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血清蛋白酶的体外作用或酸暴露对血清中可测量的免疫反应性生长调节素C的影响。

Effect of in vitro action of serum proteases or exposure to acid on measurable immunoreactive somatomedin-C in serum.

作者信息

Chatelain P G, Van Wyk J, Copeland K C, Blethen S L, Underwood L E

出版信息

J Clin Endocrinol Metab. 1983 Feb;56(2):376-83. doi: 10.1210/jcem-56-2-376.

Abstract

The proportion of immunoreactive somatomedin-C (IR-Sm-C) in blood that is available for measurement in the RIA is influenced by whether the sample is processed as serum or plasma, by how promptly the sample is chilled and frozen, by whether the reaction is carried out in glass or polystyrene tubes and by whether the incubation mixture contains protamine or heparin. Although protamine buffers and polystyrene tubes increase the availability of purified somatomedin-C (Sm-C), they decrease the detectability of Sm-C in serum. By incubating serum at neutral or acid pH, this IR-Sm-C can be made available for measurement, suggesting that incubation alters the nature of the linkage between Sm-C and its binding proteins or causes a conformational change in the binding protein, resulting in greater exposure of IR-Sm-C. The increment in measurable IR-Sm-C that occurs at neutral pH appears to be due to the action of proteolytic enzymes since it is time, temperature, and pH dependent and is inhibited by a variety of protease inhibitors and chelating agents. The increment which occurs at acid pH is not inhibited by chelating agents or elevated temperature and must be due in part to acid hydrolysis of Sm-C and its binding proteins. However, since the acid-induced increment is optimal within a narrow pH range and falls off sharply below pH 3.5, acid proteases may also be involved. These observations, which provide insight into the nature of the serum proteins with which Sm-C is associated, bear on the interpretation of results of serum somatomedin measurements carried out with different methods. They also may aid in delineating the mechanisms by which the somatomedin contained in the macromolecular complex in serum is made available to tissues.

摘要

放射免疫分析(RIA)中可用于测量的血液中免疫反应性生长调节素-C(IR-Sm-C)比例,受以下因素影响:样本处理为血清还是血浆、样本冷却和冷冻的及时性、反应在玻璃管还是聚苯乙烯管中进行,以及孵育混合物中是否含有鱼精蛋白或肝素。尽管鱼精蛋白缓冲液和聚苯乙烯管可提高纯化生长调节素-C(Sm-C)的可用性,但它们会降低血清中Sm-C的可检测性。通过在中性或酸性pH下孵育血清,这种IR-Sm-C可用于测量,这表明孵育改变了Sm-C与其结合蛋白之间连接的性质,或导致结合蛋白构象变化,从而使IR-Sm-C更多地暴露出来。在中性pH下可测量的IR-Sm-C增加似乎是由于蛋白水解酶的作用,因为它与时间、温度和pH有关,并受到多种蛋白酶抑制剂和螯合剂的抑制。在酸性pH下发生的增加不受螯合剂或温度升高的抑制,部分原因必定是Sm-C及其结合蛋白的酸水解。然而,由于酸诱导的增加在狭窄的pH范围内最佳,且在pH 3.5以下急剧下降,酸性蛋白酶可能也参与其中。这些观察结果有助于深入了解与Sm-C相关的血清蛋白的性质,对不同方法进行的血清生长调节素测量结果的解释具有重要意义。它们还可能有助于阐明血清中大分子复合物中所含生长调节素可供组织利用的机制。

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