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Nuclei Isolation Staining (NIS) Method for Imaging Chromatin-Associated Proteins in Difficult Cell Types

机译:核细胞染色蛋白相关蛋白在难量细胞类型中的核分离染色(NIS)方法

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摘要

Spatial distribution of chromatin-associated proteins provides invaluable information for understanding gene regulation. Conventional immunostaining is widely used for labeling chromatin-associated proteins in many cell types. However, for a subset ofdifficult cell types, such as differentiated human keratinocytes, achieving high-quality immunostaining for nuclear proteins remains challenging. To overcome this technical barrier, we developed the nuclei isolation staining (NIS) method. In brief, NISinvolves rapid isolation of nuclei from live cells, followed by fixation and staining of the nuclei directly on coverslips for subsequent high-magnification imaging. By removing the cytoplasmic contents and staining just the nuclei, this NIS method drastically improves antibody labeling efficiency for chromatin-associated proteins. In this article, we describe the development and a step-by-step protocol of NIS, using differentiated human keratinocytes as an example. We also discuss other applications, based on the principle of this NIS method, for understanding cell-type and cell-state specific gene regulation.
机译:染色质相关蛋白的空间分布提供了了解基因调控的宝贵信息。常规的免疫染色广泛用于在许多细胞类型中标记染色质相关蛋白。然而,对于诸如分化的人角蛋白细胞等较小的细胞类型的子集,实现核蛋白质的高质量免疫染色仍然具有挑战性。为了克服这种技术障碍,我们开发了核隔离染色(NIS)方法。简而言之,Nisinvolves从活细胞中快速分离核,然后直接在盖玻片上固定和染色核心,以用于随后的高倍率显像。通过去除细胞质含量并仅染色核,该NIS方法大大提高了染色质相关蛋白的抗体标记效率。在本文中,我们描述了NIS的开发和逐步协议,以分化的人角蛋白细胞为例。我们还基于该方法的原理讨论其他应用,用于了解细胞型和细胞状态特异性基因调控。

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