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放线菌素D类似物对核仁磷蛋白B23(37,000道尔顿/等电点5.1)的影响。

Effects of actinomycin D analogs on nucleolar phosphoprotein B23 (37,000 daltons/pI 5.1).

作者信息

Yung B Y, Busch R K, Busch H, Mauger A B, Chan P K

出版信息

Biochem Pharmacol. 1985 Nov 15;34(22):4059-63. doi: 10.1016/0006-2952(85)90387-9.

DOI:10.1016/0006-2952(85)90387-9
PMID:2415133
Abstract

Localization of protein B23 in HeLa cells after treatment with actinomycin D and its analogs was studied using indirect immunofluorescence. Bright nucleolar fluorescence was observed in control HeLa cells. After treatment with actinomycin D (250 ng/ml) for 2 hr, a uniform nucleoplasmic fluorescence was observed. Similar results were obtained with the actinomycin analogs, actinomycin Z5 and actinomycin K2T. Only after a much longer incubation (24 hr) with actinomycin 4-4'-gly was nucleoplasmic fluorescence observed. Actinomycin D, actinomycin Z5, and actinomycin K2T inhibited [3H]uridine incorporation into the trichloroacetic acid insoluble fraction of HeLa cells with IC50 values of 9.5 +/- 3.2, 59.1 +/- 19.6 and 1423.3 +/- 212.2 ng/ml respectively. No inhibition of [3H]uridine incorporation was observed using actinomycin 4-4'-gly (2000 ng/ml, 2-hr incubation). The order of potency for the loss of nucleolar fluorescence and the concurrent increase in nucleoplasmic fluorescence was actinomycin D greater than actinomycin Z5 greater than actinomycin K2T greater than actinomycin 4-4'-gly, which correlated with the order of their IC50 values for inhibition of [3H]uridine incorporation. Studies of the effects of actinomycin D and its analogs on RNA synthesis and localization of protein B23 indicated that there is a direct relationship between the B23 "translocation" from nucleolus to nucleoplasm and the inhibition of RNA synthesis. At 45-55% inhibition of RNA synthesis, both nuclear and nucleolar B23 immunofluorescence were observed. At 75-85% inhibition, only a uniform nucleoplasmic fluorescence was observed.

摘要

使用间接免疫荧光法研究了放线菌素D及其类似物处理后HeLa细胞中蛋白质B23的定位。在对照HeLa细胞中观察到明亮的核仁荧光。用放线菌素D(250 ng/ml)处理2小时后,观察到均匀的核质荧光。放线菌素类似物放线菌素Z5和放线菌素K2T也得到了类似结果。仅在用放线菌素4-4'-gly孵育更长时间(24小时)后才观察到核质荧光。放线菌素D、放线菌素Z5和放线菌素K2T抑制[3H]尿苷掺入HeLa细胞的三氯乙酸不溶性部分,IC50值分别为9.5±3.2、59.1±19.6和1423.3±212.2 ng/ml。使用放线菌素4-4'-gly(2000 ng/ml,孵育2小时)未观察到对[3H]尿苷掺入的抑制作用。核仁荧光丧失和核质荧光同时增加的效力顺序为:放线菌素D>放线菌素Z5>放线菌素K2T>放线菌素4-4'-gly,这与它们抑制[3H]尿苷掺入的IC50值顺序相关。对放线菌素D及其类似物对RNA合成和蛋白质B23定位的影响研究表明,B23从核仁“易位”到核质与RNA合成抑制之间存在直接关系。在RNA合成受到45 - 55%抑制时,观察到细胞核和核仁的B23免疫荧光。在75 - 85%抑制时,仅观察到均匀的核质荧光。

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