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克隆和鉴定编码果蝇 RNA 聚合酶 II 的 140kd 亚基的基因。

Cloning and identification of the gene coding for the 140-kd subunit of Drosophila RNA polymerase II.

机构信息

Molekulare Genetik der Universität Heidelberg, Im Neuenheimer Feld 230, 6900 Heidelberg, FRG.

出版信息

EMBO J. 1986 Apr;5(4):741-6. doi: 10.1002/j.1460-2075.1986.tb04276.x.

Abstract

Genomic clones of Drosophila melanogaster were isolated from a lambda library by cross-hybridization with the yeast gene coding for the 150-kd subunit of RNA polymerase II. Clones containing a region of approximately 2.0 kb with strong homology to the yeast gene were shown to code for a 3.9-kb poly(A)-RNA. Part of the coding region was cloned into an expression vector. A fusion protein was obtained which reacted with an antibody directed against RNA polymerase II of Drosophila. Peptide mapping of the fusion protein yielded a number of spots identical with spots derived from the 140-kd subunit of Drosophila RNA polymerase II. Sequence comparison of a segment of the Drosophila and the corresponding yeast clone yielded a high degree of homology at the protein level also, suggesting that we had isolated the gene coding for the 140-kd subunit of RNA polymerase II from Drosophila. In situ hybridization localized the DmRP140 gene at 88 A/B on chromosome 3 while the DmRP215 gene has previously been localized at 10 C on the X chromosome. Analysis of the transcripts (7.0 and 3.9 kb) in female and male flies shows dosage compensation for the transcription of the DmRP215 gene.

摘要

利用酵母基因编码的 RNA 聚合酶 II 的 150kd 亚基的杂交进行交叉杂交,从 λ 噬菌体文库中分离出黑腹果蝇的基因组克隆。含有与酵母基因强同源性的约 2.0kb 区域的克隆被证明编码 3.9kb 的 poly(A)-RNA。部分编码区被克隆到表达载体中。获得了一种融合蛋白,该蛋白与针对果蝇 RNA 聚合酶 II 的抗体反应。融合蛋白的肽图谱产生了许多与来自果蝇 RNA 聚合酶 II 的 140kd 亚基衍生的斑点相同的斑点。果蝇和相应酵母克隆的一段序列比较在蛋白质水平上也显示出高度的同源性,表明我们已经从果蝇中分离出编码 RNA 聚合酶 II 的 140kd 亚基的基因。原位杂交将 DmRP140 基因定位于染色体 3 的 88A/B 处,而 DmRP215 基因先前已被定位于 X 染色体的 10C 处。在雌性和雄性果蝇中转录本(7.0 和 3.9kb)的分析表明,DmRP215 基因的转录存在剂量补偿。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9d58/1166853/814ab63b01d7/emboj00167-0112-a.jpg

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