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人肾素原加工的分子决定因素。

Molecular determinants of human prorenin processing.

作者信息

Chu W N, Mercure C, Baxter J D, Reudelhuber T L

机构信息

Metabolic Research Unit, University of California, San Francisco.

出版信息

Hypertension. 1992 Dec;20(6):782-7. doi: 10.1161/01.hyp.20.6.782.

DOI:10.1161/01.hyp.20.6.782
PMID:1452293
Abstract

In humans, active renin is generated by the removal of a 43-amino acid prosegment from the zymogen prorenin. This cleavage event is highly specific, occurring at only one of the seven pairs of basic amino acids in the body of preprorenin. This cleavage site selectivity is also displayed by a number of other proteases in vitro and in mouse pituitary AtT-20 cells transfected with a human preprorenin expression vector, suggesting that specificity of cleavage is directed in part by the primary sequence, the higher order structure, or both of prorenin itself. To test this hypothesis, single amino acid mutations were introduced in the region of human preprorenin surrounding the natural cleavage site, and the resultant recombinant proteins were expressed in cultured Chinese hamster ovary and AtT-20 cells. The results suggest that amino acids in addition to the pair of basic amino acids surrounding the cleavage site affect the ability of both trypsin and the endogenous AtT-20 processing enzyme to cleave prorenin. Notably, although a proline at position -4 is essential for processing of prorenin in AtT-20 cells and is correlated with predicted formation of a beta-turn at this position, site-directed mutations suggest that this structural feature in addition to a pair of basic amino acids is not sufficient to lead to proteolytic activation of prorenin. Displacement of sequences surrounding the cleavage site to a position 10 amino acids toward the amino terminus led to partial processing of a mutated prorenin.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在人类中,活性肾素是通过从肾素原酶原中去除一段43个氨基酸的前体片段而产生的。这种切割事件具有高度特异性,仅发生在肾素原前体中的七对碱性氨基酸中的一对处。许多其他蛋白酶在体外以及在转染了人肾素原表达载体的小鼠垂体AtT - 20细胞中也表现出这种切割位点选择性,这表明切割的特异性部分由肾素本身的一级序列、高级结构或两者共同决定。为了验证这一假设,在人肾素原天然切割位点周围的区域引入单氨基酸突变,并在培养的中国仓鼠卵巢细胞和AtT - 20细胞中表达所得的重组蛋白。结果表明,除了切割位点周围的一对碱性氨基酸外,其他氨基酸也会影响胰蛋白酶和内源性AtT - 20加工酶切割肾素原的能力。值得注意的是,尽管 - 4位的脯氨酸对于AtT - 20细胞中肾素原的加工至关重要,并且与该位置预测的β - 转角形成相关,但定点突变表明,除了一对碱性氨基酸外,这种结构特征不足以导致肾素原的蛋白水解激活。将切割位点周围的序列向氨基末端移动10个氨基酸的位置会导致突变肾素原的部分加工。(摘要截短至250字)

相似文献

1
Molecular determinants of human prorenin processing.人肾素原加工的分子决定因素。
Hypertension. 1992 Dec;20(6):782-7. doi: 10.1161/01.hyp.20.6.782.
2
Prorenin processing by cathepsin B in vitro and in transfected cells.组织蛋白酶B在体外及转染细胞中对肾素原的加工处理
FEBS Lett. 1999 Jan 22;443(1):48-52. doi: 10.1016/s0014-5793(98)01672-x.
3
Sequence requirements for prohormone processing in mouse pituitary AtT-20 cells. Analysis using prorenins as model substrates.
Eur J Biochem. 1991 Apr 10;197(1):135-40. doi: 10.1111/j.1432-1033.1991.tb15891.x.
4
A protease processing site is essential for prorenin sorting to the regulated secretory pathway.
J Biol Chem. 1996 Aug 23;271(34):20636-40. doi: 10.1074/jbc.271.34.20636.
5
Cathepsin B is a prorenin processing enzyme.组织蛋白酶B是一种肾素原加工酶。
Hypertension. 1996 Mar;27(3 Pt 2):514-7. doi: 10.1161/01.hyp.27.3.514.
6
A targeting sequence for dense secretory granules resides in the active renin protein moiety of human preprorenin.致密分泌颗粒的靶向序列存在于人类前肾素原的活性肾素蛋白部分中。
Mol Endocrinol. 1990 Dec;4(12):1905-13. doi: 10.1210/mend-4-12-1905.
7
N-linked glycosylation affects the processing of mouse submaxillary gland prorenin in transfected AtT20 cells.N-连接糖基化影响转染的AtT20细胞中小鼠颌下腺肾素原的加工过程。
Eur J Biochem. 1991 Jun 1;198(2):535-40. doi: 10.1111/j.1432-1033.1991.tb16047.x.
8
Sequence requirements for proteolytic cleavage of precursors with paired basic amino acids.具有成对碱性氨基酸的前体蛋白水解切割的序列要求。
Biochem Biophys Res Commun. 1991 Sep 30;179(3):1181-6. doi: 10.1016/0006-291x(91)91696-a.
9
Purification of mouse Ren 2 prorenin produced in Chinese hamster ovary cells.在中国仓鼠卵巢细胞中产生的小鼠肾素2前体的纯化。
J Biochem. 1990 Jun;107(6):854-7. doi: 10.1093/oxfordjournals.jbchem.a123137.
10
Molecular analysis of human prorenin prosegment variants in vitro and in vivo.人肾素原前体片段变体的体外和体内分子分析。
J Biol Chem. 1995 Jul 7;270(27):16355-9. doi: 10.1074/jbc.270.27.16355.