- Email: [email protected]
Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods
Accepted Manuscript Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods G. Liu, F.Q. Ling, A. Magic-Knezev, W.T. Liu, J.Q.J.C. Verberk, J.C. Van Dijk PII:
S0043-1354(13)00306-0
DOI:
10.1016/j.watres.2013.03.058
Reference:
WR 9880
To appear in:
Water Research
Received Date: 16 November 2012 Revised Date:
2 March 2013
Accepted Date: 31 March 2013
Please cite this article as: Liu, G., Ling, F.Q., Magic-Knezev, A., Liu, W.T., Verberk, J.Q.J.C., Van Dijk, J.C., Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods, Water Research (2013), doi: 10.1016/ j.watres.2013.03.058. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Quantification and identification of particle-associated bacteria in unchlorinated drinking
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water from three treatment plants by cultivation-independent methods
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G. Liu1 *, F. Q. Ling2, A. Magic-Knezev3, W. T. Liu2, J.Q.J.C.Verberk1, J.C. Van Dijk1
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1. Section Sanitary Engineering, Department of Water Management, Faculty of Civil
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Engineering and Geosciences, Delft University of Technology, PO BOX 5048, 2600 GA Delft,
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the Netherlands E-mail: [email protected]
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2. Department of Civil and Environmental Engineering, University of Illinois Urbana-
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Champaign, 205 N. Mathews Ave., Urbana, Illinois 61801, U.S.A.
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3. Het Water Laboratorium, PO BOX 734, 2003 RS Haarlem, the Netherlands
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Corresponding author:
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Gang Liu
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Email: [email protected]
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Tel: 0031 15 2785457\ 0031 6 41866671
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Abstract
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Water quality regulations commonly place quantitative limits on the number of organisms
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(e.g., heterotrophic plate count and coliforms) without considering the presence of multiple
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cells per particle, which is only counted as one regardless how many cells attached. Therefore,
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it is important to quantify particle-associated bacteria (PAB), especially cells per particle. In
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addition, PAB may house (opportunistic) pathogens and have higher resistance to disinfection
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than planktonic bacteria. It is essential to know bacterial distribution on particles. However,
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limited information is available on quantification and identification of PAB in drinking water.
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In the present study, PAB were sampled from the unchlorinated drinking water at three
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treatment plants in the Netherlands, each with different particle compositions. Adenosine
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triphosphate (ATP) and total cell counts (TCC) with flow cytometry were used to quantify the
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PAB, and high-throughput pyrosequencing was used to identify them. The number and
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activity of PAB ranged from 1.0-3.5×103 cells ml-1 and 0.04-0.154 ng l-1 ATP. There were
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between 25 and 50 cells found to be attached on a single particle. ATP per cell in PAB was
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higher than in planktonic bacteria. Among the identified sequences, Proteobacteria were
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found to be the most dominant phylum at all locations, followed by OP3 candidate division
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and Nitrospirae. Sequences related to anoxic bacteria from the OP3 candidate division and
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other anaerobic bacteria were detected. Genera of bacteria were found appear to be consistent
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with the major element composition of the associated particles. The presence of multiple cells
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per particle challenges the use of quantitative methods such as HPC and Coliforms that are
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used in the current drinking water quality regulations. The detection of anoxic and anaerobic
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bacteria suggests the ecological importance of PAB in drinking water distribution systems.
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Keywords: particle associated bacteria (PAB), drinking water, adenosine triphosphate (ATP),
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flow cytometry, pyrosequencing
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1. Introduction When distributing drinking water, the regrowth of bacteria and other organisms may occur
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and lead to water quality deterioration (Ridgway and Olson, 1982; Van Der Kooij, 2000).
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Depending on the source water and water treatment, more or less planktonic bacteria (PB), as
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well as particle-associated bacteria (PAB) and biodegradable compounds, are present in the
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treated water. They enter the drinking water distribution system (DWDS) and may serve as
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“seeds” for regrowth. The generation of PAB during drinking water treatment is caused by the
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action of particles as the site for attachment and growth of bacteria (Gregory, 2005;
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Winkelmann and Harder, 2009). It has been reported that PAB represent a small number
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compared to the PB population in treated water (Brazos and O'Connor, 1996). Nevertheless,
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the PAB that may pass through or be generated during treatment have been considered an
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important source of bacteria entering the drinking water distribution systems both for bacterial
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regrowth (Camper et al., 1986) and bacteria in accumulated loose deposits (Gauthier et al.,
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1999; Vreeburg et al., 2008; Liu et al., 2013). PAB have been detected in 41.4% of the
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samples of granular activated carbon filtered water at water treatment plants (Camper et al.,
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1986), and in 17% of samples collected from fire hydrants in drinking water distribution
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systems and water well outlets (Ridgway and Olson, 1981).
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Since the attachment and growth of bacteria can lead to biofilm formation on particles
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(Winkelmann and Harder, 2009), a major concern regarding PAB is their resistance to
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disinfection (Brazos and O'Connor, 1996; Dietrich et al., 2009; Hess-Erga et al., 2008;
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Hoadley and Gould, 1977; Lin et al., 2010; Wojcicka et al., 2008). PAB have been proven to
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be more resistant to disinfection by chlorine (Ridgway and Olson, 1982), ozone (Hess-Erga et
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al., 2008) and ultraviolet (UV) (Mamane and Linden, 2006; Wu et al., 2005) than PB are. As a
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result, the regrowth or survival of pathogens in drinking water distribution systems may be
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enhanced (Herson et al., 1987). Considering the disinfection resistance of PB and PAB, the
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nutrient limitation approach (Van der Kooij, 1992) to produce biologically stable drinking
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water is likely to control the regrowth of both PB, PAB and bacteria in biofilms attached to
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pipe walls.
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Another concern regarding PAB is the potential underestimation of bacterial numbers because
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no matter how many bacteria have been attached to one particle, they will be counted as one
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by traditional culture methods (Camper et al., 1986). Water quality regulations commonly
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place quantitative limits on the number of organisms (e.g., heterotrophic plate count and
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coliforms) and particle densities (e.g., turbidity), resulting in a substantial underestimation of
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the PAB bacteria present (Dietrich et al., 2007). In addition, PAB may house (opportunistic)
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pathogens and the dose of microbes may differ significantly if PAB rather than PB are
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ingested, thereby increasing the potential risk to customers. For instance, Herson et al. (1991)
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found that a large number of coliforms added to particle-containing drinking water could not
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be reflected by plate counting because they accumulated as PAB.
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All the above-mentioned studies have improved knowledge of the importance of PAB in
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drinking water. However, limited studies on PAB in drinking water have been conducted,
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most of which applied cultivation-dependent methods (Camper et al., 1985; Ridgway and
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Olson, 1982; Wu et al., 2005) or microscopic observations (Brazos and O'Connor, 1996).
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Considerable bias and underestimation may be introduced by applying these methods.
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Consequently, PAB in drinking water have been poorly documented. Cultivation-independent
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techniques for bacterial quantification and identification offer new posibilities to reevaluate
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PAB in drinking water. The main goals of this study were to determine the presence of PAB
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in treated water from Dutch drinking water treatment plants by cultivation-independent
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methods, (i.e., use total cell count (TCC) with flow cytometry to quantify attached bacteria
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and adenosine triphosphate (ATP) to quantify activity), and use high-throughput
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pyrosequencing to identify the PAB. This study was undertaken to understand what PAB
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levels in drinking water are, what the fraction of PAB in the total bacteria levels is; how many
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bacteria are associated with a single particle; and what the PAB community is, and if the PAB
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community has a relation to the characteristics of the particles from different water treatment
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plants.
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2. Materials and Methods
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2.1 Description of water treatment plants
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Three drinking water treatment plants with different particle compositions in their treated
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water were selected: a treatment plant using artificial recharge and recovery (ARR) with river
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water as source water (TP1), and two groundwater treatment plants (TP2, TP3). TP1 takes
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source water from the Meuse River. The source water, after pre-treatment, is transported over
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30 km to a dune area of natural lakes, where it recharges the groundwater. After an average
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residence time of 2 months, the water is abstracted from the dunes. Abstracted ARR water is
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post-treated by softening, powdered activated carbon, aeration, rapid sand filtration, and slow
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sand filtration before being pumped into the distribution system.
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At TP2 anoxic groundwater is treated by aeration and rapid sand filtration, and afterwards fed
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to the distribution system. At TP3, after abstraction, the groundwater is treated by aeration,
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filtration, softening, carry-over filtration, activated carbon filtration and UV disinfection. The
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treated groundwater contains somewhat higher levels of iron, manganese and ammonia
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concentrations than at TP1. The concentrations of these elements are also different between
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TP2 and TP3 due to the different treatments applied at the two treatment plants. The quality of
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treated water is summarized in Table S1 in the supplementary data.
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2.2 Sampling
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The sampling spots are located at the treatment plants just before the water enters the
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distribution system. PAB were collected with a specially designed multiple-particle filtration
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system (MuPFiS, Figure 1). Each line of MuPFiS consists of 47mm Swinnex filter holder
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followed by a flow meter. Multiple samples can be collected at the same time, and with the
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recorded water volume, the concentration of quantified PAB can be calculated. Particles were
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pre-concentrated by filtering approximately 200 liters of water through 1.2µm pore-size glass
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fiber filters (Whatman, 1822-047). Different pore size filters (1-10µm) have been used to
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collect PAB in water systems (Power and Nagy 1999; Riemann and Winding 2001; Zhang,
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Liu et al. 2007; Parveen, Reveilliez et al. 2011). In drinking water environment, previous
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researches done by scanning electron microscope (Ridgway and Olson 1982) and differential
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size filtration experiments (Azam and Hodson 1977) have demonstrated that single bacteria
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are usually less than 1.0µm in diameter. Although bigger particles or bacteria may exist in
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source water, the multiple treatment processes applied can remove them efficiently (Brazos
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and O’Connor 1996). Brazos and O’Connor (1996) did not collect PAB successfully from
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drinking water by using 3µm filters. In this study, a pore size of 1.2µm was selected. On one
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hand, it is bigger than reported diameter of single bacteria and will not lead to losing too
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much small bio-aggregates; on the other hand, 1.2µm filters are commonly used for
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suspended solids sampling which makes it possible to interpret and combine the biological
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analysis with physiochemical analysis.
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Three samples were taken by running the MuPFiS on the same day of the week in three
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different weeks for PAB quantification. On each sampling day, water samples were taken
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before filtration at the MuPFiS-connected points. For pyrosequencing analysis, triplicate
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samples were taken by one run of MuPFiS (finished within one day for all locations). A
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particle counter (Met one, 32 channels, 1-100µm) was run parallel to MuPFiS. Every filtration
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run was standardized to 3 hours. A particle counter was run at each sampling point for weeks
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to monitor the particle load in the treated water.
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2.3 Physiochemical characteristics of collected particles 6
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The physiochemical characteristics of collected particles were studied by scanning electron
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microscopy (SEM) coupled with energy dispersive spectroscopy (EDS). SEM-EDS was used
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to obtain high resolution images and the elemental composition. The JEOL JSM-840A
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scanning electron microscope is configured with secondary and backscattered electron
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detectors as well as an energy dispersive X-ray spectrometer. The working distance was 7-39
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mm for high–resolution imaging and 39 mm for EDS analysis and element mapping
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(Echeverría et al., 2009).
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2.4 PAB quantification
The filter with pre-concentrated PAB was submerged upside down in 5 ml autoclaved tap
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water with glass beads immediately after filtration. Samples were kept in a cool box and
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transported to the laboratory within two hours. Bacteria were detached from the particles by
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low energy ultrasonic treatment for 3 mins (Branson ultrasonic water bath, 43 kHz) as
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described by (Magic-Knezev and van der Kooij, 2004). Obtained suspensions were used for
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further analyses. Cultivation-independent methods, Adenosine triphosphate (ATP) and total
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cell counts (TCC) by flow cytometry were applied to quantify collected PAB in the
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suspension. ATP was measured as previously described (Magic-Knezev and van der Kooij,
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2004); TCC was measured by C6 flow cytometer (BD Accuri C6, United States); damaged
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cells and intact cells were distinguished, as described by Hammes et al. (2008). Both ATP and
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TCC analyses were done at Het Water Laboratorium in Haarlem, the Netherlands.
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The ATP and TCC values obtained from PAB are defined as associated ATP (A-ATP) and
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associated TCC (A-TCC). Based on ATP and TCC results, ATP per cell was calculated for
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water samples and PAB samples according to the equation used by Berney et al.(2008), that is,
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dividing the cell ATP by the intact cell number. In this study, ATP was measured as total ATP.
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As for PAB, no free ATP was determined because the PAB were collected by filtration. For
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PB, it has been demonstrated that the unchlorinated drinking water samples in the Netherlands
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do not contain significant amounts of free ATP (Van der Kooij, 1992; Van der Wielen and
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Van der Kooij, 2010).
ATP per cell (10 −16 g cell −1 ) =
ATP concentration ( ng l −1 ) intact cell concentration (cells l −1 )
(1)
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To quantify bacteria attached to particles, the average number of cells per particle was
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calculated from A-TCC and particle count measurements as follows:
Cells per particle ( cells particle −1 ) =
A − TCC ( cells ml −1 ) particle count ( particles ml −1 )
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(2)
Considering PAB as a form of biofilm on a sphere, A-ATP and particle counts were used to
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calculate the ATP of PAB (pg per cm2) using Equation (3):
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ATP ( pg cm−2 ) =
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Where A-ATP represents measured PAB ATP results; N the number of particles, and S the
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surface area per particle. An average diameter of 1.5µm was used based on the particle size
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distribution in tested water, where most particles had a diameter between 1.2µm and 2µm
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(results not shown).
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2.4 454 pyrosequencing
Suspended PAB samples were further processed to study their bacterial diversity. DNA was
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extracted from the suspension using a chemical and enzymatic DNA extraction protocol as
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described by Hong et al. (2010) and was amplified with bacterium-specific forward primer
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27F and reverse primer 534R (Hong et al., 2010). DNA extraction was done at KWR Water
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Cycle Research Institute. The 454 pyrosequencing was carried out with a 454 Life Sciences
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GS FLX series genome sequencer (Roche, Switzerland). The sequences were trimmed
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(resulting in an average sequence length of 230 bp). Merged alignments of the sequences
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aligned via the infernal aligner from the Ribosomal Database Project (RDP) pyrosequencing
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pipeline (http://pyro.cme.msu.edu/) and the NAST alignment tool from Greengenes were
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obtained via software developed by the biotechnology center at the University of Illinois (UI)
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(http://acai.igb.uiuc.edu/bio/merge-nast-infernal.html). The RDP Classifier was used for
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taxonomical assignments of the aligned 454 pyrosequences at the 95% confidence level. Both
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PCR amplification and pyrosequencing were performed at the UI biotechnology center. The
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total PAB communities from the three treatment plants were analyzed for the number of
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operational taxonomic units (OTUs), and species richness by using the DOTUR program
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(Hong et al., 2010).
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3. Results and Discussion
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3.1 Physiochemical characterization of PAB
Although it was not quantifiable, SEM pictures confirmed the finding of PAB and multiple
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cells attached on a single particle (Figures 2A, 2B and 2C). Different particle sizes and
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morphologies were observed at the three treatment plants. EDS elemental analysis showed
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that particles mainly consisted of carbon (C), oxygen (O), silicon (Si), sodium (Na), calcium
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(Ca), iron (Fe), and manganese (Mn) (Figure 2D). The results complied with reported findings
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on particles in drinking water distribution systems (Gauthier et al., 2001; Matsui et al., 2007;
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Verberk et al., 2006; Vreeburg et al., 2008).
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Compared to TP2 and TP3, TP1 particles were smaller and contained mainly C, O and Si.
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This may be due to the fact that TP1 used ARR surface water as source water and larger
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particles were removed by subsequent filtration steps applied at the plant. At TP2, high
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percentages of Ca, Fe and Mn were found. The results were as expected, since the
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groundwater is treated with conventional treatments of aeration and rapid sand filtration. The
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Ca, Fe, and Mn concentrations in the treated water were also higher than that of TP1 and TP3
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(Table S1, supplementary data). At TP3, although the groundwater source is the same as at
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TP2, different particles were collected. Ca, Fe and Mn were not found, instead the highest
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concentration of carbon was found. The difference between TP2 and TP3 can be related to the
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more advanced treatments applied in TP3, such as the softening, multiple filtration steps and
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additional activated carbon filtration (ACF). The highest carbon concentration may be due to
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the last treatment step (ACF) which may release carbon fines from the activated carbon media
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into the treated water. 3.2 Quantification of PAB
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3.2.1 A-TCC and A-ATP
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ATP and TCC were analyzed for both water and PAB samples (Figure 3 and Figure 4). The
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TCC of the produced water from the three pumping stations ranged from 0.45 × 105 cells ml-1
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to 1.65 × 105 cells ml-1, while ATP ranged from 1 ng l-1 to 6 ng l-1. Both TCC and ATP results
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are typical values for public drinking water without disinfectant residuals (Hammes et al.,
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2008; Van der Wielen and Van der Kooij, 2010). For PAB, A-TCC results ranged from 1.0 ×
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103 cells ml-1 to 3.5 × 103 cells ml-1, A-ATP ranged from 0.04 ng l-1 to 0.154 ng l-1. A-TCC
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and A-ATP accounted for less than 2% of that detected in the bulk water phase. One potential
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risk of PAB over PB, as mentioned in the introduction, is that it can be protected from
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disinfection. Therefore, although it forms less than 2% of PB, it may serve as seed feed to
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drinking water distribution system that can form biofilm on pipe wall and grow during
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distribution in bulk water and sediments. In the distribution system where disinfectant
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residuals applied, growth of PB can be controlled by the residuals, whereas, persistence,
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growth and accumulation of PAB will not be limited.
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On the other hand, the amount of PAB highly depends on the particle load (Liu et al., 2013).
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In the present study, the selected treatment plants produced high quality and low particle load
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drinking water (Table S1). The monitoring of particle counts in drinking water distribution
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system of TP1 found that the particle count increased from 20 # ml-1 at treatment plant to
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1,500-2,000 # ml-1 at customers’ taps. The monitoring of PB showed stable results, as the
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water is produced with high biological stability (AOC=5.8 µg cl-1, Table S1). Particles in
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distribution network may come from treatment plant such as filter material of sand and carbon,
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or generated during drinking water distribution such as corrosion. The physiochemical
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properties of different particles will lead to different communities, as corroborated by the
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present study (will be further discussed in the following section). Furthermore, PAB may also
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be accumulated in distribution systems as loose deposits and be released to bulk water during
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hydraulic peaks (Gauthier et al., 1999; Vreeburg et al., 2008; Liu et al., 2013), while, PB is
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rapid washed out of distribution system (Boe-Hansen et al., 2002).
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The lowest A-ATP and A-TCC were found at TP1, which is reasonable since, as mentioned
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above, TP1 is using ARR and has extended post-treatment, including slow sand filtration. The
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highest A-ATP was found at TP2, where only a conventional groundwater treatment is used.
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Results also demonstrated that, for water samples, intact cells account for 95%, 92% and 85%
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for TP1, TP2 and TP3, respectively. The percentage decreased to 75%, 85% and 72% for
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PAB samples. The lower intact cell ratio of PAB can be explained by the attachment and
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accumulation of damaged cells to extracellular polymeric substances (EPS) that surround
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living cells (Liu et al., 2004).
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Though A-ATP and A-TCC results were relatively low compared to the bulk water, sufficient
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amounts of PAB were sampled successfully for further analysis. In a previous study, using
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heterotrophic plate counts (HPC), a value of 0.07 to 0.15 CFU ml-1 cultivable bacteria were
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detected, and the value seemed to depend on the particle size (Lin et al., 2010). However,
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direct comparison of results obtained between two methods is difficult because the number of
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cultivable bacteria represents only a small percentage of the total number of bacteria
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(Hammes et al., 2008; Staley and Konopka, 1985).
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The application of direct microscopy cell (DC) counting found few PAB in the treated water
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(Brazos and O'Connor, 1996). In their research, PAB was quantified by comparing DCs in
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water before and after filtering through 3µm filters. The failure of quantifying PAB may be
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related to quantifying the difference in bacterial numbers before and after filtration instead of
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direct analysis of PAB retained on the filter. As mentioned, PAB only accounted for less than
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2% of biomass in the water sample and the accuracy of most bacteria quantification methods
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make it difficult to detect such small differences.
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Although ATP has been widely used in drinking water research to quantify bacterial activity
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in bulk water and biofilm, it has not been used previously to quantify PAB in water systems.
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The ATP per surface area of particles was calculated using Equation (3). In the present study,
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9300 to 49,700 pg cm-2 ATP were derived for the PAB samples. The ATP values of pipe wall
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biofilm were reported to be from 100 to 4000 pg cm-2 (Lehtola et al., 2004; Lehtola et al.,
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2006; Yu et al., 2010). It is difficult to compare these results since they were obtained from
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different systems. It should be noted that unlike pipe wall biofilms, which are colonized on
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the pipe wall surface, PAB are suspended in the bulk water during drinking water distribution
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that can reach customers’ taps and consumed by customers. The higher ATP per surface area
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and better mobility of PAB suggest that PAB, depending on the microbial community, may
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have a higher potential health risk to customers than pipe wall biofilm. Therefore, PAB
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require more research attention than they have had thus far.
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3.2.2 Multiple cells per particle
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Cells per particle were calculated using A-TCC (Figure 3) and particle counting results (Table
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1) by Equation (2). On average, 25-50 cells per particle were found (Table 1). The values are
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higher than the previously reported number counted by microscopy counting, which is 1.7-17
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cells per particle (Brazos and O'Connor, 1996; Ridgway and Olson, 1981). It has been
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suggested that particles with five or more attached cells should be considered important
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(Brazos and O'Connor, 1996).
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It should be noted that, although TP3 had a somewhat lower number of cells per particle, the
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total amount of PAB in TP3 was higher due to a higher particle load. TP1 was just the
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opposite of TP3. TP2, on the other hand, was characterized by high particles and high cell
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counts per particle. It was reported that more particles could offer more surface area for
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bacterial cells to attach and form biofilms (Gregory, 2005), and particles with biofilms could
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promote particle aggregation (Paris et al., 2009). Thus, it is likely that high particle load in
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combination with high cell numbers per particle could result in a higher level of deposition
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and accumulation of particulate matter in the drinking water distribution system. Particle
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generating processes during water distribution such as corrosion, flocculation, aggregation
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and biofilm detachment may increase the number of PAB at the tap.
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The water quality regulations commonly place quantitative limits on the number of cultivable
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organisms (e.g., coliforms) and particle densities (e.g., turbidity). However, these regulations
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do not take into account whether bacterial cells are present in the water as PB or PAB
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(Dietrich et al., 2007). No matter how many bacteria are associated with a particle, the cells
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will likely result in only a single colony if measured by routine HPC method (Camper et al.,
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1986) and will be counted as single cell when subjected to flow cytometry without further
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processing. Microscopic methods may be able to determine PAB, but are cumbersome and
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subjective. As a result, the presence of PAB in treated water will result in the underestimation
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of both specific and total bacterial cell counts in most methods, especially for the high particle
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load drinking water systems. This will give direct influence to bacteria injected to consumers.
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Using total coliforms as an example, it has been reported that adding coliforms in drinking
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water containing particles could not be correctly counted in the water sample, due to the
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association of the added coliforms with suspended particles (Herson et al., 1991). The further
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attachment of cells to particles during water distribution will lead to increase of particle size,
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which will change the surface and settling properties, disinfectant resistance and micro-
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environments (oxygen diffusion) inside the particle.
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3.2.3 ATP content in planktonic bacteria and attached bacteria
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The average ATP per cell was calculated based on obtained total ATP and intact cell count
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results for both water and PAB samples according to Formula 1. It was found that the ATP
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per cell ranged from 0.21 × 10-16 g cell-1 to 0.33 × 10-16 g cell-1 for PB and from 0.38 × 10-16 g
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cell-1 to 0.54 × 10-16 g cell-1 for PAB (Table 1). The average ATP per cell values of PAB is
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2.5 times higher than that of PB, suggesting that PAB could have a higher metabolic activity
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(Magic-Knezev and van der Kooij, 2004). This may be due to the fact that nutrients
321
originating from treatment plant as particles can be used firstly and directly by PAB. The
322
results agreed with findings obtained in other water environments (DeBruyn and Sayler, 2009;
323
Lemarchand et al., 2006) (Table 2). The results obtained in the present study are similar to
324
that from drinking water biofilters in the Netherlands (Magic-Knezev and van der Kooij, 2004)
325
and tap water (Berney et al., 2008), but lower than that from different aquatic samples
326
(Hammes et al., 2010). This may be associated with the low nutrients concentration in treated
327
drinking water.
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3.3.1 PAB diversity
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A total of 2,988, 8,921 and 2,818 bacterial 16S rRNA gene sequences were obtained from
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TP1, TP2 and TP3, respectively. The sequences (2,818-8,921 sequences) were significantly
332
larger than that of conventional cloning and sequencing methods (generally around 200
333
sequences, Kwon et al., 2011). The increased sequences made it possible to detect more
334
microorganisms (i.e., 207-495 operational taxonomic units (OTUs) at a 3% cutoff). These
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values are higher than those reported studies on samples from freshwater based on clone
336
libraries (less than 100 OTUs, Eichler et al., 2006). Compared to available pyrosequencing
337
studies, the number of OTUs observed in the present study were higher than those from
338
biofilm in water meters sampled from drinking water distribution systems (133 and 208 OTUs)
339
(Hong et al., 2010). The number of OTUs was lower than from membrane filtration systems
340
for drinking water production (1133-1731 OTUs) (Kwon et al., 2011). The Chao1 index
341
estimated 1470, 653, and 448 OTUs at a 3% cutoff for the samples from TP1, TP2, and TP3,
342
respectively. The highest bacterial diversity for PAB was found at TP1. Other nonparametric
343
diversity indices such as the Shannon index and Evenness gave similar results (Table 3).
344
3.3.2 PAB community composition
345
Figure 5 indicates the major phyla (>3% in total sequences) found in different treatment
346
plants. The results suggest that the three treatment plants have slightly different bacterial
347
community compositions. Proteobacteria were observed to dominate in all three locations,
348
ranging from 37% to 68%, and were represented by Alphaproteobacteria, Betaproteobacteria,
349
Deltaproteobacteria, and Gammaproteobacteria.
350
Proteobacteria) and Gammaproteobacteria (23% to 34%) dominated in all three plants. At
351
TP1, Deltaproteobacteria were found to account for 22% of Proteobacteria, whereas at TP2
352
and TP3 more Alphaproteobacteria (16 - 33%) were found.
353
Among the remaining phyla, OP3 candidate phylum (OP3) and Nitrospirae were also
354
commonly found at the three treatment plants. A high percentage of OP3 was found at TP1
355
(18.7%) and TP2 (13.6%). At TP3, only Proteobacteria had an abundance > 10%. Members
356
within the Planctomycetes, Cyanobacteria, Euryarchaeota and Acidobacteria were found at
357
one or more treatment plants with a percentage > 3%. Members of the Actinobacteria,
358
Bacteroidetes, Crenarchaeota, Chloroflexi, Gemmatimonadetes, GN02, NC10 and SBR1093
Betaproteobacteria (25% to 36% of
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were also found, but had an abundance < 3%. It should be noted that significant fractions of
360
sequences were assigned as unclassified, ranging from 6.8% (TP3) to 22.2% (TP1).
361
Little is known about the diversity of the PAB community in drinking water distribution
362
systems. The typical drinking water bacteria that have been reported correspond only to PB
363
and
364
Gammaproteobacteria are repeatedly found in drinking water environment (Eichler et al.,
365
2006; Hong et al., 2010; Kalmbach et al., 1997; Magic-Knezev et al., 2009; Mathieu et al.,
366
2009). Compared to Alphaproteobacteria, Betaproteobacteria and Gammaproteobacteria,
367
species from Deltaproteobacteria, were not detected or reported. Results from this
368
investigation confirm that, similar to the bulk water and biofilm studies by (Kormas et al.,
369
2010; Tokajian et al., 2005), Proteobacteria are of central importance in the drinking water
370
environment.
371
This is also the case for PAB. The subclasses of Proteobacteria have been reported to have a
372
different resistance to disinfectants (Mathieu et al., 2009). Disinfectants can promote or
373
suppress the proliferation of certain subclasses of Proteobacteria; for instance, increased
374
chlorine in distributed water results in an increased percentage of Gammaproteobacteria and
375
a decrease in Alphaproteobacteria (Mathieu et al., 2009). Hence, the presence of all four
376
classes of Proteobacteria in the present study may reflect the fact that no chemical
377
disinfectant is applied in the Netherlands.
378
It was noted that, compared to previous water and pipe wall biofilm studies in drinking water
379
and PAB studies in other water systems, a high percentage of bacteria belonging to candidate
380
division OP3 has been detected. OP3 was originally defined based on a single 16S rRNA gene
381
sequence obtained from obsidian pool sediment in Yellowstone National Park (Hugenholtz et
382
al., 1998). Bacteria belonging to OP3 were found to thrive in anoxic environments, such as in
383
marine sediment, fresh water lakes and aquifers (Glöckner et al., 2010; Kolinko et al., 2011).
wall
biofilm
bacteria.
Alphaproteobacteria,
Betaproteobacteria
and
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Regarding the habits and characteristics of OP3 bacteria, Glöckner’s group noted that OP3
385
bacteria were frequently detected in anoxic environments that are defined by redox cycling of
386
iron, manganese and other metals, and/or sulphur as major drivers of microbial activity.
387
Groundwater originates from anoxic aquifers with high concentrations of iron and manganese.
388
This high concentration may be associated with the high prevalence of OP3, compared to
389
what is found in marine and fresh water systems.
390
This same anoxic condition is present in the ARR dune area. The contact time of more than
391
two months with dune soils may allow soil bacteria to be introduced into the water phase.
392
Considering the aerobic environment of drinking water distribution systems, it is reasonable
393
to expect less/no presence of OP3 in the community study of distribution system water and
394
the biofilm. In the present study, the percentage of OP3 becomes significant (Figure 5) by
395
sampling particulate matter from the water phase indicating that the OP3 found in our treated
396
water originated from source water and passed through the treatment systems. Another
397
possibility is that in the aerobic drinking water environment, anoxic micro-environments exist
398
in or around the PAB structure. This hypothesis was supported by the detection of specific
399
anaerobic microorganisms, such as bacteria belonging to Rhodospirillales and Chromatiales,
400
and archaea belonging to Methanosarcinales. However, the particle size examined in the
401
present study is far too small to maintain a multiple micro-environment structure.
402
Evaluation at the genus level showed that 66 genera (genera accounting for more than 1%)
403
were found, and the identified genera are listed in Table 4. There were 53, 57, and 57 genera
404
found in TP1, TP2 and TP3, respectively. In this study, most of the genera were found in all
405
the treated waters. Unidentified genera belonging to OP3 GIF10 and Comamonadeceae were
406
found at all three treatment plants in a percentage higher than 3%. At TP2, Legionella,
407
Nitrospira, Gallionella, Nitrosomonas, Crenothrix and Thermodesulfavibrionaceae LCP-6
408
were also found in (relatively) high percentages (> 3%). Rhodospirillaceae, Leptolyngbya, a
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genus belonging to unclassified Comamonadeceae and unclassified OP3 GIF10 were
410
observed at TP3.
411
As shown in the Figure 2d, iron, manganese, ammonia, and sulfate were of significant
412
concentrations in the raw water of the three treatment plants, and in the treated water at TP2.
413
Therefore, not surprisingly, bacterial groups related to Fe and Mn (Gallionella and
414
Crenothrix), sulfate (unidentified OP3 GIF10, unidentified Syntrophobacteraceae) and
415
ammonia (Nitrospira and Nitrosomonas) cycles were found at high percentages. Within the
416
two treatment plants using groundwater as source water (TP2 and TP3), a higher percentage
417
of these bacteria was found at TP2 than at TP3. This might be explained by more intensive
418
treatment and the use of subsurface aeration for iron, manganese and ammonia removal at
419
TP3 (de Vet et al., 2009). For TP1, with a higher percentage of genera belonging to
420
unclassified phyla, an even higher diversity than listed in the results can be expected.
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The results obtained by cultivation-independent methods allow us to evaluate PAB in treated
423
water at water treatment plants and to conclude that:
424
• Regardless of the sources of water and treatment processes applied in the three treatment
425
plants, treated drinking water contains PABs. Levels of A-TCC were 1.0-3.5×103 cells and A-
426
ATP 0.04-0.154 ng l-1 ATP. This represented less than 2% of the TCC and ATP in the treated
427
water.
428
• ATP per cell of PAB is higher than that of PB in bulk water. On average, 25-50 cells were
429
found attached to a single particle. The presence of multiple cells per particle challenges the
430
use of quantitative methods such as HPC and coliforms that are present in the current drinking
431
water quality regulations.
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• Members of the Proteobacteria phylum dominated in all sampled PAB communities,
433
followed by OP3 and Nitrospirae, findings that are similar to previous drinking water and
434
drinking water biofilm studies. This study is the first report of OP3 being a main part of the
435
population in drinking water and PAB in water systems. Nitrospira was the main population
436
of treated groundwater.
437
• Genera of bacteria were found in the PAB communities that appear to be consistent with the
438
particle characteristics: bacterial groups related to Fe and Mn (e.g., Gallionella and
439
Crenothrix), sulfate (e.g., unidentified OP3 GIF10, unidentified Syntrophobacteraceae) and
440
ammonia (e.g., Nitrospira and Nitrosomonas), present in groundwater and water from ARR.
441
• Although this study demonstrated complex microbial communities of PAB in treated
442
drinking water, it has not classified PAB to the species level. It is noted that the genus
443
Legionella, order Thiotrichales, and family Burkholderiaceae, all of which contain pathogenic
444
or opportunistic pathogenic species, were found through this study. To evaluate the presence
445
of (opportunistic) pathogenic bacteria, more specific studies are necessary.
446
• Since the results were observed in three treatment plants with different source water and
447
treatment processes, the study suggests that similar results would be obtained at other
448
treatment plants. However, for the PAB in distribution systems, depending on the particle
449
load, particle characteristics, pipe material and hydraulic conditions, differences can be
450
expected.
451
The data and approaches presented in this study can be useful to elucidate the complexity and
452
dynamics of PAB and PB in drinking water, both for treatment plants and distribution systems.
453
However, the mechanism behind particle-bacteria interacting phenomena is still unclear.
454
Further research is needed to study the behavior and significance of PAB during water
455
distribution and the interaction between particle properties (size, number, elemental
456
composition) and PAB, water quality changes and PAB changes in drinking water distribution
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systems. This will, in turn, improve the understanding of the potential risks associated with
458
the PAB groups present in drinking water production and distribution networks.
459
Acknowledgements
460
The authors would like to acknowledge the support from the Chinese Scholarship Council
461
(2008612022). The authors thank Oasen, Dunea and Vitens water companies for their
462
cooperation in this study. Thanks are also due to Maarten Lut, Ed van der Mark, and Geo
463
Bakker for their assistance in the study. The authors thank Gertjan Medema for his critical
464
reading of the manuscript and Yu Tao for his valuable comments.
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Table 1 Quantifiable characteristics of PAB from three treatment plants
Parameters
TP1
TP2
TP3
Particle counts (# ml-1) (on line)
20(±3)
70(±5)
120(±9)
A-TCC/particle (average cells particle-1)
50 (±14)
49 (±4)
25 (±3)
0.21
0.29
0.33
(±0.05)
(±0.04)
Average ATP/intact cell (10-16 g cell-1) (n=3)
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(n=3)
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(±0.05) Average A-ATP/intact cell (10-16 g cell-1)
0.53
0.50
0.51
(n=3)
(±0.01)
(±0.01)
(±0.01)
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Table 2 ATP per cell from reported literature
631
literature
Groundwater
0.2-4.0
(Jensen, 1989)
Groundwater
2.2-5.2
(Eydal and Pedersen, 2007)
Drinking water biofilter
0.21-3.8
(Magic-Knezev and van der Kooij,
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ATP per cell (10-16 g cell-1)
0.65-2.28
(Velten et al., 2007)
Tap water
0.31-0.55
(Berney et al., 2008)
Average aquatic
0.89
(Hammes et al., 2010)
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samples
632
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2004)
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Table 3 PAB bacterial diversity in the three treatment plants (average ± std., n=3)
Sample
TP1
Number of
Observed
Chao 1
Shannon-Wiener
Evenness
sequences analysed
OTUs (97%)
(97%)
Index (H)
(E)
2988
495 ± 12
1470 ±
8.1 ± 0.10
0.89 ± 0.01
4.9 ± 0.31
0.64 ± 0.02
103 8921
207 ± 24
653 ± 148
2818
239 ± 7
448 ± 83
6.3 ± 0.19
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0.80 ± 0.02
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Table 4 The genera identified in PAB of different treatment plants
Percentage of sequences (%) TP2
TP3
Legionella
0.34
3.03
1.0
Nitrospira
0.11
3.10
0.42
Gallionella
0.34
Planctomyces
1.00
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0.29
2.10
0.48
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4.47
CandidatusOdyssella
0.04
1.06
0.46
Caulobacter
0.17
0.22
0.11
0.16
0.20
0.31
Aquabacterium
0.27
0.71
0.07
Comamonadeceae (unclassified)
3.70
3.02
10.85
12.09
10.28
3.38
Caldilinea
0
0.02
0.08
Nitrosomonas
0.19
5.17
0.22
Crenothrix
0.13
4.49
0.30
Thermodesulfovibrionaceae LCP-6
1.90
3.50
3.71
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Hyphomicrobium
Unclassified OP3 GIF10
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0.31
0
13.79
Rhodopirellula
0
0.07
0
Leptolyngbya
0
0
3.39
Unclassified Alphaproteobacteria
1.77
6.58
6.08
Unclassified phylum bacteria
22.25
12.79
6.84
Other
55.23
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48.22
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Rhodospirillaceae (un-identified)
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637
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Figure 1 Schematic drawing of multiple particle filtration system (MuPFiS) and parallel
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running particle counter used for PAB sampling
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Figure 2 SEM pictures (a: TP1, b: TP2 and c: TP3) and elemental composition of PAB (d)
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Figure 3 Average TCC and A-TCC results at each treatment plant (n=3)
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Figure 4 Average ATP and A-ATP results of at each treatment plant (n=3)
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Figure 5 Taxonomic assignment of 16s rRNA gene sequences retrieved from PAB samples
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classified by phylum. (a: TP1; b: TP2; c: TP3)
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• The number and activity of PAB ranged from 1.0-3.5×103 cells/ml and 0.04-0.154ng/l ATP. • There were 25-50 cells found to be attached on a single particle. • Anoxic and anaerobic bacteria were detected; OP3 was a main part of the PAB population.
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• Bacterial genera associated with particles are consistent with the particle characteristics. • PAB are important to bacteria enumeration and ecology of water distribution systems.
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Supplementary data Table S1 water quality information of selected treatment plants (N.A.: not available)
TP2
Surface water
Groundwater
Extracted ARR
Treated
Raw
N.A.
12.9
N.A.
Temperature
pH
N.A.
Turbidity (NTU)
N.A.
AOC
N.A.
l-1) ATP (ng l-1)
Groundwater
Raw
12
Treated
N.A.
12
8.5
N.A.
8.3
N.A.
8.2
<0.03
N.A.
0.22
N.A.
<0.1
5.8
N.A.
12.
N.A.
5.9
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(µg c
Treated
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TP3
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TP1
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Parameters
N.A.
1
N.A.
4.5
N.A.
4.5
N.A.
0.45
N.A.
1.65
N.A.
1.62
0.60
0.0052
0.55
0.0052
0.67
<0.03
Fe (mg l-1)
0.33
<0.01
0.95
0.012
0.92
<0.01
Mn (mg l-1)
0.09
<0.01
0.79
0.023
0.085
<0.01
SO4 (mg l-1)
N.A.
50.8
N.A.
34
N.A.
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AOC of TP1 was averaged of measurements in the year 2010 (n=4). AOC of TP2 and TP3 was measured in 2010. The result of parameters were averaged results of samples taken
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Figure S1. The release of ATP during LES treatment, each LES treatment last for 2 minutes and triplicate measurements were conducted.
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Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods
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G. Liu1 *, F. Q. Ling2, A. Magic-Knezev3, W. T. Liu2, J.Q.J.C.Verberk1, J.C. Van Dijk1 1. Section Sanitary Engineering, Department of Water Management, Faculty of Civil Engineering and Geosciences, Delft University of Technology, PO BOX 5048, 2600 GA Delft, the Netherlands E-mail: [email protected]
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2. Department of Civil and Environmental Engineering, University of Illinois Urbana-
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Champaign, 205 N. Mathews Ave., Urbana, Illinois 61801, U.S.A.
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3. Het Water Laboratorium, PO BOX 734, 2003 RS Haarlem, the Netherlands
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S0043-1354(13)00306-0
DOI:
10.1016/j.watres.2013.03.058
Reference:
WR 9880
To appear in:
Water Research
Received Date: 16 November 2012 Revised Date:
2 March 2013
Accepted Date: 31 March 2013
Please cite this article as: Liu, G., Ling, F.Q., Magic-Knezev, A., Liu, W.T., Verberk, J.Q.J.C., Van Dijk, J.C., Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods, Water Research (2013), doi: 10.1016/ j.watres.2013.03.058. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Quantification and identification of particle-associated bacteria in unchlorinated drinking
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water from three treatment plants by cultivation-independent methods
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G. Liu1 *, F. Q. Ling2, A. Magic-Knezev3, W. T. Liu2, J.Q.J.C.Verberk1, J.C. Van Dijk1
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1. Section Sanitary Engineering, Department of Water Management, Faculty of Civil
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Engineering and Geosciences, Delft University of Technology, PO BOX 5048, 2600 GA Delft,
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the Netherlands E-mail: [email protected]
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2. Department of Civil and Environmental Engineering, University of Illinois Urbana-
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Champaign, 205 N. Mathews Ave., Urbana, Illinois 61801, U.S.A.
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3. Het Water Laboratorium, PO BOX 734, 2003 RS Haarlem, the Netherlands
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Corresponding author:
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Gang Liu
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Email: [email protected]
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Tel: 0031 15 2785457\ 0031 6 41866671
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Abstract
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Water quality regulations commonly place quantitative limits on the number of organisms
21
(e.g., heterotrophic plate count and coliforms) without considering the presence of multiple
22
cells per particle, which is only counted as one regardless how many cells attached. Therefore,
23
it is important to quantify particle-associated bacteria (PAB), especially cells per particle. In
24
addition, PAB may house (opportunistic) pathogens and have higher resistance to disinfection
25
than planktonic bacteria. It is essential to know bacterial distribution on particles. However,
26
limited information is available on quantification and identification of PAB in drinking water.
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In the present study, PAB were sampled from the unchlorinated drinking water at three
28
treatment plants in the Netherlands, each with different particle compositions. Adenosine
29
triphosphate (ATP) and total cell counts (TCC) with flow cytometry were used to quantify the
30
PAB, and high-throughput pyrosequencing was used to identify them. The number and
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activity of PAB ranged from 1.0-3.5×103 cells ml-1 and 0.04-0.154 ng l-1 ATP. There were
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between 25 and 50 cells found to be attached on a single particle. ATP per cell in PAB was
33
higher than in planktonic bacteria. Among the identified sequences, Proteobacteria were
34
found to be the most dominant phylum at all locations, followed by OP3 candidate division
35
and Nitrospirae. Sequences related to anoxic bacteria from the OP3 candidate division and
36
other anaerobic bacteria were detected. Genera of bacteria were found appear to be consistent
37
with the major element composition of the associated particles. The presence of multiple cells
38
per particle challenges the use of quantitative methods such as HPC and Coliforms that are
39
used in the current drinking water quality regulations. The detection of anoxic and anaerobic
40
bacteria suggests the ecological importance of PAB in drinking water distribution systems.
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Keywords: particle associated bacteria (PAB), drinking water, adenosine triphosphate (ATP),
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flow cytometry, pyrosequencing
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1. Introduction When distributing drinking water, the regrowth of bacteria and other organisms may occur
45
and lead to water quality deterioration (Ridgway and Olson, 1982; Van Der Kooij, 2000).
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Depending on the source water and water treatment, more or less planktonic bacteria (PB), as
47
well as particle-associated bacteria (PAB) and biodegradable compounds, are present in the
48
treated water. They enter the drinking water distribution system (DWDS) and may serve as
49
“seeds” for regrowth. The generation of PAB during drinking water treatment is caused by the
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action of particles as the site for attachment and growth of bacteria (Gregory, 2005;
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Winkelmann and Harder, 2009). It has been reported that PAB represent a small number
52
compared to the PB population in treated water (Brazos and O'Connor, 1996). Nevertheless,
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the PAB that may pass through or be generated during treatment have been considered an
54
important source of bacteria entering the drinking water distribution systems both for bacterial
55
regrowth (Camper et al., 1986) and bacteria in accumulated loose deposits (Gauthier et al.,
56
1999; Vreeburg et al., 2008; Liu et al., 2013). PAB have been detected in 41.4% of the
57
samples of granular activated carbon filtered water at water treatment plants (Camper et al.,
58
1986), and in 17% of samples collected from fire hydrants in drinking water distribution
59
systems and water well outlets (Ridgway and Olson, 1981).
60
Since the attachment and growth of bacteria can lead to biofilm formation on particles
61
(Winkelmann and Harder, 2009), a major concern regarding PAB is their resistance to
62
disinfection (Brazos and O'Connor, 1996; Dietrich et al., 2009; Hess-Erga et al., 2008;
63
Hoadley and Gould, 1977; Lin et al., 2010; Wojcicka et al., 2008). PAB have been proven to
64
be more resistant to disinfection by chlorine (Ridgway and Olson, 1982), ozone (Hess-Erga et
65
al., 2008) and ultraviolet (UV) (Mamane and Linden, 2006; Wu et al., 2005) than PB are. As a
66
result, the regrowth or survival of pathogens in drinking water distribution systems may be
67
enhanced (Herson et al., 1987). Considering the disinfection resistance of PB and PAB, the
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nutrient limitation approach (Van der Kooij, 1992) to produce biologically stable drinking
69
water is likely to control the regrowth of both PB, PAB and bacteria in biofilms attached to
70
pipe walls.
71
Another concern regarding PAB is the potential underestimation of bacterial numbers because
72
no matter how many bacteria have been attached to one particle, they will be counted as one
73
by traditional culture methods (Camper et al., 1986). Water quality regulations commonly
74
place quantitative limits on the number of organisms (e.g., heterotrophic plate count and
75
coliforms) and particle densities (e.g., turbidity), resulting in a substantial underestimation of
76
the PAB bacteria present (Dietrich et al., 2007). In addition, PAB may house (opportunistic)
77
pathogens and the dose of microbes may differ significantly if PAB rather than PB are
78
ingested, thereby increasing the potential risk to customers. For instance, Herson et al. (1991)
79
found that a large number of coliforms added to particle-containing drinking water could not
80
be reflected by plate counting because they accumulated as PAB.
81
All the above-mentioned studies have improved knowledge of the importance of PAB in
82
drinking water. However, limited studies on PAB in drinking water have been conducted,
83
most of which applied cultivation-dependent methods (Camper et al., 1985; Ridgway and
84
Olson, 1982; Wu et al., 2005) or microscopic observations (Brazos and O'Connor, 1996).
85
Considerable bias and underestimation may be introduced by applying these methods.
86
Consequently, PAB in drinking water have been poorly documented. Cultivation-independent
87
techniques for bacterial quantification and identification offer new posibilities to reevaluate
88
PAB in drinking water. The main goals of this study were to determine the presence of PAB
89
in treated water from Dutch drinking water treatment plants by cultivation-independent
90
methods, (i.e., use total cell count (TCC) with flow cytometry to quantify attached bacteria
91
and adenosine triphosphate (ATP) to quantify activity), and use high-throughput
92
pyrosequencing to identify the PAB. This study was undertaken to understand what PAB
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levels in drinking water are, what the fraction of PAB in the total bacteria levels is; how many
94
bacteria are associated with a single particle; and what the PAB community is, and if the PAB
95
community has a relation to the characteristics of the particles from different water treatment
96
plants.
97
2. Materials and Methods
98
2.1 Description of water treatment plants
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Three drinking water treatment plants with different particle compositions in their treated
100
water were selected: a treatment plant using artificial recharge and recovery (ARR) with river
101
water as source water (TP1), and two groundwater treatment plants (TP2, TP3). TP1 takes
102
source water from the Meuse River. The source water, after pre-treatment, is transported over
103
30 km to a dune area of natural lakes, where it recharges the groundwater. After an average
104
residence time of 2 months, the water is abstracted from the dunes. Abstracted ARR water is
105
post-treated by softening, powdered activated carbon, aeration, rapid sand filtration, and slow
106
sand filtration before being pumped into the distribution system.
107
At TP2 anoxic groundwater is treated by aeration and rapid sand filtration, and afterwards fed
108
to the distribution system. At TP3, after abstraction, the groundwater is treated by aeration,
109
filtration, softening, carry-over filtration, activated carbon filtration and UV disinfection. The
110
treated groundwater contains somewhat higher levels of iron, manganese and ammonia
111
concentrations than at TP1. The concentrations of these elements are also different between
112
TP2 and TP3 due to the different treatments applied at the two treatment plants. The quality of
113
treated water is summarized in Table S1 in the supplementary data.
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2.2 Sampling
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The sampling spots are located at the treatment plants just before the water enters the
116
distribution system. PAB were collected with a specially designed multiple-particle filtration
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system (MuPFiS, Figure 1). Each line of MuPFiS consists of 47mm Swinnex filter holder
118
followed by a flow meter. Multiple samples can be collected at the same time, and with the
119
recorded water volume, the concentration of quantified PAB can be calculated. Particles were
120
pre-concentrated by filtering approximately 200 liters of water through 1.2µm pore-size glass
121
fiber filters (Whatman, 1822-047). Different pore size filters (1-10µm) have been used to
122
collect PAB in water systems (Power and Nagy 1999; Riemann and Winding 2001; Zhang,
123
Liu et al. 2007; Parveen, Reveilliez et al. 2011). In drinking water environment, previous
124
researches done by scanning electron microscope (Ridgway and Olson 1982) and differential
125
size filtration experiments (Azam and Hodson 1977) have demonstrated that single bacteria
126
are usually less than 1.0µm in diameter. Although bigger particles or bacteria may exist in
127
source water, the multiple treatment processes applied can remove them efficiently (Brazos
128
and O’Connor 1996). Brazos and O’Connor (1996) did not collect PAB successfully from
129
drinking water by using 3µm filters. In this study, a pore size of 1.2µm was selected. On one
130
hand, it is bigger than reported diameter of single bacteria and will not lead to losing too
131
much small bio-aggregates; on the other hand, 1.2µm filters are commonly used for
132
suspended solids sampling which makes it possible to interpret and combine the biological
133
analysis with physiochemical analysis.
134
Three samples were taken by running the MuPFiS on the same day of the week in three
135
different weeks for PAB quantification. On each sampling day, water samples were taken
136
before filtration at the MuPFiS-connected points. For pyrosequencing analysis, triplicate
137
samples were taken by one run of MuPFiS (finished within one day for all locations). A
138
particle counter (Met one, 32 channels, 1-100µm) was run parallel to MuPFiS. Every filtration
139
run was standardized to 3 hours. A particle counter was run at each sampling point for weeks
140
to monitor the particle load in the treated water.
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2.3 Physiochemical characteristics of collected particles 6
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The physiochemical characteristics of collected particles were studied by scanning electron
143
microscopy (SEM) coupled with energy dispersive spectroscopy (EDS). SEM-EDS was used
144
to obtain high resolution images and the elemental composition. The JEOL JSM-840A
145
scanning electron microscope is configured with secondary and backscattered electron
146
detectors as well as an energy dispersive X-ray spectrometer. The working distance was 7-39
147
mm for high–resolution imaging and 39 mm for EDS analysis and element mapping
148
(Echeverría et al., 2009).
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2.4 PAB quantification
The filter with pre-concentrated PAB was submerged upside down in 5 ml autoclaved tap
151
water with glass beads immediately after filtration. Samples were kept in a cool box and
152
transported to the laboratory within two hours. Bacteria were detached from the particles by
153
low energy ultrasonic treatment for 3 mins (Branson ultrasonic water bath, 43 kHz) as
154
described by (Magic-Knezev and van der Kooij, 2004). Obtained suspensions were used for
155
further analyses. Cultivation-independent methods, Adenosine triphosphate (ATP) and total
156
cell counts (TCC) by flow cytometry were applied to quantify collected PAB in the
157
suspension. ATP was measured as previously described (Magic-Knezev and van der Kooij,
158
2004); TCC was measured by C6 flow cytometer (BD Accuri C6, United States); damaged
159
cells and intact cells were distinguished, as described by Hammes et al. (2008). Both ATP and
160
TCC analyses were done at Het Water Laboratorium in Haarlem, the Netherlands.
161
The ATP and TCC values obtained from PAB are defined as associated ATP (A-ATP) and
162
associated TCC (A-TCC). Based on ATP and TCC results, ATP per cell was calculated for
163
water samples and PAB samples according to the equation used by Berney et al.(2008), that is,
164
dividing the cell ATP by the intact cell number. In this study, ATP was measured as total ATP.
165
As for PAB, no free ATP was determined because the PAB were collected by filtration. For
166
PB, it has been demonstrated that the unchlorinated drinking water samples in the Netherlands
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do not contain significant amounts of free ATP (Van der Kooij, 1992; Van der Wielen and
168
Van der Kooij, 2010).
ATP per cell (10 −16 g cell −1 ) =
ATP concentration ( ng l −1 ) intact cell concentration (cells l −1 )
(1)
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To quantify bacteria attached to particles, the average number of cells per particle was
171
calculated from A-TCC and particle count measurements as follows:
Cells per particle ( cells particle −1 ) =
A − TCC ( cells ml −1 ) particle count ( particles ml −1 )
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(2)
Considering PAB as a form of biofilm on a sphere, A-ATP and particle counts were used to
174
calculate the ATP of PAB (pg per cm2) using Equation (3):
175
ATP ( pg cm−2 ) =
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A − ATP N ×S
(3)
Where A-ATP represents measured PAB ATP results; N the number of particles, and S the
177
surface area per particle. An average diameter of 1.5µm was used based on the particle size
178
distribution in tested water, where most particles had a diameter between 1.2µm and 2µm
179
(results not shown).
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2.4 454 pyrosequencing
Suspended PAB samples were further processed to study their bacterial diversity. DNA was
182
extracted from the suspension using a chemical and enzymatic DNA extraction protocol as
183
described by Hong et al. (2010) and was amplified with bacterium-specific forward primer
184
27F and reverse primer 534R (Hong et al., 2010). DNA extraction was done at KWR Water
185
Cycle Research Institute. The 454 pyrosequencing was carried out with a 454 Life Sciences
186
GS FLX series genome sequencer (Roche, Switzerland). The sequences were trimmed
187
(resulting in an average sequence length of 230 bp). Merged alignments of the sequences
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aligned via the infernal aligner from the Ribosomal Database Project (RDP) pyrosequencing
189
pipeline (http://pyro.cme.msu.edu/) and the NAST alignment tool from Greengenes were
190
obtained via software developed by the biotechnology center at the University of Illinois (UI)
191
(http://acai.igb.uiuc.edu/bio/merge-nast-infernal.html). The RDP Classifier was used for
192
taxonomical assignments of the aligned 454 pyrosequences at the 95% confidence level. Both
193
PCR amplification and pyrosequencing were performed at the UI biotechnology center. The
194
total PAB communities from the three treatment plants were analyzed for the number of
195
operational taxonomic units (OTUs), and species richness by using the DOTUR program
196
(Hong et al., 2010).
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3. Results and Discussion
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3.1 Physiochemical characterization of PAB
Although it was not quantifiable, SEM pictures confirmed the finding of PAB and multiple
200
cells attached on a single particle (Figures 2A, 2B and 2C). Different particle sizes and
201
morphologies were observed at the three treatment plants. EDS elemental analysis showed
202
that particles mainly consisted of carbon (C), oxygen (O), silicon (Si), sodium (Na), calcium
203
(Ca), iron (Fe), and manganese (Mn) (Figure 2D). The results complied with reported findings
204
on particles in drinking water distribution systems (Gauthier et al., 2001; Matsui et al., 2007;
205
Verberk et al., 2006; Vreeburg et al., 2008).
206
Compared to TP2 and TP3, TP1 particles were smaller and contained mainly C, O and Si.
207
This may be due to the fact that TP1 used ARR surface water as source water and larger
208
particles were removed by subsequent filtration steps applied at the plant. At TP2, high
209
percentages of Ca, Fe and Mn were found. The results were as expected, since the
210
groundwater is treated with conventional treatments of aeration and rapid sand filtration. The
211
Ca, Fe, and Mn concentrations in the treated water were also higher than that of TP1 and TP3
212
(Table S1, supplementary data). At TP3, although the groundwater source is the same as at
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TP2, different particles were collected. Ca, Fe and Mn were not found, instead the highest
214
concentration of carbon was found. The difference between TP2 and TP3 can be related to the
215
more advanced treatments applied in TP3, such as the softening, multiple filtration steps and
216
additional activated carbon filtration (ACF). The highest carbon concentration may be due to
217
the last treatment step (ACF) which may release carbon fines from the activated carbon media
218
into the treated water. 3.2 Quantification of PAB
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3.2.1 A-TCC and A-ATP
221
ATP and TCC were analyzed for both water and PAB samples (Figure 3 and Figure 4). The
222
TCC of the produced water from the three pumping stations ranged from 0.45 × 105 cells ml-1
223
to 1.65 × 105 cells ml-1, while ATP ranged from 1 ng l-1 to 6 ng l-1. Both TCC and ATP results
224
are typical values for public drinking water without disinfectant residuals (Hammes et al.,
225
2008; Van der Wielen and Van der Kooij, 2010). For PAB, A-TCC results ranged from 1.0 ×
226
103 cells ml-1 to 3.5 × 103 cells ml-1, A-ATP ranged from 0.04 ng l-1 to 0.154 ng l-1. A-TCC
227
and A-ATP accounted for less than 2% of that detected in the bulk water phase. One potential
228
risk of PAB over PB, as mentioned in the introduction, is that it can be protected from
229
disinfection. Therefore, although it forms less than 2% of PB, it may serve as seed feed to
230
drinking water distribution system that can form biofilm on pipe wall and grow during
231
distribution in bulk water and sediments. In the distribution system where disinfectant
232
residuals applied, growth of PB can be controlled by the residuals, whereas, persistence,
233
growth and accumulation of PAB will not be limited.
234
On the other hand, the amount of PAB highly depends on the particle load (Liu et al., 2013).
235
In the present study, the selected treatment plants produced high quality and low particle load
236
drinking water (Table S1). The monitoring of particle counts in drinking water distribution
237
system of TP1 found that the particle count increased from 20 # ml-1 at treatment plant to
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1,500-2,000 # ml-1 at customers’ taps. The monitoring of PB showed stable results, as the
239
water is produced with high biological stability (AOC=5.8 µg cl-1, Table S1). Particles in
240
distribution network may come from treatment plant such as filter material of sand and carbon,
241
or generated during drinking water distribution such as corrosion. The physiochemical
242
properties of different particles will lead to different communities, as corroborated by the
243
present study (will be further discussed in the following section). Furthermore, PAB may also
244
be accumulated in distribution systems as loose deposits and be released to bulk water during
245
hydraulic peaks (Gauthier et al., 1999; Vreeburg et al., 2008; Liu et al., 2013), while, PB is
246
rapid washed out of distribution system (Boe-Hansen et al., 2002).
247
The lowest A-ATP and A-TCC were found at TP1, which is reasonable since, as mentioned
248
above, TP1 is using ARR and has extended post-treatment, including slow sand filtration. The
249
highest A-ATP was found at TP2, where only a conventional groundwater treatment is used.
250
Results also demonstrated that, for water samples, intact cells account for 95%, 92% and 85%
251
for TP1, TP2 and TP3, respectively. The percentage decreased to 75%, 85% and 72% for
252
PAB samples. The lower intact cell ratio of PAB can be explained by the attachment and
253
accumulation of damaged cells to extracellular polymeric substances (EPS) that surround
254
living cells (Liu et al., 2004).
255
Though A-ATP and A-TCC results were relatively low compared to the bulk water, sufficient
256
amounts of PAB were sampled successfully for further analysis. In a previous study, using
257
heterotrophic plate counts (HPC), a value of 0.07 to 0.15 CFU ml-1 cultivable bacteria were
258
detected, and the value seemed to depend on the particle size (Lin et al., 2010). However,
259
direct comparison of results obtained between two methods is difficult because the number of
260
cultivable bacteria represents only a small percentage of the total number of bacteria
261
(Hammes et al., 2008; Staley and Konopka, 1985).
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The application of direct microscopy cell (DC) counting found few PAB in the treated water
263
(Brazos and O'Connor, 1996). In their research, PAB was quantified by comparing DCs in
264
water before and after filtering through 3µm filters. The failure of quantifying PAB may be
265
related to quantifying the difference in bacterial numbers before and after filtration instead of
266
direct analysis of PAB retained on the filter. As mentioned, PAB only accounted for less than
267
2% of biomass in the water sample and the accuracy of most bacteria quantification methods
268
make it difficult to detect such small differences.
269
Although ATP has been widely used in drinking water research to quantify bacterial activity
270
in bulk water and biofilm, it has not been used previously to quantify PAB in water systems.
271
The ATP per surface area of particles was calculated using Equation (3). In the present study,
272
9300 to 49,700 pg cm-2 ATP were derived for the PAB samples. The ATP values of pipe wall
273
biofilm were reported to be from 100 to 4000 pg cm-2 (Lehtola et al., 2004; Lehtola et al.,
274
2006; Yu et al., 2010). It is difficult to compare these results since they were obtained from
275
different systems. It should be noted that unlike pipe wall biofilms, which are colonized on
276
the pipe wall surface, PAB are suspended in the bulk water during drinking water distribution
277
that can reach customers’ taps and consumed by customers. The higher ATP per surface area
278
and better mobility of PAB suggest that PAB, depending on the microbial community, may
279
have a higher potential health risk to customers than pipe wall biofilm. Therefore, PAB
280
require more research attention than they have had thus far.
281
3.2.2 Multiple cells per particle
282
Cells per particle were calculated using A-TCC (Figure 3) and particle counting results (Table
283
1) by Equation (2). On average, 25-50 cells per particle were found (Table 1). The values are
284
higher than the previously reported number counted by microscopy counting, which is 1.7-17
285
cells per particle (Brazos and O'Connor, 1996; Ridgway and Olson, 1981). It has been
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suggested that particles with five or more attached cells should be considered important
287
(Brazos and O'Connor, 1996).
288
It should be noted that, although TP3 had a somewhat lower number of cells per particle, the
289
total amount of PAB in TP3 was higher due to a higher particle load. TP1 was just the
290
opposite of TP3. TP2, on the other hand, was characterized by high particles and high cell
291
counts per particle. It was reported that more particles could offer more surface area for
292
bacterial cells to attach and form biofilms (Gregory, 2005), and particles with biofilms could
293
promote particle aggregation (Paris et al., 2009). Thus, it is likely that high particle load in
294
combination with high cell numbers per particle could result in a higher level of deposition
295
and accumulation of particulate matter in the drinking water distribution system. Particle
296
generating processes during water distribution such as corrosion, flocculation, aggregation
297
and biofilm detachment may increase the number of PAB at the tap.
298
The water quality regulations commonly place quantitative limits on the number of cultivable
299
organisms (e.g., coliforms) and particle densities (e.g., turbidity). However, these regulations
300
do not take into account whether bacterial cells are present in the water as PB or PAB
301
(Dietrich et al., 2007). No matter how many bacteria are associated with a particle, the cells
302
will likely result in only a single colony if measured by routine HPC method (Camper et al.,
303
1986) and will be counted as single cell when subjected to flow cytometry without further
304
processing. Microscopic methods may be able to determine PAB, but are cumbersome and
305
subjective. As a result, the presence of PAB in treated water will result in the underestimation
306
of both specific and total bacterial cell counts in most methods, especially for the high particle
307
load drinking water systems. This will give direct influence to bacteria injected to consumers.
308
Using total coliforms as an example, it has been reported that adding coliforms in drinking
309
water containing particles could not be correctly counted in the water sample, due to the
310
association of the added coliforms with suspended particles (Herson et al., 1991). The further
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attachment of cells to particles during water distribution will lead to increase of particle size,
312
which will change the surface and settling properties, disinfectant resistance and micro-
313
environments (oxygen diffusion) inside the particle.
314
3.2.3 ATP content in planktonic bacteria and attached bacteria
315
The average ATP per cell was calculated based on obtained total ATP and intact cell count
316
results for both water and PAB samples according to Formula 1. It was found that the ATP
317
per cell ranged from 0.21 × 10-16 g cell-1 to 0.33 × 10-16 g cell-1 for PB and from 0.38 × 10-16 g
318
cell-1 to 0.54 × 10-16 g cell-1 for PAB (Table 1). The average ATP per cell values of PAB is
319
2.5 times higher than that of PB, suggesting that PAB could have a higher metabolic activity
320
(Magic-Knezev and van der Kooij, 2004). This may be due to the fact that nutrients
321
originating from treatment plant as particles can be used firstly and directly by PAB. The
322
results agreed with findings obtained in other water environments (DeBruyn and Sayler, 2009;
323
Lemarchand et al., 2006) (Table 2). The results obtained in the present study are similar to
324
that from drinking water biofilters in the Netherlands (Magic-Knezev and van der Kooij, 2004)
325
and tap water (Berney et al., 2008), but lower than that from different aquatic samples
326
(Hammes et al., 2010). This may be associated with the low nutrients concentration in treated
327
drinking water.
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3.3.1 PAB diversity
330
A total of 2,988, 8,921 and 2,818 bacterial 16S rRNA gene sequences were obtained from
331
TP1, TP2 and TP3, respectively. The sequences (2,818-8,921 sequences) were significantly
332
larger than that of conventional cloning and sequencing methods (generally around 200
333
sequences, Kwon et al., 2011). The increased sequences made it possible to detect more
334
microorganisms (i.e., 207-495 operational taxonomic units (OTUs) at a 3% cutoff). These
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values are higher than those reported studies on samples from freshwater based on clone
336
libraries (less than 100 OTUs, Eichler et al., 2006). Compared to available pyrosequencing
337
studies, the number of OTUs observed in the present study were higher than those from
338
biofilm in water meters sampled from drinking water distribution systems (133 and 208 OTUs)
339
(Hong et al., 2010). The number of OTUs was lower than from membrane filtration systems
340
for drinking water production (1133-1731 OTUs) (Kwon et al., 2011). The Chao1 index
341
estimated 1470, 653, and 448 OTUs at a 3% cutoff for the samples from TP1, TP2, and TP3,
342
respectively. The highest bacterial diversity for PAB was found at TP1. Other nonparametric
343
diversity indices such as the Shannon index and Evenness gave similar results (Table 3).
344
3.3.2 PAB community composition
345
Figure 5 indicates the major phyla (>3% in total sequences) found in different treatment
346
plants. The results suggest that the three treatment plants have slightly different bacterial
347
community compositions. Proteobacteria were observed to dominate in all three locations,
348
ranging from 37% to 68%, and were represented by Alphaproteobacteria, Betaproteobacteria,
349
Deltaproteobacteria, and Gammaproteobacteria.
350
Proteobacteria) and Gammaproteobacteria (23% to 34%) dominated in all three plants. At
351
TP1, Deltaproteobacteria were found to account for 22% of Proteobacteria, whereas at TP2
352
and TP3 more Alphaproteobacteria (16 - 33%) were found.
353
Among the remaining phyla, OP3 candidate phylum (OP3) and Nitrospirae were also
354
commonly found at the three treatment plants. A high percentage of OP3 was found at TP1
355
(18.7%) and TP2 (13.6%). At TP3, only Proteobacteria had an abundance > 10%. Members
356
within the Planctomycetes, Cyanobacteria, Euryarchaeota and Acidobacteria were found at
357
one or more treatment plants with a percentage > 3%. Members of the Actinobacteria,
358
Bacteroidetes, Crenarchaeota, Chloroflexi, Gemmatimonadetes, GN02, NC10 and SBR1093
Betaproteobacteria (25% to 36% of
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were also found, but had an abundance < 3%. It should be noted that significant fractions of
360
sequences were assigned as unclassified, ranging from 6.8% (TP3) to 22.2% (TP1).
361
Little is known about the diversity of the PAB community in drinking water distribution
362
systems. The typical drinking water bacteria that have been reported correspond only to PB
363
and
364
Gammaproteobacteria are repeatedly found in drinking water environment (Eichler et al.,
365
2006; Hong et al., 2010; Kalmbach et al., 1997; Magic-Knezev et al., 2009; Mathieu et al.,
366
2009). Compared to Alphaproteobacteria, Betaproteobacteria and Gammaproteobacteria,
367
species from Deltaproteobacteria, were not detected or reported. Results from this
368
investigation confirm that, similar to the bulk water and biofilm studies by (Kormas et al.,
369
2010; Tokajian et al., 2005), Proteobacteria are of central importance in the drinking water
370
environment.
371
This is also the case for PAB. The subclasses of Proteobacteria have been reported to have a
372
different resistance to disinfectants (Mathieu et al., 2009). Disinfectants can promote or
373
suppress the proliferation of certain subclasses of Proteobacteria; for instance, increased
374
chlorine in distributed water results in an increased percentage of Gammaproteobacteria and
375
a decrease in Alphaproteobacteria (Mathieu et al., 2009). Hence, the presence of all four
376
classes of Proteobacteria in the present study may reflect the fact that no chemical
377
disinfectant is applied in the Netherlands.
378
It was noted that, compared to previous water and pipe wall biofilm studies in drinking water
379
and PAB studies in other water systems, a high percentage of bacteria belonging to candidate
380
division OP3 has been detected. OP3 was originally defined based on a single 16S rRNA gene
381
sequence obtained from obsidian pool sediment in Yellowstone National Park (Hugenholtz et
382
al., 1998). Bacteria belonging to OP3 were found to thrive in anoxic environments, such as in
383
marine sediment, fresh water lakes and aquifers (Glöckner et al., 2010; Kolinko et al., 2011).
wall
biofilm
bacteria.
Alphaproteobacteria,
Betaproteobacteria
and
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Regarding the habits and characteristics of OP3 bacteria, Glöckner’s group noted that OP3
385
bacteria were frequently detected in anoxic environments that are defined by redox cycling of
386
iron, manganese and other metals, and/or sulphur as major drivers of microbial activity.
387
Groundwater originates from anoxic aquifers with high concentrations of iron and manganese.
388
This high concentration may be associated with the high prevalence of OP3, compared to
389
what is found in marine and fresh water systems.
390
This same anoxic condition is present in the ARR dune area. The contact time of more than
391
two months with dune soils may allow soil bacteria to be introduced into the water phase.
392
Considering the aerobic environment of drinking water distribution systems, it is reasonable
393
to expect less/no presence of OP3 in the community study of distribution system water and
394
the biofilm. In the present study, the percentage of OP3 becomes significant (Figure 5) by
395
sampling particulate matter from the water phase indicating that the OP3 found in our treated
396
water originated from source water and passed through the treatment systems. Another
397
possibility is that in the aerobic drinking water environment, anoxic micro-environments exist
398
in or around the PAB structure. This hypothesis was supported by the detection of specific
399
anaerobic microorganisms, such as bacteria belonging to Rhodospirillales and Chromatiales,
400
and archaea belonging to Methanosarcinales. However, the particle size examined in the
401
present study is far too small to maintain a multiple micro-environment structure.
402
Evaluation at the genus level showed that 66 genera (genera accounting for more than 1%)
403
were found, and the identified genera are listed in Table 4. There were 53, 57, and 57 genera
404
found in TP1, TP2 and TP3, respectively. In this study, most of the genera were found in all
405
the treated waters. Unidentified genera belonging to OP3 GIF10 and Comamonadeceae were
406
found at all three treatment plants in a percentage higher than 3%. At TP2, Legionella,
407
Nitrospira, Gallionella, Nitrosomonas, Crenothrix and Thermodesulfavibrionaceae LCP-6
408
were also found in (relatively) high percentages (> 3%). Rhodospirillaceae, Leptolyngbya, a
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genus belonging to unclassified Comamonadeceae and unclassified OP3 GIF10 were
410
observed at TP3.
411
As shown in the Figure 2d, iron, manganese, ammonia, and sulfate were of significant
412
concentrations in the raw water of the three treatment plants, and in the treated water at TP2.
413
Therefore, not surprisingly, bacterial groups related to Fe and Mn (Gallionella and
414
Crenothrix), sulfate (unidentified OP3 GIF10, unidentified Syntrophobacteraceae) and
415
ammonia (Nitrospira and Nitrosomonas) cycles were found at high percentages. Within the
416
two treatment plants using groundwater as source water (TP2 and TP3), a higher percentage
417
of these bacteria was found at TP2 than at TP3. This might be explained by more intensive
418
treatment and the use of subsurface aeration for iron, manganese and ammonia removal at
419
TP3 (de Vet et al., 2009). For TP1, with a higher percentage of genera belonging to
420
unclassified phyla, an even higher diversity than listed in the results can be expected.
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The results obtained by cultivation-independent methods allow us to evaluate PAB in treated
423
water at water treatment plants and to conclude that:
424
• Regardless of the sources of water and treatment processes applied in the three treatment
425
plants, treated drinking water contains PABs. Levels of A-TCC were 1.0-3.5×103 cells and A-
426
ATP 0.04-0.154 ng l-1 ATP. This represented less than 2% of the TCC and ATP in the treated
427
water.
428
• ATP per cell of PAB is higher than that of PB in bulk water. On average, 25-50 cells were
429
found attached to a single particle. The presence of multiple cells per particle challenges the
430
use of quantitative methods such as HPC and coliforms that are present in the current drinking
431
water quality regulations.
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• Members of the Proteobacteria phylum dominated in all sampled PAB communities,
433
followed by OP3 and Nitrospirae, findings that are similar to previous drinking water and
434
drinking water biofilm studies. This study is the first report of OP3 being a main part of the
435
population in drinking water and PAB in water systems. Nitrospira was the main population
436
of treated groundwater.
437
• Genera of bacteria were found in the PAB communities that appear to be consistent with the
438
particle characteristics: bacterial groups related to Fe and Mn (e.g., Gallionella and
439
Crenothrix), sulfate (e.g., unidentified OP3 GIF10, unidentified Syntrophobacteraceae) and
440
ammonia (e.g., Nitrospira and Nitrosomonas), present in groundwater and water from ARR.
441
• Although this study demonstrated complex microbial communities of PAB in treated
442
drinking water, it has not classified PAB to the species level. It is noted that the genus
443
Legionella, order Thiotrichales, and family Burkholderiaceae, all of which contain pathogenic
444
or opportunistic pathogenic species, were found through this study. To evaluate the presence
445
of (opportunistic) pathogenic bacteria, more specific studies are necessary.
446
• Since the results were observed in three treatment plants with different source water and
447
treatment processes, the study suggests that similar results would be obtained at other
448
treatment plants. However, for the PAB in distribution systems, depending on the particle
449
load, particle characteristics, pipe material and hydraulic conditions, differences can be
450
expected.
451
The data and approaches presented in this study can be useful to elucidate the complexity and
452
dynamics of PAB and PB in drinking water, both for treatment plants and distribution systems.
453
However, the mechanism behind particle-bacteria interacting phenomena is still unclear.
454
Further research is needed to study the behavior and significance of PAB during water
455
distribution and the interaction between particle properties (size, number, elemental
456
composition) and PAB, water quality changes and PAB changes in drinking water distribution
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systems. This will, in turn, improve the understanding of the potential risks associated with
458
the PAB groups present in drinking water production and distribution networks.
459
Acknowledgements
460
The authors would like to acknowledge the support from the Chinese Scholarship Council
461
(2008612022). The authors thank Oasen, Dunea and Vitens water companies for their
462
cooperation in this study. Thanks are also due to Maarten Lut, Ed van der Mark, and Geo
463
Bakker for their assistance in the study. The authors thank Gertjan Medema for his critical
464
reading of the manuscript and Yu Tao for his valuable comments.
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Table 1 Quantifiable characteristics of PAB from three treatment plants
Parameters
TP1
TP2
TP3
Particle counts (# ml-1) (on line)
20(±3)
70(±5)
120(±9)
A-TCC/particle (average cells particle-1)
50 (±14)
49 (±4)
25 (±3)
0.21
0.29
0.33
(±0.05)
(±0.04)
Average ATP/intact cell (10-16 g cell-1) (n=3)
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(±0.05) Average A-ATP/intact cell (10-16 g cell-1)
0.53
0.50
0.51
(n=3)
(±0.01)
(±0.01)
(±0.01)
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Table 2 ATP per cell from reported literature
631
literature
Groundwater
0.2-4.0
(Jensen, 1989)
Groundwater
2.2-5.2
(Eydal and Pedersen, 2007)
Drinking water biofilter
0.21-3.8
(Magic-Knezev and van der Kooij,
RI PT
ATP per cell (10-16 g cell-1)
0.65-2.28
(Velten et al., 2007)
Tap water
0.31-0.55
(Berney et al., 2008)
Average aquatic
0.89
(Hammes et al., 2010)
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2004)
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Table 3 PAB bacterial diversity in the three treatment plants (average ± std., n=3)
Sample
TP1
Number of
Observed
Chao 1
Shannon-Wiener
Evenness
sequences analysed
OTUs (97%)
(97%)
Index (H)
(E)
2988
495 ± 12
1470 ±
8.1 ± 0.10
0.89 ± 0.01
4.9 ± 0.31
0.64 ± 0.02
103 8921
207 ± 24
653 ± 148
2818
239 ± 7
448 ± 83
6.3 ± 0.19
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0.80 ± 0.02
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Table 4 The genera identified in PAB of different treatment plants
Percentage of sequences (%) TP2
TP3
Legionella
0.34
3.03
1.0
Nitrospira
0.11
3.10
0.42
Gallionella
0.34
Planctomyces
1.00
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TP1
0.29
2.10
0.48
M AN U
4.47
CandidatusOdyssella
0.04
1.06
0.46
Caulobacter
0.17
0.22
0.11
0.16
0.20
0.31
Aquabacterium
0.27
0.71
0.07
Comamonadeceae (unclassified)
3.70
3.02
10.85
12.09
10.28
3.38
Caldilinea
0
0.02
0.08
Nitrosomonas
0.19
5.17
0.22
Crenothrix
0.13
4.49
0.30
Thermodesulfovibrionaceae LCP-6
1.90
3.50
3.71
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Unclassified OP3 GIF10
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0.31
0
13.79
Rhodopirellula
0
0.07
0
Leptolyngbya
0
0
3.39
Unclassified Alphaproteobacteria
1.77
6.58
6.08
Unclassified phylum bacteria
22.25
12.79
6.84
Other
55.23
SC 39.19
48.22
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Rhodospirillaceae (un-identified)
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Figure 1 Schematic drawing of multiple particle filtration system (MuPFiS) and parallel
639
running particle counter used for PAB sampling
640
Figure 2 SEM pictures (a: TP1, b: TP2 and c: TP3) and elemental composition of PAB (d)
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Figure 3 Average TCC and A-TCC results at each treatment plant (n=3)
SC
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Figure 4 Average ATP and A-ATP results of at each treatment plant (n=3)
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Figure 5 Taxonomic assignment of 16s rRNA gene sequences retrieved from PAB samples
648
classified by phylum. (a: TP1; b: TP2; c: TP3)
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• The number and activity of PAB ranged from 1.0-3.5×103 cells/ml and 0.04-0.154ng/l ATP. • There were 25-50 cells found to be attached on a single particle. • Anoxic and anaerobic bacteria were detected; OP3 was a main part of the PAB population.
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• Bacterial genera associated with particles are consistent with the particle characteristics. • PAB are important to bacteria enumeration and ecology of water distribution systems.
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Supplementary data Table S1 water quality information of selected treatment plants (N.A.: not available)
TP2
Surface water
Groundwater
Extracted ARR
Treated
Raw
N.A.
12.9
N.A.
Temperature
pH
N.A.
Turbidity (NTU)
N.A.
AOC
N.A.
l-1) ATP (ng l-1)
Groundwater
Raw
12
Treated
N.A.
12
8.5
N.A.
8.3
N.A.
8.2
<0.03
N.A.
0.22
N.A.
<0.1
5.8
N.A.
12.
N.A.
5.9
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(µg c
Treated
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(°C)
TP3
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TP1
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Parameters
N.A.
1
N.A.
4.5
N.A.
4.5
N.A.
0.45
N.A.
1.65
N.A.
1.62
0.60
0.0052
0.55
0.0052
0.67
<0.03
Fe (mg l-1)
0.33
<0.01
0.95
0.012
0.92
<0.01
Mn (mg l-1)
0.09
<0.01
0.79
0.023
0.085
<0.01
SO4 (mg l-1)
N.A.
50.8
N.A.
34
N.A.
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TCC (cells ml-1)
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NH4 (mg l-1)
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AOC of TP1 was averaged of measurements in the year 2010 (n=4). AOC of TP2 and TP3 was measured in 2010. The result of parameters were averaged results of samples taken
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together with PAB sampling (n=3).
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Figure S1. The release of ATP during LES treatment, each LES treatment last for 2 minutes and triplicate measurements were conducted.
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Quantification and identification of particle-associated bacteria in unchlorinated drinking water from three treatment plants by cultivation-independent methods
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G. Liu1 *, F. Q. Ling2, A. Magic-Knezev3, W. T. Liu2, J.Q.J.C.Verberk1, J.C. Van Dijk1 1. Section Sanitary Engineering, Department of Water Management, Faculty of Civil Engineering and Geosciences, Delft University of Technology, PO BOX 5048, 2600 GA Delft, the Netherlands E-mail: [email protected]
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2. Department of Civil and Environmental Engineering, University of Illinois Urbana-
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Champaign, 205 N. Mathews Ave., Urbana, Illinois 61801, U.S.A.
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3. Het Water Laboratorium, PO BOX 734, 2003 RS Haarlem, the Netherlands
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