4.8 Article

Degradation and Deactivation of Bacterial Antibiotic Resistance Genes during Exposure to Free Chlorine, Monochloramine, Chlorine Dioxide, Ozone, Ultraviolet Light, and Hydroxyl Radical

Journal

ENVIRONMENTAL SCIENCE & TECHNOLOGY
Volume 53, Issue 4, Pages 2013-2026

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.est.8b04393

Keywords

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Funding

  1. National Science Foundation [CBET-1254929]

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This work investigated degradation (measured by qPCR) and biological deactivation (measured by culture based natural transformation) of extra- and intracellular antibiotic resistance genes (eARGs and iARGs) by free available chlorine (FAC), NH2Cl, O-3, ClO2, and UV light (254 nm), and of eARGs by (OH)-O-center dot, using a chromosomal ARG (blt) of multidrug-resistant Bacillus subtilis 1A189. Rate constants for degradation of four 266-1017 bp amplicons adjacent to or encompassing the acfA mutation enabling blt overexpression increased in proportion to #AT+GC bps/amplicon, or in proportion to #5'-GG-3' or 5'-TT-3' doublets/amplicon, with respective values ranging from 0.59 to 2.3 (x10(11) M-1 s(-1)) for (OH)-O-center dot, 1.8-6.9 (x10(4) s(-1)) for O-3, 3.9-9.2 (x10(3) M-1 s(-1)) for FAC, 0.35-1.2(x10(1) M-1 s(-1)) for ClO2, and 2.0-8.8 (x10(-2) cm(2)/mJ) for UV at pH 7, and from 1.7-4.4 M(-1)s(-1) for NH2Cl at pH 8. For FAC, NH2Cl, O-3, ClO2, and UV, ARG deactivation paralleled degradation of amplicons approximating a similar to 800-1000 bp acfA-flanking sequence required for natural transformation in B. subtilis, whereas deactivation outpaced degradation for (OH)-O-center dot. At practical disinfectant exposures, eARGs and iARGs were >= 90% degraded/deactivated by FAC, O-3, and UV, but recalcitrant to NH2Cl and ClO2. iARG degradation/deactivation always lagged cell inactivation. These findings provide a quantitative framework for evaluating ARG fate during disinfection/oxidation, and support using qPCR as a proxy for tracking ARG deactivation under carefully selected circumstances.

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