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从仓鼠胎盘中纯化松弛素及其前体并进行部分特性分析。

Purification and partial characterization of relaxin and relaxin precursors from the hamster placenta.

作者信息

Renegar R H, Owens C R, Chalovich J M

机构信息

Department of Anatomy and Cell Biology, East Carolina University, School of Medicine, Greenville, North Carolina 27858.

出版信息

Biol Reprod. 1993 Jul;49(1):154-61. doi: 10.1095/biolreprod49.1.154.

Abstract

Previous immunological studies have indicated that the molecular structure of hamster relaxin is quite different from that of porcine relaxin. In the present study, hamster relaxin was purified from placentas and characterized in order to investigate its biochemical properties. Placentas from Days 14 and 15 of gestation were homogenized in 0.26 N HCl-62.5% acetone containing protease inhibitors. After centrifugation, soluble proteins were acetone precipitated. Soluble proteins were applied to a carboxymethyl cellulose ion-exchange column and bound proteins were eluted with 0.1 and 0.3 M NaCl. Western blot analysis detected 16.5-, 18.7-, and 36.0-kDa relaxin-immunoreactive (IR) proteins within the 0.1 M NaCl eluant and detected a 5.6-kDa relaxin-IR protein within the 0.3 M NaCl eluant. The 5.6-kDa protein was purified to homogeneity by gel filtration (Sephadex G-50), ion-exchange HPLC, and C18-HPLC. Reduction of the 5.6-kDa protein prior to electrophoresis resulted in a single band of lower molecular mass, suggesting that hamster relaxin consists of two chains of approximately equal molecular mass. Isoelectric point of the 5.6-kDa protein was 7.78. The 16.5- and 18.7-kDa IR proteins were copurified by gel filtration and ion-exchange HPLC. At least five isoelectric point variants were observed for the 16.5- and 18.7-kDa proteins. The N-terminal amino acid for the 5.6 and 18.7 relaxin-IR proteins was arginine, and subsequent cycles indicated an identical partial sequence that was consistent with that for relaxins from other species.

摘要

先前的免疫学研究表明,仓鼠松弛素的分子结构与猪松弛素的分子结构有很大不同。在本研究中,从胎盘纯化仓鼠松弛素并对其进行表征,以研究其生化特性。将妊娠第14天和第15天的胎盘在含有蛋白酶抑制剂的0.26N HCl-62.5%丙酮中匀浆。离心后,将可溶性蛋白质用丙酮沉淀。将可溶性蛋白质应用于羧甲基纤维素离子交换柱,并用0.1和0.3M NaCl洗脱结合的蛋白质。蛋白质印迹分析在0.1M NaCl洗脱液中检测到16.5、18.7和36.0kDa的松弛素免疫反应性(IR)蛋白,在0.3M NaCl洗脱液中检测到5.6kDa的松弛素IR蛋白。通过凝胶过滤(葡聚糖G-50)、离子交换HPLC和C18-HPLC将5.6kDa的蛋白质纯化至同质。电泳前对5.6kDa的蛋白质进行还原,得到一条较低分子量的单条带,表明仓鼠松弛素由两条分子量大致相等的链组成。5.6kDa蛋白质的等电点为7.78。通过凝胶过滤和离子交换HPLC共纯化16.5和18.7kDa的IR蛋白。对于16.5和18.7kDa的蛋白质,观察到至少五个等电点变体。5.6和18.7松弛素IR蛋白的N端氨基酸为精氨酸,随后的循环表明其部分序列相同,与其他物种的松弛素一致。

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