Nucleic Acid‐based Electrochemical Sensors Facilitate the Study of DNA Binding by Platinum (II)‐based Antineoplastics

Author:

Wu Yao1ORCID,Arroyo‐Currás Netzahualcóyotl1ORCID

Affiliation:

1. Department of Pharmacology and Molecular Sciences Johns Hopkins University School of Medicine 21205 Baltimore Maryland United States

Abstract

AbstractDNA crosslinking agents such as cisplatin and related platinum(II) analogs are effective drugs to treat solid tumors. However, these therapeutics can cause high toxicity in the body, and tumors can develop resistance to them. To develop less toxic and more effective DNA crosslinkers, medicinal chemists have focused on tuning the ligands in square planar platinum(II) complexes to modulate their bioavailability, targeted cell penetration, and DNA binding rates. Unfortunately, linking in vitro DNA binding capacity of DNA crosslinkers with their in vivo efficacy has proven challenging. Here we report an electrochemical biosensor strategy that allows the study of platinum(II)‐DNA binding in real time. Our biosensors contain a purine‐rich deoxynucleotide sequence, T6(AG)10, modified with a 5’ hexylthiol linker for easy self‐assembly onto gold electrodes. The 3’ terminus is functionalized with the redox reporter methylene blue. Electron transfer from methylene blue to the sensor is a function of platinum(II) compound concentration and reaction time. Using these biosensors, we resolve DNA binding mechanisms including monovalent and bivalent binding, as well as base stacking. Our approach can measure DNA binding kinetics in buffers and in 50 % serum, offering a single‐step, real‐time approach to screen therapeutic compounds during drug development.

Funder

National Institute of General Medical Sciences

Publisher

Wiley

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