Influence of Azo Dye on Metabolism of Phosphorus Accumulating Organisms Linked to Transformation of Intracellular Storage Products ()
1. Introduction
Enhanced biological phosphorus removal (EBPR) process is considered as one of the most economical and sustainable methods for phosphorus removal in wastewater treatment plants [1] [2] . In this process, activated sludge was under the alternating anaerobic and aerobic conditions and polyphosphate accumulating organisms (PAOs) could be enriched in this system. Generally, under anaerobic conditions, PAOs take up volatile fatty acids and store them to intracellular polyhydroxyalkanotes (PHAs), with the energy obtained from glycogen utilization and poly-phosphate (poly-P) hydrolysis and simultaneously released of ortho-phosphorus into solution. However, under aerobic conditions, PAOs take up excess phosphorus as intracellular poly-P formation and simultaneously glycogen is replenished by the oxidation of stored PHA. With wasted activated sludge enriched in poly-P discharging, the net removal of phosphorus in activated sludge can be achieved [1] .
In EBPR system, many operational factors would influence the performance of this system, especially the variation of the wastewater quality. At present, much municipal wastewater often contains large amount of industrial wastewater, especially includes certain amount of heavy metals, dyes and antibiotics, which has detrimental effect on nutrient removal [2] . For example, poor performance of P removal in EBPR system had been found to be related with the presence of heavy metals or antibiotics in wastewater [3] - [9] . However, few studies have been considered the influence of dye, especially azo dye on EBPR system performance.
In activated sludge system, azo dye is often complete removed under sequencing anaerobic-aerobic biological treatment process [10] . Under anaerobic conditions, with the help of azoreductase enzymes, reductive cleavage of the azo bonds resulted in the formation of potentially hazardous aromatic amines. Then under aerobic conditions, the produced aromatic amines can be further degraded [11] [12] [13] [14] . The azo dyes or their cleavage products would change the characteristics of sludge or had biological toxicity on microorganisms [15] . However, the influence of dye on the performance of EBPR system is still unknown yet.
Therefore, in this study, the influence of azo dye of methyl med (MR) on EBPR system were investigated. The COD, phosphorus and dye removal as well as intracellular storage products of PHA and glycogen were evaluated at different dye concentrations. Hopefully, the results would provide a better understanding of dye on EBPR system.
2. Materials and Methods
2.1. Reactor, Sludge and Wastewater
An anaerobic-aerobic sequencing batch reactor (SBR) with a working volume of 3.2 L was used for the cultivation of activated sludge. The reactor was operated with a cycle time of 12 h, consisted of 7 min of influent filling, 6 h of anaerobic, 5 h of aeration, 40 min of settling, 7 min of effluent withdrawal and 6 min of standing idle. The hydraulic retention time (HRT) and the sludge retention time (SRT) were set at 24 h and 12 days, respectively. Nitrogen gas was purged into the reactor with mechanical mixing for anaerobic conditions. Air was introduced through an air diffuser by an air pump for aeration. The temperature was kept at 25˚C with water jacket. The azo dye of MR was introduced to activated sludge gradually from 5 to 40 mg/L.
The seed sludge was obtained from a secondary sedimentation tank of the sewage treatment station in Han Bai Textile Company, Nanjing, China. The seed sludge had a mixed liquor suspended solids (MLSS) concentration of about 3000 mg/L. Synthetic wastewater used in this work comprised (mg/L): sodium acetate 1000, NH4Cl 170, CaCl2・2H2O 7.5, NaH2PO4 48, MgCl2 11, and KCl 25. In addition, 2.5 mL microelement solution was added, which contained (mg/L): H3BO3 2, FeCl2・4H2O 2, EDTA 2, ZnCl2・4H2O 0.4, MnCl2・4H2O 0.8, CuCl2・2H2O 0.2, (NH4)6MoO7・4H2O 1.1 and NiCl2・6H2O 1.
2.2. Batch Experiments
The batch experiments were carried out in a 2.0 L batch reactor. When the reactor reached the steady state, the activated sludge with a mixed liquor volatile suspended solids (MLVSS) of 2700 - 2800 mg/L was withdrawn from the SBR to batch reactor after starved for several hours and then washed twice with distilled water. A required amount of MR solution was added to batch reactors at the beginning of cycle to provide a constant MR concentration of 5, 10, 20, and 40 mg/L for each treatment cycle, respectively. The reactor without MR was used as the control. The influent chemical oxygen demand (COD) concentration was 400 mg/L and the medium pH was adjusted at around 7.0 through the addition of 1M HCl or NaOH. The argon gas was filled into the synthetic wastewater for 20 min to remove the oxygen before into the reactor. In the aerobic condition, the SBR was aerated continuously to keep the dissolved oxygen (DO) concentration around 6 mg/L. Samples of the activated sludge mixture were withdrawn from the reactor at set intervals for the analysis of COD, dye, phosphorus, and intracellular storage products of PHA and glycogen.
2.3. Analytical Methods
The measurements of COD, phosphorus (PO43−-P), MLSS, and MLVSS were conducted according to the Standard Methods [16] . The concentration of azo dye was determined using the modified method of Wong and Yuen [17] . Aliquots from the test solution were centrifuged at 5200 rpm for 5 min. The dye solution was measured at 430 nm, which is the absorbance maximum for the orange color of methyl red, using a spectrophotometer (ALPHA-1506, Pu Yuan, China).
The PHA was determined according to Fang et al. [18] , and glycogen was measured according to Smolders et al. [19] with minor modification. Glycogen was extracted and hydrolyzed from activated sludge by heating a sample of a known amount of freeze-dried activated sludge (typically 50 mg) in a known volume of 0.6M HCl (typically 5 mL) for 5 h at 100˚C. The glycogen content in the supernatant was determined by anthrone method [20] with glucose as the standard.
3. Results and Discussion
3.1. COD and Dye Removal at Different Dye Concentration
The influences of dye on COD and dye removal efficiencies are shown in Figure 1. At the MR concentration of 5 mg/L, the COD removal efficiency was almost the same as that in control experiment. However, with the increase of MR concentration, COD removal efficiency decreased slightly. The increase of MR concentration from 0 to 40 mg/L led to the decrease of COD removal efficiency from 97.9% to 84.0% (Figure 1(a)). The inhibition of PAOs and other heterotrophic microorganisms might be the reason for this phenomenon.
The dye removal efficiency was also decreased from 99.7% to 86.9% with the increase of MR concentration from 5 to 40 mg/L (Figure 1(b)), and the result was consistent with that reported by Hakimelahi et al. [21] . The decrease of dye removal efficiency was probably due to the lessening of the COD removal caused a lower production of reducing equivalents, negatively affecting the color removal [22] . Furthermore, main color was removed at the anaerobic condition and the contribution of aerobic condition to decolorization was low. The results were in good agreement with other results in the sequencing anaerobic-aerobic conditions [13] [23] .
Figure 1. Effects of dye concentration on COD and dye removal: (a) COD removal efficiency; and (b) MR removal efficiency.
To further confirm the biodegradation of MR by activated sludge, the UV-Vis spectra of the samples taken at different time are illustrated in Figure 2. The peak in the visible region at 430 nm which represents the azo linkage of MR was decreased at anaerobic condition. Correspondingly, the appearance of the absorbance peak at 241 nm and 305 nm is probably due to the production of intermediate products of N, N’ dimethyl-p-phenyle-nediamine (DMPD) and 2-aminobenzoic acid (2-ABA) [24] . At aerobic condition, the two absorbance peaks were decreased. This indicated that the ability of the activated sludge for the biodegradation of MR.
3.2. Influence of Dye Concentration on P Release and Uptake
The P release at anaerobic condition and P uptake at aerobic condition at different MR concentrations are shown in Figure 3. It was found that P removal efficiency was almost 100% in the control experiment. At low MR concentration of 5 mg/L, the P release and uptake were almost the same as those in control experiments, which indicated that low MR concentration had no inhibitory effect on P removal in the EBPR system. At MR concentration of 10 mg/L, P removal efficiency decreased slightly to 93.6%. However, when MR concentration was further increased to 20 and 40 mg/L, P removal efficiency decreased to 59.9% and 19.9%, respectively. Under anaerobic conditions, P release decreased significantly at MR concentration of 20 and 40 mg/L, suggesting that polyphosphate degradation was inhibited at high MR concentration [3] . Correspondingly, P uptake at aerobic condition was inhibited due to the shortage of energy provided by PHA degradation [25] . Thus, the increase of MR concentration severely decreased P removal capacity and had a toxic effect on the activity of PAOs.
3.3. Influence of Dye Concentration on the Transformation of PHA
The changes of intracellular storage product of PHA at anaerobic condition at different MR concentrations are illustrated in Figure 4. Under the control experiment, the content of PHA stored at anaerobic condition was 152.4 mg/gVSS. With the increase of MR concentration from 5 to 40 mg/L, the content of PHA stored at anaerobic condition decreased from 147.2 to 79.0 mg/gVSS. The linear regression analysis indicated that the stored PHA content at anaerobic condition was linearly decreased with the increase in MR concentration (R2 = 0.978). The results indicated that high dye concentration could inhibit the PHA synthesis at anaerobic condition in EBPR system, especially at high MR concentration. Due to the inhibitions of high concentration of intermediate aromatic amide on substrate uptake and poly-phosphate degradation at anaerobic condition, insufficient energy available can be used for PHA synthesis, leading to less PHA stored at higher MR concentration [1] [5] .
Figure 4 also gives the content of PHA degradation at aerobic condition with different concentrations of MR. The content of PHA consumption at aerobic condition was 146.8 mg/gVSS for the control experiment, and similar PHA degradation
Figure 2. UV-Vis spectra analysis of MR at anaerobic and aerobic conditions.
Figure 3. The P release and uptake in batch experiments at different MR concentrations.
Figure 4. The transformation of PHA in batch experiments at different MR concentrations.
was displayed at MR concentration of 5 mg/L. However, with the increase of MR concentration from 10 to 40 mg/L, PHA degradation content decreased sharply, indicating that high concentration of MR had severely inhibition effect on PHA degradation at aerobic condition. The results demonstrated that the mechanism of aerobic PHA degradation was more sensitive to MR dosing than that of anaerobic PHA synthesis, which was in agreement with the findings of Tsai and Chen [4] and Wang et al. [5] .
3.4. Influence of Dye Concentration on the Transformation of Glycogen
Figure 5 depicts the variation of intracellular storage product of glycogen at different MR concentrations. Under the control experiment, the hydrolyzed-glycogen was 46.7 mg/g VSS at anaerobic condition. At low MR concentrations (5 and 10 mg/L), the amount of glycogen hydrolysis at anaerobic condition was similar with that in the control experiment, indicating that low concentration of MR had no effect on the hydrolysis of glycogen at anaerobic condition in EBPR system. However, glycogen contents at anaerobic condition increased when dye concentrations were increased from 20 and 40 mg/L. The higher glycogen content at anaerobic condition was probably due to the maintenance adenosine triphosphate required by the cell [5] .
At aerobic condition, the content of glycogen was 54.9 mg/g VSS for the control experiment (Figure 5). At low MR concentrations (5 and 10 mg/L), the content of glycogen at aerobic condition was similar with that in the control experiment, indicating that low concentration of MR had no effect on glycogen replenishment at aerobic condition in EBPR system. However, the glycogen content decreased sharply at MR concentrations of 20 and 40 mg/L. Due to the accumulated PHA at anaerobic condition decreased at high MR concentration, less available PHA could be used for glycogen reproduction, resulting in the decrease in glycogen content [3] .
Figure 5. The transformation of glycogen in batch experiments at different MR concentrations.
4. Conclusion
The pollution removal and transformation of PHA and glycogen at different MR concentrations in EBPR system were investigated in this study. The COD, dye and phosphorus removal efficiencies were all decreased with the increase of MR concentration. For intracellular storage products, PHA synthesis and consumption, and glycogen replenishment was seriously inhibited at high MR concentration. Oppositely, glycogen hydrolysis was increased at MR concentration of 20 and 40 mg/L. The transformations of PHA and glycogen at aerobic condition were more sensitive to high MR concentration than those at anaerobic condition.
Acknowledgements
The work is financially supported by the “Fundamental Research Funds for the Central Universities, No: 2017B13214”, “National Natural Science Foundation of China (No: 51578210)”, “Guangzhou Key Laboratory of Environmental Exposure and Health (No. GZKLEEH201603)” and the “Priority Academic Program Development of Jiangsu Higher Education Institutions (PAPD), China”.