A new method was developed using the carbon dioxide detected in the headspace of a batch reactor to determine the carbon source addition in the biological nutrient removal (BNR) process. The activated sludge used in this study was taken from the University of British Columbia (UBC) Wastewater Treatment Pilot Plant aerobic tanks undergoing simplified UCT process. Experiments showed that detectable changes of carbon dioxide concentration in the headspace reflected the acetate utilization in the anaerobic condition, i.e. the P release reaction. In the sodium acetate addition cases, the elapsed time (E Time) of carbon dioxide evolution rate changes was proportional to the amount of acetate added in solution. Results were successfully used to estimate the amount of acetate added in tests. This new methodology was also capable of estimating the amount of VFAs recovered from the thermophilic aerobic digestion (TAD) supernatant. This on-line “E Time” monitoring approach has the potential to optimize the carbon source addition in BNR processe
Trang 1A New Technique Using Headspace Gas Monitoring
to Determine Carbon Source Addition in a BNR Process
Jowitt Z Li*, Donald S Mavinic*, and Harlan G Kelly**
* University of British Columbia, Department of Civil Engineering, Environmental Engineering Group, Vancouver, B C V6T 1Z4, Canada
** Dayton & Knight Ltd., West Vancouver, B C V7V 3N9, Canada
ABSTRACT
A new method was developed using the carbon dioxide detected in the headspace of a batch reactor to determine the carbon source addition in the biological nutrient removal (BNR) process The activated sludge used in this study was taken from the University of British Columbia (UBC) Wastewater Treatment Pilot Plant aerobic tanks undergoing simplified UCT process Experiments showed that detectable changes
of carbon dioxide concentration in the headspace reflected the acetate utilization in the anaerobic condition, i.e the P release reaction In the sodium acetate addition cases, the elapsed time (E Time) of carbon dioxide evolution rate changes was proportional to the amount of acetate added in solution Results were successfully used to estimate the amount of acetate added in tests This new methodology was also capable
of estimating the amount of VFAs recovered from the thermophilic aerobic digestion (TAD) supernatant This on-line “E Time” monitoring approach has the potential to optimize the carbon source addition in BNR processes
KEYWORDS
Biological nutrient removal (BNR), carbon dioxide evolution, carbon source determination, on-line
headspace monitoring, thermophilic aerobic digestion (TAD), volatile fatty acids (VFAs)
INTRODUCTION
Available carbon is an essential component for biological nutrient removal (BNR) enhancement Volatile fatty acids (VFAs, C2-C4) recovered from the thermophilic aerobic digested (TAD) sludge supernatant, under a microaerated operation, is a potential carbon source for denitrification and enhanced biological phosphorus removal (Chu, et al, 1996) However, high soluble COD and ammonia-N recovered from the TAD supernatant could disrupt the system performance and deteriorate effluent quality Meanwhile, the VFA concentration in TAD supernatant fluctuates due to varied sludge conditions, such as the sludge age and ORP TAD supernatant addition must be optimized to maximize the benefit of VFA utilization and prevent system overloading (Li, Mavinic, and Kelly, 1999) A quick and reliable method to estimate the available carbon source on-line would be considerably beneficial in optimizing the BNR performance
A new method, using the headspace carbon dioxide (CO2) monitoring of a batch reaction under the anaerobic condition, was proposed to estimate the amount of carbon source addition The fundamental concept was derived from the observation of P release corresponding to the acetate utilization Complexity and interference of the carbonate-bicarbonate species and pH in the system were discussed elsewhere (Spérandio and Paul, 1997) The observed CO2
concentration in the headspace is the overall outcome of various mechanisms, such as endogenous respiration, carbonate-bicarbonate balance, CO2 reserve, and BNR The objective of this study was to access the correlation between the carbon dioxide profiles observed in the headspace and the amount of acetate added in the activated sludge
Trang 2METHODOLOGY
Experiment Apparatus
The experiment apparatus, equipped with carbon dioxide (Vaislal GMD20), ORP
(Broadley-James, Ag/Ag-Cl), pH (Oakton, Ag/Ag-Cl), and temperature probes/sensors, is
illustrated in Figure 1 Nitrogen gas was sparged through the entire test course to provide sufficient mixing of solution, prevent oxygen interference, and carry the gas for detection Internal circulation was designed to enhance the transfer mixing in the headspace The carbon dioxide sensor readings were verified by different volumes of air samples using a Shimadzu
TOC-500 inorganic carbon analyzer (samples taken at 1 atm, 100% relative humidity), the calibration curve is shown in Figure 2
Batch Tests
The activated sludge used in this study was taken from the University of British Columbia (UBC) Wastewater Treatment Pilot Plant aerobic tank Sludge was pre-sparged with nitrogen gas, at a 5 L/min rate for 10 minutes in a preparation tank, to remove the foam, if any, and carbon dioxide reserve in solution; then the sludge was transferred to the experimental reactor (3.6 L in total with 1.6 L headspace volume) The nitrogen flow rate was maintained at 1,200 mL/min in the experiment reactor In each batch test, a certain volume of sodium acetate (1,000 mg/L as HAc) was added and the carbon dioxide profiles were monitored until the reaction completed Unknown concentrations of sodium acetate were tested using the same procedure; their concentrations were estimated using the calibration curve generated from the known concentration tests TAD supernatant samples were tested to derive CO2 monitoring information, and this was compared with the known NaAc calibration curve, to estimate their VFA content Due to the variance of sludge characteristics and activity, the comparison was made only on the basis of tests using the same batch of sludge sample Acetate and VFAs concentrations were verified using a Hewlett-Packard® 5880A gas chromatograph, equipped with a flame ionization detector (FID)
Figure 1 Experiment setup of CO 2 headspace monitoring
Spike and sampling
ORP pH Temp.
Data logger
CO 2 sensor
KOH
Nitrogen
gas
V ent Sampling
Gauge
Internal circulation P
Data logger
Trang 3Figure 2 Carbon dioxide sensor calibration with air samples
TAD operation
A pilot-scale, single-stage TAD (75L) equipped with a Turborator® aerator (Turborator® Technologies Inc.) was operated to produce digested sludge for tests TAD operations in this study were deliberately maintained at a microaerated condition (typically the ORP below –300 mV) to accumulate VFAs (Chu, et al., 1996) Temperature was maintained within the range of 50
to 60 ºC and volatile solid destruction averaged about 30% at 7 days of HRT Digested sludge was centrifuged for 10 minutes at 3,000 rpm and supernatant was withdrawn for tests VFAs concentration in supernatant averaged about 490 (100-1,230) mg/L as HAc
RESULTS AND DISCUSSIONS
Figure 3 shows a typical CO2/pH profile of sodium acetate addition in the CO2 profile; the rising time between the left foot of the slope and right edge of the peak was defined as the “E Time” (elapsing time) Chemical tracing studies demonstrated that the CO2 change was highly reflective of VFA utilization upon the spiking and depletion in solution Results indicated that the CO2 changes accompanied to the typical enhanced biological P release reaction The pH profile showed a mirror image to the CO2 and decreased (less than 0.01/minute in rate) after the addition; this implied that the pH change was due to the biological reaction A 14
C tracing study suggested that the CO2 monitoring was not practical in a biological phosphorus release reaction, because of insignificant CO2 changes (Bordacs and Chiesa, 1989) However, in comparison with pH-buffered tests in this study, it was confirmed that the pH change in the reaction helped to result in distinguishing overall CO2 change
The “E Times” of different acetate concentration additions are shown in Figure 4 There was a high linear correlation between the initial acetate concentrations and determined “E Times” Results suggested that the unknown concentration could be estimated by interpolation Unknown sodium acetate concentrations were estimated using this linear correlation and their verification (by gas chromatograph analysis) are shown in Table 1 The estimated error was less than 2 %, in four out of five tests At lower concentrations, this method appeared to overestimate the concentration slightly Results revealed that the CO2 monitored using this approach and experimental design was able to estimate the initial acetate concentration in the reactor
CO2 verify-1 (n=16)
y = 175.54x
R 2 = 0.9998
0 200 400 600 800 1000 1200 1400
Reading (V)
Trang 4Figure 3 CO 2 and pH profiles of NaAc addition
Table 1: Acetate concentration estimation and analytical verification
Sample
#
E Times (minutes)
Estimated conc
(mg/L as HAc)
Analytical conc
(mg/L as HAc)
Error in % *
*Error estimation in percentage: (estimated conc – analytical conc.)/analytical conc ×100
Slight foaming was also observed but in this study, its accumulation was not severe Foaming had to be eliminated during the testing, to prevent the gas been trapped and affecting the
CO2 profiles The carrier gas sparging rate also played a key role in deliver a distinguishable
CO2 profile, and it had to be carefully selected for each specific test condition Occasionally, a short plateau was observed in the CO2 profile; this was probably due to the dynamic equilibrium established in the system A time lag after the acetate spike was consistently observed in every case Transfer mechanisms inside the reactor and the carrier gas flow rate were probably the key factors resulting in this delay However, according to ORP and pH profiles, this time lag seemed
to be consistent and it did not have a significant effect on the determination of the “E Time”
defined in this study
Preliminary experiments showed that the TAD supernatant addition resulted in comparable BNR enhancement, as the sodium acetate addition cases A higher P/VFAs molar ratio, observed in TAD addition case, suggested there were other potential carbon substrate available for P release (Li, Mavinic and Kelly, 1999) TAD supernatant samples were tested using this CO2 monitoring approach, to estimate its VFA concentrations Figure 5 shows a typical comparison of CO2 profile of TAD supernatant and NaAc addition Observed CO2
evolution rates were similar in both cases, and the TAD supernatant VFA estimations are shown
in Table 2 Estimations showed a substantial overestimation, compared with the analytical results using the GC method However, this is explained by the fact that the TAD supernatant contains other potential carbon sources, which could be converted to VFAs or utilized directly in the reactions
J1206-0-CO2
110
120
130
140
150
160
170
180
190
200
210
100 120 140 160 180 200
Tim e elapsed (m in.)
E T im e
J1206-0-pH
7.30 7.35 7.40 7.45 7.50 7.55 7.60 7.65 7.70
100 120 140 160 180 200
Tim e elapsed (m in.)
Trang 5Figure 4: NaAc conc vs the “E Time” Figure 5: Comparison of CO 2 profile of
TAD supernatant and NaAc additions
Table 2: TAD supernatant VFAs estimation based on “E Time” approach
Estimated VFAs Analytical
VFAs
Analytical HAc
Comparison in VFAs
Comparison in HAc J0413-2-1 185 mg/L 169 mg/L 166 mg/L +9.5 % +11.4 % J0413-2-2 199 mg/L 169 mg/L 166 mg/L +17.8 % +19.9 % J0418-3 533 mg/L 507 mg/L 421 mg/L +5.1 % +26.6 % J0515-1 367 mg/L 343 mg/L 343 mg/L +7.0 % +7.0 % J0516-1 448 mg/L 399 mg/L 397 mg/L +12.2 % +12.8 % Average
(S.D.)
+10.3% (5.0%) +15.5% (7.7%)
SUMMARY
Headspace CO2 information derived in this study was found to correspond highly to the VFA utilization and P release in anaerobic conditions This new CO2 monitoring technique showed promise in being able to determine the initial VFA concentration using the “E Time” approach The CO2 change in headspace was detectable with the help of the pH change during the P release reaction This method was also able to estimate the TAD supernatant VFA concentration, or more specifically, the available carbon sources in the supernatant from a thermophilic aerobic digestion process With the sludge directly withdrawn from the system and reacting with the carbon supplements in this batch-based test, results revealed the real state of utilizable carbon substrates involved in the particular BNR reaction It also showed the potential, using the observed CO2 profiles and “E Time” correlations with the carbon source concentrations,
to determine on-line the carbon substrates in TAD samples, as well the BNR process performance
of the P release reaction under anaerobic conditions In a sequencing batch reactor, CO2
J0515-1 and -2
0 50 100 150 200 250 300
Tim e elapsed (m in.)
TAD NaAc
R 2 = 0.9977 n=7 0
5
10
15
20
25
NaAc Conc m g/L as HAc
Trang 6monitoring information could be used to regulate the sequencing time, especially the stage of anaerobic conditions In a continuous process, this semi-on-line CO2 measurement could be
applied to optimize the external carbon source dosing rates
ACKNOWLEDGEMENTS
This research was supported by grants form the National Science and Engineering
Research Council (NSERC) of Canada and the Dayton and Knight Ltd., West Vancouver, BC, Canada The excellent technical support provided by the Environmental Engineering Laboratory and Wastewater Treatment Pilot Plant at the University of British Columbia is acknowledged and appreciated
REFERENCES
Bordacs, K and S C Chiesa (1989), Carbon flow patterns in enhanced biological phosphorus accumulating activated sludge cultures, Water Science and Technology, v21, n1, p387-396 Chu, A, D S Mavinic, W D Ramey, and H G Kelly (1996), A Biological Model Describing Volatile fatty Acid Metabolism in thermophilic Aerobic Digestion of Wastewater Sludge, Water Research, v30, n8, p1759
Li, J Z., D S Mavinic and H G Kelly (1999), Using Thermophilic Aerobic Digested Sludge Supernatant as a Potential Carbon Source in Biological Nutrient Removal System, The 7th IAWQ Asia-Pacific Regional Conference Proceeding Volume I, Taipei, p 289-p295
Spérandio, M and E Paul (1997), Determination of Carbon Dioxide Evolution Rate Using On-Line Gas Analysis During Dynamic Biodegradation Experiments, Biotechnology & Bioengineering, v53, n3, Feb p243-p252