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核糖体编辑的计算机模拟

Computer simulation of ribosome editing.

作者信息

Menninger J R

出版信息

J Mol Biol. 1983 Dec 25;171(4):383-99. doi: 10.1016/0022-2836(83)90036-0.

DOI:10.1016/0022-2836(83)90036-0
PMID:6559207
Abstract

A stochastic model of protein synthesis was modified by including the process of dissociating peptidyl-tRNA from ribosomes. To simulate ribosome editing, the probability of dissociation was assumed to be high if the peptidyl-tRNA was erroneous; that is, if it resulted from transfer of a peptide to an aminoacyl-tRNA that was inappropriate relative to the mRNA codon. The effects of amino acid starvation on protein synthesis were simulated both by increasing the probability of such erring at and by reducing the conditional probability of elongation at "hungry" codons, those whose correct amino acid was in short supply. These probabilities were varied systematically to simulate tryptophan limitation during synthesis of coat protein from bacteriophage MS2. Significant reduction, during starvation, in the synthesis of complete coat protein required large reductions in the probability of elongation at hungry codons but only small increases in the probability of erring. Enhanced dissociation of peptidyl-tRNA during starvation, followed rapidly by dissociation of ribosomes from mRNA, led to reductions in mean polysome size, a result that had been interpreted by others as due to some effect of starvation on the initiation of protein synthesis. Results from experiments by Goldman (1982) on the cell-free synthesis of MS2 coat protein during tryptophan starvation could be mimicked in detail by the computer simulations. A simple competition between correct and erroneous amino acids was sufficient to explain the tryptophan dependence of complete coat protein and internal peptide syntheses. Values for the Michaelis constants were derived from the computer simulations.

摘要

通过纳入肽基 - tRNA从核糖体解离的过程,对蛋白质合成的随机模型进行了修改。为了模拟核糖体编辑,如果肽基 - tRNA错误,则假定其解离概率很高;也就是说,如果它是由肽转移到相对于mRNA密码子不合适的氨酰 - tRNA上导致的。通过增加此类错误发生的概率以及降低“饥饿”密码子(即其正确氨基酸供应短缺的密码子)处延伸的条件概率,来模拟氨基酸饥饿对蛋白质合成的影响。系统地改变这些概率,以模拟从噬菌体MS2合成外壳蛋白期间色氨酸的限制情况。在饥饿期间,完整外壳蛋白合成的显著减少需要大幅降低饥饿密码子处延伸的概率,但错误发生的概率只需小幅增加。饥饿期间肽基 - tRNA的解离增强,随后核糖体迅速从mRNA上解离,导致平均多核糖体大小减小,其他人将此结果解释为饥饿对蛋白质合成起始的某种影响。Goldman(1982年)关于色氨酸饥饿期间MS2外壳蛋白无细胞合成的实验结果可以通过计算机模拟详细模仿。正确和错误氨基酸之间的简单竞争足以解释完整外壳蛋白和内部肽合成对色氨酸的依赖性。米氏常数的值是从计算机模拟中得出的。

相似文献

1
Computer simulation of ribosome editing.核糖体编辑的计算机模拟
J Mol Biol. 1983 Dec 25;171(4):383-99. doi: 10.1016/0022-2836(83)90036-0.
2
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Control of RNA and protein synthesis by the concentration of Trp-tRNATrp in Escherichia coli infected with bacteriophage MS2.噬菌体MS2感染的大肠杆菌中色氨酸-tRNA色氨酸浓度对RNA和蛋白质合成的调控
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Miscoding-induced stalling of substrate translocation on the bacterial ribosome.诱导的错译导致细菌核糖体上底物易位停滞。
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Changes produced by bound tryptophan in the ribosome peptidyl transferase center in response to TnaC, a nascent leader peptide.结合色氨酸在核糖体肽基转移酶中心响应TnaC(一种新生的前导肽)而产生的变化。
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Activity of methoxyamine-modified f2 RNA in initiation and elongation steps of protein synthesis.甲氧基胺修饰的f2 RNA在蛋白质合成起始和延伸步骤中的活性。
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Initiation of polypeptide synthesis with various NH2-blocked aminoacyl-tRNAs under the direction of alfalfa mosaic virus RNA 4.在苜蓿花叶病毒RNA 4的指导下,用各种氨基被封闭的氨酰-tRNA起始多肽合成。
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引用本文的文献

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Effects of consecutive AGG codons on translation in Escherichia coli, demonstrated with a versatile codon test system.
利用通用密码子测试系统证明连续AGG密码子对大肠杆菌翻译的影响。
J Bacteriol. 1993 Feb;175(3):716-22. doi: 10.1128/jb.175.3.716-722.1993.
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Genetic and physical location of the Escherichia coli rap locus, which is essential for growth of bacteriophage lambda.大肠杆菌rap基因座的遗传和物理位置,该基因座对噬菌体λ的生长至关重要。
J Bacteriol. 1987 Nov;169(11):5188-92. doi: 10.1128/jb.169.11.5188-5192.1987.
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Relationship between protein synthesis and concentrations of charged and uncharged tRNATrp in Escherichia coli.大肠杆菌中蛋白质合成与带电荷和不带电荷的色氨酸转运RNA浓度之间的关系。
Proc Natl Acad Sci U S A. 1990 Feb;87(4):1511-5. doi: 10.1073/pnas.87.4.1511.