An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency

DNA cloning requires two steps: the assembly of recombinant DNA molecules and the transformation of the product into a host organism for replication. High efficiencies in both processes can increase the success rate. Recently, we developed an Escherichia coli BW3KD strain with higher transformation...

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Autores principales: Yang, Yuqing, Liu, Menghui, Wang, Tianqi, Wang, Qian, Liu, Huaiwei, Xun, Luying, Xia, Yongzhen
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Microbiology 2022
Materias:
Methods and Protocols
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9769673/
https://www.ncbi.nlm.nih.gov/pubmed/36317996
http://dx.doi.org/10.1128/spectrum.02497-22
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author Yang, Yuqing
Liu, Menghui
Wang, Tianqi
Wang, Qian
Liu, Huaiwei
Xun, Luying
Xia, Yongzhen
author_facet Yang, Yuqing
Liu, Menghui
Wang, Tianqi
Wang, Qian
Liu, Huaiwei
Xun, Luying
Xia, Yongzhen
author_sort Yang, Yuqing
collection PubMed
description DNA cloning requires two steps: the assembly of recombinant DNA molecules and the transformation of the product into a host organism for replication. High efficiencies in both processes can increase the success rate. Recently, we developed an Escherichia coli BW3KD strain with higher transformation efficiency than commonly used cloning strains. Here, we further developed a simple method named TSS-HI (transformation storage solution optimized by Hannahan and Inoue method) for competent cell preparation, which combined the advantages of three common methods for operational simplicity and high transformation efficiency. When competent BW3KD cells were prepared using this developed method, the transformation efficiency reached up to (7.21 ± 1.85) × 10(9) CFU/μg DNA, which exceeded the levels of commercial chemically competent cells and homemade electrocompetent cells. BW3KD cells formed colonies within 7 h on lysogeny broth agar plates, quicker than the well-known fast-growing E. coli cloning strain Mach1. The competent cells worked effectively for the transformation of assembled DNA of 1 to 7 fragments in one step and promoted efficiencies of transformation or cloning with large plasmids. The cloning efficiency of BW3KD cells prepared by this method increased up to 828-fold over that of E. coli XL1-Blue MRF′ cells prepared by a common method. Thus, competent cells are suitable for different cloning jobs and should help with the increased demand for DNA assembly in biological studies and biotechnology. IMPORTANCE DNA transformation is commonly used in cloning; however, high transformation efficiency becomes a limiting factor in many applications, such as the construction of CRISPR and DNA libraries, the assembly of multiple fragments, and the transformation of large plasmids. We developed a new competent cell preparation method with unmatched transformation efficiency. When the BW3KD strain, derived from Escherichia coli BW25113 cells, was prepared by this method, its transformation efficiency reached up to (7.21 ± 1.85) × 10(9) CFU/μg DNA, which broke the record for chemically prepared competent cells. Routine cloning could be completed in 1 day due to the high growth rate of this strain. The competent cells were shown to be highly efficient for transformation or cloning with large plasmids and for the assembly of multiple fragments. The results highlight the effectiveness of the new protocol and the usefulness of the BW3KD strain as the host.
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spelling pubmed-97696732022-12-22 An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency Yang, Yuqing Liu, Menghui Wang, Tianqi Wang, Qian Liu, Huaiwei Xun, Luying Xia, Yongzhen Microbiol Spectr Methods and Protocols DNA cloning requires two steps: the assembly of recombinant DNA molecules and the transformation of the product into a host organism for replication. High efficiencies in both processes can increase the success rate. Recently, we developed an Escherichia coli BW3KD strain with higher transformation efficiency than commonly used cloning strains. Here, we further developed a simple method named TSS-HI (transformation storage solution optimized by Hannahan and Inoue method) for competent cell preparation, which combined the advantages of three common methods for operational simplicity and high transformation efficiency. When competent BW3KD cells were prepared using this developed method, the transformation efficiency reached up to (7.21 ± 1.85) × 10(9) CFU/μg DNA, which exceeded the levels of commercial chemically competent cells and homemade electrocompetent cells. BW3KD cells formed colonies within 7 h on lysogeny broth agar plates, quicker than the well-known fast-growing E. coli cloning strain Mach1. The competent cells worked effectively for the transformation of assembled DNA of 1 to 7 fragments in one step and promoted efficiencies of transformation or cloning with large plasmids. The cloning efficiency of BW3KD cells prepared by this method increased up to 828-fold over that of E. coli XL1-Blue MRF′ cells prepared by a common method. Thus, competent cells are suitable for different cloning jobs and should help with the increased demand for DNA assembly in biological studies and biotechnology. IMPORTANCE DNA transformation is commonly used in cloning; however, high transformation efficiency becomes a limiting factor in many applications, such as the construction of CRISPR and DNA libraries, the assembly of multiple fragments, and the transformation of large plasmids. We developed a new competent cell preparation method with unmatched transformation efficiency. When the BW3KD strain, derived from Escherichia coli BW25113 cells, was prepared by this method, its transformation efficiency reached up to (7.21 ± 1.85) × 10(9) CFU/μg DNA, which broke the record for chemically prepared competent cells. Routine cloning could be completed in 1 day due to the high growth rate of this strain. The competent cells were shown to be highly efficient for transformation or cloning with large plasmids and for the assembly of multiple fragments. The results highlight the effectiveness of the new protocol and the usefulness of the BW3KD strain as the host. American Society for Microbiology 2022-11-01 /pmc/articles/PMC9769673/ /pubmed/36317996 http://dx.doi.org/10.1128/spectrum.02497-22 Text en Copyright © 2022 Yang et al. https://creativecommons.org/licenses/by/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Methods and Protocols
Yang, Yuqing
Liu, Menghui
Wang, Tianqi
Wang, Qian
Liu, Huaiwei
Xun, Luying
Xia, Yongzhen
An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title_full An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title_fullStr An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title_full_unstemmed An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title_short An Optimized Transformation Protocol for Escherichia coli BW3KD with Supreme DNA Assembly Efficiency
title_sort optimized transformation protocol for escherichia coli bw3kd with supreme dna assembly efficiency
topic Methods and Protocols
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9769673/
https://www.ncbi.nlm.nih.gov/pubmed/36317996
http://dx.doi.org/10.1128/spectrum.02497-22
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