Which Drinking Water Disinfection Process Generates the Least Toxic DBP Mixture: Chlorination, Chloramination, Ozonation, or Chlorine Dioxide Treatment?

Xiangru Zhang JCEE editorial board member, Department of Civil and Environmental Engineering, The Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, Hong Kong SAR, China *Corresponding author: Xiangru Zhang JCEE editorial board member Department of Civil and Environmental Engineering The Hong Kong University of Science and Technology Clear Water Bay, Kowloon, Hong Kong SAR, China E-mail: xiangru@ust.hk Complexity and Unknowns of Disinfection Byproducts (DBPs) in Drinking Waters Chlorine, chloramines, chlorine dioxide, and ozone are widely used drinking water disinfectants. The use of these disinfectants affords great success in eliminating harmful microorganisms and acute waterborne diseases, but in the disinfection process, they may react with Natural Organic Matter (NOM), bromide, and iodide in source waters to produce DBPs. NOM in natural waters mainly originates from the decomposition of plants. It consists of a wide variety of complex organic compounds with molecular weights ranging from hundreds to hundreds of thousands of Da. The complexity of NOM determines a higher magnitude of complexity of the reaction products from disinfectants and NOM with/without bromide and iodide. Since Rook [2] first found trihalomethanes as DBPs in finished drinking water in 1974, numerous DBPs have been identified in real or simulated drinking waters. Commonly known DBPs include trihalomethanes, haloacetic acids, haloacetonitriles, haloketones, cyanogen halides, chloropicrin, chloral hydrate, N-nitrosodimethylamine, bromate, and chlorite. Richardson compiled a review on drinking water DBPs formed from using four major disinfectants, in which she listed about 600 DBPs that were identified by gas chromatography/mass spectrometry (GC/MS). Of the 600 DBPs, some are commonly known DBPs and occur at low-μg/L levels, some occur at sub-μg/L or ng/L levels, and some may still not be quantifiable. The non-quantifiable DBPs are because of no corresponding standard compounds for calibration or their concentrations below detection limits. In addition, there are a countless number of unidentified/unknown DBPs. A collective parameter for all the organic halogenated DBPs is total organic halogen (TOX). Only a fraction of TOX formed during disinfection has been chemically identified or even well characterized. By simulating a typical drinking water disinfection condition, Zhang et al. [7] demonstrated that the percentages of total organic chlorine (TOCl) that could be represented by the commonly known chlorinated DBPs in the chlorine, chlorine dioxide, and chloramine treated samples were 50, 31, and 17%, respectively; the percentages of total organic bromine (TOBr) that could be represented by the commonly known brominated DBPs in the chlorine, chlorine dioxide, chloramine, and ozone treated samples were 60, 26, 14, and 8.2%, respectively. The uncounted parts of TOX, TOCl and TOBr are mainly ascribed to unknown/unidentified DBPs in drinking waters, which may exist due to limitations of GC/MS because GC/MS is not amenable to identification of highly polar compounds, and compounds with molecular weights of more than 650 Da [8]. Recently, novel precursor ion scan methods using ultra performance liquid chromatography/ electrospray ionization-triple quadrupole mass spectrometry have been developed for fast selective detection of polar chloro-/bromo-/ iodo-DBPs in drinking waters. Status Quo and Existing Problems of Toxicologic Studies on DBPs in Drinking Waters Although DBP levels in most finished drinking waters are very low, “the large absolute amount of water (about 50,000 liters) ingested by an individual over a lifetime means that human exposure to chemical contaminants may be significant”. Epidemiological studies suggest that human consumption of chlorinated drinking water is somewhat associated with increased spontaneous abortions, stillbirth, birth defects, bladder cancer, and rectal cancer. Some DBPs have been regulated in Stage I of the Disinfectants/Disinfection By-Products (D/ DBP) Rule by the U.S. Environmental Protection Agency. A vast majority of laboratory-based toxicologic studies have been conducted with individual DBPs . Richardson et al.  reviewed 30 years of research on the occurrence, genotoxicity, and carcinogenicity of 85 DBPs. A systematic assessment of individual DBPs for genotoxicity has been performed for 60 DBPs for DNA damage in mammalian cells and 16 for mutagenicity in Salmonella. The results show that eight of them have some or all of the toxicologic characteristics of human carcinogens, and 29 of them are genotoxic; brominated DBPs are both more genotoxic and carcinogenic than their chlorinated analogues, and iodinated DBPs were the most genotoxic of all. Most toxicologic studies on individual DBPs are conducted with bacterial or mammalian cell assays, i.e., the cytotoxicity and mutagenicity assays using Salmonella typhimurium strain TA100 , or the cytotoxicity and genotoxicity assays using Chinese hamster ovary cells . Both types of assays have been used to quantitatively compare cytotoxicity, mutagenicity or genotoxicity of known individual DBPs. In cytotoxicity assays, for instance, the DBP concentration that induces 50% repression of growth is LC50. With LC50 values, the cytotoxicity rank order of individual DBPs can be assigned. Although toxicologic results of individual DBPs can be indicative of mechanisms of health effects, they cannot be directly linked to the toxicity of a whole DBP mixture. This is because: (a) for the individual DBPs that have been performed with the bacterial or mammalian cell assays, the concentrations that induce the cytotoxicity, mutagenicity or genotoxicity are around 4−6 orders of magnitude higher than their actual concentrations in drinking water; (b) the number of DBPs in drinking water is countless and most of them are unknown, unidentified or non-quantifiable, and thus it is prohibitive and unlikely to achieve the occurrence and toxicologic data of all individual DBPs; (c) even if the occurrence and toxicologic data of all individual DBPs are achievable, the toxicity of the whole DBP mixture may still not be achievable owing to potential interactions among the DBPs. These interactions can be addition, synergy, and antagonism. Synergy (or antagonism) is a phenomenon where two or more agents in combination have an overall effect which is greater (or less) than the sum of their individual effects. Accordingly, evaluation of the toxicity of each individual DBP alone is insufficient for understanding the biological effects of the whole DBP mixture. Importance of estimating the overall toxicity of DBP mixtures has been increasingly recognized in most recent years. Despite numerous toxicologic reports on individual DBPs, significantly fewer investigations have been done on DBP mixtures. Only a couple of studies have examined the cytotoxicity and mutagenicity of drinking water extracts in Salmonella or mammalian-cell assays. A disinfected drinking water sample itself seems to be an ideal DBP mixture, but it cannot be used directly for the bacterial or mammaliancell assay because either the bacterial or the mammalian-cell assay is not sensitive enough. To perform the bacterial or mammalian-cell assay of a drinking water DBP mixture, it is most critical to concentrate the drinking water sample. There are two procedures for concentrating a drinking water sample for the bioassays. (a) Solid phase extraction: 20−200 L of disinfected drinking waters (with source water DOC of 1.6−9.0 mg/L as C) → acidified to pH 2 → filtrated by XAD-2 / CHP20P resin or by C18 / CSP-800 cartridge → the resin or cartridge eluted with methanol / acetonitrile / dichloromethane / acetone / ethyl acetate / DMSO → the eluates evaporated to dryness → dissolved in 0.8-2.0 mL DMSO. The samples were concentrated by 10,000-200,000 times. (b) Liquid phase extraction : 70 mL of a simulated chlorinated water sample (with source water DOC of 108 mg/L as C) → lyophilized to dryness → extracted with ethyl acetate → the organic layer evaporated to dryness → dissolved in 200 μL DMSO. The highly dosed simulated sample was concentrated by 350 times. Compared to the typical DOC level in source water, this sample was concentrated by ~10,000 times. For either the solid or liquid phase extraction of a typical drinking water sample or a highly dosed drinking water sample, concentration of organic DBPs up to 10,000−200,000 times and removal of dissolved inorganic salts are the prerequisites for the bacterial or mammalian-cell assays. In the extraction procedure, apart from the tedious and timeconsuming steps involved, a major problem is that part or all of certain specific types of DBPs may be lost. For the solid phase extraction, all inorganic DBPs (such as bromate in ozonated water and chlorite in chlorine dioxide treated water) and some polar/highly polar organic DBPs may not be adsorbed on the resin/cartridge, some organic DBPs strongly adsorbed on the resin/cartridge may not be desorbed during eluting with the organic solvent(s), and all volatile organic DBPs are lost during solvent evaporation to dryness. For the liquid phase extraction, a similar problem may occur. Therefore, the extracts involve significant losses in DBP species and levels, and thus cannot accurately reflect the toxicity of drinking water DBP mixtures. A New Approach Needed to Evaluate the Toxicity of Drinking Water DBP Mixtures Chlorine is the most widely used disinfectant. Chlorination generates relatively high levels of chlorinated/brominated organic DBPs including chloro-/bromo- trihalomethanes and haloacetic acids, 9 of which have been regulated in Stage I of the D/DBP Rule. To reduce the formation of chlorinated/brominated organic DBPs, some drinking water utilities have switched to alternative disinfectants such as ozone, chlorine dioxide, and chloramine, however, other DBPs are formed. For instances, ozonation and chlorine dioxide treatment generate bromate and chlorite, respectively, both of which have also been regulated in Stage I of the D/DBP Rule; chloramination generates relatively high levels of iodo-DBPs. Only a few early studies examined the Salmonella mutagenicity of solid phase extraction extracts of drinking waters prepared with alternative disinfectants, and the results showed that drinking water with alternative disinfectants was less mutagenic than chlorinated drinking water. However, as aforementioned, the organic extracts by solid phase extraction involve significant losses in DBP species and levels (e.g. they completely exclude bromate and chlorite), and thus cannot adequately represent the toxicity of the DBP mixtures of drinking waters. Now that the solid or liquid phase extraction may cause significant DBP losses, a new approach to evaluating the toxicity of drinking water DBP mixtures should involve a better procedure for concentrating all types of DBPs, including organic and inorganic, and volatile and polar ones. Also, since the bacterial or the mammalian-cell assay is not sensitive enough, a new approach should entail a more sensitive bioassay species to the DBPs mixtures. It is expected that, with the new approach, the long-lasting issue in drinking water disinfection—which disinfection process generates the least toxic DBP mixture, chlorination, chloramination, ozonation, or chlorine dioxide treatment?—can be resolved.

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