Sancar G B, Smith F W, Sancar A
Nucleic Acids Res. 1983 Oct 11;11(19):6667-78. doi: 10.1093/nar/11.19.6667.
We have constructed a series of multicopy plasmids that complement mutations in the phr gene of Escherichia coli. By subcloning into a tac plasmid vector we obtained a phr plasmid that upon induction overproduces two proteins of Mr's 49,000 and 20,000. Tn1000 insertions into the phr gene caused the disappearance of the 49,000 dalton protein, thus demonstrating this protein to be the phr gene product, DNA photolyase. The photolyase encoded by the phr gene makes up about 15% of total cellular proteins after induction of cells carrying a tac-phr plasmid. This protein binds specifically to UV (254 nm) irradiated DNA and upon exposure to near UV (300-500 nm) illumination repairs the UV damage and dissociates from DNA.
我们构建了一系列多拷贝质粒,这些质粒可互补大肠杆菌phr基因中的突变。通过亚克隆到一个tac质粒载体中,我们获得了一个phr质粒,该质粒在诱导后会过量产生分子量分别为49,000和20,000的两种蛋白质。Tn1000插入phr基因导致49,000道尔顿蛋白质消失,从而证明该蛋白质是phr基因产物——DNA光解酶。在携带tac-phr质粒的细胞诱导后,phr基因编码的光解酶约占细胞总蛋白的15%。这种蛋白质特异性结合紫外线(254 nm)照射的DNA,并在近紫外线(300 - 500 nm)照射下修复紫外线损伤并从DNA上解离。
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