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[应用双抗体放射免疫分析法测定缓激肽的研究]

[The research of radioimmunoassay using double Abs for bradykinin].

作者信息

Cheng J, Wang L, Duan J, Han F, Wang Z

机构信息

Institute of Basic Medical Sciences, CAMS, Beijing.

出版信息

Zhongguo Yi Xue Ke Xue Yuan Xue Bao. 1996 Dec;18(6):411-5.

PMID:9388945
Abstract

Bradykinin (BK) is a potent vasodilative substance, and plays great physiological and pathological roles in animals and human beings. To measure the quantity of BK, the radioimmunoassay (RIA) has been devised, but the traditional RIA method has certain defects, such as presence of numerows interfering factors and errors and time consuming. Now, we produce anti-BK serum in rabbits by using BK-ovalbumin conjugate as an immunogen, and the 125I labeled Tyr8-BK by using a modified chloramine-T method. High specific activity has been obtained after purification with DEAE-Sephadex A-25 column chromatography. We use the donkey anti-rabbit Ab and PEG 6000 to separate the bound from the free 125I-Tyr8-BK. The limitation range of standard curve is from 25 to 1600 pg, NSB is 3.1% affinity constant (K) is 0.8 x 10(10) L/mol, and there is no significant interference with other biological BK analogues. The blood samples are treated by adding Polybrene (inhibitor) and PEG 6000 to deposit the big serum proteins in order to reduce the disturbing substances. This method has been shown to be a sensitive, specific, reliable, simple and convenient measure of the serum BK level. By this method, the serum BK quantities in men, women and rats are respectively 1584 +/- 347 pg/ml, 1642 +/- 302 pg/ml and 1805 +/- 225 pg/ml, the recycling rate is 95%, the intergroup CV is 5.0% and outergroup CV = 9.2%.

摘要

缓激肽(BK)是一种强效血管舒张物质,在动物和人类中发挥着重要的生理和病理作用。为了测定BK的量,人们设计了放射免疫分析(RIA)方法,但传统的RIA方法存在一些缺陷,如存在众多干扰因素、误差大且耗时。现在,我们以BK - 卵清蛋白偶联物作为免疫原在兔体内制备抗BK血清,并采用改良氯胺 - T法制备125I标记的Tyr8 - BK。经DEAE - 葡聚糖A - 25柱层析纯化后获得了高比活性。我们使用驴抗兔抗体和聚乙二醇6000(PEG 6000)来分离结合态和游离态的125I - Tyr8 - BK。标准曲线的线性范围为25至1600 pg,非特异性结合(NSB)为3.1%,亲和常数(K)为0.8×10(10) L/mol,并且对其他生物BK类似物无明显干扰。血液样本通过添加鱼精蛋白(抑制剂)和PEG 6000进行处理,以沉淀大分子血清蛋白,从而减少干扰物质。该方法已被证明是一种灵敏、特异、可靠、简便且方便的测定血清BK水平的方法。通过该方法,男性、女性和大鼠血清中的BK量分别为1584±347 pg/ml、1642±302 pg/ml和1805±225 pg/ml,回收率为95%,组内变异系数(CV)为5.0%,组间变异系数(CV)= 9.2%。

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