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大鼠下丘脑的肽酶活性:利用亮氨酸 - 对硝基苯胺监测降解促黄体生成素释放激素的活性。

Peptidase activity in the hypothalamus of the rat: utilization of leucine-p-nitroanilide to monitor the activity degrading luteinizing hormone releasing hormone.

作者信息

Lapp C A, O'Conner J L

出版信息

Biol Reprod. 1984 May;30(4):848-54. doi: 10.1095/biolreprod30.4.848.

Abstract

Previous studies by other investigators have shown that luteinizing hormone releasing hormone (LHRH) and amino acid derivatives of p-nitroanilide are probably degraded by a common enzymatic activity; however, most of these studies are inferential in that they are largely based upon kinetic inhibition data derived from relatively crude tissue preparations. The purpose of this work was to determine whether the synthetic substrate leucine-p- nitroanilide (Leu-p-NA) and LHRH were degraded by the same peptidase activity. Supernatants (10,000 X g) from homogenates of rat hypothalami were eluted from Sephadex G-200, and the resultant fractions were assayed for degrading activity toward LHRH and Leu-p-NA. Radioimmunoassay (RIA) indicated that loss of immunologically active LHRH occurred in the same fractions in which maximal Leu-p-NA degrading activity eluted. Kinetically, exogenous LHRH inhibited degradation of Leu-p-NA in a concentration-dependent manner. When fractions evidencing Leu-p-NA degrading activity were incubated with 125I-LHRH, polyacrylamide gel electrophoresis (PAGE) indicated a time-dependent loss of LHRH with the concomitant production of a radioactive peptide fragment. High-performance liquid chromatography (HPLC) analysis of unlabeled LHRH incubations revealed, within the Leu-p-NA degrading fractions, the formation of two peptide fragments. These studies have further substantiated the likelihood that LHRH and Leu-p-NA are degraded by a common enzyme activity as indicated not only by kinetic inhibition data, but also by cofractionation of activity toward both substrates and by two analytical methods capable of detecting LHRH fragmentation (PAGE and HPLC).

摘要

其他研究人员之前的研究表明,促黄体生成激素释放激素(LHRH)和对硝基苯胺的氨基酸衍生物可能被一种共同的酶活性降解;然而,这些研究大多是推断性的,因为它们很大程度上基于从相对粗糙的组织制备物中获得的动力学抑制数据。这项工作的目的是确定合成底物亮氨酸 - 对硝基苯胺(Leu-p-NA)和LHRH是否被相同的肽酶活性降解。从大鼠下丘脑匀浆的上清液(10,000×g)在Sephadex G - 200上进行洗脱,然后对所得馏分进行针对LHRH和Leu-p-NA的降解活性测定。放射免疫分析(RIA)表明,免疫活性LHRH的损失发生在与最大Leu-p-NA降解活性洗脱相同的馏分中。从动力学角度来看,外源性LHRH以浓度依赖的方式抑制Leu-p-NA的降解。当将显示Leu-p-NA降解活性的馏分与125I - LHRH一起孵育时,聚丙烯酰胺凝胶电泳(PAGE)表明LHRH随时间逐渐损失,同时产生一个放射性肽片段。对未标记的LHRH孵育物进行高效液相色谱(HPLC)分析发现,在Leu-p-NA降解馏分中形成了两个肽片段。这些研究进一步证实了LHRH和Leu-p-NA被一种共同酶活性降解的可能性,这不仅由动力学抑制数据表明,还通过对两种底物的活性共分级以及两种能够检测LHRH片段化的分析方法(PAGE和HPLC)得以证明。

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