Study sites and study samples.

This cross-sectional study was carried out to investigate L. pneumophila contamination in 160 water samples collected from 72 cooling towers located at 4 hospitals (21 cooling towers), 7 department stores (35 cooling towers), and 3 hotels (16 cooling towers) in Bangkok. The study was reviewed and approved by the ethics committee of the Faculty of Public Health, Mahidol University, with a Research with Exemption category.

Approximately 2 L of water in sterile screw-cap bottles was collected aseptically from two or three points on each cooling tower (water-in, water-out, and reservoir). The sample size was calculated from a formula: n = Z²_α/2 PQ/d² (Z is the standard score of normal distribution at α = 0.05 and two tails = 1.96, d = allowable error at 0.075, P is the probability of L. pneumophila positivity in cooling tower water by real-time PCR from a previous study = 63%¹⁴ or P = 0.63, Q = 1-P, 0.37). Each water sample was divided into two equal parts, one to test for the Legionella culture and one to perform real-time PCR for L. pneumophila, following a study by Yaradou et al (2007).¹⁴ Cooling tower characteristics, including design or model and size, maintenance system, and duration of use were recorded. Some water parameters including temperature, pH, and residual free chlorine were measured. All water samples were transferred using ice-boxes to the Department of Microbiology at the Faculty of Public Health, Mahidol University, within four hours and kept at 4-10°C until total bacterial count (TBC), Legionella culture, and real-time PCR were performed.

Detection of Legionella spp. by culture.

To each water sample, 0.5 mL of 0.1 mol/L sodium thiosulfate (Na₂S₂O₃ 0.5 mL/sample water 1000 mL) was added, to neutralize disinfectants, following Majid et al (2007).¹⁵ The water samples were concentrated by filtration through 0.45 µm pore-size cellulose nitrate filters, following the study of Yaradou et al (2007).¹⁴ Each filter was cut and transferred into a micro-centrifuge tube. Then, 1.5 mL of sterile distilled water was added to the tube and vortexed for two minutes to recover bacterial cells. Portions of the concentrated sample were treated with 0.2 mol/L HCl-KCl, pH 2.2 at room temperature for 20 minutes to eliminate non-Legionella organisms. Next, 100 µL of the concentrate (undiluted and 10-fold diluted samples) were plated onto modified buffered charcoal yeast extract (MBCYE) agar. The inoculated plates were kept in a humidified incubator at 35-37°C for 7 days, and the grayish-white, shiny colonies were counted as suspected Legionella spp. Then, suspected colonies were sub-cultured onto normal BCYE agar and BCYE agar without L-cysteine for verification. If the isolate could grow only on BCYE and the Gram stain was negative, it was determined to be a Legionella spp.

Detection of L. pneumophila by real-time PCR.

Sample preparation for PCR.

Following the Roche method, 1000 mL water samples were concentrated by filtration through 0.45 µm pore-size cellulose nitrate filters. The filter was placed into a centrifuge tube. Then, 1.5 mL of sterile distilled water was added to each centrifuge tube and vortexed for bacterial release for 2 minutes. Next, 1 mL of the concentrate was transferred to a 1.5 mL micro-centrifuge tube and centrifuged at 10,000 g for 5 minutes. The supernatant was discarded. The sediment was used for DNA extraction with a High pure PCR template preparation kit (Roche, Germany). The Roche kit protocol was followed step by step for enzymatic lysis and DNA extraction. Then, the supernatant containing the DNA was stored at -20°C until use.

Real-time PCR. Real-time PCR used in this study followed the study of Yaradou et al (2007).¹⁴ The method is highly specific and sensitive for environmental water samples.^14,16 LightCycler version 1.1 instruments from Roche Applied Science (Roche, Mannheim, Germany) were used with a final volume of 20 µL of total reaction mixture, which consisted of 15 µL of master mix and 5 µL of template. The master mix was prepared with the following final concentrations per capillary tube: 0.5 µL (both) primers, 10 µL LightCycler 480 SYBR Green I Master, 2x conc. (2x-concentrated master mix that contains FastStart Taq DNA polymerase, reaction buffer, nucleotides—dATP, dCTP, dGTP, dUTP—and SYBR Green I), 4 µL PCR-grade. Primers for PCR amplification of Legionella spp. (16S rRNA gene) and L. pneumophila (mip gene) were used in the reaction. The experimental LightCycler protocol consisted of 10 minutes at 95°C for Taq polymerase activation, 45 cycles of PCR amplification (95°C for 15 seconds, 60°C for 15 seconds, and 72°C for 20 seconds), melting (65 to 97°C at 0.1°C/second), and a cooling step (40°C for 30 seconds). This process is shown in Figure 1. A positive control (L. pneumophila Sg1 strain ATCC 33152) and a negative control (purified PCR grade water) were included in all PCR assays. All the runs were completed with a melt curve analysis to confirm the specificity of amplification by slowly ramping the instrument from a low temperature to a high temperature. The range of between 80°C and 81°C was mip gene. The range of between 84°C and 85°C was 16s rRNA gene. Crossing point (Cp) values were determined by LightCycler 480 software version 1.2 and put into an MS Excel data sheet (Microsoft) for analysis after background subtraction. Cp cycles were plotted with log of input DNA quantities to calculate the slope (see Fig. 1).

Figure 1.

The optimal condition for L. pneumophila detection by real-time PCR.

Detection of physicochemical parameters and total bacterial counts of water samples.

Water temperature, pH (direct reading pH meter, probe and meter) and residual free chlorine using the DPD method (N, N-diethyl-p-phenylenediamine, and colorimeter Protronics Intertrade Co., Ltd) were determined at the time of water sample collection. Additionally, the total bacterial count was detected using 0.1 mL of water samples with a 10-fold dilution series of the concentrated water samples (10⁻¹, 10⁻² and 10⁻³) inoculated on plate count agar in duplicate tests. All plates were incubated at 35°C for 24-48 hours. The number of colonies were counted, and reported in colony forming units/mL (CFU/mL).

Statistical analysis.

Data about cooling tower characteristics and parameters of water samples with and without L. pneumophila were compared and analyzed to search for factors associated with the contamination and predictive factors using univariate analysis (χ²-test), odds ratio and 95% confidence interval, and stepwise logistic regression analysis. The statistically significant level was set at α = 0.05.

Cooling tower characteristics and parameters of studied water samples.

The present study found two models of cooling towers used in the studied buildings, a counter-flow model (16 cooling towers) and a cross-flow model (56 cooling towers). Approximately 50% of studied cooling towers had a size less than 500 tons, ranging from 300 to 600 tons (average = 450 tons). Half of them had been in use for at least 10 years, and ages of towers ranged from 3 to 12 years (average = 7 years). The mean maintenance frequency was 6 times a year, ranging from 1 to 12 times a year. However, most of the studied cooling towers were not treated with biocide or ozone to inhibit the growth of Legionella spp. The ratio of using biocides, ozone, or none was 1:2.6. It was found that the mean value of residual free chlorine was 0.1 ppm, ranging from 0.0 to 0.5 ppm. The mean pH was 7.0, ranging from 6.0 to 8.5. Average water temperature was 32.2°C, and average total bacterial count was 6.6 × 10⁵ CFU/mL, ranging from 2.0 × 10³ to 5.0 × 10⁶ CFU/mL, as shown in Table 1.

Table 1.

Summary of physicochemical and biological parameters of studied cooling towers and water samples.

Legionella Spp. and L. Pneumophila Contamination in Cooling Tower Water.

In total 160 water samples, 32 (20.0%) were positive for Legionella spp. by culture, and 98 (61.3%) were positive for L. pneumophila by real-time PCR. The sensitivity of real-time PCR was higher than that of the culture. Water samples collected from the reservoirs of the cooling towers had the highest percentage of L. pneumophila contamination by real-time PCR compared with those collected from the water-in and the water-out flow areas of the cooling towers (reservoirs: 76.0%, water-in: 44.9%, and water-out: 52.8%). It was statistically significant with P < 0.05 as shown in more details in Table 2.

Table 2.

Prevalence of Legionella spp. and L. pneumophila contamination in water samples by culture and real-time PCR distributed by places and sites of water collection.

Predictive factors and risk probability of L. pneumophila contamination.

From univariate analysis, the cooling tower characteristics and parameters found to be significantly associated factors for L. pneumophila contamination were: (1) cross-flow model, P = 0.005 (crude OR = 2.82, 95% CI = 1.26-6.37); (2) size <500 tons, P = 0.010 (crude OR = 2.37, 95% CI = 1.16-4.88); (3) use duration >5 years, P = 0.005 (crude OR = 3.79, 95% CI = 1.32-11.23); (4) pH > 6, P = 0.019 (crude OR = 2.88, 95% CI = 1.07-7.87); (5) no use of biocide or ozone, P = 0.018 (crude OR = 2.32, 95% CI = 1.08-4.97); (6) residual free chlorine <0.2 ppm, P = 0.009 (crude OR = 4.52, 95% CI = 1.22-20.53); and (7) water temperature <29.4°C, P = 0.005 (crude OR = 4.45, 95% CI = 1.40-18.52). After stepwise logistic regression analysis, 4 significantly predictive factors remained including: the cooling tower model as a cross-flow type, P = 0.017 (OR = 3.09, 95% CI = 1.22-7.84); use duration >5 years, P = 0.016 (OR = 3.59, 95% CI = 1.27-10.14); residual free chlorine <0.2 ppm, P = 0.003 (OR = 8.49, 95% CI = 2.06-34.93); and water temperature < 29.4°C, P = 0.002 (OR = 7.87, 95% CI = 2.09-29.59). (See Table 3). Additionally, the risk probability for L. pneumophila contamination was estimated using four predictive factors. It was found that the risk probability ranged from 13.9 to 97.1%, depending on the combination of predictive factors, as shown in Table 4.

Table 3.

Risk factors for Legionella pneumophila contamination in cooling tower water detected by real-time PCR, univariate and multivariate analyses.

Table 4.

The risk probability of L. pneumophila contamination in cooling tower water.

A cooling tower is a heat rejecting device, which includes both direct (open) and indirect (closed) circuits. It transmits waste heat to the atmosphere through the cooling of a water stream to a lower temperature.¹⁷ In general, there are two models of cooling towers used in buildings, a cross-flow type and a counter-flow type. In a cross-flow cooling tower, air flows horizontally through the fill as the water moves downward, and in a counter-flow model, air flows upwardly through the fill or tube bundles, opposite to the downward movement of the water.^17,18 The present study found that most of the studied cooling towers were cross-flow types and the ratio of cross-flow models to counter-flow models was 3.5:1. The findings from analysis of risk factors for the contamination of L. pneumophila in cooling tower water indicated that the cross-flow model significantly increased the risk of L. pneumophila contamination when compared to the counter-flow model (adjusted OR = 3.09, 95% CI = 1.22-7.84, P = 0.017). The water movement in the cross-flow model probably increased the settlement of organic particles and sludge in the reservoir of the cooling towers. Sediment, sludge, and some organic matter could be nutrient sources for Legionella spp.^19,20

Cooling towers frequently generate droplets by distributing water over a packing material through which there is a counter-current flow of air.^17,18 A previous study reported that major Legionella outbreaks have been associated with relatively small systems (i.e. <100 tons).²¹ This present study supported that finding, with the smaller cooling towers (<500 tons) having higher risk of L. pneumophila contamination in the cooling tower water (crude OR = 2.37, 95% CI = 1.16-4.88, P = 0.010), but it was not statistically significant after multivariate analysis (P > 0.05). Additionally, the recommended schedule for cooling tower maintenance is at least twice a year and determination of total bacterial count should be frequently performed to evaluate proper water treatment. In this study, the average maintenance frequency was six times per year, and surprisingly, the total bacterial count in cooling tower water was rather high with a mean of 6.6 × 10⁵ CFU/ml. However, both parameters showed no significant association with the L. pneumophila contamination (P > 0.05) after univariate and multivariate analyses. These findings supported previous reports from World Health Organization (2007)¹⁷ and Bentham and Broadbent (1993).²¹

Two other factors, including duration of use and pH, had an effect, since findings indicated that water pH was a significant risk factor for contamination after univariate analysis (P = 0.019) and was not significant after multivariate analysis (P > 0.05), whereas, the use duration of cooling towers was a significant risk factor for the contamination after univariate and multivariate analyses (crude OR = 3.79, 95% CI = 1.32-11.23, P = 0.005 and adjusted OR = 3.59, 95% CI = 1.27-10.14, P = 0.016). This might be due to the longer usage, the more accumulation of sediments, sludge, nutrients, and biofilm formation.^19,20 Cooling tower users frequently apply biocides to the circulating cooling tower water for controlling the growth of micro-organisms and other macro-organisms. Oxidizing biocides such as chlorine and bromine are more widely used in the electrical power and refining industries because of their effectiveness, moderate cost and easy treatability. Ozone is also highly effective, but there is more difficulty concerning maintenance than using chlorine.^22232425 Results from this study showed significance in univariate analysis (P = 0.018), however there was no significance in multivariate analysis (P > 0.05). In Thailand, the Metropolitan Waterworks Authority recommended the standard level of free chlorine to be at 0.2-0.5 ppm for inhibition of microbial growth in the water.²⁶ This recommendation was supported by data from the present study since residual free chlorine less than 0.2 ppm was a risk factor for L. pneumophila contamination (crude OR = 4.52, 95% CI = 1.22-20.53, P = 0.009 and adjusted OR = 8.49, 95% CI = 2.06-34.93, P = 0.003). Nevertheless residual free chlorine 0.5-1.0 ppm was recommended by Zhang, et al (2007) for controlling the L. pneumophila growth in hospital water systems.²³

Operating temperatures in the range of 25.0°C to 42.2°C are likely to be favorable in amplifying the growth of Legionella spp.^27,28 This study found that water temperature at 16.7-38.2°C, with the average of 32.2°C, probably supported the growth of Legionella spp. When a cut-off temperature of 29.4°C (85°F) was used for determining the risk factors in L. pneumophila contamination of cooling tower water, it was found that water temperature less than 29.4°C was a significant risk factor by univariate and multivariate analyses (crude OR = 4.45, 95% CI = 1.40-18.52, P = 0.005 and adjusted OR = 7.87, 95% CI = 2.09-29.59, P = 0.002). This evidence remains unexplained.

Additionally, the risk probability for L. pneumophila contamination was estimated using four significant factors from multivariate analysis (cooling tower model, use duration, residual free chlorine, and water temperature). It was found that the risk probability ranged from 13.9 to 97.1% depending on the combination of predictive factors. The lowest risk for contamination (13.9%) was for counter-flow type cooling towers, use duration <5 years, residual free chlorine ≥20.2 ppm, and water temperature ≥229.4°C. Alternatively, the highest risk for contamination (97.1%) was the condition of the cooling tower model being a cross-flow type, use duration ≥25 years, residual free chlorine <0.2 ppm, and water temperature <29.4°C. Therefore, cooling tower users should provide the optimal conditions and maintenance methods to minimize the risk of L. pneumophila contamination in cooling tower water.

Finally, the findings in this study showed higher sensitivity using real-time PCR than using the culture (61.3% and 20.0%). The culture remains the standard method for detecting Legionella spp. from environmental sources, but this technique yields low sensitivity and requires up to 10 days to complete. The PCR method provides a very sensitive and powerful screening test for the detection of L. pneumophila in environmental samples and requires a few hours to complete.^14,16,29 Even though the PCR method does not distinguish between living and dead cells, it is usually indicative of an existing or potential future problem and helps to prevent future exposure when it is positive.

The cleanliness of cooling towers is important for public health and should be ensured.^14,29 Results of the present study revealed that water samples collected from the reservoir of the cooling towers had significantly higher percentages of L. pneumophila contamination compared to those collected from the water-in and water-out areas of the cooling towers (reservoir: 76.0%, water-in: 44.9%, and water-out: 52.8%, P < 0.05). For routine maintenance of cooling towers, testing for L. pneumophila contamination should be done frequently and the reservoirs of cooling towers should receive focus as the predominant sampling point.