Author:
Qin Jilong,Hong Yaoqin,Pullela Karthik,Morona Renato,Henderson Ian R.,Totsika Makrina
Abstract
AbstractThe study of clinically relevant bacterial pathogens relies on molecular and genetic approaches. However, the generally low transformation frequency among natural isolates poses technical hurdles to widely applying common methods in molecular biology, including transformation of large constructs, chromosomal genetic manipulation, and dense mutant library construction. Here we demonstrate that culturing clinical isolates in the presence of polymyxin B nonapeptide (PMBN) improves their transformation frequency via electroporation by up to 100-fold in a dose-dependent and reversible manner. The effect was observed for PMBN-binding uropathogenicEscherichia coli(UPEC) andSalmonella entericastrains but not naturally polymyxin resistantProteus mirabilis. Using our PMBN electroporation method we show efficient delivery of large plasmid constructs into UPEC, which otherwise failed using a conventional electroporation protocol. Moreover, we show a fivefold increase in the yield of engineered mutant colonies obtained inS. entericawith the widely used lambda-Red recombineering method, when cells are cultured in the presence of PMBN. Lastly, we demonstrate that PMBN treatment can enhance the delivery of DNA-transposase complexes into UPEC and increase transposon mutant yield by eightfold when constructing Transposon Insertion Sequencing (TIS) libraries. Therefore, PMBN can be used as a powerful electropermeabilisation adjuvant to aid the delivery of DNA and DNA–protein complexes into clinically important bacteria.
Funder
Australian National Health and Medical Research Council Project Grant
Clive and Vera Ramaciotti Health Investment Grant
Georgina Sweet Award for Women in Quantitative Biomedical Science
Publisher
Springer Science and Business Media LLC
Cited by
6 articles.
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