Introduction

There has been growing interest in control of the emission of volatile organic compounds (VOCs) because of their potential to harm the environment and human health toxicity (Zheng et al. 2013). Recently, waste gases emitted in high volume containing complex VOCs at low concentration have hindered performance enhancement of related treatments (Cheng et al. 2016). This has led to increased interest in biofiltration systems, which have advantages of high efficiency, minimal secondary pollution and low costs (Khan and Ghoshal 2000).

Microorganisms play an important role in biodegradation, having direct interactions with contaminants. In previous studies, significant shifts in the bacterial community were observed during biodegradation, especially in the initial period (Qiu et al. 2013). Increasing doses also impact microbial communities (Li et al. 2017). Efforts were also paid on microbial community structures analysis to determine microbial indicators of contaminants (Obi et al. 2017). Evaluation of the influence of different degrading conditions on microbial communities also revealed significant effects (Techtmann et al. 2017). However, it is worth noting that previous studies were predominantly conducted using simple and stable inlet chemicals, while few investigations have focused on microbial changes with contaminant shifts.

Various VOCs have physical and chemical characteristics that differ significantly. Water-solubility and biodegradability are the two main factors that influence the removal efficiency of biofilters (Deshusses and Webster 2000). Low water-solubility limits mass transfer prior degradation (Alonso et al. 1998), while biodegradability influences the degradation of soluble VOCs. Among all pollutants, hydrocarbons (i.e., alcohols, ketones, esters etc.) have been shown to be the easiest degraded compounds, before alkene and aromatic hydrocarbon (Delhomenie and Heitz 2005). Therefore, different types of VOCs alter biofilter performances and microbial community structures significantly. However, precise analyses and conclusive studies are not yet available, especially for waste air treatments.

Few studies have investigated the interactions between environments and microorganisms (Zhang et al. 2018); therefore, the present study was conducted to elucidate these interactions. Specifically, this study investigated a biofilter applied to treat a variety of volatile organic compounds (toluene, ethylbenzene, chlorobenzene, acetone, isopropyl alcohol, ethyl acetate, n-hexane and tetrahydrofuran) in sequence. Differences in degrading performance and the changes in microbial structures during the process were then evaluated. The data obtained in this study will provide insight into microbial community function, functional diversity, and other aspects of the biofilter operation.

Materials and methods

Biofilter configuration and operation

Biofilter set up

The system had a height of 335 mm and an internal diameter of 118, giving an effective height of packing material of 150 mm with an approximately 1.7 L volume (Additional file 1: Figure S1). The air flow was pressurized and controlled with an electromagnetic air compressor (ACO-318, Hailea Co., Ltd., Guangdong, China) and a flowmeter (LZB-WB, Zhenxing Flowmeter Factory, China). Pressurized airflow entered the mixing chamber, which contained multiple vials of evaporating VOCs. The quantity of the vials, volume and volatile area of the VOCs was used to control the inlet concentration. Mixed air flow then entered the biofilter from the bottom and passed through the packing materials containing the microorganisms, after which the treated air was discharged from the top of the biofilter. An electromagnetic flowmeter (Iwaki Co., Ltd, EH-B20VC-220R1) was used to control the liquid flow rate and a microcomputer time controlled switch (Toone Co., Ltd., Shanghai, China) was used to control the spraying rate.

Eight common volatile organic compounds were selected in this study for biofilter performances and microbial community analyses. The selected compounds, including aromatic and non-aromatic hydrocarbons, were common industrial materials or organic solvents (Additional file 1: Table S1). Different VOCs were applied one by one in the order toluene, ethylbenzene, chlorobenzene, acetone, isopropyl alcohol, ethyl acetate, n-hexane and tetrahydrofuran. The duration of operation for each compound ranged from 12 to 17 days, depending on the time spent to reach a stable state.

Biofilter operation

The inlet air flow rate was 2.2 L min−1 with an empty bed residence time of 46 s. Spraying was conducted for 1 min every 3 h, giving a total sprayed volume of 90 mL. The nutrient medium was renewed every 3–4 days, the pH of the medium was controlled at 6.5–7.2, and temperature ranged from 25 to 32 °C.

Nutrient medium and inoculation

The nutrient medium used consisted of 10 g NaNO3, 2.56 g Na2HPO3 and 1.66 g KH2PO3 per L water, and the pH values ranged from 6.5 to 7.2. The medium was inoculated with suspended activated sludge, and 1.7 L packing materials were filled into the biofilter after being soaked in 1 L of the activated sludge suspension for an hour.

Analytical methods

VOCs, CO2 and biomass concentration

The concentrations of the chemicals were analyzed by gas chromatography (GC-14C, Shimadzu Co. Ltd., Shanghai, China). The temperatures of the inlet, column (HICRON HP-1, 50 m × 0.25 mm) and detector were 150 °C, 100 °C and 150 °C, respectively.

The concentration of CO2 was tested using a portable CO2 m (Testo 535, Testo China Co. Ltd., China), while decreases in pressure were analyzed with a manometer (Testo 512, Testo China Co. Ltd., China).

Biomass in different periods was tested 2 h after spraying to minimize the influence of sprayed nutrient medium. The growth of biomass was compared among treatments to evaluate increases in microorganisms.

DNA extraction

DNA extraction was performed during the stable phase using a Fast DNA™ SPIN Kit for Soil (MP Biomedicals, Canada), after which the extracted DNA was sequenced using the Illumina MiSeq sequencing platform (Novogene Co., Beijing, China) and the 515F (5′-GTGCCAGCAGCCGCGGTAA-3′) and 806R (5′-GGACTACCAGGGTATCTAAT-3′) targeting the V4 region of the 16S rRNA gene. Each reverse primer contained a 6-bp error-correcting unique barcode and PCR amplification was conducted by subjecting the samples to 98 °C for 5 min, followed by 40 cycles of 94 °C for 30 s, 55 °C for 30 s and 72 °C for 45 s, and then final extension at 72 °C for 10 min. Sequences were then analyzed using the Illumina MiSeq platform (Novogene Co., Beijing, China).

DNA sequencing

Illumina MiSeq original DNA sequence data were processed and analyzed by Qiime (http://qiime.org/) and UPARSE (http://drive5.com/uparse/). Paired-end reads from the original DNA fragments were combined using FLASH18. All sequences were aligned with the SILVA bacterial 16S rRNA database. Sequences were clustered into operational taxonomic units (OTUs) at a cutoff of 97% sequence identity, after which the unweighted UniFrac in principal coordinate analysis (PCoA) was determined by Qiime. Some indices (rarefaction curves, Chao, Simpson, Shannon, coverage) were calculated to reveal Alpha diversity using mothur v.1.32. (http://www.mothur.org).

The Illumina MiSeq sequencing raw data have been deposited in the NCBI Sequence Read Archive database, and the SRA accession is SRP148831.

Biolog test

BIOLOG ECO Plates and high-throughput sequencing were used in this study to monitor microbial communities. High-throughput sequencing has helped investigators identify changes in the microbial structure and diversity (Alpana et al. 2017).

BIOLOG Eco-plates were used to investigate Sole-Carbon-Source Utilization (SCSU) of different microbial communities. Each plate contained a total of 31 carbon sources in triplicate. The suspension samples required a 5-min resting after they were obtained from the biofilter. Then, the supernatant was diluted to make the OD600 close to 0.05. Next, 150 µL aliquots of the diluted supernatants were added to the wells of the microplate and incubated at 30 °C for 3–4 days.

Data from the Biolog experiments were subsequently analyzed for metabolic function of microbial communities. The ability to degrade each of the 31 carbon source was indicated by average well color developments (AWCD):

$${\text{AWCD}} = \frac{{\sum_{{{\text{i = }}1}}^{96} {\left( {{\text{A}}_{\text{i}} - \frac{{{\text{A}}_{ 1} {\text{ + A}}_{ 3 3} {\text{ + A}}_{ 6 5} }}{3}} \right)} }}{93}.$$

In this equation, Ai refers to the OD600 value in well number “i”, among which No. 1, 33, and 66 were blank values.

Metabolic activities were indicated by changes in the AWCD rate (v) obtained in during the rapid growth rate as follows (Choi and Dobbs 1999):

$$v = \frac{{{\text{AWCD}}_{1} - {\text{AWCD}}_{0} }}{t},$$

where AWCD0 is the AWCD value at the beginning of the rapid growth period, AWCD1 is the AWCD value at the end of the rapid growth period and t is the length of the rapid growth period in hours.

The results were then subjected to principal component analysis (PCA) using SPSS 22.

Results

Removal and mineralization of VOCs

Shifting of inlet VOCs influenced removal efficiencies were observed (Fig. 1). Specifically, significant declines in removal efficiency were obtained after shifting VOCs; however, it recovered several days later, indicating that the system required time to adapt to the new conditions. Differences in molecular structures are known to impact the biodegradability of different compounds. For example, simpler compounds such as ethanol are more readily degraded by microorganisms than more complex materials (Sempere et al. 2008). In the present study, the removal efficiency varied from 18.2% (chlorobenzene) to 92.3% (isopropyl alcohol). The maximum elimination capacities of different volatile organic compounds are listed in Table 1. Alcohols, ketones, esters and ethers appeared to be more easily removed, whose eliminated capacities were higher than 600 mg m−3 min−1. Moreover, the system showed satisfactory performance for degrading toluene (678.11 mg m−3 min−1) and tetrahydrofuran (401.53 mg m−3 min−1). Conversely, chlorobenzene and n-hexane were not easily degraded by microorganisms, as indicated by removal efficiencies lower than 30%. Overall, considerable differences in degradation performance were seen among different VOCs.

Fig. 1
figure 1

Removal efficiencies (RE) and average mineralization rates (MR) of the biofilter with shifting of VOCs (inlet VOCs were changed every 15 days with the order of toluene, ethylbenzene, chlorobenzene, acetone, isopropyl alcohol, ethyl acetate, n-hexane and tetrahydrofuran)

Table 1 Performances of the biofilter with different inlet VOCs

Similar results were observed among VOC mineralization rates (Fig. 1). Surprisingly, the mineralization rate of tetrahydrofuran was lowest among all tested compounds. More tetrahydrofuran was degraded into intermediates or microorganisms instead of CO2 and H2O.

Different performance was observed for different inlet VOCs, suggesting that the characteristics of the microbial community changed with inlet VOCs.

Microbial diversity

The microbial community was analyzed following changes in VOCs (Table 2). The highest OTU value of 690 was observed for toluene, while all other VOCs had OTU values of less than 380. The ACE and Chao1 index values showed a similar trend, confirming that there was higher microbial diversity when treating toluene.

Table 2 Indexes of microbial following treatment with different types of VOCs

Shannon’s index was lower for compounds of aromatic hydrocarbons, indicating lower microbial diversity. A similar trend was observed for Simpson’s index, indicating that a higher microbial diversity led to lower dominance of the dominant species, as occurred with toluene. High consistency was seen between degrading performance and microbial community. As previously mentioned, higher microbial diversity was observed for toluene, which had the highest biodegradability among the aromatic hydrocarbons.

Microbial community structure

During the course of varying inlet VOCs, 21 phyla were found. Ten known phyla and two unidentified phyla were found to account for over 98% of the abundance (Fig. 2a).

Fig. 2
figure 2

Figure 3-2 Microbial community structures (a relative abundances of microorganisms at the phylum level following the inlet of different volatile organic compounds; b relative abundances at the genus level when treating different volatile organic compounds. 22 genera were included, including the five genera with the highest abundance in each stage)

Actinobacteria and Proteobacteria remained dominant throughout the experimental period. Upon further analysis, the abundance of Actinobacteria was found to fluctuate from 17 to 72%, while that of Proteobacteria varied from 19 to 57%. As the inlet VOCs were changed from toluene to ethylbenzene and chlorobenzene, the abundance of Actinobacteria increased in a stepwise fashion to 33.2%, 63.9% and 71.1%, respectively, while that of Proteobacteria decreased from 56.4 to 24.6% and then 19.8%. Surprisingly, the sum of the two phyla remains stable, with values of 89.6%, 88.5% and 90.9% being observed for toluene, ethylbenzene and chlorobenzene, respectively.

The changes in the microbial community occurred when the VOCs were switched from aromatic to non-aromatic hydrocarbons. The sum of Actinobacteria and Proteobacteria decreased from 90% to approximately 60%–70%, while the abundances of Planctomycetes and Thermi increased significantly after the hydrocarbons were changed. The abundance of the phylum Planctomycetes increased when some aromatic chemicals were removed. Moreover, their abundance increased when the aromatic hydrocarbons were replaced with non-aromatic chemicals such as acetone. Thermi remained stable during purification of non-aromatic hydrocarbons, fluctuating at levels of 5.0–8.0%. The abundance of Bacteroidetes peaked at 14.6% in response to acetone and then decreased to 1.0% upon application of n-hexane. These findings indicate that acetone was a better carbon and energy source for species in the phylum Bacteroidetes than n-hexane. The abundance of Cyanobacteria tripled in the presence of tetrahydrofuran when compared to other compounds. It has been speculated that members of the phylum Cyanobacteria could include more tetrahydrofuran degraders than other phyla.

A total of 264 genera were obtained during the operation, 21 of which were present in high abundance. The sum of these dominant genera accounted for 75%–91% of the total biomass (Fig. 2b). All genera belonged to the top seven phyla, with most belonging to the phyla Actinobacteria and Proteobacteria. Four genera, including Rhodococcus, Pseudonocardia and other two unidentified genera from the phylum Actinobacteria, had high abundances. Among them, Rhodococcus had significant advantages in abundance throughout the experimental period. The phylum Proteobacteria, which contained Pseudomonas, Devosia, Aquimonas, Marinobacter and eight other genera, showed high stability and uniformity with increased abundance when treating various contaminants, as opposed to genera belonging to the phylum Actinobactria.

The genus Rhodococcus, which belongs to the phylum Actinobacteria, was obtained in high abundance (> 10%) throughout the operation. Surprisingly, higher values of relative abundance were observed when aromatic hydrocarbons were being eliminated. Similarly, the abundance of Devosia sp. increased in response to the inlet of aromatic hydrocarbons. During the operation, specific degraders were identified. Specifically, high abundance (18.8%) of Thauera was observed in the presence of ethyl acetate, while less than 1% was observed in the presence of other VOCs. In addition, the genus Pseudomonas showed highest abundance during the inlet of toluene, while it comprised less than 0.5% in the presence of other VOCs.

Microbial metabolic profile

The values of average well color development (hereafter AWCD, Fig. 3) were affected by density and activity of bacterial community (Preston-Mafham et al. 2002; Rutgers et al. 2016). The results showed that carbon source metabolic capacity of the microbial community decreased gradually with time. Initially, the AWCD values of toluene and ethylbenzene were higher than those observed for other VOCs. The rate of AWCD increase was 0.042 cm−1 h−1 for toluene and 0.035 cm−1 h−1 for ethylbenzene, which illustrated that the microbial community had higher activity in the presence of purified toluene than ethylbenzene. Growth rate declined to approximately 0.025 cm−1 h−1 when treating acetone and chlorobenzene and carbon source metabolic capacities and activities declined with time. The increase rate of AWCD when treating isopropyl alcohol, ethyl acetate, hexane and tetrahydrofuran were 0.013 cm−1 h−1, 0.014 cm−1 h−1, 0.010 cm−1 h−1 and 0.015 cm−1 h−1, respectively. Taken together, these results suggested that some measures might be taken to increase the activities of microorganisms after a long-term operation.

Fig. 3
figure 3

AWCD changes in microbial community under different inlet VOCs

The duration between hours 20 and 30 was a period when the highest AWCD increasing rates were obtained. Therefore, principle component analysis was conducted in this study to obtain further insight (Fig. 4) based on data obtained between hours 20 and 30.

Fig. 4
figure 4

Carbon metabolism principle component analysis of microbial community with different inlet VOCs: No. 1–8 referred to stages of toluene, ethylbenzene, chlorobenzene, acetone, isopropyl alcohol, ethyl acetate, n-hexane and tetrahydrofuran

Discussion

The dominant phyla Actinobacteria and Proteobacteria are the most commonly reported prokaryotic degraders (Coleman et al. 2006). As reported in previous studies, many members of the phylum Actinobacteria have aromatic hydrocarbon degrading abilities, and some species can utilize complicated chemicals as carbon or energy sources for growth; however, the capability for degradation decreases with increasing carbon chain length (Wen et al. 2014; Zylstra et al. 2000). Proteobacteria has previously been widely applied in bioremediation for hydrocarbon purification in combination with Actinobacteria, which is another dominant phylum commonly seen in aromatic hydrocarbon biodegradation (Fuentes et al. 2014). Hence, we can conclude that Actinobacteria and Proteobacteria played crucial roles in aromatic hydrocarbon purification in this study. Increasing abundance of the phylum Planctomycetes when some aromatic chemicals were being removed have also been confirmed in previous study (Delgado-Balbuena et al. 2016).

On genus level, it was previously reported that Rhodococcus can utilize and removal a large variety of pollutants (Maia et al. 2018; Warhurst and Fewson 1994). Members of the genus Rhodococcus were found to have the considerable ability to degrade a great number of aromatic hydrocarbons several decades ago (Sorkhoh et al. 1990). As well-known VOCs degraders, Rhodococcus species can utilize various chemicals and have therefore been applied frequently in VOCs purifications (Li et al. 2016). It was also confirmed that Rhodococcus species can degrade complicated chemicals like three to five rings polycyclic aromatic hydrocarbons (PAHs) (Song et al. 2011). Moreover, some strains of Rhodococcus were shown to have broad degradation capacities toward a mixture of 16 VOCs including benzene, toluene, ethylbenzene, m-xylene, p-xylene, o-xylene, and octane (Auffret et al. 2009). Because of its efficient and broad degradation capacities, Rhodococcus was used to remediate heavily PAH-contaminated soil with total PAHs of 375 mg, and up to 55% was removed (Sun et al. 2012). These performances could explain the high abundance of Rhodococcus throughout the experimental period and likely contributed greatly to the biodegradation performance in this system.

In consideration of other genera, the findings in this study are consistent with those of previous reports. High abundances of Devosia sp. were previously observed in aromatic compounds purification systems (Ramos et al. 2015), and they have been used as aromatic compounds degraders in previous studies (Papale et al. 2017). Ethyl acetate can be utilized as carbon resources by Thauera sp. (Du et al. 2017). The genus Pseudomonas was previously reported to be a toluene utilizer and degrader (Hernandez and Torre 2011; Su et al. 2014). Pseudomonas sp. was previously proposed to be indicators of biodegradation because of their sensitivity to substrate change (Obi et al. 2017; Yakimov et al. 2007).

The significant differences observed in this study indicated that target VOCs had significant effects on microorganisms, particularly at the genus level. The population of utilizers and degraders increased rapidly in the response to VOCs, with some becoming dominant species. Subsequently, changes in inlet VOCs caused dramatic decreases shifts in these populations. Taken together, these results indicate that the microbial community has the ability to adapt to new environmental conditions. Accordingly, there is the potential to develop specific measures to facilitate such adaptation to optimize biodegradation, such as increasing the abundance of specific degraders artificially.

The results revealed that the microbial community was significantly different when purifying toluene then when treating other VOCs. Surprisingly, the communities were highly similar in the presence of all other test compounds. This might have occurred because of significant microbial community shifts in the initial operations (Qiu et al. 2013). After the initial operation, the system became relatively stable, possibly indicating that the community stabilized with time.

Biodegradability of different VOCs has remarkable influences on microbial elimination performance, community structures and metabolic profiles. The highest diversity was obtained at the beginning of the operation while eliminating toluene. Diversity declined with prolonged operation, and significant differences were found in microbial community structures at both the phylum and genus levels. As the experiment continued, the carbon source metabolic capacity declined gradually. The metabolic characteristics of carbon source utilization differed significantly following toluene input, while it was similar among all other treatment groups. Artificial addition of degraders and measures to increase microbial activity might optimize biofiltration.