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关于HeLa S3核基质的分离与特性的综合研究。

A comprehensive study on the isolation and characterization of the HeLa S3 nuclear matrix.

作者信息

Belgrader P, Siegel A J, Berezney R

机构信息

Department of Biological Sciences, State University of New York, Buffalo 14260.

出版信息

J Cell Sci. 1991 Mar;98 ( Pt 3):281-91. doi: 10.1242/jcs.98.3.281.

DOI:10.1242/jcs.98.3.281
PMID:1711534
Abstract

Different agents have been employed to extract the histones and other soluble components from isolated HeLa S3 nuclei during nuclear matrix isolation. We report that 0.2M (NH4)2SO4 is a milder extracting agent than NaCl and LIS (lithium 3,5-diiodosalicylate), on the basis of the apparent preservation of the elaborate fibrogranular network and the residual nucleolus that resemble the in situ structures in whole cells and nuclei, minimal aggregation, and sufficient solubilization of DNA and histones. The importance of intermolecular disulfide bonds, RNA and 37 degrees C stabilization on the structural integrity of the nuclear matrix was examined in detail using sulfydryl alkylating, reducing and oxidizing agents, and RNase A. The data suggest that any disulfides formed during the isolation are not essential for maintaining the structural integrity of the in vitro matrix. However, structural integrity of the matrix is dependent upon RNA and to some degree on disulfides that presumably existed in situ. Sodium tetrathionate and 37 degrees C stabilization of isolated nuclei resulted in nuclear matrices containing an approximately twofold greater amount of protein, RNA and DNA than control preparations. The 37 degrees C incubation, unlike the sodium tetrathionate stabilization, does not appear to induce intermolecular disulfide bond formation. Neither stabilizations resulted in significant differences of the major matrix polypeptide pattern on two-dimensional (2-D) gels stained with Coomassie Blue as compared to that of unstabilized matrix. The major nuclear matrix proteins, other than the lamins, did not react to the Pruss murine monoclonal antibody (IFA) that recognizes all known intermediate filament proteins, suggesting that the internal matrix proteins are not related to the lamins in intermediate filament-like quality.

摘要

在核基质分离过程中,人们使用了不同的试剂从分离的HeLa S3细胞核中提取组蛋白和其他可溶性成分。我们报告称,基于精细的纤维颗粒网络和残留核仁的明显保留(它们类似于完整细胞和细胞核中的原位结构)、最小程度的聚集以及DNA和组蛋白的充分溶解,0.2M硫酸铵是一种比氯化钠和LIS(3,5 - 二碘水杨酸锂)更温和的提取剂。使用巯基烷基化、还原和氧化剂以及核糖核酸酶A详细研究了分子间二硫键、RNA和37℃稳定化对核基质结构完整性的重要性。数据表明,在分离过程中形成的任何二硫键对于维持体外基质的结构完整性并非必不可少。然而,基质的结构完整性取决于RNA,并且在某种程度上取决于可能原位存在的二硫键。连四硫酸钠和37℃对分离细胞核的稳定作用导致核基质中蛋白质、RNA和DNA的含量比对照制剂大约多两倍。与连四硫酸钠稳定化不同,37℃孵育似乎不会诱导分子间二硫键的形成。与未稳定化的基质相比,两种稳定化处理在考马斯亮蓝染色的二维凝胶上均未导致主要基质多肽模式出现显著差异。除核纤层蛋白外,主要的核基质蛋白不与识别所有已知中间丝蛋白的普鲁士鼠单克隆抗体(免疫荧光分析)发生反应,这表明内部基质蛋白在中间丝样性质方面与核纤层蛋白无关。

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