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制备单体抗原-酶偶联物以研究滤泡免疫复合物捕获的要求。

Production of monomeric antigen-enzyme conjugate to study requirements for follicular immune complex trapping.

作者信息

Laman J D, ter Hart H, Boorsma D M, Claassen E, Van Rooijen N

机构信息

Department of Immunology and Medical Microbiology, Medical Biological Laboratory TNO, Rijswijk, The Netherlands.

出版信息

Histochemistry. 1992;97(2):189-94. doi: 10.1007/BF00267310.

DOI:10.1007/BF00267310
PMID:1373127
Abstract

Studies concerning the localization of immune complexes in lymphoid follicles and the involvement of these trapped immune complexes in the regulation of the immune response have thus far been performed with poorly defined complexes in terms of size and composition. For that reason, the minimum requirements for trapping in terms of number of antigen- and antibody molecules present in immune complexes could not be determined. We here describe the production and in vivo use of a monomeric HSA-HRP antigen-enzyme conjugate, readily demonstrable in cryostat sections and ELISA. This conjugate was obtained by combining the glutaraldehyde coupling-method with chromatography to fractionate monomeric and multimeric constituents. SDS-PAGE analysis showed that the conjugate consisted of a single molecular species of 109 kDa, whereas the often used periodate oxidation coupling method yielded a heterogeneous population of multimeric, oligomeric and monomeric molecules. We investigated the minimal size requirements for the composition of immune complexes to be trapped in murine spleen follicles using three different conjugates (monomeric HSA-HRP, multimeric HSA-HRP and multimeric HSA-HRP-Penicillin) and a panel of anti-HSA and anti-Penicillin monoclonal antibodies. We demonstrate that the smallest immune complexes, consisting of one antibody and two conjugate molecules, do not localize in splenic follicles. Immune complexes prepared with a single monoclonal antibody localize in follicles only if the epitope recognized occurs repeatedly on the antigen. The relevance of these results for physiological follicular trapping of protein antigens is discussed.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

迄今为止,有关免疫复合物在淋巴滤泡中的定位以及这些被困免疫复合物在免疫反应调节中的作用的研究,所使用的复合物在大小和组成方面定义并不明确。因此,无法确定免疫复合物中抗原和抗体分子数量对于被困的最低要求。我们在此描述了一种单体HSA-HRP抗原-酶偶联物的制备及其在体内的应用,该偶联物在低温切片和酶联免疫吸附测定中易于检测。这种偶联物是通过将戊二醛偶联法与色谱法相结合来分离单体和多聚体成分而获得的。十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析表明,该偶联物由一种分子量为109 kDa的单一分子组成,而常用的高碘酸盐氧化偶联法产生的是多聚体、寡聚体和单体分子的异质群体。我们使用三种不同的偶联物(单体HSA-HRP、多聚体HSA-HRP和多聚体HSA-HRP-青霉素)以及一组抗HSA和抗青霉素单克隆抗体,研究了免疫复合物组成被捕获在小鼠脾脏滤泡中的最小尺寸要求。我们证明,由一个抗体和两个偶联物分子组成的最小免疫复合物不会定位在脾脏滤泡中。仅当抗原上反复出现被识别的表位时,用单克隆抗体制备的免疫复合物才会定位在滤泡中。讨论了这些结果与蛋白质抗原生理性滤泡捕获的相关性。(摘要截短于250字)

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