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非白血病小鼠腹水肿瘤细胞表面的核糖体RNA。

Ribosomal RNA on the surfaces of nonleukemic mouse ascites tumor cells.

作者信息

Terasaki T, Izawa M, Shimosato Y

出版信息

Cell Struct Funct. 1986 Mar;11(1):43-51. doi: 10.1247/csf.11.43.

DOI:10.1247/csf.11.43
PMID:3513969
Abstract

RNAs on the cell surfaces of two nonleukemic and two leukemic strains of mouse ascites tumor cells were studied by fractionating the RNAs released from the cell surface by gentle pronase treatment after sucrose density gradient centrifugation, by indirect membrane immunofluorescence that used anti-RNA antibody and by cell electrophoresis. RNA was extracted from the cell supernatants of Ehrlich ascites tumor and sarcoma 180 cells (nonleukemic) that had been treated or not treated with pronase (1 microgram/ml, 37 degrees C, 20 min) followed by sucrose density gradient centrifugation. It was clearly demonstrated that the amounts of ribosomal RNA (18S and 28S) released after pronase treatment were approximately 80% greater than that of nonpronase-treated cells. Ehrlich ascites tumor cells that had been treated with actinomycin D (100 micrograms/kg body weight of mouse, 16 h) in vivo released an amount of ribosomal RNA after pronase treatment only 20% greater than the value for untreated cells. Actinomycin D treatment greatly reduced both the cell surface negative charge and the cell surface immunofluorescence when rabbit anti-RNA antibody was used. Under the same experimental conditions with actinomycin D, only ribosomal RNA synthesis showed preferential inhibition, not the syntheses of poly A-containing messenger RNA, 4S or other small-size RNAs. In contrast, L1210 and C1498 cells (leukemic) showed no change in the amounts of ribosomal RNA released after pronase treatment. L1210 cells also showed no change in the surface negative charge after being treated with actinomycin D.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过以下方法研究了两种非白血病和两种白血病小鼠腹水肿瘤细胞系细胞表面的RNA:在蔗糖密度梯度离心后,用温和的链霉蛋白酶处理从细胞表面释放的RNA进行分级分离;使用抗RNA抗体的间接膜免疫荧光法;以及细胞电泳法。从艾氏腹水瘤和肉瘤180细胞(非白血病)的细胞上清液中提取RNA,这些细胞经或未经链霉蛋白酶(1微克/毫升,37℃,20分钟)处理,随后进行蔗糖密度梯度离心。结果清楚地表明,链霉蛋白酶处理后释放的核糖体RNA(18S和28S)的量比未用链霉蛋白酶处理的细胞大约多80%。在体内用放线菌素D(100微克/千克小鼠体重,16小时)处理过的艾氏腹水瘤细胞,经链霉蛋白酶处理后释放的核糖体RNA量仅比未处理细胞的值高20%。当使用兔抗RNA抗体时,放线菌素D处理大大降低了细胞表面负电荷和细胞表面免疫荧光。在与放线菌素D相同的实验条件下,只有核糖体RNA合成表现出优先抑制,而含多聚A的信使RNA、4S或其他小尺寸RNA的合成则没有受到抑制。相比之下,L1210和C1498细胞(白血病)经链霉蛋白酶处理后释放的核糖体RNA量没有变化。L1210细胞在用放线菌素D处理后表面负电荷也没有变化。(摘要截短于250字)

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