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小鼠线粒体DNA重链和轻链上初级转录本的特征分析及转录起始位点的鉴定。

Characterization of primary transcripts and identification of transcription initiation sites on the heavy and light strands of mouse mitochondrial DNA.

作者信息

Bhat K S, Avdalovic N, Avadhani N G

机构信息

Department of Animal Biology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia 19104-6048.

出版信息

Biochemistry. 1989 Jan 24;28(2):763-9. doi: 10.1021/bi00428a052.

DOI:10.1021/bi00428a052
PMID:2713342
Abstract

Total RNA from Ehrlich ascites mitochondria pretreated with RNase-free DNase was capped in vitro with [alpha-32P]GTP and guanylyl transferase. The cappable RNAs representing the primary transcripts show a heterogeneous size distribution with four major species of 46, 63, 94, and 152 nucleotides and four minor species of 19, 24, 104, and 790 nucleotides in size. Hybridization with the D-loop DNA probes shows that the 19-nucleotide-long capped RNA is coded by the H-strand of mitochondrial DNA while the rest are coded by the L-strand. S1 nuclease mapping and primer extension analyses suggest the occurrence of a transcription initiation of H-strand at about 19 nucleotides upstream from the start of the tRNA(Phe) gene. All of the L-strand cappable RNAs have a common 5' end mapping to nucleotide 16,183 +/- 5 of the genome. The 3' ends of four major cappable RNA species line up to the conserved sequence boxes, putative start sites of DH-DNA; and in fact about 2% of these cappable species are found to exist as DNA-linked RNA under steady-state conditions. The 3' end of the 790-nucleotide cappable RNA lies close to the start of the tRNA(Pro) gene, suggesting that it may be the true precursor of L-strand transcript endonucleolytically processed at the 3' end. The level of L-strand-coded cappable RNAs varies markedly under different growth conditions. Treatment with cycloheximide results in a reduction while chloramphenicol caused over 3-fold induction, suggesting that these "primer" RNAs may have an additional regulatory function.

摘要

用无核糖核酸酶的脱氧核糖核酸酶预处理的艾氏腹水癌细胞线粒体的总核糖核酸,在体外与[α-32P]鸟苷三磷酸和鸟苷酸转移酶进行加帽反应。代表初级转录本的可加帽核糖核酸显示出大小不均一的分布,有四种主要的分别为46、63、94和152个核苷酸的种类,以及四种较小的分别为19、24、104和790个核苷酸的种类。与D环脱氧核糖核酸探针杂交表明,19个核苷酸长的加帽核糖核酸由线粒体脱氧核糖核酸的重链编码,而其余的由轻链编码。S1核酸酶图谱分析和引物延伸分析表明,重链转录起始于tRNA(Phe)基因起始位点上游约19个核苷酸处。所有可加帽的轻链核糖核酸都有一个共同的5'端,定位于基因组的16,183±5核苷酸处。四种主要可加帽核糖核酸种类的3'端与保守序列框对齐,保守序列框是DH-DNA的假定起始位点;实际上,在稳态条件下,约2%的这些可加帽种类以与脱氧核糖核酸相连的核糖核酸形式存在。790个核苷酸可加帽核糖核酸的3'端靠近tRNA(Pro)基因的起始位点,这表明它可能是在轻链转录本3'端进行内切核酸酶加工的真正前体。在不同的生长条件下,轻链编码的可加帽核糖核酸的水平有显著变化。用环己酰亚胺处理会导致其减少,而氯霉素则会引起超过3倍的诱导,这表明这些“引物”核糖核酸可能具有额外的调节功能。

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