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通过免疫组织化学对组织切片中的酶进行定位。传统抗体和混合聚集技术。

The localization of enzymes in tissue sections by immuno-histochemistry. Conventional antibody and mixed aggregation techniques.

作者信息

Wachsmuth E D

出版信息

Histochem J. 1976 May;8(3):253-70. doi: 10.1007/BF01003815.

Abstract

Methods for detecting enzymes in tissue sections by antibody techniques are reviewed. In all these techniques, sections are first incubated with antibody. The bound antibody is visualized in one of four ways: identifying a label such as fluorescein linked to the antibody; using a labelled anti-antibody; employing complement and labelled anti-complement; or making use of a mixed aggregation immuno-cytochemical method. The last technique consists of three steps. A section is first incubated with antiserum, and secondly with the soluble enzyme under investigation. Thirdly the desired enzyme is "stained" using a conventional cytochemical method. The method is specific since, for example, the soluble enzyme used in the second step can bind only to antigenic determinants which are identical to those of the enzyme localized in the tissue. Thus purification of antigen and antibody sources is simplified, and chemical modifications of the antigen and antibody are avoided. Antibody also acts as a selective fixative for tissue antigen. It will inhibit the catalytic activity of its antigen and, in this way, permit the enzyme activity arising after the reaction of tissue enzyme-antibody complex with soluble enzyme to be amplified selectively. The mixed aggregation immuno-cytochemical technique has been used successfully with membrane-bound enzymes and cytoplasmic enzymes and for the demostration of catalytically inactive enzyme precursors.

摘要

本文综述了通过抗体技术检测组织切片中酶的方法。在所有这些技术中,首先将切片与抗体孵育。结合的抗体通过以下四种方式之一进行可视化:识别与抗体相连的荧光素等标记物;使用标记的抗抗体;使用补体和标记的抗补体;或利用混合聚集免疫细胞化学方法。最后一种技术包括三个步骤。首先将切片与抗血清孵育,其次与所研究的可溶性酶孵育。第三步,使用传统的细胞化学方法对所需的酶进行“染色”。该方法具有特异性,例如,第二步中使用的可溶性酶只能与与组织中定位的酶相同的抗原决定簇结合。因此,简化了抗原和抗体来源的纯化,并避免了抗原和抗体的化学修饰。抗体还可作为组织抗原的选择性固定剂。它会抑制其抗原的催化活性,并以这种方式选择性地放大组织酶-抗体复合物与可溶性酶反应后产生的酶活性。混合聚集免疫细胞化学技术已成功用于膜结合酶和细胞质酶,并用于证明无催化活性的酶前体。

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