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作为基因调控研究模型的原噬菌体抑制。I. λ阻遏物的滴定

Prophage repression as a model for the study of gene regulation. I. Titration of the lambda repressor.

作者信息

Wiesmeyer H

出版信息

J Bacteriol. 1966 Jan;91(1):89-94. doi: 10.1128/jb.91.1.89-94.1966.

Abstract

Wiesmeyer, Herbert (Vanderbilt University, Nashville, Tenn.). Prophage repression as a model for the study of gene regulation. I. Titration of the lambda repressor. J. Bacteriol. 91:89-94. 1966.-The concentration of lambda repressor molecules within a lambda lysogenic cell was estimated from the multiplicity of superinfecting homologous phage necessary to permit replication and release of plaque-forming units. A multiplicity of 20 superinfecting phage was found sufficient to permit replication to occur in the normal lambda lysogen. The phage released after lysis of the superinfected lysogen was composed of both prophage and superinfecting phage types. Superinfection of the lysogen at lower multiplicities resulted in the lysis of only a small percentage of infected cells and is thought to represent a possible heterogeneity of repressor concentration in the lysogenic population. Viability of the superinfecting particle was found to be unnecessary for titration of the repressor. The repressor concentration in three lysogens of the nonultraviolet-inducible mutant of lambda, lambda(ind-), was found to be greater than 20 regardless of the host bacterium. However, the number of cells yielding phage after superinfection was found to vary with the particular host. The specificity of the lambda repressor was shown to be limited to homologous phage, as determined following heterologous superinfection experiments with phages T6r, 82c, 434c, 434hy, and 424. In all instances except that of superinfection with phage 434hy, only heterologous phage replication occurred. Superinfection by phage 434hy resulted in the release of both prophage and superinfecting phage types. The latter type represented approximately 80% of the total phage released.

摘要

威斯迈尔,赫伯特(范德比尔特大学,田纳西州纳什维尔)。原噬菌体阻遏作为基因调控研究的模型。I. λ阻遏物的滴定。《细菌学杂志》91:89 - 94。1966年。——通过允许形成噬菌斑单位的复制和释放所需的超感染同源噬菌体的复数来估计λ溶原细胞内λ阻遏物分子的浓度。发现20个超感染噬菌体的复数足以使正常的λ溶原菌发生复制。超感染溶原菌裂解后释放的噬菌体由原噬菌体和超感染噬菌体类型组成。以较低复数对溶原菌进行超感染仅导致一小部分受感染细胞裂解,并且被认为代表了溶原群体中阻遏物浓度可能存在的异质性。发现超感染颗粒的活力对于阻遏物的滴定并非必需。发现λ的非紫外线诱导型突变体λ(ind -)的三个溶原菌中的阻遏物浓度大于20,与宿主细菌无关。然而,发现超感染后产生噬菌体的细胞数量因特定宿主而异。如用噬菌体T6r、82c、434c、434hy和424进行异源超感染实验后所确定的,λ阻遏物的特异性仅限于同源噬菌体。在除用噬菌体434hy进行超感染的所有情况下,仅发生异源噬菌体复制。用噬菌体434hy进行超感染导致原噬菌体和超感染噬菌体类型都释放。后一种类型约占释放的总噬菌体的80%。

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