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一种用于检测红细胞上补体成分的酶联免疫吸附测定法。

An enzyme-linked immunosorbent assay for the detection of complement components on red blood cells.

作者信息

Sirois M, Chartier C, Brun G, Hamel Y, Petitclerc C, Delage J M

出版信息

Am J Clin Pathol. 1984 Jul;82(1):67-73. doi: 10.1093/ajcp/82.1.67.

Abstract

A new technic using the principle of enzyme-linked immunoassay (ELISA) has been developed for the detection of complement components on red blood cells sensitized in vivo or in vitro. Using a double-antibody technic, anticomplement antisera (anti-C3c or anti-C3c/C3d) produced in rabbits was incubated with the red blood cells, followed by incubation with antirabbit alkaline phosphatase conjugated antiglobulin. The amount of the enzyme fixed was measured spectrophotometrically by the enzymatic hydrolysis of the substrate PNPP. A calibration curve was made from red blood cells on which complement was deposited by the method of Fruitstone . The technic showed a greater sensitivity than the standard antiglobulin tests and allowed simultaneous qualitative and semiquantitative estimates. The technic can be performed in any laboratory equipped with the standard equipment found in a blood bank, including a spectrophotometer. The authors made a modification of Alsever 's solution, which allowed the safe and stable preservation of complement coated red blood cells for 15 days. Significant positive results were obtained clinically using this technic, while negative or weakly positive reactions were obtained by the conventional antiglobulin tests.

摘要

一种利用酶联免疫吸附测定(ELISA)原理的新技术已被开发出来,用于检测体内或体外致敏红细胞上的补体成分。采用双抗体技术,将兔产生的抗补体抗血清(抗C3c或抗C3c/C3d)与红细胞孵育,然后再与抗兔碱性磷酸酶偶联抗球蛋白孵育。通过底物PNPP的酶促水解,用分光光度法测定固定的酶量。用弗鲁斯托内方法在红细胞上沉积补体后制作校准曲线。该技术比标准抗球蛋白试验具有更高的灵敏度,并且可以同时进行定性和半定量评估。该技术可以在任何配备血库标准设备(包括分光光度计)的实验室中进行。作者对阿尔塞弗溶液进行了改良,使得补体包被的红细胞能够安全稳定地保存15天。临床上使用该技术获得了显著的阳性结果,而传统抗球蛋白试验则得到阴性或弱阳性反应。

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