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大鼠血管紧张素原和去(血管紧张素I)血管紧张素原:纯化、特性鉴定及部分测序

Rat angiotensinogen and des(angiotensin I)angiotensinogen: purification, characterization, and partial sequencing.

作者信息

Bouhnik J, Clauser E, Strosberg D, Frenoy J P, Menard J, Corvol P

出版信息

Biochemistry. 1981 Nov 24;20(24):7010-5. doi: 10.1021/bi00527a036.

DOI:10.1021/bi00527a036
PMID:6797467
Abstract

Rat angiotensinogen was completely purified by a six-step procedure including (1) ammonium sulfate precipitation, (2) affinity chromatography on Affi-gel blue, (3) chromatography on DEAE-Sephacel, (4) chromatography on hydroxylapatite, (5) chromatography on Ultrogel AcA 54, and (6) isoelectric focusing. Two peaks of pure angiotensinogen were obtained, distinguishable by their isoelectric points (4.55 and 4.75). Both contained 23 microgram of angiotensin I/mg of protein. Sodium dodecyl sulfate--polyacrylamide gel electrophoresis of the peak with pI = 4.55 revealed two protein bands (respectively Mr 57000 and 59000) and a single protein band (Mr 57000) for the peak with pI = 4.75. The molecular weight of the latter homogeneous form, as determined by sedimentation equilibrium, was 55000. Only one immunoprecipitin line was observed when antiserum reacted with the heterogeneous angiotensinogen in Ouchterlony gels. The first 17 amino acids of the N-terminal region of the angiotensinogen with pI = 4.75 are reported. The amino acids in positions 10 and 11 which correspond to the renin cleavage site are leucyl-leucyl. The des(angiotensin I)angiotensinogen obtained after hydrolysis of angiotensinogen with pure mouse submaxillary gland renin was found to consist of a single protein band with an Mr of 56000 as revealed by sodium dodecyl sulfate--polyacrylamide gel electrophoresis. Only one N-terminal residue (leucyl) was obtained for this des(angiotensin I)angiotensinogen. These findings establish that renin only cleaves angiotensinogen at a single site.

摘要

大鼠血管紧张素原通过六步程序完全纯化,包括:(1)硫酸铵沉淀;(2)Affi - 凝胶蓝亲和层析;(3)DEAE - 葡聚糖凝胶层析;(4)羟基磷灰石层析;(5)Ultrogel AcA 54层析;(6)等电聚焦。获得了两个纯血管紧张素原峰,可通过它们的等电点(4.55和4.75)区分。两者每毫克蛋白质均含23微克血管紧张素I。十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳显示,等电点为4.55的峰有两条蛋白带(分别为Mr 57000和59000),等电点为4.75的峰有一条单一蛋白带(Mr 57000)。通过沉降平衡测定,后一种均一形式的分子量为55000。当抗血清与Ouchterlony凝胶中的异质血管紧张素原反应时,仅观察到一条免疫沉淀线。报告了等电点为4.75的血管紧张素原N端区域的前17个氨基酸。对应于肾素裂解位点的第10和11位氨基酸是亮氨酰 - 亮氨酰。用纯小鼠颌下腺肾素水解血管紧张素原后得到的去(血管紧张素I)血管紧张素原,经十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳显示由一条Mr为56000的单一蛋白带组成。该去(血管紧张素I)血管紧张素原仅获得一个N端残基(亮氨酰)。这些发现证实肾素仅在一个位点裂解血管紧张素原。

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