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果蝇热休克基因座在细胞核系统中的转录

Transcription of heat shock loci of Drosophila in a nuclear system.

作者信息

Miller D W, Elgin S C

出版信息

Biochemistry. 1981 Aug 18;20(17):5033-42. doi: 10.1021/bi00520a033.

Abstract

We have investigated transcription in nucleic isolated from 6-18-h Drosophila melanogaster embryos. Kinetic aspects and specific products of the reaction have been analyzed; in particular, we have examined whether or not a faithful representation of an induced state, in this case the heat shock response, is maintained in the isolated nucleic. RNA polymerase II is active for at least 30 min. The combined RNA polymerase I and III activities are seen to continue synthesis for 60 min. Maximal synthesis by all enzymes is obtained in the absence of Mn2+. Transcripts from the 5S DNA have been characterized. These consist of two species, of 135 and 120 nucleotides, apparently the precursor and mature forms of 5S RNA. Extensive initiation by RNA polymerase III occurs on 5S DNA in this system. Transcription from the heat shock loci at 87A and 87Cl has been analyzed by hybridization of the newly synthesized RNA (selected by using 5'-mercuri-UTP) to plasmids containing the hsp 70 gene and adjacent regions. Only those segments of the DNA to which transcripts have been mapped in vivo hybridized with the in vitro synthesized RNA, and this transcription was observed only in nuclei isolated from heat-shocked embryos; no transcripts are detected in nuclei isolated from control embryos. These RNA species are synthesized by RNA polymerase II. Further analysis of transcription of the hsp68 gene (at locus 95D) has also been carried out. We conclude that in this system RNA polymerases II and II transcribe the chromatin template accurately and that the changes related to gene activation by heat shock are stable during nuclear isolation.

摘要

我们研究了从6至18小时的黑腹果蝇胚胎中分离出的核酸的转录情况。分析了该反应的动力学方面和特定产物;特别是,我们检查了在分离出的核酸中是否保持了诱导状态(在这种情况下是热休克反应)的忠实表征。RNA聚合酶II至少活跃30分钟。RNA聚合酶I和III的联合活性在60分钟内持续进行合成。在没有Mn2+的情况下,所有酶都能获得最大合成量。已对5S DNA的转录本进行了表征。这些转录本由两种类型组成,分别为135和120个核苷酸,显然是5S RNA的前体和成熟形式。在该系统中,RNA聚合酶III在5S DNA上广泛起始转录。通过将新合成的RNA(使用5'-汞尿苷三磷酸选择)与含有hsp 70基因及相邻区域的质粒杂交,分析了87A和87Cl处热休克基因座的转录情况。只有那些在体内已将转录本定位到的DNA片段与体外合成的RNA杂交,并且这种转录仅在从热休克胚胎中分离出的细胞核中观察到;在从对照胚胎中分离出的细胞核中未检测到转录本。这些RNA种类是由RNA聚合酶II合成的。还对hsp68基因(位于95D基因座)的转录进行了进一步分析。我们得出结论,在该系统中,RNA聚合酶II和III准确地转录染色质模板,并且与热休克引起的基因激活相关的变化在细胞核分离过程中是稳定的。

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