Harvesting and amplifying gene cassettes confers cross-resistance to critically important antibiotics

Author:

Dulyayangkul Punyawee,Beavis Thomas,Lee Winnie WY,Ardagh Robbie,Edwards Frances,Hamilton Fergus,Head Ian,Heesom Kate J.,Mounsey Oliver,Murarik Marek,Reding CarlosORCID,Satapoomin Naphat,Shaw John M.,Takebayashi Yuiko,Tooke Catherine L.,Spencer James,Williams Philip B.,Avison Matthew B.

Abstract

AbstractAmikacin and piperacillin/tazobactam are frequent antibiotic choices to treat bloodstream infection, which is commonly fatal and most often caused by bacteria from the familyEnterobacterales. Here we show that two gene cassettes located side-by-side in and ancestral integron similar to In37have been “harvested” by insertion sequence IS26as a transposon that is already globally disseminated among theEnterobacterales. This transposon encodes the enzymes AAC(6’)-Ib-cr and OXA-1, reported, respectively, as amikacin and piperacillin/tazobactam resistance mechanisms. However, by studying bloodstream infection isolates from 769 patients from, three hospitals serving a population of 1.5 million people in South West England, we show that increased enzyme production due to mutation in an IS26/In37-derived hybrid promoter or, more commonly, transposon copy number amplification is required to simultaneously remove these two key therapeutic options; in many cases leaving only the last-resort antibiotic, meropenem. These findings may help improve the accuracy of predicting piperacillin/tazobactam treatment failure, allowing stratification of patients to receive meropenem or piperacillin/tazobactam, which may improve outcome and slow the emergence of meropenem resistance.

Publisher

Cold Spring Harbor Laboratory

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