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Immunonucleochemistry: a new method for in situ detection of antigens in the nucleus of cells in culture

机译:免疫核化学:原位检测培养细胞核中抗原的新方法

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摘要

The advancement of immunocytochemistry (ICC) allows one to observe detailed spatial distribution of cellular antigens, but, with some limitations. Using conventional ICC, it is difficult to distinguish the nuclear localization from cytoplasm, as two large subcellular compartments overlap on the z-axis. In this study, we have investigated whether in situ immunostaining of ‘naked’ nuclei could provide an unambiguous method for detection of nuclear antigens. We have designed a protocol that efficiently lyses plasmalemma, while keeping the nuclear envelope intact. The optimal condition for lysing the plasmalemma was 0.5% Nonidet P-40 for 5 min in both neuronal and non-neuronal cultured cells. Using this protocol, we could unambiguously isolate nuclear from cytoplasmic ICC signals. Since the present protocol has been designed for immunostaining of ‘naked’ nuclei from cultured or isolated cells, we have coined a new term to refer to this procedure as ‘immunonucleochemistry’ (‘INC’ for abbreviation).
机译:免疫细胞化学(ICC)的发展使人们能够观察到细胞抗原的详细空间分布,但存在一些局限性。使用传统的ICC,由于两个大的亚细胞区室在z轴上重叠,因此很难将核定位与细胞质区分开。在这项研究中,我们调查了“裸”核的原位免疫染色是否可以提供明确的检测核抗原的方法。我们设计了一种协议,该协议可有效裂解血浆病,同时保持完整的核膜。在神经元和非神经元培养细胞中,溶解血浆的最佳条件是0.5%Nonidet P-40 5分钟。使用此协议,我们可以明确地从细胞质ICC信号中分离核。由于本协议是为从培养或分离的细胞中“裸”核进行免疫染色而设计的,因此我们创造了一个新术语,称为“免疫核化学”(简称“ INC”)。

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