AI Article Synopsis

  • Previous studies linked 23S rRNA gene mutations to macrolide resistance in M. catarrhalis, but new research suggests there may be other mechanisms involved.
  • This study focused on two isolated strains of M. catarrhalis—one resistant and one susceptible—to find differences in genes and single nucleotide polymorphisms (SNPs) that might be associated with drug resistance.
  • Of the genes and SNPs analyzed, 10 genes and 6 SNPs were identified that may contribute to macrolide resistance, mainly through processes related to ribosomal RNA and DNA methylation, indicating a need for further research on their roles.

Article Abstract

Although previous studies have confirmed that 23S rRNA gene mutation could be responsible for most of macrolide resistance in M. catarrhalis, a recent study suggested otherwise. Next generation sequence based comparative genomics has revolutionized the mining of potential novel drug resistant mechanisms. In this study, two pairs of resistant and susceptible M. catarrhalis isolates with different multilocus sequence types, were investigated for potential differential genes or informative single nucleotide polymorphisms (SNPs). The identified genes and SNPs were evaluated in 188 clinical isolates. From initially 12 selected differential genes and 12 informative SNPs, 10 differential genes (mboIA, mcbC, mcbI, mboIB, MCR_1794, MCR_1795, lgt2B/C, dpnI, mcbB, and mcbA) and 6 SNPs (C619T of rumA, T140C of rplF, G643A of MCR_0020, T270G of MCR_1465, C1348A of copB, and G238A of rrmA) were identified as possibly linked to macrolide resistance in M. catarrhalis. Most of the identified differential genes and SNPs are related to methylation of ribosomal RNA (rRNA) or DNA, especially MCR_0020 and rrmA. Further studies are needed to determine the function and/or evolution process, of the identified genes or SNPs, to establish whether some novel or combined mechanisms are truly involved in M. catarrhalis macrolide resistance mechanism.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5075928PMC
http://dx.doi.org/10.1038/srep35711DOI Listing

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