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The cl repressor of bacteriophage P1 operator-repressor interaction of wild-type and mutant repressor proteins

机译:野生型和突变型阻遏蛋白的噬菌体P1操纵基因-阻遏物相互作用的cl阻遏物

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The cl repressor gene of bacteriophage P1 and the temperature-sensitive mutants P1cl.100 and P1cl.162 was cloned into an expression vector and the repressor proteins were overproduced. A rapid purification procedure was required for the isolation of the thermolabile repressor proteins. Identification of the highly purified protein of an apparent molecular weight of 33,000 as the product of the cl gene was verified by (i) the coincidence of partial amino acid sequences determined experimentally to that deduced from the cl DNA sequence, and (ii) the temperature-sensitive binding to the operator DNA of the thermolabile repressor proteins. Analysis of the products of cl-cl.100 recombinant DNAs relates the thermolability to an unknown alteration in the C-terminal half of the cl.100 repressor. Binding to the operator DNA of cl repressor is sensitive to N-ethylmaleimide. Since the only three cysteine residues are located in the C-terminal half of the repressor it is suggested that this part of the molecule is important for the binding to the operator DNA. This assumption is supported by the findings that a 14-kDa C-terminal repressor fragment obtained by cyanogen bromide cleavage retains DNA binding properties.
机译:将噬菌体P1的cl阻遏基因以及温度敏感突变体P1cl.100和P1cl.162克隆到表达载体中,从而过量产生了阻遏蛋白。需要快速纯化程序来分离热不稳定的阻遏蛋白。通过(i)实验确定的部分氨基酸序列与从cl DNA序列推导的部分氨基酸序列的一致性,验证了表观分子量为33,000的高度纯化的蛋白作为cl基因的产物的鉴定。与耐热性阻遏蛋白的操纵子DNA敏感结合。对cl-cl.100重组DNA产物的分析将可热性与cl.100阻遏物C端一半的未知变化联系起来。与C1阻遏物的操纵子DNA结合对N-乙基马来酰亚胺敏感。由于仅三个半胱氨酸残基位于阻遏物的C末端一半,因此建议分子的这一部分对于与操纵子DNA的结合很重要。这一假设得到了以下发现的支持:通过溴化氰裂解获得的14 kDa C末端阻遏物片段保留了DNA结合特性。

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