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通过分离的红白血病细胞核进行体外珠蛋白RNA合成:红系分化过程中转录增加的直接证据。

Globin RNA synthesis in vitro by isolated erythroleukemic cell nuclei: direct evidence for increased transcription during erythroid differentiation.

作者信息

Orkin S H, Swerdlow P S

出版信息

Proc Natl Acad Sci U S A. 1977 Jun;74(6):2475-9. doi: 10.1073/pnas.74.6.2475.

Abstract

Murine erythroleukemic cells accumulate cytoplasmic globin mRNA during differentiation induced in tissue culture by dimethyl sulfoxide. Cellular accumulation of globin RNA may reflect transcriptional activation of the globin genes and/or posttranscriptional stabilization of globin RNA during differentiation. To evaluate possible transcriptional controls directly; globin RNA synthesis by isolated erythroleukemic cell nuclei was studied. Conditions were established for optimal nuclear RNA synthesis in vitro in the presence of a mercurinucleotide (Hg-CTP). Mercurated RNA synthesized in vitro was purified free of endogenous RNA by affinity chromatography on sulfhydryl-Sepharose, and analyzed for the presence of newly synthesized globin RNA sequences by molecular hybridization to globin complementary [32P]DNA. The results demonstrate markedly increased synthesis of globin RNA by nuclei isolated from dimethyl sulfoxide-treated cells, even within 5 min of nuclear transcription in vitro. These findings are most consistent with transcriptional activation of the globin genes upon induction of differentiation.

摘要

在组织培养中,用二甲基亚砜诱导分化时,小鼠红白血病细胞会积累细胞质珠蛋白mRNA。珠蛋白RNA的细胞积累可能反映了分化过程中珠蛋白基因的转录激活和/或珠蛋白RNA的转录后稳定。为了直接评估可能的转录控制;研究了分离的红白血病细胞核合成珠蛋白RNA的情况。在存在汞核苷酸(Hg-CTP)的情况下,建立了体外最佳核RNA合成的条件。通过巯基琼脂糖亲和层析纯化体外合成的汞化RNA,去除内源性RNA,并通过与珠蛋白互补[32P]DNA的分子杂交分析新合成的珠蛋白RNA序列的存在情况。结果表明,从经二甲基亚砜处理的细胞中分离的细胞核合成珠蛋白RNA的量显著增加,即使在体外核转录的5分钟内也是如此。这些发现与分化诱导后珠蛋白基因的转录激活最为一致。

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