Yan Pu scite author profile

Yan Pu

3Publications

143Citation Statements Received

71Citation Statements Given

How they've been cited

217

143

How they cite others

Affiliations

Ministry of Agriculture and Rural Affairs, Chinese Academy of Tropical Agricultural Sciences, Sichuan University

Publications

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Nimble Cloning: A Simple, Versatile, and Efficient System for Standardized Molecular Cloning

Zeng

Shen

et al. 2020

Front. Bioeng. Biotechnol.

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Molecular cloning is one of the most fundamental technologies in molecular biology, and has been critical for driving biotechnological advances. In this study, we have developed a novel method for standardized molecular cloning. The cloning technique known as "Nimble Cloning" uses the restriction enzyme, SfiI, in combination with the T5 exonuclease, to linearize the vector and generate 3 ′-overhangs simultaneously. Both PCR products and plasmids can be used for the cloning reaction in the Nimble Cloning system. The cloning system is highly efficient, suitable for gene expression in both prokaryotic and eukaryotic expression systems, and enables the reuse of DNA fragments or plasmid entry clones. Nimble Cloning is applicable for the cloning of single or multiple fragments, as well as multi-site cloning. Due also to its simplicity and versatility, the cloning method has great potential for the modular assembly of DNA constructs.

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High-Throughput Construction of Intron-Containing Hairpin RNA Vectors for RNAi in Plants

Shen

Gao

et al. 2012

PLoS ONE

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With the wide use of double-stranded RNA interference (RNAi) for the analysis of gene function in plants, a high-throughput system for making hairpin RNA (hpRNA) constructs is in great demand. Here, we describe a novel restriction-ligation approach that provides a simple but efficient construction of intron-containing hpRNA (ihpRNA) vectors. The system takes advantage of the type IIs restriction enzyme BsaI and our new plant RNAi vector pRNAi-GG based on the Golden Gate (GG) cloning. This method requires only a single PCR product of the gene of interest flanked with BsaI recognition sequence, which can then be cloned into pRNAi-GG at both sense and antisense orientations simultaneously to form ihpRNA construct. The process, completed in one tube with one restriction-ligation step, produced a recombinant ihpRNA with high efficiency and zero background. We demonstrate the utility of the ihpRNA constructs generated with pRNAi-GG vector for the effective silencing of various individual endogenous and exogenous marker genes as well as two genes simultaneously. This method provides a novel and high-throughput platform for large-scale analysis of plant functional genomics.

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Evaluation of the Microhaplotypes panel for DNA mixture analyses

Chen

Yin

et al. 2018

Forensic Science International: Genetics

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Yan Pu

Nimble Cloning: A Simple, Versatile, and Efficient System for Standardized Molecular Cloning

High-Throughput Construction of Intron-Containing Hairpin RNA Vectors for RNAi in Plants

Evaluation of the Microhaplotypes panel for DNA mixture analyses

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