大鼠肝脏和胸腺核染色质组分中几种非组蛋白的鉴别。

Acta biologica et medica Germanica Pub Date : 1982-01-01
A Weihe, G Schmidt, C U von Mickwitz, R Lindigkeit
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引用次数: 0

摘要

采用sds -聚丙烯酰胺凝胶电泳法研究了大鼠肝脏和胸腺的盐溶性染色质(染色质S)和残核(染色质P)的非组蛋白(NHPs)。肝脏的两个染色质部分在NHP模式上表现出显著差异,大部分hnRNP和基质蛋白发生在染色质p中。由于胸腺核蛋白含量低,相应的胸腺部分表现出NHPs数量明显低于肝脏的电泳模式。与肝脏部分相比,胸腺的染色质P显示只有非常低的分子量为30,000-40,000 (30 K至40 K)的hnrnp特异性蛋白(信息染色体蛋白)含量,这与胸腺细胞核的RNA含量显著降低相一致。在基质蛋白(60-75 K)区域,染色质P在胸腺中仅表现出约64 K和73 K的两条强带,而在肝脏中则表现出64、66、69、73和75 K的五条强带。RNase酶切用于从“真正的”染色体NHPs中区分hnrnp特异性蛋白。肝脏染色质P和S中至少65%和25%的NHPs分别是rnp特异性的。用蔗糖梯度离心和甲咪唑胺的异氰酸带进一步分离两个染色质组分。离心后,染色质S和P的主峰只含有少量的NHPs,其主导蛋白为38 K。通过本文描述的离心程序,可以分离出一小部分染色质,这些染色质富含新合成的RNA、信息染色体蛋白、基质和其他高分子量蛋白质。这个亚组分可能与转录活性染色质有关。
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Discrimination of several classes of nonhistone proteins in chromatin fractions from liver and thymus nuclei of rats.

Nonhistone proteins (NHPs) of salt-soluble chromatin (Chromatin S) and of the residual nuclei (Chromatin P) from rat liver and thymus were studied by SDS-polyacrylamide gel electrophoresis. The two chromatin fractions of the liver showed significant differences in their NHP patterns with most of the hnRNP and matrix proteins occurring in Chromatin P. In accordance with the low protein content of thymus nuclei, the corresponding thymus fractions exhibited electrophoretic patterns with a markedly lower amount of NHPs than in liver. Chromatin P from thymus, in contrast to the liver fraction, revealed only a very low content of hnRNP-specific proteins of molecular weight 30,000-40,000 (30 K to 40 K) (informosomal proteins) consistent with the significantly lower RNA content of thymus nuclei. In the region of the matrix proteins (60-75 K) Chromatin P showed only two bands of about 64 K and 73 K in thymus, whereas in liver five strong bands at 64 K, 66 K, 69 K, 73 K, and 75 K were found. RNase digestion was employed to discriminate hnRNP-specific protein from "real" chromosomal NHPs. At least about 65% and 25% of the NHPs from Chromatin P and S of liver, respectively, were found to be RNP-specific. The two chromatin fractions were further fractionated by sucrose gradient centrifugation and isopycnic banding in metrizamide. After centrifugation the main peaks, both of Chromatin S and P, contained only minor amounts of NHPs with a predominating protein of 38 K. By the centrifugation procedures described in this paper, a small subfraction of chromatin could be separated which was enriched in newly synthesized RNA, informosomal proteins, matrix- and other high molecular weight proteins. This subfraction might be related to transcriptionally active chromatin.

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