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Multicopy suppression by asd gene and osmotic stress-dependent complementation by heterologous proA in proA mutants.

机译:proA突变体中asd基因的多拷贝抑制和异源proA的渗透胁迫依赖性互补。

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摘要

Auxotrophic proA mutants of Escherichia coli were complemented by two different classes of Corynebacterium glutamicum genes. One of these was the asd gene. The E. coli asd gene also complements the same proA alleles. Complementation of proA by the asd+ gene requires a high asd dosage and the proB and the proC gene products. The reciprocal complementation pattern (asd by the proA+ gene) was not observed. This complementation appears to be due to multicopy suppression by a proline biosynthetic gene whose product was expected to play a negligible role in this pathway. The other class of complementing clones carries the C. glutamicum proA gene. Complementation of E. coli proA mutants by the C. glutamicum proA+ gene was optimal at high osmolarity.
机译:大肠杆菌的营养缺陷型proA突变体由两种不同类型的谷氨酸棒状杆菌基因补充。其中之一是asd基因。大肠杆菌的asd基因还补充了相同的proA等位基因。由asd +基因对proA的补充需要高asd剂量以及proB和proC基因产物。没有观察到相互的互补模式(由proA +基因鉴定)。这种互补似乎是由于脯氨酸生物合成基因的多拷贝抑制作用,脯氨酸生物合成基因的产物在该途径中起着微不足道的作用。另一类互补克隆携带谷氨酸棒杆菌proA基因。谷氨酸棒杆菌proA +基因对大肠杆菌proA突变体的补充在高渗透压下是最佳的。

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