酶的免疫电子显微镜,多酶复合物,和选定的其他寡聚蛋白

Heinrich Lünsdorf , Henri Tiedge
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引用次数: 1

摘要

“免疫电子显微镜”这一统称包含了许多技术,在这些技术中,在电子显微镜中可视化之前,生物材料被特异性抗体修饰。在这篇文章中,我们回顾了有关免疫电子显微镜的文献,重点是分析蛋白质的分子结构,特别是酶和多酶复合物。分子免疫电子显微镜在复杂的四元结构的多亚基酶上取得了显著的成功,在许多情况下,这些数据已成为最终详细的三维分子模型发展的基础。对特定酶的亚基组成和并置的阐明,本身就是一项重要的成就,反过来又刺激和指导了对催化机制的讨论;说明性的例子包括F1 atp酶和柠檬酸裂解酶等。在这里,我们选择了多种酶、多酶复合物和非酶蛋白来展示免疫电子显微镜的多功能性,说明方法的先决条件和局限性,并讨论个体免疫电子显微镜研究的意义和含义。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Immunoelectron microscopy of enzymes, multienzyme complexes, and selected other oligomeric proteins

The collective term “immunoelectron microscopy” subsumes a number of techniques in which the biological material is decorated with specific antibodies, prior to being visualized in the electron microscope. In this article, we have reviewed literature on immunoelectron microscopy that focusses on the analysis of the molecular architecture of proteins, in particular of enzymes and of multienzyme complexes. Molecular immunoelectron microscopy has been remarkably successful with multi-subunit enzymes of complex quaternary structures, and in many cases the data have been the basis for the eventual development of detailed three-dimensional molecular models. The elucidation of subunit composition and juxtaposition of a given enzyme, an important accomplishment in itself, has in turn stimulated and guided discussions on the catalytic mechanism; illustrative examples include F1 ATPase and citrate lyase, among others. Here we have chosen a variety of enzymes, multienzyme complexes, and non-enzymatic proteins to demonstrate the versatility of immunoelectron microscopy, to illustrate methodological prerequisites and limitations, and to discuss significance and implications of individual immunoelectron microscopy studies.

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