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RNA聚合酶B在分离的母鸡输卵管细胞核中对卵清蛋白基因进行优先转录。

Preferential transcription of the ovalbumin gene in isolated hen oviduct nuclei by RNA polymerase B.

作者信息

Nguyen-Huu M C, Sippel A A, Hynes N E, Groner B, Schütz G

出版信息

Proc Natl Acad Sci U S A. 1978 Feb;75(2):686-90. doi: 10.1073/pnas.75.2.686.

Abstract

The synthesis of ovalbumin mRNA sequences was studied in isolated nuclei from hen oviduct. Two different methods of analysis were used to distinguish in vitro synthesized from preexisting mRNA sequences: (i) Mercurated ribonucleotides were used for in vitro RNA synthesis, and the newly synthesized RNA was purified by chromatography on sulfhydryl-agarose and hybridized to radioactive ovalbumin cDNA. (ii) [3H]UTP was used to label the in vitro synthesized RNA. Hybridization to unlabeled mercurated cDNA, RNase A digestion, and subsequent purification of the hybrids on SH-agarose allowed the quantitation of newly synthesized ovalbumin mRNA sequences. Approximately 0.1% of the newly synthesized RNA was identified as ovalbumin RNA by both methods. The synthesis of ovalbumin RNA progressed during the incubation of nuclei and was sensitive to actinomycin D and low concentrations of alpha-amanitin. The preferential in vitro transcription of the ovalbumin gene (1000-fold over random transcription of the chicken genome) by RNA polymerase B (nucleosidetriphosphate:RNA nucleotidyltransferase, EC 2.7.7.6) suggests that the specificity of in vitro RNA synthesis is retained in isolated nuclei.

摘要

在从母鸡输卵管分离出的细胞核中研究了卵清蛋白mRNA序列的合成。使用两种不同的分析方法来区分体外合成的mRNA序列和预先存在的mRNA序列:(i)用汞化核糖核苷酸进行体外RNA合成,新合成的RNA通过在巯基琼脂糖上的层析进行纯化,并与放射性卵清蛋白cDNA杂交。(ii)用[3H]UTP标记体外合成的RNA。与未标记的汞化cDNA杂交、用核糖核酸酶A消化,随后在SH-琼脂糖上纯化杂交体,从而可以对新合成的卵清蛋白mRNA序列进行定量。两种方法均将约0.1%的新合成RNA鉴定为卵清蛋白RNA。在细胞核孵育过程中,卵清蛋白RNA的合成持续进行,并且对放线菌素D和低浓度的α-鹅膏蕈碱敏感。RNA聚合酶B(核苷三磷酸:RNA核苷酸基转移酶,EC 2.7.7.6)对卵清蛋白基因的优先体外转录(比鸡基因组的随机转录高1000倍)表明,体外RNA合成的特异性在分离的细胞核中得以保留。

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RNA synthesis in isolated hen oviduct nuclei.分离的母鸡输卵管细胞核中的RNA合成
Biochemistry. 1976 Feb 24;15(4):824-9. doi: 10.1021/bi00649a015.

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