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Genome editing and transcriptional repression in Pseudomonas putida KT2440 via the type II CRISPR system
by
Wu, Jianping
, Wang, Qingzhuo
, Yang, Lirong
, Yang, Sheng
, Sun, Jun
, Wen, Zhiqiang
, Jiang, Yu
in
Applied Microbiology
/ Biotechnology
/ Chemistry
/ Chemistry and Materials Science
/ CRISPR-Cas Systems
/ CRISPR–Cas9 system
/ CRISPR–Cpf1 system
/ Endonucleases - metabolism
/ Enzymology
/ Gene Deletion
/ Gene Editing
/ Gene Expression
/ Genetic aspects
/ Genetic Engineering
/ Genetic transcription
/ Genome editing
/ Green Fluorescent Proteins
/ Methods
/ Microbial genetic engineering
/ Microbial Genetics and Genomics
/ Microbiology
/ Mutagenesis, Insertional
/ Physiological aspects
/ Pseudomonas putida
/ Pseudomonas putida - genetics
/ Pseudomonas putida - metabolism
/ Pseudomonas putida KT2440
/ Single nucleotide mutation
/ Technology application
/ Transcriptional engineering
2018
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Genome editing and transcriptional repression in Pseudomonas putida KT2440 via the type II CRISPR system
by
Wu, Jianping
, Wang, Qingzhuo
, Yang, Lirong
, Yang, Sheng
, Sun, Jun
, Wen, Zhiqiang
, Jiang, Yu
in
Applied Microbiology
/ Biotechnology
/ Chemistry
/ Chemistry and Materials Science
/ CRISPR-Cas Systems
/ CRISPR–Cas9 system
/ CRISPR–Cpf1 system
/ Endonucleases - metabolism
/ Enzymology
/ Gene Deletion
/ Gene Editing
/ Gene Expression
/ Genetic aspects
/ Genetic Engineering
/ Genetic transcription
/ Genome editing
/ Green Fluorescent Proteins
/ Methods
/ Microbial genetic engineering
/ Microbial Genetics and Genomics
/ Microbiology
/ Mutagenesis, Insertional
/ Physiological aspects
/ Pseudomonas putida
/ Pseudomonas putida - genetics
/ Pseudomonas putida - metabolism
/ Pseudomonas putida KT2440
/ Single nucleotide mutation
/ Technology application
/ Transcriptional engineering
2018
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Genome editing and transcriptional repression in Pseudomonas putida KT2440 via the type II CRISPR system
by
Wu, Jianping
, Wang, Qingzhuo
, Yang, Lirong
, Yang, Sheng
, Sun, Jun
, Wen, Zhiqiang
, Jiang, Yu
in
Applied Microbiology
/ Biotechnology
/ Chemistry
/ Chemistry and Materials Science
/ CRISPR-Cas Systems
/ CRISPR–Cas9 system
/ CRISPR–Cpf1 system
/ Endonucleases - metabolism
/ Enzymology
/ Gene Deletion
/ Gene Editing
/ Gene Expression
/ Genetic aspects
/ Genetic Engineering
/ Genetic transcription
/ Genome editing
/ Green Fluorescent Proteins
/ Methods
/ Microbial genetic engineering
/ Microbial Genetics and Genomics
/ Microbiology
/ Mutagenesis, Insertional
/ Physiological aspects
/ Pseudomonas putida
/ Pseudomonas putida - genetics
/ Pseudomonas putida - metabolism
/ Pseudomonas putida KT2440
/ Single nucleotide mutation
/ Technology application
/ Transcriptional engineering
2018
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Genome editing and transcriptional repression in Pseudomonas putida KT2440 via the type II CRISPR system
Journal Article
Genome editing and transcriptional repression in Pseudomonas putida KT2440 via the type II CRISPR system
2018
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Overview
Background
The soil bacterium
Pseudomonas putida
KT2440 is a “generally recognized as safe”-certified strain with robust property and versatile metabolism. Thus, it is an ideal candidate for synthetic biology, biodegradation, and other biotechnology applications. The known genome editing approaches of
Pseudomonas
are suboptimal; thus, it is necessary to develop a high efficiency genome editing tool.
Results
In this study, we established a fast and convenient CRISPR–Cas9 method in
P. putida
KT2440. Gene deletion, gene insertion and gene replacement could be achieved within 5 days, and the mutation efficiency reached > 70%. Single nucleotide replacement could be realized, overcoming the limitations of protospacer adjacent motif sequences. We also applied nuclease-deficient Cas9 binding at three locations upstream of enhanced green fluorescent protein (eGFP) for transcriptional inhibition, and the expression intensity of eGFP reduced to 28.5, 29.4, and 72.1% of the control level, respectively. Furthermore, based on this CRISPR–Cas9 system, we also constructed a CRISPR–Cpf1 system, which we validated for genome editing in
P. putida
KT2440.
Conclusions
In this research, we established CRISPR based genome editing and regulation control systems in
P. putida
KT2440. These fast and efficient approaches will greatly facilitate the application of
P. putida
KT2440.
Publisher
BioMed Central,BioMed Central Ltd,BMC
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