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Probing and regulating the activity of cellular enzymes by using DNA tetrahedron nanostructures

机译:利用DNA四面体纳米结构探测和调节细胞酶的活性

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摘要

Given the essential role of apurinic/apyrimidinic endonuclease (APE1) in gene repair and cancer progression, we report a novel approach for probing and regulating cellular APE1 activity by using DNA tetrahedrons. The tetrahedron with an AP site-containing antenna exhibits high sensitivity and specificity to APE1. It is suitable for APE1 in vitro detection (detection limit 5 pM) and cellular fluorescence imaging without any auxiliary transfection reagents, which discriminates the APE1 expression level of cancer cells and normal cells. In contrast, the tetrahedron with an AP site on its scaffold exhibits high binding affinity to APE1 but limits enzymatic catalysis making this nanostructure an APE1 inhibitor with an IC50 of 14.8 nM. It suppresses the APE1 activity in living cells and sensitizes cancer cells to anticancer drugs. We also demonstrate that the APE1 probe and inhibitor can be switched allosterically via stand displacement, which holds potential for reversible inhibition of APE1. Our approach provides a new way for fabricating enzyme probes and regulators and new insights into enzyme–substrate interactions, and it can be expanded to regulate other nucleic acid related enzymes.
机译:考虑到嘌呤/嘧啶内切核酸酶(APE1)在基因修复和癌症进展中的重要作用,我们报告了一种通过使用DNA四面体探测和调节细胞APE1活性的新方法。具有包含AP位置的天线的四面体对APE1表现出高灵敏度和特异性。它适用于APE1体外检测(检测限5 pM)和无任何辅助转染试剂的细胞荧光成像,可区分癌细胞和正常细胞的APE1表达水平。相反,在其支架上具有AP位点的四面体对APE1表现出高结合亲和力,但限制了酶催化作用,从而使该纳米结构成为APE1抑制剂,IC50为14.8 nM。它抑制活细胞中的APE1活性并使癌细胞对抗癌药敏感。我们还证明了APE1探针和抑制剂可以通过支架位移进行变构转换,从而可逆地抑制APE1。我们的方法为制造酶探针和调节剂提供了新途径,并为了解酶与底物之间的相互作用提供了新的见解,并且可以扩展为调控其他核酸相关酶。

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