a message specifying a single DBH polypeptide chain.

摘要

多巴胺-β-羟化酶(DBH)是催化多巴胺转化为去甲肾上腺素的酶,仍然是许多未解问题的主题。我们从载体λgt10中的牛肾上腺髓质cDNA文库中分离出DBH cDNA克隆。最长的cDNA具有一个开放阅读框,编码一条完整的成熟DBH 578个氨基酸(64,808道尔顿)的多肽链,不过缺少一部分信号肽。通过聚合酶链反应获得的额外5'端克隆确定了一个19个氨基酸的信号肽序列。成熟蛋白序列与人类嗜铬细胞瘤DBH的序列同源性为84%,包括保留了四个潜在的铜配体位点(HH或HXH)和底物结合结构域。除了信号肽外,没有其他疏水(假定的跨膜)结构域。所有可用的DBH肽和蛋白质序列数据都可以由cDNA推导的578个氨基酸的成熟蛋白一级结构来解释。原核DBH表达产生了一个65千道尔顿的DBH免疫反应性肽,它与真核肾上腺DBH的区别仅在于后者的N-连接、内切糖苷酶F敏感的糖基化。Southern分析表明有一个DBH基因,而Northern分析表明有一个单一的2.6 kb组织特异性DBH转录本。将DBH一级结构与其他已报道的序列[蛋白质鉴定资源(PIR)、新图谱(NEWAT)]进行比较,并未表明DBH是任何已知基因家族的成员。结果表明单个DBH基因编码一个指定单一DBH多肽链的信息。

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