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脂质体与免疫测定法。

Liposomes and immunoassays.

作者信息

Rongen H A, Bult A, van Bennekom W P

机构信息

Department of Pharmaceutical Analysis, Faculty of Pharmacy, Utrecht University, Netherlands.

出版信息

J Immunol Methods. 1997 May 26;204(2):105-33. doi: 10.1016/s0022-1759(97)00041-0.

Abstract

Various aspects of the application of liposomes as a label in immunoassays are reviewed. Methods for the preparation of liposomes, from the basic film method to the more advanced dehydration-rehydration method, are discussed. Furthermore, the markers used in liposome labels, as well as the methods to conjugate liposomes to antigens or antibodies, are summarized. Liposome immunoassays are applied as homogeneous or heterogeneous assays. Homogeneous assays often rely on the lytic activity of complement on antibody-associated liposomes. Another group of homogeneous assays utilizes the inhibitory action of antibodies on the activity of conjugates of mellitin (a bee venom protein) with a hapten. Free mellitin conjugates are able to lyse liposomes effectively. Heterogeneous liposome immunoassays, performed either competitively or non-competitively, resemble more closely standard enzyme linked immunosorbent assays, with the enzyme being replaced by a liposome label. Washing steps are used to separate antigen-specifically bound liposomes from unbound liposomes. All bound liposomes are lysed with a detergent, giving an instantaneous amplification. Flow-injection liposome immunoassays and liposome immunosensors are also described as examples of other possible immunoassay formats.

摘要

本文综述了脂质体作为免疫测定标记物应用的各个方面。讨论了脂质体制备方法,从基本的薄膜法到更先进的脱水再水化法。此外,总结了脂质体标记物中使用的标记以及将脂质体与抗原或抗体偶联的方法。脂质体免疫测定可作为均相或异相测定应用。均相测定通常依赖补体对抗体相关脂质体的裂解活性。另一组均相测定利用抗体对蜂毒素(一种蜂毒蛋白)与半抗原偶联物活性的抑制作用。游离的蜂毒素偶联物能够有效地裂解脂质体。异相脂质体免疫测定,无论是竞争性还是非竞争性进行,更类似于标准酶联免疫吸附测定,只是酶被脂质体标记物取代。洗涤步骤用于将抗原特异性结合的脂质体与未结合的脂质体分离。所有结合的脂质体用去污剂裂解,实现瞬间放大。流动注射脂质体免疫测定和脂质体免疫传感器也作为其他可能的免疫测定形式的例子进行了描述。

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