Premium
Double Click Reaction for the Acquisition of a Highly Potent and Selective mPTPB Inhibitor
Author(s) -
He Rongjun,
Yu Zhihong,
He Yantao,
Zeng LiFan,
Xu Jie,
Wu Li,
Gunawan Andrea M.,
Wang Lina,
Jiang ZhongXing,
Zhang ZhongYin
Publication year - 2010
Publication title -
chemmedchem
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.817
H-Index - 100
eISSN - 1860-7187
pISSN - 1860-7179
DOI - 10.1002/cmdc.201000348
Subject(s) - protein tyrosine phosphatase , mycobacterium tuberculosis , enzyme , docking (animal) , mode of action , small molecule , phosphatase , biochemistry , active site , chemistry , click chemistry , drug discovery , biology , stereochemistry , combinatorial chemistry , tuberculosis , medicine , nursing , pathology
Tuberculosis (TB), which is caused by Mycobacterium tuberculosis (Mtb), is a major worldwide threat to public health. Mycobacterium protein tyrosine phosphatase B (mPTPB) is a virulent phosphatase secreted by Mtb, which is essential for the survival and persistence of the bacterium in the host. Consequently, small‐molecule inhibitors of mPTPB are expected to serve as anti‐TB agents with a novel mode of action. Herein, we report the discovery of highly potent and selective mPTPB inhibitors using a novel, double Click chemistry strategy. The most potent mPTPB inhibitor from this approach possesses a K i value of 160 n M and a >25‐fold selectivity for mPTPB over 19 other protein tyrosine phosphatases (PTBs). Molecular docking study of the enzyme–inhibitor complex provides a rationale for the high potency and selectivity of the lead compound and reveals an unusual binding mode, which may guide further optimization effort.