222 nm causes greater protein damage and repair inhibition of E. coli than 254 nm for water disinfection

PLOS water Pub Date : 2024-07-24 DOI:10.1371/journal.pwat.0000238

David McDonald, Daniel Ma, Natalie M. Hull

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Abstract

Germicidal ultraviolet (UV) light has been widely used to inactivate pathogens in water. Emerging alternatives to conventional low pressure (LP) mercury lamps emitting at 254 nm, such as krypton chloride (KrCl) excimer lamps emitting at 222 nm, are gaining acceptance and popularity due to advantages in human safety and disinfection mechanisms. Cyclobutane pyrimidine dimer (CPD) formation kinetics and photolyase damage kinetics were quantified in E. coli for 222 nm and 254 nm UV. Molecular damage and cell regrowth were also quantified after UV irradiation under photorepair and dark repair incubation conditions using a standardized photorepair fluence response protocol. CPDs and photolyase were measured using enzyme linked immunosorbent assays (ELISA). A novel ELISA for photolyase was developed for this study. Culture-based log inactivation UV fluence responses were similar for 254 nm and 222 nm, with Geeraerd model estimates for rate constants of 1.18±0.09 and 1.24±0.08 cm2 mJ−1 for LP and KrCl lamps, respectively. Molecular UV fluence kinetics showed that the rate of CPD formation was greater by LP, but the rate of photolyase damage was greater by KrCl, as supported by the intercepts of repair kinetics. Compared to LP irradiated samples, KrCl irradiated samples exhibited less repair overall. For a given lamp, similar repair was observed between light and dark repair incubations. Percent reactivation rates with respect to photorepair fluence were (3.7±1.4)×10−5 and (–1.3±2.5)×10−5 cm2 mJ-1 for LP and KrCl lamps, respectively. CPDs decreased at a higher rate during repair incubations in LP samples than KrCl samples, and photolyase concentration increased in LP samples but decreased in KrCl samples. The results quantify contributions of photolyase protein damage to disinfection and repair prevention mechanism of KrCl lamps. This study mechanistically demonstrates why KrCl lamps can be applied for UV water disinfection to limit photorepair after treatment. Synopsis: This study used a novel photolyase assay to demonstrate photolyase damage inflicted by krypton chloride excimer lamps contributes to disinfection of bacteria to prevent bacterial photorepair of damaged DNA and regrowth in drinking water treatment.

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用于水消毒时，222 纳米比 254 纳米对大肠杆菌的蛋白质破坏和修复抑制作用更大

紫外线（UV）杀菌灯已被广泛用于灭活水中的病原体。由于在人类安全和消毒机制方面的优势，传统的 254 纳米低压汞灯的新兴替代品，如 222 纳米的氯化氪（KrCl）准分子灯，正逐渐被接受和普及。对大肠杆菌在 222 纳米和 254 纳米紫外线下的环丁烷嘧啶二聚体（CPD）形成动力学和光解酶损伤动力学进行了量化。在光修复和暗修复孵育条件下，还使用标准化的光修复通量响应协议对紫外线照射后的分子损伤和细胞再生进行了量化。使用酶联免疫吸附试验（ELISA）测量了 CPDs 和光解酶。本研究开发了一种新型的光解酶 ELISA。基于培养基的对数失活紫外线通量反应在 254 纳米和 222 纳米波长下相似，Geeraerd 模型估计 LP 灯和 KrCl 灯的速率常数分别为 1.18±0.09 和 1.24±0.08 cm2 mJ-1。分子紫外通量动力学表明，LP 的 CPD 形成率更高，但 KrCl 的光解酶破坏率更高，这一点可以从修复动力学的截距中得到证实。与 LP 辐照样品相比，KrCl 辐照样品的总体修复率较低。对于特定的灯管，在光照和黑暗修复培养条件下观察到的修复情况相似。LP 灯和 KrCl 灯的光修复通量百分比再活化率分别为 (3.7±1.4)×10-5 和 (-1.3±2.5)×10-5 cm2 mJ-1。与 KrCl 样品相比，LP 样品在修复过程中 CPDs 的下降率更高，LP 样品中的光解酶浓度增加，而 KrCl 样品中的光解酶浓度下降。研究结果量化了光解酶蛋白质损伤对氯化氢灯的消毒和修复预防机制的贡献。这项研究从机理上证明了为什么氯化氪灯可用于紫外线水消毒，以限制处理后的光修复。简要说明：这项研究使用了一种新型光解酶测定法，证明了氯化氪准分子灯造成的光解酶损伤有助于细菌消毒，以防止细菌对受损 DNA 进行光修复，并在饮用水处理过程中防止细菌再生。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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PLOS water

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