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Article

A Two-Stage Biogas Desulfurization Process Using Cellular Concrete Filtration and an Anoxic Biotrickling Filter

by
Morgane Poser
1,2,
Luis Rodolfo Duarte E. Silva
1,
Pascal Peu
3,
Éric Dumont
2 and
Annabelle Couvert
1,*
1
Ecole Nationale Supérieure de Chimie de Rennes, CNRS, Université Rennes, ISCR—UMR 6226, 35000 Rennes, France
2
IMT Atlantique, CNRS, GEPEA, Nantes Université, UMR 6144, 44000 Nantes, France
3
INRAe, 17, Avenue de Cucillé—CS 64427, 35044 Rennes, France
*
Author to whom correspondence should be addressed.
Energies 2022, 15(10), 3762; https://doi.org/10.3390/en15103762
Submission received: 21 April 2022 / Revised: 17 May 2022 / Accepted: 19 May 2022 / Published: 20 May 2022
(This article belongs to the Special Issue Innovative Biodegradation Processes for Environmental Contaminants Removal)
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Abstract

:
A two-stage desulfurization process including an abiotic filtration using cellular concrete waste (first stage) and an anoxic biotrickling filter filling with an inoculated expanded schist material (second stage) was investigated to remove H2S in mimic biogas with limited O2 amount (ranged from 0.5 to 0.8%). The two-stage process was able to satisfactorily remove H2S for all experimental conditions (RE > 97%; H2S concentration = 1500 mg m−3; total Empty Bed Residence Time (EBRT) = 200 s; removal capacity (RC) = 26 g m−3 h−1). Moreover, at a total EBRT = 360 s (i.e., 180 s for each stage), the H2S loading rate (LR) was almost treated by the bed of cellular concrete alone, indicating that abiotic filtration could be applied to satisfactorily remove H2S contained in the gas. According to the H2S concentration entering the biotrickling filter, the majority end-product was either elemental sulfur (S0) or sulfate (SO42−). Thus, the ability of the abiotic filter to remove a significant part of H2S would avoid the clogging of the biotrickling filter due to the deposit of S0. Consequently, this two-stage desulfurization process is a promising technology for efficient and economical biogas cleaning adapted to biogas containing limited O2 amounts, such as landfill biogas.

1. Introduction

According to the European directives, such as the Directive (EU) 2018/2001, the energy from renewable sources constitutes an important part of the package of measures needed to reduce greenhouse gas emissions and comply with the 2015 Paris Agreement on Climate Change (Union 2030 energy and climate framework). Moreover, the increased use of energy from renewable sources also has a fundamental part to play in promoting the security of energy supply and sustainable energy at affordable prices [1]. The most important renewable energy sources are wind power, solar photovoltaics and biomass energy [2]. Among the biomass energy sources, biogas from anaerobic digestion is largely used both on European and global scales. Depending on its production origin (anaerobic digestion, landfills), methane (CH4) and carbon dioxide (CO2) are the major constituents of biogas. However, trace amounts of other components such as nitrogen (N2), water vapor (H2O), ammonia (NH3), oxygen (O2), hydrogen sulfide (H2S) and other sulfur compounds are also found [3,4]. In order to avoid SO2 formation during biogas combustion, protect combined heat and power and avoid H2S injection in natural gas network, H2S removal is needed. Indeed, H2S is known as a corrosive and hazardous pollutant whose gaseous concentrations in biogas can vary significantly from some ppm to several thousands of ppm [3,5]. According to the fields of biogas utilization, different purification stages are applied to remove unwanted gases and substances [6]. The first stage involves the removal of H2S (<1000 ppmv [7]), which is sufficient for the production of heat and steam in boilers, as well as combustion in cogeneration engines. The second stage of purification includes the removal of CO2. The third stage involves the removal of various components and pollutants (biogas to biomethane) to levels required for the injection into the natural gas grid and uses as a vehicle fuel [8,9,10,11]. The present paper is dedicated to the first stage of biogas purification. H2S can be removed using physical–chemical methods (scrubbing, adsorption processes, etc.) and biotechnological ones [3,4,12,13]. By considering these latter, it was established that biofiltration, mainly biofilters and biotrickling filters, is a mature technology to efficiently remove H2S in the air, whereas biological desulfurization of biogas is currently considered a promising technology [14]. In the air, i.e., in the presence of atmospheric oxygen acting as an electron acceptor, the ability of bioreactors to remove H2S is largely reported in the literature, even under extremely acidic conditions [15]. However, for biogas desulfurization in aerobic conditions, i.e., using atmospheric oxygen from air flow rate additions, significant efforts have to be still placed on developing control strategies to avoid biogas dilution [16]. In the absence of atmospheric oxygen, solutions based on alternative electron acceptors, such as nitrates, exist to biologically remove H2S under anoxic conditions. Consequently, anaerobic biotrickling filtration appears a suitable solution to overcome the main drawbacks of aerobic bioprocesses, i.e., biogas dilution with nitrogen and safety problems due to potential explosive mixtures of oxygen/methane. In both cases, H2S must be first absorbed in the aqueous phase in which sulfide oxidizing bacteria carry out the substrate oxidation. The products of the oxidation are either elemental sulfur (H2S + 0.5O2 → S0 + H2O) or sulfate (H2S + 2O2 → SO42− + 2H+) according to the H2S/electron acceptor ratio. Between the air addition way and the anoxic way, a third way consisting of taking advantage of the possible presence of oxygen in the raw gas also has to be considered since oxygen concentrations up to 1% are reported in landfill gases [3]. The amount of oxygen is usually lower in biogas produced through anaerobic digestion since preventive treatment based on a simple micro-aeration of the digester headspace allows the development of aerobic thiobacteria oxidizing H2S into elemental sulfur S0 [5,7,17]. According to the stoichiometric equations abovementioned, the first product of the H2S oxidation is elemental sulfur S0, which can be converted into sulfate SO42− in the case of excess oxygen amounts (S0 + 1.5O2 + H2O → SO42− + 2H+). It was admitted that the accumulation of S0 in a biotrickling filter leading to bed clogging is the main drawback of these bioreactors [18,19]. As the washing of the filter bed is difficult, and as S0 is insoluble in the recirculating liquid, it is preferable to operate in oxygen excess to oxidize S0 into SO42− [20,21]. Moreover, the literature reports that H2S removal efficiency (RE) depends on the O2/H2S molar ratio. Thus, RE of 95% was obtained for an O2/H2S ratio of 2:1, against 63% and 50% for 1:1 and 1:2 ratios, respectively [22]. As a result, according to the H2S and O2 concentrations characterizing the biogas, efficient desulfurization could be directly achieved in a biotrickling filter without any electron acceptor addition, atmospheric oxygen or nitrates. The objective of this study was consequently to study the feasibility of a biotrickling filter filled with expanded schist as packing material to removed H2S from a biogas with trace amounts of oxygen. Among the materials commonly used in H2S biofiltration (peat, pouzzolane, wood bark, etc.), expanded schist has widely proved to be a good carrier material, showing high removal H2S performances both in aerobic and anoxic conditions, but also good lifetime due to its mechanical resistance and its non-alteration during chemical or biological reactions [15,23,24]. However, as biotrickling filters are sensitive to H2S loading rate changes due to concentration or flow rate fluctuations, a basic filtration using cellular concrete, an inexpensive waste material from construction, was used beforehand to buffer the shock loads and avoid the inhibition of the bacterial community. Indeed, cellular concrete waste was demonstrated to be efficient for partial H2S removal in abiotic conditions, i.e., without any microbial population [25,26]. Chemical reactions involving the components of the cellular concrete (mainly CaO, CaCO3 and Fe2O3) would explain the ability of this material to react with H2S. The H2S removal was therefore investigated using a two-stage desulfurization process for different operating conditions of H2S concentrations and Empty Bed Residence Time (EBRT).

2. Materials and Methods

2.1. Materials

Both of the materials, expanded schist and cellular concrete waste, were described in previous studies [25,26]. Expanded schist is an inorganic material provided by the Granulex company (France), and cellular concrete waste, called “copolight”, is a mineral material provided by the Florentaise company (France). Properties and pictures of both materials are given in Table 1 and Figure 1, respectively. The ability of biotrickling filters filled with expanded schist to remove H2S was demonstrated in aerobic and anoxic conditions, as well as under extremely acidic conditions in relation to the production of large amounts of SO42− [15]. Maximum removal capacity RCmax of 30.3 g m−3 h−1 was recorded for H2S concentrations up to 1100 ppmv (EBRT of 300 s) [23]. Moreover, compared with other biofiltration materials, the good mechanical stability of the expanded schist observed over time is a great advantage in avoiding technical maintenance. As no bed compaction was observed during long-running periods, bed pressure drops are limited to some Pa per meter of material [15].
The ability of cellular concrete waste to react with H2S in air and in abiotic conditions was recently highlighted [26]. It was reported that in wet conditions, reactions occurring between H2S and calcium carbonate lead to gypsum formation (CaSO4·2H2O). This abiotic H2S filtration could thus be beneficially used as a first step of biofiltration systems, e.g., to soften the change in H2S loading rate. To date, cellular concrete waste has not yet been studied for H2S biogas filtration.

2.2. Experimental Setup

The experimental setup is described in Figure 2. The pilot plant consisted of 2 PVC cylindrical columns (internal diameter of 100 mm) filled with 7.8 L of material (1 m in height). The “abiotic filter” was filled with cellular concrete waste (Figure 1), and the “biotrickling filter” was filled with expanded schist inoculated with 4 L of activated sludge from a wastewater treatment plant (Procanar, Lauzach, France). Prior to inoculation, sludge was not H2S acclimatized. For safety reasons, mimic biogas was used, and CH4 was replaced by N2. The use of mimic biogas without CH4 and CO2 was successfully considered in several studies, with the presence or absence of methane having no effect on the microorganisms using H2S as substrate [22]. A nitrogen generator BrezzaNiGen LC–MS (40-1) (purity up to 99.9%) from Gengaz Company (Wasquehal, France) was used to supply N2 continuously into the columns. In spite of the ability of the generator to efficiently purify N2 from the air, a weak fraction of oxygen ranging from 0.5 to 0.8% was always measured in the nitrogen gas. The N2 flow rate entering the two-stages process was controlled and measured by a mass flowmeter (Model 58500, Brooks Instruments, Hatfield, MA, USA). A stream of H2S (99.7% purity) controlled by another mass flow meter (Model 5850S, Brooks Instruments, Hatfield, PA, USA) was mixed with the N2 flow rate before entering the abiotic filter. As a result, the gas entering the two-stage process was a mixture of N2-H2S-O2 mimicking raw biogas. Thermocouples (K type) were installed on each column to measure temperatures. In order to maintain optimal bed humidity, both columns were fed with tap water. For the abiotic filter, cellular concrete waste was humidified by a drop-by-drop system. For the biotrickling filter, expanded schist was sprinkled (water flow rate of 60 mL min−1) by water recirculating in the column. The water was discharged once a week to prevent its electrical conductivity from exceeding 10 mS cm−1. As a result, all experiments were carried out in wet conditions controlled by humidity sensors (Model EE08, E + E Electronik, Sevres, France) located at the top of columns. Relative humidity measurements of the gas at the outlet of the first stage were always higher than 94%. H2S and O2 concentrations were measured by an electrochemical analyzer (Biogas 5000, QED Environmental Systems Ltd., Coventry, UK) along all the columns, which were equipped with 6 sampling ports located at 0, 20, 40, 60, 80 and 100 cm from the bottom. These sampling ports were also used to measure the pressure drops (pressure sensor Setra, Setra Systems, Inc, Boxborough, MA, USA; 0–700 Pa). No nutritive solution was added to the tap water for the inoculated biotrickling filter. Indeed, it was assumed that the minerals contained in the tap water would be sufficient for the growth of autotrophic biomass.
The biotrickling filter washing liquid parameters, such as (i) temperature, (ii) pH and (iii) electrical conductivity, were measured daily using a multi-channel analyzer consort C834 (Consort bvba, Turnhout, Belgium) with temperature correction. The sulfate concentration was measured daily using a High-Pressure Ion Chromatography (940 Professional IC Vario, Metrohm, detection by conductivity, eluent: 3.2 mM Na2CO3 + 1 mM NaHCO3, column: metrosep A supp 5 150/4.0). For this study, no specific measurement were made on the abiotic filter washing liquid.
The cellular concrete composition over time (at days 0 and 43) was determined using an Energy Dispersive X-ray Fluorescence Spectrometer (EDX-800HS, Shimadzu Company, Kyoto, Japan).

2.3. Operating Parameters

The parameters used to determine the performance of the two-stage process are detailed in Table 2. Two parameters influencing the H2S loading rate were studied during the 68 days of operation: (i) the influence of pollutant concentration change at a constant EBRT; (ii) the influence of the change in EBRT for a given H2S concentration. The H2S concentrations selected for the study (up to 1500 mg m−3) were chosen according to the concentrations usually encountered in raw biogas. The operating conditions of the study are summarized in Table 3. Temperatures of gas and materials were measured, not controlled. For the running period, recorded temperatures ranged from 17 to 27 °C according to the climatic conditions (June to August 2021). Before the beginning of this measurement campaign (June 2021), the two-stage process was operated continuously for several months in order to fix the different problems encountered. Consequently, it can be considered that the biomass inoculating the biotrickling filter was H2S acclimatized.

2.4. Analysis of Microbial Community

Biofilm samples were taken on day 0 (after acclimatization) and after 55 days in operation. They were centrifuged at 3000× g for 10 min, the supernatant was removed, and the pellet was stored at −20 °C until DNA extraction.
DNA was extracted from 200 mg of pellet using the Macherey Nagel NucleoSpin Soil kit according to the manufacturer’s instructions. The extracted DNA was eluted in 100 µL of sterile water and stored at −20 °C for further analysis. Microbial community dynamics were investigated by high throughput DNA sequencing using Ion Torrent Personal Genome Machine methods and technologies (ThermoFisher Scientific, MA, USA) as described in Madigou et al. [27] with a few adaptations. The analysis targeted the V4-V5 hypervariable regions of the bacterial and archaeal 16S rRNA genes using PCR amplification (Platinium SuperFi PCR protocol from Life Technologies) and fusion primers 515F (5′-Ion A adapter–Barcode–GTGYCAGCMGCCGCGGTA-3′) and 928R (5′-Ion trP1 adapter–CCCCGYCAATTCMTTTRAGT-3′) [28], which includes a barcode and sequencing adapters. The resulting amplicons were purified and quantified according to the manufacturer’s instructions using, respectively, the Agencourt AMPure XP magnetic beads (Beckman Coulter, Lane Cove West, NSW, Australia), DNA 1000 kit and 2100 Bioanalyzer (Agilent Technologies, Les Ulis, France). Template preparation for emulsion PCR and subsequent sequencing were performed using the Ion PGM Hi-Q View OT2 Kit and Ion PGM Hi-Q View Sequencing kit (Life Technologies, West Sacramento, CA, USA) as described in [27]. The high-throughput DNA sequencing produced an average of 3369/10071 +/− 2291 sequence reads of about 380 base pairs length for each sample.
These sequences were processed with the FROGS pipeline [29], following the authors’ recommendations on the MIGALE Galaxy instance (INRAE, Jouy-en-Josas, France). Operational Taxonomic Unit (OTUs) abundance and microbial community diversity indices calculations were performed using Easy16S (https://shiny.migale.inrae.fr/app/easy16S (accessed on 7 April 2022)), a shiny web interface based on the phyloseq R package [30].

3. Results and Discussion

Results of the two-stage process are reported in Figure 3. The two-stage process was able to satisfactorily remove H2S (RE > 97%) for all experimental conditions. Basically, the measured H2S outlet concentration was never higher than 14 mg m−3. At EBRT = 360 s, H2S removal was mainly achieved by the abiotic filter, whereas at lower EBRT, most of the removal was performed by the biotrickling filter. Figure 4a shows that the removal capacity (RC) was always close to the loading rate (LR) for the two-stage process, in agreement with the high RE value. Therefore, it can be concluded that a total EBRT of 200 s is sufficient for the complete H2S removal. Moreover, it can be argued that lower EBRT would make it possible to efficiently treat H2S concentrations higher than 1500 mg m−3. It is interesting to note that RC of 26 g m−3 h−1 was achieved by the abiotic filter alone at EBRT of 180 s (Figure 4b). In this case, RE ranged from 75 to 100%. These results are significantly higher than those reported in air by Lebrun et al. [26] (RC = 7.8 g m−3 h−1 at EBRT of 56 s, C G in = 70 mg m−3) and Ben Jaber et al. [25] (RC = 5.6 g m−3 h−1 at EBRT of 63 s, C G in = 140 mg m−3). Indeed, in these previous studies, the humidity of the material was not controlled, and consequently, recorded performances were not optimized. It can thus be concluded that an efficient H2S filtration through only a bed of cellular concrete waste is possible at moderate H2S concentrations. In other words, this abiotic H2S filtration could be used instead of biofiltration for many H2S gas treatment applications with equal performance. For LR > 30 g m−3 h−1, the removal efficiency dropped to values lower than 50% in relation to the decrease in EBRT (Figure 4b). Consequently, it can be suggested that EBRT seems to be the main parameter governing H2S removal in the abiotic filter, rather than H2S concentration. However, investigations must be continued to refine the parameters influencing H2S removal.
By considering results achieved in the biotrickling filter alone during the first 37 days of operation (Figure 5), the H2S inlet concentration was lower than 200 mg m−3 because part of H2S was previously removed by the cellular concrete filter. As a result, the loading rate to be treated was limited to 5 g m−3 h−1. However, for days 37 to 68, corresponding to a decrease in the total EBRT, the H2S inlet concentration reached up to 1000 mg m−3, and consequently, LR increased to 35 g m−3 h−1. As observed in Figure 5, the removal capacity was always close to LR, confirming the ability of the biotrickling filter to remove H2S. In terms of RE and RC values, these results are in the same order of magnitude as those reported in the recent literature dedicated to the anoxic removal of H2S using conventional biotrickling filters [31,32,33,34]. Bearing in mind that the maximal RC of the two-stage process was not reached, these results can be compared with those obtained by means of others technologies. For instance, using an anoxic bioscrubber (absorption column + stirred tank), Quijano et al. [35] reported a maximum RC of 35.7 ± 2.0 g m−3 h−1 (RE from 92 to 99%). Using a 3D-printed honeycomb monolith as a biotrickling filter, Qiu and Deshusses [22] obtained for the first time an RC of 122 g m−3 h−1 (RE 95%). However, after the cleaning procedure, the performance of the system decreases significantly (RC = 63 g m−3 h−1 and RE = 49%) to reach some values close to RC obtained in this study. Anoxic desulfurization was also performed by González-Cortés et al. in a 3 L inner loop jacketed gas-lift bioreactor fed with mimic biogas (N2 + H2S) and nitrogen species (NO2, NO3) as the electron acceptor [36]. A maximum RC of 141.18 g m−3 h−1 (RE = 95.0%) was achieved. However, these authors indicated that the high operating costs of this technology, due to the high requirements of nitrite or nitrate, make its full-scale application difficult. Thus, the major difference between the results of the present study and the literature data lies in the fact that H2S removal under anoxic conditions was obtained without any addition of electron acceptors such as nitrates or nitrites. Thus, it can be reasonably suggested that the amount of oxygen present in the mimic biogas is sufficient for H2S oxidation (it is unlikely that oxygen comes from reactions occurring between H2S and the cellular concrete during the abiotic filtration [26]). EBRT applied in the biotrickling filter was high enough to provide both the mass transfer of H2S and oxygen from the gas phase to the liquid phase and the H2S biodegradation by microorganisms, as revealed by high RE values. However, the oxygen availability in relation to the H2S concentration to be treated determines the degradation products (S0 or SO42−). Elemental sulfur S0, the first product of the H2S degradation, is transformed into SO42− if O2 is in excess. The oxygen fraction in the mimic biogas entering the biotrickling filter ranged from 0.5 to 0.8%, i.e., from 5000 to 8000 ppm. According to the H2S concentration entering the biotrickling filter, it can then be argued that the O2/H2S ratio value was around 50–100 at the bottom for low H2S concentrations (some ppm) and close to 5–10 for high concentrations (some hundreds of ppm). As O2 is progressively consumed along all the biotrickling filter, values lower than five can be reasonably assumed at the outlet, especially as oxygen is 80 times less soluble in water than H2S [31]. According to the literature, half of H2S degraded is converted into S0 for an O2/H2S ratio of 6 [21], and complete H2S oxidation to SO42− is achieved for an O2/H2S ratio of 23.6 [37]. The sulfate production, expressed as the ratio (S–SO42− accumulated in the leachate/S–H2S removed from the biogas) as a function of the H2S concentration entering the biotrickling filter is displayed in Figure 6. As observed, SO42− production decreased with the increase in the H2S concentrations and the removal capacity, in agreement with the literature data. SO42− production, ranged between 70% and 100% for H2S concentrations lower than 100 mg m−3 (corresponding to RC lower than 2 g m−3 h−1), tended to a plateau of around 25–30% for H2S concentrations reaching 1000 mg m−3 (RC tending toward 40 g m−3 h−1). In parallel of these findings, it can be added that the concentration of sulfate in the leachate, measured from ion chromatography, can also be deduced from the measurement of the electrical conductivity of water, on the basis that SO42− is the majority ionic species in water since other sulfur ionic species, which could derive from H2S oxidation, such as sulfide (S2), sulfite (SO32−) and thiosulfate (S2O32−), are insignificant in water. Indeed, Qiu and Deshusses [22] measured that sulfide produced by H2S oxidation was less than 1% of the total species detected in the liquid. Moreover, formation of thiosulfate (S2O32−) is unfavorable at pH lower than 8 [38]. Thus, in acidic conditions (pH = 1.8), Rodriguez et al. [21] observed that the presence of sulfite and thiosulfate was below the detection limit of the analyzer. In the present study, the pH value ranged between 1.5 and 3 during the operating conditions. As a result, it can be claimed that the change in the electrical conductivity of water was due to change in the sulfate concentration in water (SO42−(gS/L) = 0.058 × electrical conductivity(mS/cm); R2 = 0.98; not shown). Note that a part of leachate was periodically removed and replaced by fresh water in order to keep the pH higher than 1.5; such a condition avoiding a performance decay. Acidic conditions also influenced the microbial communities in the biotrickling filter. Figure 7 exhibits genus level NGS (next-generation sequencing) analysis results for microbial diversity in the biofilm harvested at the surface of the expanded schist sampled in the middle of the biotrickling filter. After the acclimatization period, Illumina Miseq sequencing revealed that the microbial community at the beginning of experiment (day 0) contained high abundance of H2S-affinity genera including mainly Alicyclobacillus, Thionomas, Acidithiobacillus and Metallibacterium. The total proportion of these four genera exceeded 95%, which indicated a microbial community with low diversity, but high enrichment of functional bacteria proving that the activated sludge used to inoculate the biotrickling filter was well H2S acclimatized. All these OTUs are involved in the sulfur cycle and were previously described in acid mining environments as sulfur-oxidizing bacteria [39]. Amongst the most common genera are acidophiles which exhibit mesophilic growth optima. These bacteria possess chemolithotrophic metabolism, by which they are able to use sulfur under oxic conditions. Therefore, high H2S concentrations and low pH helped shape a microbial community well adapted to H2S degradation, as reported in the literature [40,41]. After 55 days in operation under severe acidic conditions (pH 1.5–3), the microbial diversity was simplified to extremophile Acidithiobacillus spp. and Metallibacterium spp., with Acidithiobacillus being the most abundant bacterial group (95%), confirming that this genus dominates for this range of acidic pH [42]. These two genera are acidophile bacteria with optimal growth at pH 2–3 and autotrophic metabolism.
Pictures of the two packing materials extracted from columns at the end of the experiment are displayed in Figure 8. The yellow color suggests a sulfur deposit, which was confirmed by the analysis of cellular concrete composition over time. For this material, the mass percentage of sulfur was 6.8% at the beginning of the study and increased progressively to reach 15.4% on day 43. For the biotrickling filter, a sulfur deposit was clearly observed on the material pieces extracted at the bottom of the bed (Figure 8b), whereas the material pieces extracted at the top were cleaner. This finding is consistent with the explanation given above for Figure 6 concerning the predominant S0 production at high loading rates due to high H2S inlet concentration. Despite the sulfur deposits, no clogging was observed on both bed materials, as illustrated by the measurement of pressure drops. Thus, at the end of the experiment, pressure drops were below 20 Pa m−1 for the biotrickling filter and below 30 Pa m−1 for the abiotic filter, respectively. These results are in agreement with those reported by Ben Jaber et al. [25] and Lebrun et al. [26], where pressure drops were less than 40 Pa m−1 and around 12 Pa m−1, respectively.
Moreover, given that the sulfate production by the biotrickling filter mainly depends on the H2S concentration at the inlet of the column, i.e., at the outlet of the abiotic filter filled with cellular concrete, it is possible to consider that the ability of the abiotic filter to remove a significant part of H2S would allow reducing the clogging of the biotrickling filter. Indeed, Rodriguez et al. [21] demonstrated that it is possible to partially remove the deposited S0 by bio-oxidation (40.3%) when the biotrickling filter is not fed by biogas. In other words, the expanded schist filling the biotrickling filter could be partially cleaned, thus regenerated, during phases when the abiotic filter would be highly effective, depending on the fluctuations of the H2S loading rate of the two-stage process.
EBRT is one of the critical parameters for the mass transfer of H2S required for high removal efficiency. The objective is always to find a good compromise between short EBRT in order to limit the size of the equipment and high RE. At a total EBRT of 200 s (100 s for each stage), the present study demonstrated that the two-stage process was efficient in treating H2S concentration of 1500 mg m−3 (RE > 97%; Figure 3). Consequently, future works will be performed to reduce the total EBRT. However, for these operating conditions, Figure 3 reveals that the part of H2S removed by the abiotic filtration stage was around 30%. Considering the ability of the cellular concrete to react with H2S, it could be emphasized to adapt the EBRT of the first stage in order to reduce the EBRT of the second stage. Indeed, the design of the two stages is significantly different since the first one is based on chemical reactions, whereas the second one is based on biological reactions. Thus, the first stage could be designed as a compact horizontal mode system allowing to easily adjust the EBRT to operating changes, while the second stage would be designed as a more classical biofiltration system governed by a given EBRT value imposed by the height of expanded schist filling the system.
The two-stage process could be an interesting way to overcome current difficulties with typical desulfurization bioprocesses of landfill gas. Bioprocesses such as BTF are simple, environmentally benign, cost-effective and ease scalability [4], but some issues can be encountered, such as (i) handling bacteria during high inlet H2S concentration or stops, (ii) controlling the chemicals nutrients feeding and (iii) avoiding the premature clogging due to sulfur accumulation. Therefore, the cellular concrete as a first-stage abiotic filter could be a solution to protect the biotrickling filter from H2S shock loads and reduce the premature clogging risk of the second-stage BTF concomitantly. Moreover, as expanded schist has widely proved to be a good carrier material with a long lifetime due to its mechanical resistance during biological reactions, the management of the BTF is limited, and the possible handling of the saturated or degraded media will be avoided. Admittedly, the cellular concrete should be changed periodically, but the management of the first abiotic stage is largely easier than the BTF management. Currently, this two-stage desulfurization process allows reaching the maximal H2S concentration for numerous applications, i.e., fuel cells, heating and Stirling engines, internal combustion engine, turbines and microturbines [3]. Moreover, the process probably reduces the amount of oxygen in the biogas. Consequently, it can be considered an alternative to biogas purification based on activated carbon. Pragmatically, the process should be tested in situ on real biogas to assess the efficiency of the process, to evaluate its ability to remove other elements such as NH3 and CO2, and to carry out an economic study.

4. Conclusions

It was demonstrated that a two-stage desulfurization process including an abiotic filtration using cellular concrete waste and an anoxic biotrickling filter using an inoculated expanded schist material is efficient in removing H2S in mimic biogas without any addition of electron acceptors such as nitrite or nitrate (RE > 97%; H2S concentration = 1500 mg m−3). Bio-oxidation of H2S is achieved provided that the biogas to be treated contains a small fraction of oxygen (up to 0.8% in the present study). The drop in pH in the biotrickling filter (1.5–3) simplified the microbial diversity mainly to extremophile Acidithiobacillus spp. At EBRT = 200 s, the removal capacity of the two-stage process was 26 g m−3 h−1, and consequently, it appears as a promising technology for efficient and economical biogas cleaning adapted to biogas containing limited O2 amounts, such as landfill biogas. Moreover, at H2S concentrations up to 1200 mg m−3 and longer EBRT (180 s for the first stage only), the abiotic H2S filtration alone using cellular concrete waste was shown to be equally efficient. Therefore, this abiotic filtration could be used instead of biofiltration for many H2S gas treatment applications (not limited to biogas) in aerobic or anoxic conditions.
This promising two-stage desulfurization process has to be now investigated in situ in real conditions for the treatment of real biogas containing CH4, CO2, NH3, O2 and H2S. Only the use in real conditions will allow studying the influence of EBRT and H2S concentration, the main operating parameters.

Author Contributions

Conceptualization, É.D. and A.C.; methodology, É.D. and M.P.; software, M.P. and L.R.D.E.S.; validation, É.D., A.C., P.P. and M.P.; formal analysis, M.P. and L.R.D.E.S.; investigation, M.P. and L.R.D.E.S.; data curation, M.P. and L.R.D.E.S.; writing—original draft preparation, É.D. and M.P.; writing—review and editing, É.D., A.C., P.P. and M.P.; supervision, É.D., A.C. and P.P.; project administration, A.C.; funding acquisition, A.C. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by the French governmental agency ADEME (N°TEZ19-041) and the Region of Brittany (N°1169).

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

Data are contained within the article.

Acknowledgments

To the Département Systèmes Energétiques et Environnement of IMT Atlantique (Nantes, France) and also special thanks to Yvan Gouriou for his continuous support in process management.

Conflicts of Interest

The authors declare no conflict of interest.

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Figure 1. Materials used in this study; (a) cellular concrete waste; (b) expanded schist.
Figure 1. Materials used in this study; (a) cellular concrete waste; (b) expanded schist.
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Figure 2. Experimental setup; (a) flow sheet; (b) picture of experimental columns (left: first stage, abiotic filter; right: second stage, biotrickling filter).
Figure 2. Experimental setup; (a) flow sheet; (b) picture of experimental columns (left: first stage, abiotic filter; right: second stage, biotrickling filter).
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Figure 3. H2S removal efficiency of the two-stage process.
Figure 3. H2S removal efficiency of the two-stage process.
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Figure 4. RC vs. LR: (a) two-stage process (LR and RC calculated using both the abiotic filter bed and the biotrickling filter bed); (b) abiotic filter only (EBRT, LR and RC calculated using the abiotic filter bed volume only).
Figure 4. RC vs. LR: (a) two-stage process (LR and RC calculated using both the abiotic filter bed and the biotrickling filter bed); (b) abiotic filter only (EBRT, LR and RC calculated using the abiotic filter bed volume only).
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Figure 5. Loading rate (LR) and removal capacity (RC) of the biotrickling filter alone at different EBRT and H2S inlet concentrations.
Figure 5. Loading rate (LR) and removal capacity (RC) of the biotrickling filter alone at different EBRT and H2S inlet concentrations.
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Figure 6. Biotrickling filter results: sulfate production and removal capacity according to the H2S concentration at the inlet of the second stage.
Figure 6. Biotrickling filter results: sulfate production and removal capacity according to the H2S concentration at the inlet of the second stage.
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Figure 7. Genus level NGS analysis results for microbial diversity in biotrickling filter using the prokaryotic universal primer. The bar charts show taxonomic profiles obtained at the beginning of experiment (day 0) and after 55 days in operation.
Figure 7. Genus level NGS analysis results for microbial diversity in biotrickling filter using the prokaryotic universal primer. The bar charts show taxonomic profiles obtained at the beginning of experiment (day 0) and after 55 days in operation.
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Figure 8. Change in aspect of both packing materials over time; (a) Cellular concrete waste (left to right: blank material, extracted from the top of the abiotic filter, extracted from the bottom); (b) expanded schist (left to right: blank material, extracted from the bottom of the biotrickling filter, extracted from the top).
Figure 8. Change in aspect of both packing materials over time; (a) Cellular concrete waste (left to right: blank material, extracted from the top of the abiotic filter, extracted from the bottom); (b) expanded schist (left to right: blank material, extracted from the bottom of the biotrickling filter, extracted from the top).
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Table
Table 1. Physico-chemical properties and composition of materials (Adapted with permission from Refs. [23,25]).
Table 1. Physico-chemical properties and composition of materials (Adapted with permission from Refs. [23,25]).
PropertiesCellular Concrete WasteExpanded Schist
Density (kg m−3)547 ± 51248 ± 12
Porosity (%)6447
pH of surface9.0 ± 0.17.0 ± 0.1
Composition (weight %)
SiO250.556.4
Fe2O31.312.4
Al2O32.220.5
CaO24.60.9
K2O0.25
SO319.71.6
TiO2(nd)(nd)
P2O51.412.4
Table
Table 2. Parameters used in this study.
Table 2. Parameters used in this study.
ParameterDefinitionNomenclature
Loading Rate LR (g m−3 h−1) Q   V   C G in C G in : Inlet concentration (g m−3)
Removal Capacity RC (g m−3 h−1) Q V   ( C G in C G out ) C G out : Outlet concentration (g m−3)
Empty Bed Residence Time EBRT (s) V Q Q: Gas flow rate (m3 s−1)
Removal Efficiency RE (%) 100   C G in C G out C G in V: Packing bed volume (m3)
Table
Table 3. Operating conditions.
Table 3. Operating conditions.
Duration (Day)Inlet H2S Concentration (mg m−3)Abiotic Filter EBRT (s)Biotrickling Filter EBRT (s)Total
EBRT (s)		Loading Rate
LR (g m−3 h−1)
83501801803603.5
85005.0
89009.0
6120012.0
8150014.5
11150015015030018.0
1012012024022.5
1010010020027.0
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Poser, M.; Silva, L.R.D.E.; Peu, P.; Dumont, É.; Couvert, A. A Two-Stage Biogas Desulfurization Process Using Cellular Concrete Filtration and an Anoxic Biotrickling Filter. Energies 2022, 15, 3762. https://doi.org/10.3390/en15103762

AMA Style

Poser M, Silva LRDE, Peu P, Dumont É, Couvert A. A Two-Stage Biogas Desulfurization Process Using Cellular Concrete Filtration and an Anoxic Biotrickling Filter. Energies. 2022; 15(10):3762. https://doi.org/10.3390/en15103762

Chicago/Turabian Style

Poser, Morgane, Luis Rodolfo Duarte E. Silva, Pascal Peu, Éric Dumont, and Annabelle Couvert. 2022. "A Two-Stage Biogas Desulfurization Process Using Cellular Concrete Filtration and an Anoxic Biotrickling Filter" Energies 15, no. 10: 3762. https://doi.org/10.3390/en15103762

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