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大鼠肝癌细胞系中核糖体RNA基因多样性显著增加。

Marked increase in ribosomal RNA gene multiplicity in a rat hepatoma cell line.

作者信息

Miller O J, Tantravahi R, Miller D A, Yu L C, Szabo P, Prensky W

出版信息

Chromosoma. 1979 Feb 21;71(2):183-95. doi: 10.1007/BF00292822.

Abstract

An H4-IIE-C3 hepatoma cell line derived from an ACI rat has been shown to have differentially stained regions attached to the short arms of chromosomes 3, 11 and 13 and the long arm of an unidentified small chromosome. There is cell to cell variability in the number and size of the differentially stained regions, which contain, on the average, about 5% of the total DNA. A series of secondary constrictions occur at intervals along the length of each differentially stained region. These stain with silver by the Ag-AS method, indicating that the differentially stained regions contain sites of active 45S ribosomal precursor RNA transcription. In situ hybridization to metaphase chromosomes shows that the hepatoma cells have a 10 fold increase in DNA coding for 18S and 28S ribosomal RNA, 90% of it located in the differentially stained regions, and no change in the number of genes coding for 5S RNA. These results have been confirmed by filter disc hybridization.

摘要

源自ACI大鼠的H4-IIE-C3肝癌细胞系已显示出与3号、11号和13号染色体短臂以及一条未鉴定的小染色体长臂相连的差异染色区域。差异染色区域的数量和大小在细胞之间存在差异,这些区域平均包含约5%的总DNA。一系列次级缢痕沿着每个差异染色区域的长度间隔出现。这些区域通过Ag-AS法用银染色,表明差异染色区域包含活跃的45S核糖体前体RNA转录位点。对中期染色体的原位杂交显示,肝癌细胞中编码18S和28S核糖体RNA的DNA增加了10倍,其中90%位于差异染色区域,而编码5S RNA的基因数量没有变化。这些结果已通过滤膜杂交得到证实。

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