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1
Evidence against an Interaction between the mRNA downstream box and 16S rRNA in translation initiation.反对mRNA下游框与16S rRNA在翻译起始过程中存在相互作用的证据。
J Bacteriol. 2001 Jun;183(11):3499-505. doi: 10.1128/JB.183.11.3499-3505.2001.
2
Downstream box-anti-downstream box interactions are dispensable for translation initiation of leaderless mRNAs.下游框与反下游框的相互作用对于无前导mRNA的翻译起始并非必需。
EMBO J. 1996 Sep 2;15(17):4740-8.
3
The downstream box: an efficient and independent translation initiation signal in Escherichia coli.下游框:大肠杆菌中一种高效且独立的翻译起始信号
EMBO J. 1996 Feb 1;15(3):665-74.
4
Complementarity of the 16S rRNA penultimate stem with sequences downstream of the AUG destabilizes the plastid mRNAs.16S rRNA倒数第二个茎与AUG下游序列的互补性使质体mRNA不稳定。
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5
Enhancement of translation by the downstream box does not involve base pairing of mRNA with the penultimate stem sequence of 16S rRNA.下游框对翻译的增强作用并不涉及mRNA与16S rRNA倒数第二个茎序列的碱基配对。
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7
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Protein synthesis in Giardia lamblia may involve interaction between a downstream box (DB) in mRNA and an anti-DB in the 16S-like ribosomal RNA.蓝氏贾第鞭毛虫中的蛋白质合成可能涉及mRNA中的下游框(DB)与16S样核糖体RNA中的抗DB之间的相互作用。
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Comparative genomic analysis of translation initiation mechanisms for genes lacking the Shine-Dalgarno sequence in prokaryotes.原核生物中缺乏Shine-Dalgarno序列的基因的翻译起始机制的比较基因组分析。
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Organization and expression of a Thermus thermophilus arginine cluster: presence of unidentified open reading frames and absence of a Shine-Dalgarno sequence.嗜热栖热菌精氨酸簇的组织与表达:存在未鉴定的开放阅读框且缺少SD序列
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Selective stimulation of translation of leaderless mRNA by initiation factor 2: evolutionary implications for translation.起始因子2对无帽mRNA翻译的选择性刺激:翻译的进化意义
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Solution structure of the E. coli 70S ribosome at 11.5 A resolution.分辨率为11.5埃的大肠杆菌70S核糖体的溶液结构。
Cell. 2000 Mar 3;100(5):537-49. doi: 10.1016/s0092-8674(00)80690-x.
9
Cis-acting signals controlling translational initiation in the thermophilic archaeon Sulfolobus solfataricus.控制嗜热古菌嗜热栖热菌中翻译起始的顺式作用信号。
Mol Microbiol. 1999 Oct;34(2):377-84. doi: 10.1046/j.1365-2958.1999.01615.x.
10
A sequence downstream of the initiation codon is essential for cold shock induction of cspB of Escherichia coli.起始密码子下游的序列对于大肠杆菌cspB的冷休克诱导至关重要。
J Bacteriol. 1999 Sep;181(18):5852-4. doi: 10.1128/JB.181.18.5852-5854.1999.

反对mRNA下游框与16S rRNA在翻译起始过程中存在相互作用的证据。

Evidence against an Interaction between the mRNA downstream box and 16S rRNA in translation initiation.

作者信息

Moll I, Huber M, Grill S, Sairafi P, Mueller F, Brimacombe R, Londei P, Bläsi U

机构信息

Institute of Microbiology and Genetics, University of Vienna, Vienna Biocenter, Dr. Bohrgasse 9, 1030 Vienna, Austria.

出版信息

J Bacteriol. 2001 Jun;183(11):3499-505. doi: 10.1128/JB.183.11.3499-3505.2001.

DOI:10.1128/JB.183.11.3499-3505.2001
PMID:11344158
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC99648/
Abstract

Based on the complementarity of the initial coding region (downstream box [db]) of several bacterial and phage mRNAs to bases 1469 to 1483 in helix 44 of 16S rRNA (anti-downstream box [adb]), it has been proposed that db-adb base pairing enhances translation in a way that is similar to that of the Shine-Dalgarno (SD)/anti-Shine-Dalgarno (aSD) interaction. Computer modeling of helix 44 on the 30S subunit shows that the topography of the 30S ribosome does not allow a simultaneous db-adb interaction and placement of the initiation codon in the ribosomal P site. Thus, the db-adb interaction cannot substitute for the SD-aSD interaction in translation initiation. We have always argued that any contribution of the db-adb interaction should be most apparent on mRNAs devoid of an SD sequence. Here, we show that 30S ribosomes do not bind to leaderless mRNA in the absence of initiator tRNA, even when the initial coding region shows a 15-nucleotide complementarity (optimal fit) with the putative adb. In addition, an optimized db did not affect the translational efficiency of a leaderless lambda cI-lacZ reporter construct. Thus, the db-adb interaction can hardly serve as an initial recruitment signal for ribosomes. Moreover, we show that different leaderless mRNAs are translated in heterologous systems although the sequence of the putative adb's within helix 44 of the 30S subunits of the corresponding bacteria differ largely. Taken our data together with those of others (M. O'Connor, T. Asai, C. L. Squires, and A. E. Dahlberg, Proc. Natl. Acad. Sci. USA 96:8973-8978, 1999; A. La Teana, A. Brandi, M. O'Connor, S. Freddi, and C. L. Pon, RNA 6:1393-1402, 2000), we conclude that the db does not base pair with the adb.

摘要

基于几种细菌和噬菌体mRNA的起始编码区(下游框[db])与16S rRNA螺旋44中第1469至1483位碱基(反下游框[adb])的互补性,有人提出db - adb碱基配对以类似于Shine - Dalgarno(SD)/反Shine - Dalgarno(aSD)相互作用的方式增强翻译。对30S亚基上螺旋44的计算机建模表明,30S核糖体的拓扑结构不允许同时发生db - adb相互作用以及起始密码子位于核糖体P位点。因此,db - adb相互作用不能在翻译起始中替代SD - aSD相互作用。我们一直认为,db - adb相互作用的任何贡献在缺乏SD序列的mRNA上应该最为明显。在此,我们表明在没有起始tRNA的情况下,30S核糖体不会与无 leader的mRNA结合,即使起始编码区与假定的adb显示出15个核苷酸的互补性(最佳匹配)。此外,优化后的db并不影响无 leader的λ cI - lacZ报告构建体的翻译效率。因此,db - adb相互作用几乎不能作为核糖体的初始招募信号。而且,我们表明不同的无 leader的mRNA在异源系统中能够被翻译,尽管相应细菌30S亚基螺旋44内假定的adb序列差异很大。综合我们的数据以及其他人的数据(M. O'Connor、T. Asai、C. L. Squires和A. E. Dahlberg,《美国国家科学院院刊》96:8973 - 8978,1999;A. La Teana、A. Brandi、M. O'Connor、S. Freddi和C. L. Pon,《RNA》6:1393 - 1402,2000),我们得出结论,db不会与adb进行碱基配对。