Lund E, Dahlberg J E
Proc Natl Acad Sci U S A. 1979 Nov;76(11):5480-4. doi: 10.1073/pnas.76.11.5480.
The 5'-terminal sequences of Escherichia coli ribosomal RNA precursors (pre-rRNAs) synthesized in vivo were characterized by RNA oligonucleotide sequence analysis. The 60- to 170-nucleotide-long 5'-end-specific fragments were produced by RNase III treatment of 30S and 18S pre-rRNAs. Comparison of the RNA oligonucleotides of these fragments with known DNA sequences of the promoter regions of several ribosomal RNA operons allows us to determine the start points of transcription of each operon. We conclude that transcription of most (and perhaps all) rRNA operons is initiated in vivo at two tandem promoters, called P1 and P2, which have recently been identified by in vitro transcription studies of several groups. Depending on the transcription unit, the initiating nucleotide at P1 promoters is either ATP or GTP, whereas at P2 promoters it is either CTP or GTP.
通过RNA寡核苷酸序列分析对体内合成的大肠杆菌核糖体RNA前体(pre-rRNA)的5'-末端序列进行了表征。通过用RNase III处理30S和18S pre-rRNA产生了长度为60至170个核苷酸的5'-末端特异性片段。将这些片段的RNA寡核苷酸与几个核糖体RNA操纵子启动子区域的已知DNA序列进行比较,使我们能够确定每个操纵子的转录起始点。我们得出结论,大多数(也许是所有)rRNA操纵子的转录在体内是在两个串联启动子处起始的,这两个启动子称为P1和P2,最近几组体外转录研究已经鉴定出了它们。根据转录单位的不同,P1启动子处的起始核苷酸要么是ATP,要么是GTP,而在P2启动子处则是CTP或GTP。
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