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噬菌体λ pL操纵子中的转录终止和加工位点。

Transcription termination and processing sites in the bacteriophage lambda pL operon.

作者信息

Hyman H C, Honigman A

出版信息

J Mol Biol. 1986 May 5;189(1):131-41. doi: 10.1016/0022-2836(86)90386-4.

DOI:10.1016/0022-2836(86)90386-4
PMID:3023619
Abstract

S1 nuclease mapping was performed on transcripts from the major leftward operon of the bacteriophage lambda in order to locate the 3' ends of stable RNA species produced in vivo. The analysis was carried out on RNA purified from either an induced lambda prophage or bacteria carrying a plasmid containing a large segment of lambda including the intact PL operon through the bet gene. The S1 nuclease mapping was performed on transcripts produced in the presence and the absence of the N antitermination function, and in the presence and the absence of either the RNase III processing enzyme or the Rho factor. The results of this work indicate that the intercistronic region between the N and ral genes of lambda contains three sites at which transcripts end under N-Rho+ conditions (positions on the lambda sequence: 34,826, 34,558 and 34,393). The distal two correspond to the two sites previously described in this region as tL1 (on both sides of the BamHI site). In the region between ral and Ea10, we mapped the 3' ends of three species of RNA. The 3' end of one species was found to be located 90 nucleotides proximal to tL2a, at 34,000 in the lambda sequence. The terminator at this site may be partially N-resistant. In an RNase III deficient host, an additional RNA species is formed. The 3' end of this RNA species is located at tL2a (33,910 on the lambda sequence). In the presence of the antitermination N gene product, the readthrough transcripts are processed to form a 3' end at position 33,980 on the lambda sequence. These results suggest that elongation of transcription of the lambda PL operon is reduced gradually by clusters of termination located between genes and that the expression of the terminated products is further controlled by processing of the mRNA.

摘要

为了确定体内产生的稳定RNA种类的3'末端,对噬菌体λ主要左向操纵子的转录本进行了S1核酸酶图谱分析。分析是在从诱导的λ原噬菌体或携带质粒的细菌中纯化的RNA上进行的,该质粒包含λ的大片段,包括完整的PL操纵子直至bet基因。在有和没有N抗终止功能的情况下,以及在有和没有RNase III加工酶或Rho因子的情况下,对产生的转录本进行S1核酸酶图谱分析。这项工作的结果表明,λ的N和ral基因之间的顺反子间区域包含三个位点,在N-Rho+条件下转录本在此处终止(λ序列上的位置:34,826、34,558和34,393)。最远端的两个位点对应于该区域先前描述的两个位点tL1(在BamHI位点的两侧)。在ral和Ea10之间的区域,我们绘制了三种RNA的3'末端图谱。发现一种RNA的3'末端位于tL2a近端90个核苷酸处,在λ序列的34,000处。该位点的终止子可能部分抗N。在缺乏RNase III的宿主中,会形成另一种RNA。这种RNA的3'末端位于tL2a(λ序列上的33,910)。在抗终止N基因产物存在的情况下,通读转录本被加工形成λ序列上33,980位置的3'末端。这些结果表明,λ PL操纵子转录的延伸因基因间的终止簇而逐渐减少,并且终止产物的表达通过mRNA的加工进一步受到控制。

相似文献

1
Transcription termination and processing sites in the bacteriophage lambda pL operon.噬菌体λ pL操纵子中的转录终止和加工位点。
J Mol Biol. 1986 May 5;189(1):131-41. doi: 10.1016/0022-2836(86)90386-4.
2
The tL2 cluster of transcription termination sites between genes bet and ral of coliphage lambda.大肠杆菌噬菌体λ的bet基因和ral基因之间的转录终止位点的tL2簇。
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Tandem transcription-termination sites in the late rightward operon of bacteriophage lambda.噬菌体λ晚期右向操纵子中的串联转录终止位点。
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Initiation, attenuation and RNase III processing of transcripts from the Escherichia coli operon encoding ribosomal protein S15 and polynucleotide phosphorylase.编码核糖体蛋白S15和多核苷酸磷酸化酶的大肠杆菌操纵子转录本的起始、衰减及核糖核酸酶III加工过程
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Mutations of bacteriophage lambda that define independent but overlapping RNA processing and transcription termination sites.定义独立但重叠的RNA加工和转录终止位点的噬菌体λ突变。
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NusA protein is necessary and sufficient in vitro for phage lambda N gene product to suppress a rho-independent terminator placed downstream of nutL.在体外,NusA蛋白对于噬菌体λ N基因产物抑制位于nutL下游的一个不依赖ρ因子的终止子而言是必需且充分的。
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Transcription termination: sequence and function of the rho-independent tL3 terminator in the major leftward operon of bacteriophage lambda.转录终止:噬菌体λ主要向左操纵子中ρ非依赖型tL3终止子的序列与功能
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Antitermination and termination functions of the cloned nutL, N, and tL1 modules of coliphage lambda.
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Antitermination of E. coli rRNA transcription is caused by a control region segment containing lambda nut-like sequences.大肠杆菌核糖体RNA转录的抗终止作用是由一个含有λ nut样序列的控制区片段引起的。
Cell. 1984 Oct;38(3):851-60. doi: 10.1016/0092-8674(84)90280-0.

引用本文的文献

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Bacteriophage lambda: a paradigm revisited.λ噬菌体:重温一个范例
J Virol. 2010 Jul;84(13):6876-9. doi: 10.1128/JVI.02177-09. Epub 2010 Apr 7.
2
RNase III stimulates the translation of the cIII gene of bacteriophage lambda.核糖核酸酶III刺激噬菌体λ的cIII基因的翻译。
Proc Natl Acad Sci U S A. 1987 Sep;84(18):6511-5. doi: 10.1073/pnas.84.18.6511.
3
Overexpression of N antitermination proteins of bacteriophages lambda, 21, and P22: loss of N protein specificity.噬菌体λ、21和P22的N抗终止蛋白的过表达:N蛋白特异性丧失。
J Bacteriol. 1989 May;171(5):2513-22. doi: 10.1128/jb.171.5.2513-2522.1989.
4
Genetic analysis of the rnc operon of Escherichia coli.大肠杆菌rnc操纵子的遗传分析。
J Bacteriol. 1989 May;171(5):2581-90. doi: 10.1128/jb.171.5.2581-2590.1989.
5
Retroregulation of the bacteriophage lambda int gene: limited secondary degradation of the RNase III-processed transcript.噬菌体λ整合酶基因的反向调控:核糖核酸酶III加工转录本的有限二级降解
J Bacteriol. 1989 Jan;171(1):588-92. doi: 10.1128/jb.171.1.588-592.1989.
6
Readthrough transcription occurs at the rho dependent signal F1 TIV in suppressor cells.通读转录发生在抑制细胞中依赖于ρ因子的信号F1 TIV处。
Nucleic Acids Res. 1990 Feb 25;18(4):865-70. doi: 10.1093/nar/18.4.865.