Establishment of a markerless multiple-gene deletion method based on Cre/loxP mutant system for Bacillus pumilus

Zheng-Bing Guan; Kai-Qiang Wang; Yan Shui; Xiang-Ru Liao

doi:10.1002/jobm.201700370

Establishment of a markerless multiple-gene deletion method based on Cre/loxP mutant system for Bacillus pumilus

J Basic Microbiol. 2017 Dec;57(12):1065-1068. doi: 10.1002/jobm.201700370. Epub 2017 Oct 20.

Authors

Zheng-Bing Guan¹, Kai-Qiang Wang¹, Yan Shui², Xiang-Ru Liao¹

Affiliations

¹ The Key Laboratory of Industrial Biotechnology, Ministry of Education, School of Biotechnology, Jiangnan University, Wuxi, P. R. China.
² The Key Laboratory of Freshwater Fisheries and Germplasm Resources Utilization, Ministry of Agriculture, Freshwater Fisheries Research Center, Chinese Academy of Fishery Sciences, Wuxi, P. R. China.

PMID: 29052235
DOI: 10.1002/jobm.201700370

Abstract

In this study, we established a Cre/loxP mutant recombination system (Cre/lox71-66 system) for markerless gene deletion to facilitate our follow-up rational genetic engineering to the strain Bacillus pumilus W3. This modified method uses two mutant loxP sites, which after recombination creates a double-mutant loxP site that is poorly recognized by Cre recombinase, facilitating multiple gene deletions in a single genetic background. Two selected genes, cotA and sigF, were continuously knocked out and verified at different levels using this method. This method is simple and efficient and can be easily implemented for multiple gene deletions in B. pumilus.

Keywords: Bacillus pumilus; Cre/loxP system; gene deletion; recombination.

MeSH terms

Bacillus pumilus / genetics*
Binding Sites
DNA, Bacterial / metabolism
Gene Deletion
Gene Knockout Techniques*
Genes, Bacterial
Integrases / metabolism
Mutagenesis, Site-Directed / methods*
Recombination, Genetic

Substances

DNA, Bacterial
Cre recombinase
Integrases