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具有改变的甘氨酰转移核糖核酸合成酶的大肠杆菌突变体的分离与部分特性分析

Isolation and partial characterization of Escherichia coli mutants with altered glycyl transfer ribonucleic acid synthetases.

作者信息

Folk W R, Berg P

出版信息

J Bacteriol. 1970 Apr;102(1):193-203. doi: 10.1128/jb.102.1.193-203.1970.

Abstract

Isolates with mutations in glyS, the structural gene for glycyl-transfer ribonucleic acid (tRNA) synthetase (GRS) in Escherichia coli, are frequently found among glycine auxotrophs. Extracts of glyS mutants have altered GRS activities. The mutants grow with normal growth rates in minimal media when high levels of glycine are provided. No other metabolite of a variety tested is capable of restoring normal growth. The glyS mutants fail to make ribonucleic acid (RNA) when depleted of exogenous glycine in strains which are RC(str) but do so when the cells are RC(rel). In contrast, biosynthetic mutants which are unable to synthesize glycine (glyA mutants) do not make RNA when deprived of glycine even if they are RC(rel); in this case, RNA is synthesized upon glycine deprivation only when the nucleic acid precursors made from glycine are provided in the medium. The level of serine transhydroxymethylase is unaltered in extracts of any of the glyS mutants, even though the level of charged tRNA(Gly) is at least 20-fold lower than that found in a prototrophic parent; this indicates that, if there is control over the synthesis of serine transhydroxymethylase, it is not modified by reduced levels of charging of the major species of tRNA(Gly).

摘要

在大肠杆菌中,甘氨酰转移核糖核酸(tRNA)合成酶(GRS)的结构基因glyS发生突变的分离株,在甘氨酸营养缺陷型菌株中经常被发现。glyS突变体的提取物具有改变的GRS活性。当提供高水平的甘氨酸时,这些突变体在基本培养基中以正常生长速率生长。所测试的其他代谢物均不能恢复正常生长。在RC(str)菌株中,当耗尽外源甘氨酸时,glyS突变体无法合成核糖核酸(RNA),但当细胞为RC(rel)时则可以合成。相比之下,无法合成甘氨酸的生物合成突变体(glyA突变体),即使它们是RC(rel),在缺乏甘氨酸时也不会合成RNA;在这种情况下,只有当培养基中提供由甘氨酸制成的核酸前体时,在缺乏甘氨酸时才会合成RNA。在任何glyS突变体的提取物中,丝氨酸转羟甲基酶的水平都没有改变,尽管带电荷的tRNA(Gly)水平比原养型亲本中发现的水平至少低20倍;这表明,如果对丝氨酸转羟甲基酶的合成有控制,它不会因tRNA(Gly)主要种类的电荷水平降低而被修饰。

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