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Detection of a key tertiary interaction in the highly conserved GTPase center of large subunit ribosomal RNA.在大亚基核糖体RNA高度保守的GTP酶中心检测到一个关键的三级相互作用。
Proc Natl Acad Sci U S A. 1991 Jul 15;88(14):6308-12. doi: 10.1073/pnas.88.14.6308.
2
Recognition of the highly conserved GTPase center of 23 S ribosomal RNA by ribosomal protein L11 and the antibiotic thiostrepton.核糖体蛋白L11和抗生素硫链丝菌素对23S核糖体RNA高度保守的GTP酶中心的识别。
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3
On the role of rRNA tertiary structure in recognition of ribosomal protein L11 and thiostrepton.关于核糖体RNA三级结构在核糖体蛋白L11和硫链丝菌素识别中的作用
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4
Ribosomal proteins L11 and L10.(L12)4 and the antibiotic thiostrepton interact with overlapping regions of the 23 S rRNA backbone in the ribosomal GTPase centre.核糖体蛋白L11和L10(L12)4以及抗生素硫链丝菌素与核糖体GTP酶中心23 S rRNA主链的重叠区域相互作用。
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The antibiotic thiostrepton inhibits a functional transition within protein L11 at the ribosomal GTPase centre.抗生素硫链丝菌素可抑制核糖体GTP酶中心的蛋白质L11内的功能转变。
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Replacement of the L11 binding region within E.coli 23S ribosomal RNA with its homologue from yeast: in vivo and in vitro analysis of hybrid ribosomes altered in the GTPase centre.将大肠杆菌23S核糖体RNA中的L11结合区域替换为酵母中的同源区域:对GTP酶中心发生改变的杂交核糖体进行体内和体外分析。
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Characterization of the binding sites of protein L11 and the L10.(L12)4 pentameric complex in the GTPase domain of 23 S ribosomal RNA from Escherichia coli.蛋白质L11与L10·(L12)4五聚体复合物在大肠杆菌23S核糖体RNA GTPase结构域中的结合位点表征。
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The RNA-binding domain of ribosomal protein L11 recognizes an rRNA tertiary structure stabilized by both thiostrepton and magnesium ion.核糖体蛋白L11的RNA结合结构域识别由硫链丝菌素和镁离子稳定的rRNA三级结构。
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8
Expansion of the 16S and 23S ribosomal RNA mutation databases (16SMDB and 23SMDB).16S和23S核糖体RNA突变数据库(16SMDB和23SMDB)的扩充。
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Throwing a spanner in the works: antibiotics and the translation apparatus.破坏计划:抗生素与翻译装置
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The phylogenetically conserved doublet tertiary interaction in domain III of the large subunit rRNA is crucial for ribosomal protein binding.大亚基核糖体RNA结构域III中系统发育保守的双重三级相互作用对于核糖体蛋白结合至关重要。
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本文引用的文献

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Site of action of a ribosomal RNA methylase conferring resistance to thiostrepton.赋予对硫链丝菌素抗性的核糖体RNA甲基化酶的作用位点。
J Biol Chem. 1982 Jul 25;257(14):7915-7.
2
Functional homology between E. coli ribosomal protein L11 and B. megaterium protein BM-L11.大肠杆菌核糖体蛋白L11与巨大芽孢杆菌蛋白BM-L11之间的功能同源性。
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Immunoelectron microscopy of ribosomes.核糖体的免疫电子显微镜检查。
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The structure of rat 28S ribosomal ribonucleic acid inferred from the sequence of nucleotides in a gene.从一个基因中的核苷酸序列推断出的大鼠28S核糖体核糖核酸的结构。
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The binding site for ribosomal protein L11 within 23 S ribosomal RNA of Escherichia coli.核糖体蛋白L11在大肠杆菌23S核糖体RNA内的结合位点。
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Secondary structure of 16S ribosomal RNA.16S核糖体RNA的二级结构
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Concerning the mode of action of micrococcin upon bacterial protein synthesis.关于微球菌素对细菌蛋白质合成的作用方式。
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Detailed molecular model for transfer ribonucleic acid.转移核糖核酸的详细分子模型。
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9
NMR analysis of DNA junctions: imino proton NMR studies of individual arms and intact junction.DNA连接体的核磁共振分析:单个臂和完整连接体的亚氨基质子核磁共振研究
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Comparative anatomy of 16-S-like ribosomal RNA.16S 样核糖体 RNA 的比较解剖学
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在大亚基核糖体RNA高度保守的GTP酶中心检测到一个关键的三级相互作用。

Detection of a key tertiary interaction in the highly conserved GTPase center of large subunit ribosomal RNA.

作者信息

Ryan P C, Draper D E

机构信息

Department of Chemistry, Johns Hopkins University, Baltimore, MD 21218.

出版信息

Proc Natl Acad Sci U S A. 1991 Jul 15;88(14):6308-12. doi: 10.1073/pnas.88.14.6308.

DOI:10.1073/pnas.88.14.6308
PMID:2068110
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC52072/
Abstract

Searches of ribosomal RNA sequences for compensatory base changes preserving Watson-Crick base pairing have led to detailed models of the conserved secondary structures of these RNAs. In principle, tertiary interactions can also be detected by searches for phylogenetically covariant bases. Within a highly conserved region of the large subunit ribosomal RNA termed the "GTPase center," the bases G-1056-U-1082.A-1086 are found in all eubacteria (Escherichia coli numbering), while A-1056.C-1082.G-1086 are found at the homologous positions in eukaryotes; archaebacteria fall into either category with some exceptions. Either sequence can potentially form a similar set of hydrogen bonds connecting the 3 bases. To determine the contribution of these 3 bases to RNA tertiary structure, sequence variants were made in RNA fragments covering the GTPase center. Correct folding of the RNA fragments was assayed by measuring the binding affinities of two different ligands that recognize the RNA tertiary structure: the highly conserved ribosomal protein L11, which is normally associated with the GTPase center RNA, and the peptide antibiotic thiostrepton, which inhibits the GTPase activity of eubacterial and some archaebacterial ribosomes. The results strongly support the existence of a base pair between positions 1082 and 1086: single mutations at either position weaken both L11 and thiostrepton binding by approximately 10-fold or more, while compensatory double mutations bind the ligands nearly as well as the wild-type E. coli sequence. Variants at position 1056 have little effect on either L11 or thiostrepton binding; a 3-base interaction is therefore not supported by these experiments. A base pair between positions 1082 and 1086 strongly constrains the geometry with which three helical segments join in the middle of the GTPase center.

摘要

通过搜索核糖体RNA序列中能保持沃森-克里克碱基配对的补偿性碱基变化,已得出这些RNA保守二级结构的详细模型。原则上,三级相互作用也可通过搜索系统发育协变碱基来检测。在被称为“GTP酶中心”的大亚基核糖体RNA的一个高度保守区域内,所有真细菌(以大肠杆菌编号)中都存在碱基G-1056-U-1082.A-1086,而在真核生物的同源位置则是A-1056.C-1082.G-1086;古细菌除了一些例外情况,属于这两类中的任何一类。这两种序列都有可能形成一组类似的氢键来连接这三个碱基。为了确定这三个碱基对RNA三级结构的贡献,对覆盖GTP酶中心的RNA片段进行了序列变异。通过测量两种识别RNA三级结构的不同配体的结合亲和力,来检测RNA片段的正确折叠:高度保守的核糖体蛋白L11,它通常与GTP酶中心RNA相关联;以及肽抗生素硫链丝菌素,它抑制真细菌和一些古细菌核糖体的GTP酶活性。结果有力地支持了1082位和1086位之间存在碱基对:这两个位置上的单个突变会使L11和硫链丝菌素的结合能力减弱约10倍或更多,而补偿性双突变结合配体的能力几乎与野生型大肠杆菌序列一样好。1056位的变异对L11或硫链丝菌素的结合几乎没有影响;因此这些实验不支持存在三碱基相互作用。1082位和1086位之间的碱基对强烈限制了GTP酶中心中部三个螺旋段连接的几何形状。