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一种新的荧光检测系统,用于在凝胶电泳后使用单克隆抗体免疫结合来鉴定变异血红蛋白。

A new fluorescent detection system for identifying variant hemoglobins after gel electrophoresis using immunobinding with monoclonal antibodies.

作者信息

Smith R E

出版信息

J Histochem Cytochem. 1986 May;34(5):585-91. doi: 10.1177/34.5.3084625.

Abstract

This paper describes a low-resolution system for identifying variant hemoglobins with great sensitivity and specificity. After electrophoresis of the hemoglobin sample in a gel, fixation is used to entrap the hemoglobin. The gel is dried, incubated with a monoclonal antibody against the desired hemoglobin, then incubated with a second antibody against the first antibody which is conjugated with the enzyme beta-d-galactosidase. An enzyme overlay membrane containing a fluorogenic substrate is then placed on the gel surface, incubated, and removed, yielding an immunofluorescent print. The entire procedure takes only two hours, and by virtue of fluorescent detection gives sharper band resolution and greater sensitivity than conventional dye methods. The system clearly distinguishes SS sickle-cell hemoglobin from heterozygous and "S-like" hemoglobins. The technique therefore holds promise as a powerful probe for allelic variants.

摘要

本文介绍了一种用于识别变异血红蛋白的低分辨率系统,该系统具有高灵敏度和特异性。在凝胶中对血红蛋白样本进行电泳后,通过固定来捕获血红蛋白。将凝胶干燥,与针对所需血红蛋白的单克隆抗体孵育,然后与针对与β - d - 半乳糖苷酶缀合的第一抗体的第二抗体孵育。然后将含有荧光底物的酶覆盖膜放置在凝胶表面,孵育后移除,从而得到免疫荧光印记。整个过程仅需两小时,并且通过荧光检测,与传统染色方法相比,能提供更清晰的条带分辨率和更高的灵敏度。该系统能够清晰地区分SS镰状细胞血红蛋白与杂合及“类S”血红蛋白。因此,这项技术有望成为一种强大的等位基因变异探测工具。

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