RH2Fusion: A universal tool for precise DNA fragment assembly

Despite its limitations, restriction enzyme (RE)-mediated cleavage remains the prevalent method for generating sticky ends in DNA assembly. Here, we present RNase HII Fusion (RH2Fusion), a robust system for user-defined sticky ends, enabling scarless assembly of multiple DNA fragments alongside simu...

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Published in:International journal of biological macromolecules 2024-12, Vol.288, p.138788, Article 138788
Main Authors: Liu, Benchao, Zhao, Junru, Chen, Hui, Dong, Yan, Zhang, Xiandan, Lv, Min, Yang, Yunruo, Liu, Huaqing, Zhang, Jianhui, Zheng, Hualei, Zhang, Yongyou
Format: Article
Language:English
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DNA assembly
Molecular cloning
RH2Fusion
Ribonuclease
RNase HII
YgdG
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container_title International journal of biological macromolecules
container_volume 288
creator Liu, Benchao
Zhao, Junru
Chen, Hui
Dong, Yan
Zhang, Xiandan
Lv, Min
Yang, Yunruo
Liu, Huaqing
Zhang, Jianhui
Zheng, Hualei
Zhang, Yongyou
description Despite its limitations, restriction enzyme (RE)-mediated cleavage remains the prevalent method for generating sticky ends in DNA assembly. Here, we present RNase HII Fusion (RH2Fusion), a robust system for user-defined sticky ends, enabling scarless assembly of multiple DNA fragments alongside simultaneous site-directed mutagenesis (SDM) at multiple sites. In bacterial cells, DNA fragments with ribonucleotide modifications are expected to form complementary 3′ overhangs after RNase HII treatment, followed by annealing and recombination via the bacterial self-repair system. In vitro, RNase HII-mediated cleavage produces similar overhangs, which are subsequently processed and ligated by YgdG and T4 DNA ligase, enabling efficient DNA assembly. We report for the first time that Escherichia coli Exonuclease IX (YgdG) possesses ribonuclease-specific cleavage activity, selectively cleaving ribonucleotides without cleaving deoxyribonucleotides. Through the fusion of RNase HII and YgdG, novel constructs RNase RY (RNase HII-YgdG) and RNase YR (YgdG-RNase HII) are generated, each showcasing dual enzyme functionality. In conclusion, RH2Fusion offers a rapid, effective, and versatile alternative for DNA assembly, empowering researchers across diverse fields like synthetic biology and genetic engineering. This transformative tool is poised to significantly enhance the capabilities of DNA manipulation and advance molecular biology research.
doi_str_mv 10.1016/j.ijbiomac.2024.138788
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subjects DNA assembly
Molecular cloning
RH2Fusion
Ribonuclease
RNase HII
YgdG
title RH2Fusion: A universal tool for precise DNA fragment assembly
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