Electronically controlled deprotection chemistry for multiplex enzymatic DNA synthesis on a chip with single-base resolution

Abstract

Enzymatic deoxyribonucleic acid (DNA) synthesis (EDS) is an environmentally friendly approach capable of generating longer and more complex sequences than chemical synthesis, making it a promising next-generation technology for high-throughput single-stranded DNA production. However, precise sequence control at high throughput remains a key challenge. Here, we present a novel electronically controlled deprotection chemistry (ECDC) integrated with a hydrogel–primer modification system on-chip for efficient multiplexed EDS. Electrochemically generated HNO2 at the working electrodes selectively converts the 3′-oxyamino group of DNA into a hydroxyl group, enabling precise spatiotemporal control of a multipixel synthesis array and facilitating future automation. This platform enables parallel EDS with single-base resolution on silicon chips. In four-nucleotide validation experiments, single-sequence synthesis could achieve 100% accuracy, while dual-sequence synthesis reached an average accuracy of approximately 96%. Our approach provides a highly accurate solution for high-throughput ssDNA synthesis, laying the foundation for scalable and automated enzymatic DNA manufacturing.

Graphical abstract: Electronically controlled deprotection chemistry for multiplex enzymatic DNA synthesis on a chip with single-base resolution

Supplementary files

Article information

Article type
Paper
Submitted
04 Jun 2025
Accepted
27 Aug 2025
First published
05 Sep 2025

Lab Chip, 2025, Advance Article

Electronically controlled deprotection chemistry for multiplex enzymatic DNA synthesis on a chip with single-base resolution

L. Zhao, Q. Sun, J. Jiang, X. Wu, Y. Dong, D. Wu, L. Wu and X. Zhao, Lab Chip, 2025, Advance Article , DOI: 10.1039/D5LC00548E

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