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Molecular cloning of human testicular angiotensin-converting enzyme: the testis isozyme is identical to the C-terminal half of endothelial angiotensin-converting enzyme.

机译:人睾丸血管紧张素转化酶的分子克隆:睾丸同工酶与内皮血管紧张素转化酶的C端一半相同。

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摘要

Angiotensin-converting enzyme (ACE; EC 3.4.15.1) is a zinc-containing dipeptidyl carboxypeptidase widely distributed in mammalian tissues and is thought to play a critical role in blood pressure regulation. Testis contains a unique, androgen-dependent ACE isozyme of unknown function. We have determined the cDNA sequence for human testicular ACE; it encodes a protein that is identical, from residue 37 to its C terminus, to the second half or C-terminal domain of the endothelial ACE sequence [Soubrier, F., Alhenc-Gelas, F., Hubert, C., Allegrini, J., John, M., Tregear, G. & Corvol, P. (1988) Proc. Natl. Acad. Sci. USA 85, 9386-9390]. The full-length human testis ACE cDNA was constructed from a composite of cloned cDNAs, obtained by a combination of (i) immunoscreening and hybridization screening of a human testicular cDNA library in lambda gt11 and (ii) hybridization screening of human testis cDNAs constructed with ACE-specific primers and amplified by the polymerase chain reaction. The protein sequence inferred consists of a 732-residue preprotein including a 31-residue signal peptide. The mature polypeptide has a molecular weight of 80,073. The testis enzyme contains the second of the two putative metal-binding sites (His-Glu-Met-Gly-His) identified in endothelial ACE. This indicates that the functionally active catalytic site is within the C-terminal domain of the endothelial enzyme, accounting for the previous finding that these two structurally dissimilar isozymes are virtually identical catalytically. Of 22 testis ACE cDNAs cloned and sequenced, 3 have unique 5' regions, consisting of inserted, deleted, or substituted sequences up to 328 base pairs long, which have apparently arisen by alternative pre-mRNA splicing.
机译:血管紧张素转换酶(ACE; EC 3.4.15.1)是一种含锌的二肽基羧肽酶,广泛分布于哺乳动物组织中,被认为在血压调节中起着至关重要的作用。睾丸含有功能未知的独特的雄激素依赖性ACE同工酶。我们已经确定了人类睾丸ACE的cDNA序列;它编码的蛋白质在内皮ACE序列中从残基37到其C末端,到后半部分或C端结构域都是相同的[Soubrier,F.,Alhenc-Gelas,F.,Hubert,C.,Allegrini, J.,John,M.,Tregear,G.&Corvol,P.(1988)美国国家科学院院刊。 Natl。学院科学美国85,9386-9390]。全长人睾丸ACE cDNA由克隆的cDNA的复合物构建而成,该复合物是通过(i)在λgt11中对人睾丸cDNA文库的免疫筛选和杂交筛选,以及(ii)对构建的人睾丸cDNA进行杂交筛选而获得的ACE特异的引物通过聚合酶链反应而扩增。推测的蛋白质序列由包含31个残基的信号肽的732个残基的前蛋白组成。成熟多肽的分子量为80073。睾丸酶包含在内皮ACE中鉴定的两个假定的金属结合位点中的第二个(His-Glu-Met-Gly-His)。这表明功能活性催化位点在内皮酶的C-末端结构域内,这解释了先前的发现,即这两种结构不同的同工酶在催化上实际上是相同的。在克隆和测序的22种睾丸ACE cDNA中,有3个具有独特的5'区,由长达328个碱基对的插入,缺失或取代序列组成,这显然是由mRNA前期剪接产生的。

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