| Literature DB >> 28120472 |
Ji Luo1, Muwen Kong2,3, Lili Liu3, Subhas Samanta1, Bennett Van Houten2,3, Alexander Deiters1,3.
Abstract
Nucleotide excision repair (NER) is a general DNA repair mechanism that is capable of removing a wide variety of DNA lesions induced by physical or chemical insults. UvrD, a member of the helicase SF1 superfamily, plays an essential role in bacterial NER by unwinding the duplex DNA in the 3' to 5' direction to displace the lesion-containing strand. In order to achieve conditional control over NER, we generated a light-activated DNA helicase. This was achieved through a site-specific incorporation of a genetically encoded hydroxycoumarin lysine at a crucial position in the ATP-binding pocket of UvrD. The resulting caged enzyme was completely inactive in several functional assays. Moreover, enzymatic activity of the optically triggered UvrD was comparable to that of the wild-type protein, thus demonstrating excellent OFF to ON switching of the helicase. The developed approach provides optical control of NER, thereby laying a foundation for the regulation of ATP-dependent helicase functions in higher organisms. In addition, this methodology is applicable to the light-activation of a wide range of ATPases.Entities:
Keywords: DNA damage; caged compounds; helicase; light activation; unnatural amino acids
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Year: 2017 PMID: 28120472 PMCID: PMC5516474 DOI: 10.1002/cbic.201600624
Source DB: PubMed Journal: Chembiochem ISSN: 1439-4227 Impact factor: 3.164