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大肠杆菌中精氨酸生物合成酶翻译抑制的证据:链霉素抗性突变体中的调控改变

Evidence for translational repression of arginine biosynthetic enzymes in Escherichia coli: altered regulation in a streptomycin-resistant mutant.

作者信息

Vogel R H, Devine E A, Vogel H J

出版信息

Mol Gen Genet. 1978 Jun 14;162(2):157-62. doi: 10.1007/BF00267872.

Abstract

The formation and repressibility of the arginine biosyntietic enzymes acetylornithine delta-aminotransferase (EC 2.6.1.11), acetylornithine deacetylase (EC 3.5.1.16), ornithine carbamoyltransferase (EC 2.1.3.3), and argininosuccinate lyase (EC 4.3.2.1) were studied in an Escherichia coli W derivative (strain 250-10) that carries (a) a mutant allele of the argR regulatory gene causing a diminished repression-derepression range and (b) a streptomycin resistance mutation. In comparison with the streptomycin-sensitive parent 250, all four enzymes (a) are formed as smaller proportions of the total protein (overall range, 12% to 71%), whether the conditions are repressive (arginine excess) or derepressive (arginine restriction), and (b) show increased repressibility ratios, the carbamoyltransferase giving the largest increase (from 5.7 to 25.0). These effects appear to depend on the concurrent expression of the regulatory-gene and streptomycin resistance mutations, as indicated by analogous experiments with canavanine-resistant mutants of 250-10 that have partial argR- character. The results provide evidence for translational repression in the arginine system, and are interpreted in terms of a functional interaction of a mutant arginine repressor with a mutant S12 ribosomal protein. The locale of translational repression may be near the site of S12, and this mode of regulation may involve initiational selectivity of groupwise recognizable arginine messenger RNA's.

摘要

在携带(a)导致阻遏 - 去阻遏范围减小的argR调控基因突变等位基因和(b)链霉素抗性突变的大肠杆菌W衍生物(菌株250 - 10)中,研究了精氨酸生物合成酶乙酰鸟氨酸δ - 氨基转移酶(EC 2.6.1.11)、乙酰鸟氨酸脱乙酰酶(EC 3.5.1.16)、鸟氨酸氨甲酰转移酶(EC 2.1.3.3)和精氨琥珀酸裂解酶(EC 4.3.2.1)的形成及可阻遏性。与链霉素敏感的亲本250相比,无论条件是阻遏性的(精氨酸过量)还是去阻遏性的(精氨酸限制),所有这四种酶(a)在总蛋白中所占比例较小(总体范围为12%至71%),并且(b)表现出增加的阻遏率,氨甲酰转移酶的增加幅度最大(从5.7增至25.0)。如对具有部分argR特性的250 - 10的刀豆氨酸抗性突变体进行的类似实验所示,这些效应似乎取决于调控基因突变和链霉素抗性突变的同时表达。结果为精氨酸系统中的翻译阻遏提供了证据,并根据突变的精氨酸阻遏物与突变的S12核糖体蛋白的功能相互作用进行了解释。翻译阻遏的位点可能在S12附近,并且这种调控模式可能涉及成组可识别的精氨酸信使RNA的起始选择性。

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