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藤黄微球菌中组氨酸生物合成的遗传与生化研究。

A genetic and biochemical study of histidine biosynthesis in Micrococcus luteus.

作者信息

Kane-Falce C, Kloos W E

出版信息

Genetics. 1975 Mar;79(3):361-76. doi: 10.1093/genetics/79.3.361.

Abstract

Histidine auxotrophs of Micrococcus luteus strain ATCC 27141 were induced by treatment of the parent strain with N-methyl-N'-nitro-N-nitrosoguanidine. Auxotrophs were biochemically characterized by examining culture accumulations of histidine intermediates, using paper chromatography and the Bratton-Marshall test, and growth responses to L-histidinol. his(IG) mutants failed to accumulate Pauly-positive imidazoles; his(EAHF) mutants accumulated 5-amino-1-ribosyn-4-imidazole carboxamide; hisB mutants accumulated imidazoleglycerol; hisC mutants accumulated imidazoleacetol; hisD mutants, but did stimulate all other histidine mutants, blocked at earlier steps in the biosynthetic pathway. In addition, imidazoleglycerol phosphate dehydrase activity was assayed in representative mutants of each class. hisB mutants lacked activity for this enzyme.--Two -point, three-point, and cotransformation analyses resolved linkage relationships of histidine genes and in two gene clusters aided in determining their sequences. Histidine biosynthetic genes exist in at least four separate, unlinked regions of the chromosome. One histidine gene cluster linked to a tryptophan gene cluster and appears to be contiguous in the sequence his(IG) -his(EAHF)-trpE-trpC-trpA. A second and unlinked histidine cluster has the tentative gene sequence his(EAHF)-hisB-hisC-his(EAHF). The hisD gene and an unclassified mutant site his-94 are not linked to any of the other histidine genes examined in this study or to each other.

摘要

用N-甲基-N'-硝基-N-亚硝基胍处理藤黄微球菌菌株ATCC 27141的亲本菌株,诱导出了组氨酸营养缺陷型菌株。通过纸层析和布拉顿-马歇尔试验检测组氨酸中间体的培养积累情况,以及对L-组氨醇的生长反应,对营养缺陷型菌株进行了生化特性分析。his(IG)突变体未能积累保利阳性咪唑;his(EAHF)突变体积累了5-氨基-1-核糖基-4-咪唑甲酰胺;hisB突变体积累了咪唑甘油;hisC突变体积累了咪唑乙醇;hisD突变体在生物合成途径的早期步骤受阻,但确实刺激了所有其他组氨酸突变体。此外,还对每个类别的代表性突变体测定了咪唑甘油磷酸脱水酶活性。hisB突变体缺乏这种酶的活性。两点、三点和共转化分析解析了组氨酸基因的连锁关系,并且在两个基因簇中有助于确定它们的序列。组氨酸生物合成基因存在于染色体的至少四个独立、不连锁的区域。一个组氨酸基因簇与一个色氨酸基因簇相连,并且在序列his(IG)-his(EAHF)-trpE-trpC-trpA中似乎是连续的。第二个不连锁的组氨酸簇具有暂定的基因序列his(EAHF)-hisB-hisC-his(EAHF)。hisD基因和一个未分类的突变位点his-94与本研究中检测的任何其他组氨酸基因都不连锁,它们彼此之间也不连锁。

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