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Abstract

Objectives:

To investigate the transcriptional response of bla_OXA-48 and the copy number alteration of IncF_repB plasmid carrying bla_OXA-48 under an antibiotic concentration gradient.

Methods:

Escherichia coli strains harboring bla_OXA-48 on an IncFrep_B plasmid were isolated from Silchar Medical College and Hospital, Silchar, India. Sequence type and common resistance determinants were determined by PCR assay. Plasmid copy number alteration and the transcriptional expression of bla_OXA-48 under different antibiotic pressures were determined by quantitative real-time PCR, and the relative fold change was measured by the ΔΔCT method.

Results and Conclusion:

The plasmid that carried bla_OXA-48 in E. coli ST448 was characterized as IncFrep_B and found to be conjugatively transferable. The isolates were found to coexist with bla_NDM-1 within the IncX3-type plasmid. It was observed that the copy number and transcriptional response of bla_OXA-48 were directly proportional to the increasing concentration of meropenem and ertapenem, whereas in the case of imipenem, it was reversed. The identification of bla_OXA-48 through IncF_repB-type plasmid in this study indicates the potential route of spread of this resistance determinant in this area and also the insights we gained from the transcriptional changes of bla_OXA-48 in response to different antibiotic pressures could also facilitate the development of novel or alternative therapeutic options needed for multidrug-resistant infections.

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Transcriptional Analysis of IncF repB -Mediated bla OXA-48 -Positive Plasmid Characterized from Escherichia coli ST448

Abstract

Objectives:

Methods:

Results and Conclusion:

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References

Supplementary Material