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L-刀豆氨酸对大肠杆菌精氨酰转移核糖核酸合成酶突变体中精氨酸生物合成酶的抑制作用。

Repression of enzymes of arginine biosynthesis by L-canavanine in arginyl-transfer ribonucleic acid synthetase mutants of Escherichia coli.

作者信息

Faanes R, Rogers P

出版信息

J Bacteriol. 1972 Oct;112(1):102-13. doi: 10.1128/jb.112.1.102-113.1972.

DOI:10.1128/jb.112.1.102-113.1972
PMID:4562386
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC251385/
Abstract

We show that the arginine analogue, l-canavanine, repressed the accumulation of translatable messenger ribonucleic acid (RNA) for three arginine biosynthetic enzymes in Escherichia coli. The method used to determine the level of translatable messenger RNA depended upon measurement of a burst of enzyme synthesis as described previously. E. coli strains with defective arginyltransfer ribonucleic acid (tRNA) synthetase (argS mutants) were insensitive to canavanine repression. When deprived of leucine, a leu argS strain regained normal sensitivity to canavanine repression. The level of in vivo canavanyl-tRNA(arg) was determined for a normal strain and an argS mutant. After 20 min of growth with canavanine only 9% of tRNA(arg) from the argS strain was protected from periodate oxidation, while 42% of the tRNA(arg) from an argS(+) strain was charged. When deprived of leucine, leu argS or leu argS(+) strains grown with canavanine contained more than 60% charged tRNA(arg). Reverse phase column chromatography of periodate-oxidized tRNA from canavanine-grown argS and argS(+) strains showed no preferential charging of any isoaccepting species of tRNA(arg). Therefore, we failed to detect a specific arginyl-tRNA species that might be involved in repression by canavanine. However, the data suggest that canavanine repression of the arginine pathway occurs only when high levels of canavanyl-tRNA are present, and thus support the notion that arginyl-tRNA synthetase plays a role in generating a repression signal.

摘要

我们发现,精氨酸类似物L-刀豆氨酸可抑制大肠杆菌中三种精氨酸生物合成酶的可翻译信使核糖核酸(RNA)的积累。用于确定可翻译信使RNA水平的方法取决于如前所述对酶合成爆发的测量。精氨酰转移核糖核酸(tRNA)合成酶有缺陷的大肠杆菌菌株(argS突变体)对刀豆氨酸抑制不敏感。当缺乏亮氨酸时,leu argS菌株恢复了对刀豆氨酸抑制的正常敏感性。测定了正常菌株和argS突变体体内刀豆氨酰-tRNA(arg)的水平。仅用刀豆氨酸培养20分钟后,argS菌株中只有9%的tRNA(arg)能免受高碘酸盐氧化的影响,而argS(+)菌株中有42%的tRNA(arg)被氨酰化。当缺乏亮氨酸时,用刀豆氨酸培养的leu argS或leu argS(+)菌株含有超过60%被氨酰化的tRNA(arg)。对用刀豆氨酸培养的argS和argS(+)菌株的高碘酸盐氧化tRNA进行反相柱色谱分析,结果表明tRNA(arg)的任何同工受体种类都没有优先氨酰化。因此,我们未能检测到可能参与刀豆氨酸抑制作用的特定精氨酰-tRNA种类。然而,数据表明,只有当存在高水平的刀豆氨酰-tRNA时,刀豆氨酸才会对精氨酸途径产生抑制作用,从而支持了精氨酰-tRNA合成酶在产生抑制信号中起作用的观点。

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Repression of enzymes of arginine biosynthesis by L-canavanine in arginyl-transfer ribonucleic acid synthetase mutants of Escherichia coli.L-刀豆氨酸对大肠杆菌精氨酰转移核糖核酸合成酶突变体中精氨酸生物合成酶的抑制作用。
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