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Merck
CN

Biochemical assays for the discovery of TDP1 inhibitors.

Molecular cancer therapeutics (2014-07-16)
Christophe Marchand, Shar-yin N Huang, Thomas S Dexheimer, Wendy A Lea, Bryan T Mott, Adel Chergui, Alena Naumova, Andrew G Stephen, Andrew S Rosenthal, Ganesha Rai, Junko Murai, Rui Gao, David J Maloney, Ajit Jadhav, William L Jorgensen, Anton Simeonov, Yves Pommier
摘要

Drug screening against novel targets is warranted to generate biochemical probes and new therapeutic drug leads. TDP1 and TDP2 are two DNA repair enzymes that have yet to be successfully targeted. TDP1 repairs topoisomerase I-, alkylation-, and chain terminator-induced DNA damage, whereas TDP2 repairs topoisomerase II-induced DNA damage. Here, we report the quantitative high-throughput screening (qHTS) of the NIH Molecular Libraries Small Molecule Repository using recombinant human TDP1. We also developed a secondary screening method using a multiple loading gel-based assay where recombinant TDP1 is replaced by whole cell extract (WCE) from genetically engineered DT40 cells. While developing this assay, we determined the importance of buffer conditions for testing TDP1, and most notably the possible interference of phosphate-based buffers. The high specificity of endogenous TDP1 in WCE allowed the evaluation of a large number of hits with up to 600 samples analyzed per gel via multiple loadings. The increased stringency of the WCE assay eliminated a large fraction of the initial hits collected from the qHTS. Finally, inclusion of a TDP2 counter-screening assay allowed the identification of two novel series of selective TDP1 inhibitors.

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Sigma-Aldrich
氯化镁 溶液, for molecular biology, 1.00 M±0.01 M
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