大肠杆菌recC基因产物的分子扩增与纯化
Molecular amplification and purification of the E. coli recC gene product.
作者信息
Hickson I D, Atkinson K E, Hutton L, Tomkinson A E, Emmerson P T
出版信息
Nucleic Acids Res. 1984 May 11;12(9):3807-19. doi: 10.1093/nar/12.9.3807.
The level of recC gene expression has been analysed using Mud(bla lac) fusions to the recC promoter. The constitutive level of expression is very low and remains so even under SOS inducing conditions. The recC gene product has been amplified by harnessing the gene to the phage lambda leftward promoter in a plasmid. From cells harbouring this plasmid, RecC protein, which represented approximately 6% of the total cellular protein, was purified to electrophoretic homogeneity.
已使用与recC启动子的Mud(bla lac)融合体分析了recC基因的表达水平。组成型表达水平非常低,即使在SOS诱导条件下也是如此。通过将该基因与质粒中的噬菌体λ左向启动子连接,扩增了recC基因产物。从含有该质粒的细胞中,将占细胞总蛋白约6%的RecC蛋白纯化至电泳纯。
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