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首页> 外文期刊>Journal of bacteriology >Analysis of functional domains of Rts1 RepA by means of a series of hybrid proteins with P1 RepA.
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Analysis of functional domains of Rts1 RepA by means of a series of hybrid proteins with P1 RepA.

机译:通过一系列具有P1 RepA的杂交蛋白分析Rts1 RepA的功能域。

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The RepA protein of the plasmid Rts1, consisting of 288 amino acids, is a trans-acting protein essential for initiation of plasmid replication. To study the functional domains of RepA, hybrid proteins of Rts1 RepA with the RepA initiator protein of plasmid P1 were constructed such that the N-terminal portion was from Rts1 RepA and the C-terminal portion was from P1 RepA. Six hybrid proteins were examined for function. The N-terminal region of Rts1 RepA between amino acid residues 113 and 129 was found to be important for Rts1 ori binding in vitro. For activation of the origin in vivo, an Rts1 RepA subregion between residues 177 and 206 as well as the DNA binding domain was required. None of the hybrid initiator proteins activated the P1 origin. Both in vivo and in vitro studies showed, in addition, that a C-terminal portion of Rts1 RepA was required along with the DNA binding and ori activating domains to achieve autorepression, suggesting that the C-terminal region of Rts1 RepA is involved in dimer formation. A hybrid protein consisting of the N-terminal 145 amino acids of Rts1 and the C-terminal 142 amino acids from P1 showed strong interference with both Rts1 and P1 replication, whereas other hybrid proteins showed no or little effect on P1 replication.
机译:包含288个氨基酸的Rts1质粒的RepA蛋白是启动质粒复制所必需的反式作用蛋白。为了研究RepA的功能结构域,构建了Rts1 RepA与质粒P1的RepA启动子蛋白的杂合蛋白,使得N-末端部分来自Rts1 RepA,C-末端部分来自P1 RepA。检查了六个杂合蛋白的功能。发现在氨基酸残基113和129之间的Rts1 RepA的N末端区域对于体外的Rts1 ori结合很重要。为了激活体内来源,需要残基177和206之间的Rts1 RepA子区域以及DNA结合结构域。杂种起始蛋白均未激活P1起源。此外,体内和体外研究均显示,Rts1 RepA的C末端部分以及DNA结合域和ori激活域均需要实现自抑制,这表明Rts1 RepA的C末端区域参与了二聚体编队。由Rts1的N端145个氨基酸和P1的C端142个氨基酸组成的杂合蛋白对Rts1和P1复制均表现出强烈的干扰,而其他杂合蛋白则对P1复制没有影响或影响很小。

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