Bio-treatment of phosphate from synthetic wastewater using Pseudomonas sp YLW-7

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In this study, the efficient phosphate utilizing isolates were used to remove phosphate from synthetic phosphate wastewater was tested using batch scale process. Hence the objective of the present study was to examine the efficiency of bacterial species individually for the removal of phosphate from synthetic phosphate wastewater. The most efficient phosphate reducers were isolated and screened from eutrophic lake water samples. The total heterotrophic bacterial analysis of the samples showed the presence of about 22 phosphate reducers. Among them, Pseudomonas sp YLW-7 were found to be efficient in phosphate reduction based on the maximum phosphate ultization which was observed by plate screening method using the minimum inhibitory concentration (MIC) test. The effect of carbon sources (glucose, starch, sucrose and lactose) at 0.5% on the removal of phosphate by Pseudomonas sp YLW7 was estimated. The maximum growth of Pseudomonas sp YLW7 was observed to be 0.9886 OD in glucose followed by starch (0.9456 OD), Sucrose (0.9095 OD) and lactose (0.8407 OD). The pH change in culture medium after 72 h treatment was found to be 6.0 in glucose, starch, lactose sources and 5.8 in sucrose carbon source. The phosphate removal was observed to be maximum of 68 % in synthetic phosphate wastewater with glucose carbon source followed by starch (66%), sucrose (65%) and lactose (62%) after 72 h at neutral pH (7.0± 2) by Pseudomonas sp YLW-7. Thus the Pseudomonas sp YLW-7 may use the contaminants as nutrients source and might be used in the remediation of phosphate contaminated environments. @ JASEM The addition of phosphorus as phosphate ion is one of the most serious environmental problems because of its contribution to the increased eutrophication process of lakes and other natural waters. The possible entry of this ion into aquatic environment is through household sewage water and industrial effluentsparticularly fertilizer and soap industries. Nitrogen and phosphorus are the primary causes of cultural eutrophication (i.e., nutrient enrichment due to human activities) in surface waters. The most recognizable manifestations of this eutrophication are algal blooms that occur during the summer. Chronic symptoms of over-enrichment include low dissolved oxygen, fish kills, murky water, and depletion of desirable flora and fauna. In addition, the increase in algae and turbidity increases the need to chlorinate drinking water, which, in turn, leads to higher levels of disinfection by-products that have been shown to increase the risk of cancer. Excessive amounts of nutrients can also stimulate the activity of microbes, such as P fisteria, which may be harmful to human health (U.S. EPA, 2001). Approximately 25% of all water body impairments are due to nutrient-related causes (e.g., nutrients, oxygen depletion, algal growth, ammonia, harmful algal blooms, biological integrity, and turbidity) (U.S. EPA, 2007). In efforts to reduce the number of nutrient impairments, many point source dischargers have received more stringent effluent limits for nitrogen and phosphorus. To achieve these new, lower effluent limits, facilities have begun to look beyond traditional treatment technologies. An important group of contaminants for which efficient treatment methods are needed are phosphates, since they may adversely affect and pose a threat to aquatic ecosystems. According to federal government standards, phosphate levels in water should not exceed 0.01 – 0.1 mgl -1 (EPA, 1991). Therefore it is essential to control the emission of phosphates from discharge of wastewater and reducing phosphorus concentrations to the lowest possible level is vital to the maintenance of unpolluted water supplies. Biotreatment is a cost-effective method for wastewater before being discharged into the streams and rivers. Microbial strategies for the removal of environmental pollutants from waste streams or contaminated sites can provide an attractive alternative to traditional methods such as incineration or disposal in landfills. Currently, phosphates are biologically removed by wastewater treatment facilities by absorption of dissolved orthophosphate, polyphosphate and organic phosphate by living microorganisms, such as bacteria, microalgae, yeast, protozoa, fungi, and macrophytes. Hence the objective of the present study was to examine the efficiency of individual bacterial species isolated from eutrophic lake water for the removal of phosphate from wastewater. MATERIALS AND METHODS Sample Collection: The eutrophic lake waters were collected in sterile glass bottles from four different sampling stations of Yercaud and Kodaikanal Lakes (Tamil Nadu, South India). Isolation and identification of phosphate reducers: Pour plate technique was employed to enumerate total heterotrophic bacteria using Nutrient Agar (Hi-Media, Mumbai, India). Minimum inhibitory concentration (MIC) test with plate screening method was carried out to screen phosphate reducers using phosphate agar. The bacterial cultures isolated from nutrient agar and phosphate agar plates were classified to various Bio-treatment of phosphate..... SHARANI, K; LAKSHMANAPERUMALSAMY, P genera based on their morphological and biochemical characters as given in Bergey's Manual of Determinative Bacteriology (Buchanan and Gibbons, 1994). The phosphate reducers screened from the different sample source were given symbols (code name) based on the source of isolation; Kodaikanal Lake WaterKLW, Yercaud Lake Water – YLW. Preparation of inoculums: Nutrient broth (Hi-Media, Mumbai, India) was prepared and selected bacterial isolates were inoculated separately and incubated for 24 h at room temperature. The cells were recovered by centrifugation (10,000 rpm for 15 min) and were transferred to sterile saline. The cell concentration of each strain was adjusted to an optical density at 600 nm (OD 600) of 0.1 and used as inoculum. The efficient phosphate reducers (Pseudomonas sp YLW7) were used for removal of phosphate. About 105 (YLW-7) X 10 4 CFU/100ml (1ml of 0.1OD) of the cells was used as an inoculum. Experimental study: Shake flask batch culture experiments were performed. Phosphate removal was carried out by adding phosphate to synthetic wastewater (mineral salts dissolve in plain distilled water with phosphate concentration of 100mgl -1 ; pH7.2) and 0.5% of different carbon substrates such as sucrose, starch, glucose and lactose were prepared. Phosphate was added to the medium as KH2PO4 and K2HPO4 at a 1.2:1 weight ratio to obtain P concentrations of 100 mg/liter. The nutrient solution contained (per liter) 1.5 g of FeCl36H2O, 0.15 g of H3BO3, 0.03 g of CuSO4 5H2O, 0.18 g of KI, 0.12 g of MnCl2 4H2O, 0.06 g of Na2MoO4 2H2O, 0.12 g of ZnSO4 7H2O, 0.15 g of CoCl2 6H2O, and 10 g of EDTA. Then the medium containing flasks were sterilized at 121°C and at 15 lbs for 15 min in an autoclave. One ml of inoculum (0.1 OD) from the selected phosphate reducers (Pseudomonas sp YLW7) was inoculated in the individual flasks. They were incubated at room temperature in a shaker maintained at 150 rpm for a period of three days. Samples were collected at 0, 24, 48, 72 h and analyzed for growth of bacteria, pH change and change in total phosphate concentration of the medium. All experiments were performed in triplicates. Growth of bacteria and pH change: The increase in growth of bacteria for every 24 h was monitored by measuring OD at 600nm on a UV-Visible Spectrophotometer (UV-VIS Hitachi U3210). The pH change in the culture medium after treatment was measured using a pH meter. Estimation of phosphate: The phosphate uptake activities of different strains were quantified by stannous chloride reduced molybdophosphoric acid blue method. The soluble phosphate content in the culture medium was estimated after 24, 42, and 72 h of incubation by using the stannous chloride calorimetric method (Saxena, 1994) and (APHA, 1998). After every 24 h, 10 ml of the agitated sample was drawn from the series of individual flask and transferred into the centrifuge tubes of 15ml capacity under aseptic conditions. Then the tubes containing samples were centrifuged at 10,000 rpm at 15 min and the clear supernatant was used for soluble phosphate estimation at 690 nm by using spectrophotometer (UV-VIS Hitachi U3210). Phosphate uptake efficiency (E) was calculated using the formula, E = [(I-F)/I] x 100 Where, I and F are the initial and final concentrations of phosphorous respectively. An efficiency value of 100% was obtained when no phosphate appeared in the water sample (i.e., F = 0). RESULTS AND DISCUSSION The isolation and screening of phosphate reducers from the samples mentioned above were carried out to determine the efficient phosphate removal which showed that wide range of these bacteria was occurred in eutrophic lake water. Table.1 shows the maximum population of total heterotrophic bacterial (THB) population of 28.5 CFU x 10 3 ml -1 and phosphate reducing bacterial population of 3.3 CFU x 10 3 ml -1 was noticed in Yercaud lake water sample. It was found that among the 22 isolates, Pseudomonas sp (YLW-7) was screened and identified as predominant phosphate utilizers based on the minimum inhibitory concentration (MIC) test after 72 h of incubation, Yercaud Lake Water-YLW as in Fig.1. These isolates were used in this study to remove phosphate in synthetic phosphate wastewater. Phosphate utilizing bacteria were known to be present in various environments (Illmer and Schinner, 1992) and (Illmer et al., 1995). The removal efficiency of soluble phosphates varied with strains. Various microorganisms are capable of utilizing phosphate as a sole source carbon or phosphorus (Malacinski et al., 1967) and these microbial transformations have been proposed as key steps in the phosphorous cycle in nature. Table.1 Enumeration of Total heterotrophic bacteria (THB) and Phosphate reducers present in different samples Source of Isolation THB Population Phosphate reducers Kodikanal Lake Water (KLW) 17.8 cfu x10 ml 2.2 cfu x10 ml Yercaud Lake Water (YLW) 28.5 cfu x10 ml 3.3 cfu x10 ml The growth of bacterial species was analyzed using different carbon sources in phosphate medium after 72 h of incubation period. In synthetic phosphate wastewater with 0.5% carbon sources, the individual 76 Bio-treatment of phosphate..... SHARANI, K; LAKSHMANAPERUMALSAMY, P strain of Pseudomonas sp YLW7 was observed a maximum growth of 0.9886 OD in glucose followed by starch (0.9456 OD), Sucrose (0.9095 OD) and lactose (0.8407 OD) as in Fig.2. The phosphate was taken up by cells for growth and to reform polyphosphate under aerobic condition. Increase in biomass concentrations showed a greater phosphate uptake capacity and enhances the efficiency of phosphate removal. Fig.1. Screening of efficient phosphate reducers based on the Minimum Inhibitory Concentration test (Pseudomonas sp YLW-7) In order to find the relationship between metabolic activities and reduction of phosphate, pH of the culture medium was monitored. The pH change in culture medium from the initial pH 7 after 72h was found to be 6.0 in glucose, starch, lactose and 5.8 in sucrose carbon source as in Fig.3. The pH value of the culture medium with 0.5% of carbon source was reduced during the process. In contrast, there is no significant change of pH was monitored in the medium without carbon source. The culture medium, pH 6.0 was favored for acid phosphatase secretion was reported (Bouquet et al., 1987). Burkholderia cepacia maximum phosphate removal and accumulation of polyphosphate at pH 5.5 reported (Mullan et al., 2002). In contrast, high phosphate utilization was observed without detectable pH change (Asea et al., 1998). In synthetic phosphate wastewater with 0.5% carbon source, the Pseudomonas YLW-7 showed maximum phosphate removal of 68% when compared to control in glucose carbon source followed by starch (66%), sucrose (65%) and lactose (62%) as in Fig.4. Among the carbon sources, the glucose source showed maximum phosphate removal (68%) by the Pseudomonas sp in synthetic phosphate wastewater at initial pH 7, the glucose may be oxidized to gluconate which is further converted to other compounds. Glucose carbon source could induce good enhanced biological phosphate removal performance reported (Jeon and Park, 2000). The carbon, i.e. glucose is oxidized to gluconate, which is converted into other compounds, such as 2-keto-3-deoxygluconate, pyruvate or glyceraldehydes was reported (Kim et al, 1998) and (Reyes et al., 1999). Kim et al (1998) suggested that the presence of organic acids (formate) and the mechanism such as the release of protons associated with biological ammonium assimilation that enhances the utilization of phosphates. In synthetic phosphate solution at 100 mgl -1 of phosphate concentration in 0.5% carbon source, it was found to be maximum removal of 68% with maximum growth of 0.9886 OD at initial pH 7.0± 2, by Pseudomonas sp in glucose carbon source (Fig. 5). The results showed that the strain could grow rapidly and remove phosphate efficiently in synthetic phosphate solution with 0.5% carbon source. 0 0.1 0.2 0.3 0.4 0.5 0.6 0.7 0.8 0.9 1 1.1 1.2 0 24 48 72 Time (h) O p ti c a l D e n s it y ( O D 6 0 0 n m ) Sucrose Starch Lactose Glucose Control Fig.2 Effect of carbon source on the growth of Pseudomonas sp YLW-7 in synthetic phosphate wastewater 77 Bio-treatment of phosphate..... SHARANI, K; LAKSHMANAPERUMALSAMY, P 4.4 4.8 5.2 5.6 6 6.4 6.8 7.2 0 24 48 72 Time (h) p H

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تاریخ انتشار 2010