Facile and Sensitive Fluorescence Assay of DNA Polymerase Activity Using Cu 2+ and Ascorbate as Signal Developers

We report herein a label‐free and turn‐on fluorescence approach for detecting DNA polymerase activity. In the presence of DNA polymerase, the DNA primer could be elongated to produce one long double‐stranded DNA (dsDNA). Then, the produced dsDNA acted as the template for in‐situ synthesizing fluorescent copper nanoclusters (CuNCs) via Cu 2+ –ascorbate reaction (10 min at room temperature), and the fluorescent intensity of the CuNCs was used to quantify the activity of DNA polymerase. In this strategy, cheap CuSO 4 and ascorbate acted as fluorescence developers, so this method is low‐cost and easy to carry out. Interestingly, based on the sequence‐dependent fluorescence of DNA‐templated CuNCs, we rationally designed the sequence of DNA substrate to decrease the background and increase the signal of this assay. Therefore, this proposed method exhibited a high sensitivity toward DNA polymerase, and the limit of detection was 3.7×10 –7 U/μL for Klenow Fragment (KF) polymerase. The strategy suggests a “mix‐and‐detect” homogenous assay format without precipitation, separation and washing. The whole process (including enzyme reaction and synthesizing CuNCs) can be completed in a single tube. This fluorescence method is low‐cost and simple, and shows potential application in some biomedical studies and clinical diagnostics.