Fernando Eustace Y
Environmental Technology Unit, Industrial Technology Institute, 363 Bauddhaloka Mawatha, Colombo 00700, Sri Lanka.
Enzyme Microb Technol. 2025 Dec;191:110724. doi: 10.1016/j.enzmictec.2025.110724. Epub 2025 Jul 24.
Poly and per fluorinated substances (PFAS) are emerging contaminants of concern that are thought to be involved in causing numerous adverse health effects, such as immunosuppression, increased chance of cancer development, and altered levels of hepatic enzyme levels in humans. However, PFAS are considered highly persistent and resistant to biodegradation given the fact that the C-F bond can have a bond dissociation energy of up to 544 kJ/mol. Though many studies have reported PFAS biodefluorination by bacterial isolates and microbial communities, little is known regarding the molecular foundations for biodefluorination. In this study, a novel defluorinase was identified, that is responsible for the biodefluorination of 6:2 fluorotelomer carboxylic acid (6:2 FTCA) in R.jostii RHA1 using the combination of transposome-based insertional mutagenesis and heterologous expression. From a library of 417 R.jostii RHA1. mutants, 3 individual mutants lost their ability for defluorination when they were exposed to 6:2 FTCA (mutant # 15, 32 and 38 - Table S2). The disruption of the genetic locus in all 3 non-defluorinating mutants was identified coding for a putative MhPC superfamily protein. The MhPC superfamily of proteins is known to harbor other proteins such as fluoroacetate dehalogenase (UniProt - Q6NAM1) that are capable of -C-F bond cleavage. This identified gene was cloned into the heterologous expression host M. smegmatis MC-155. After induction, the M. smegmatis MC-155 transformant exhibited the ability to defluorinate 6:2 FTCA at a rate of 13 µmol/h (V = 80.9 µmol/min and K = 5.04 mM in Michaelis-Menten models). In contrast, defluorination was not observed in either abiotic or biotic controls. Further characterization of the novel defluorinase indicated that it could moderately defluorinate the unsaturated PFAS compound 6:2 FTCUA (4.9 µmol/h fluoride) and minimally defluorinate 5:2 sFTOH (1.3 µmol/h fluoride). The novel defluorinase indicated a maximal specific activity of 12.9 ± 1.9 µmol F/hr/g protein, against its primary PFAS substrate, 6:2 FTCA. However, it showed no activity with 5:3 FTCA or sulfonated PFAS compounds such as 6:2 FTS and 8:2 FTS. The wild-type Rhodococcus could defluorinate 6:2 FTCA at a rate of 2.2 µmol/h. The discovery of this MhPC class novel defluorinase in WT R.jostii RHA1. has substantial value since it is responsible for the critical step that initiates defluorination of PFAS compounds such as 6:2 FTCA.
多氟和全氟化合物(PFAS)是备受关注的新兴污染物,被认为与多种不良健康影响有关,如免疫抑制、癌症发生几率增加以及人体肝酶水平改变。然而,鉴于碳氟键的键解离能高达544 kJ/mol,PFAS被认为具有高度持久性且抗生物降解。尽管许多研究报道了细菌分离株和微生物群落对PFAS的生物脱氟作用,但对于生物脱氟的分子基础知之甚少。在本研究中,通过基于转座体的插入诱变和异源表达相结合的方法,在约氏不动杆菌RHA1中鉴定出一种新型脱氟酶,该酶负责6:2氟调聚物羧酸(6:2 FTCA)的生物脱氟。在417个约氏不动杆菌RHA1突变体文库中,有3个单独的突变体在接触6:2 FTCA时失去了脱氟能力(突变体#15、32和38 - 表S2)。在所有3个非脱氟突变体中,鉴定出编码一种假定的MhPC超家族蛋白的基因座被破坏。已知MhPC超家族蛋白包含其他能够裂解碳氟键的蛋白,如氟乙酸脱卤酶(UniProt - Q6NAM1)。将该鉴定出的基因克隆到异源表达宿主耻垢分枝杆菌MC - 155中。诱导后,耻垢分枝杆菌MC - 155转化体表现出以13 μmol/h的速率对6:2 FTCA进行脱氟的能力(在米氏模型中V = 80.9 μmol/min,K = 5.04 mM)。相比之下,在非生物或生物对照中均未观察到脱氟现象。对这种新型脱氟酶的进一步表征表明,它可以适度地对不饱和PFAS化合物6:2 FTCUA进行脱氟(4.9 μmol/h氟化物),对5:2 sFTOH的脱氟作用最小(1.3 μmol/h氟化物)。这种新型脱氟酶对其主要PFAS底物6:2 FTCA的最大比活性为1十二点九±一点九μmol F/hr/g蛋白。然而,它对5:3 FTCA或磺化PFAS化合物如6:2 FTS和8:2 FTS没有活性。野生型红球菌可以以2.2 μmol/h的速率对6:2 FTCA进行脱氟。在野生型约氏不动杆菌RHA1中发现这种MhPC类新型脱氟酶具有重要价值,因为它负责启动PFAS化合物如6:2 FTCA脱氟的关键步骤。
