Pretreatment of Miscanthus with biomass‐degrading bacteria for increasing delignification and enzymatic hydrolysability

Summary Biomass recalcitrance is still a main challenge for the production of biofuels and high‐value products. Here, an alternative Miscanthus pretreatment method by using lignin‐degrading bacteria was developed. Six efficient Miscanthus‐degrading bacteria were first cultured to produce laccase by using 0.5% Miscanthus biomass as carbon source. After 1–5 days of incubation, the maximum laccase activities induced by Miscanthus in the six strains were ranged from 103 to 8091 U l−1. Then, the crude enzymes were directly diluted by equal volumes of citrate buffer and added Miscanthus biomass to a solid concentration at 4% (w/v). The results showed that all bacterial pretreatments significantly decreased the lignin content, especially in the presence of two laccase mediators (ABTS and HBT). The lignin removal directly correlated with increases in total sugar and glucose yields after enzymatic hydrolysis. When ABTS was used as a mediator, the best lignin‐degrading bacteria (Pseudomonas sp. AS1) can remove up to 50.1% lignin of Miscanthus by obtaining 2.2‐fold glucose yield, compared with that of untreated biomass. Therefore, this study provided an effective Miscanthus pretreatment method by using lignin‐degrading bacteria, which may be potentially used in improving enzymatic hydrolysability of biomass.


Introduction
Various sources of lignocellulosic feedstocks have been regarded as emerging biofuels to partly replace the fossil fuels in the near future. However, their complicated cell wall structure makes the production of biofuels more difficult and costly due to the existence of biomass recalcitrance (Pauly and Keegstra, 2008). Among the three main polymeric components (cellulose, hemicellulose and lignin) constituting lignocellulosic biomass, lignin, which covers the cellulose and hemicellulose in various ways, is the most stable and complex polymer and acts as an obstacle in the enzymatic hydrolysis of cellulose (Mussatto et al., 2008;Lee et al., 2014). To make more cellulose and hemicellulose available before enzymatic hydrolysis, a pretreatment step is necessary to weaken and remove lignin (Lee et al., 2014). The lignin can be disrupted via physical, chemical and biological processes (Alvira et al., 2010). Various pretreatments methods through physical and chemical processes (Hu and Wen, 2008), alkaline and dilute acid (Si et al., 2015), organic solvent (Sun et al., 2000), steam explosion ( € Ohgren et al., 2007) and wet oxidation (Hendriks and Zeeman, 2009) are available to remove lignin from lignocellulosic biomass. However, high energy input, high costs of chemicals and increased environmental risk make these methods challenging to scale up (Millati et al., 2011). In addition, the lignin degraded by physical and chemical processes will release some inhibiting compounds, such as furfurals, 5-hydroxymethyl furfurals and other volatile products, which inhibit the next stages of enzymatic hydrolysis and yeast fermentation (Hendriks and Zeeman, 2009;Camesasca et al., 2015). Organosolv pretreatment may cause severe damage like fire explosions in the absence of proper safety measures, although it can achieve a biomass fractionation to lignin, hemicellulosic sugars and a relatively pure cellulose fraction (Kumar and Sharma, 2017;Li et al., 2017). These are the disadvantages for large-scale application.
Lignin removal via biological pretreatment has received increasing attention as an alternative to physical and chemical pretreatment for enhancing cellulose digestibility due to its environmental and economical benefits (Wan and Li, 2012;Sindhu et al., 2016). Among the various biological pretreatments adopted for lignin removal from lignocellulosic biomass, fungal pretreatments have been widely studied because fungi, especially white-rot fungi, were thought to be excellent laccase and peroxidase producers (Wesenberg et al., 2003;Wan and Li, 2012). However, fungi usually grow slowly and require a long time to produce lignolytic enzymes like laccase, manganese peroxidase (MnP) and lignin peroxidase (LiP), which means that long pretreatment time is necessary for lignin removal by fungi (Leonowicz et al., 1999;Wan and Li, 2012). Moreover, large loss of cellulose and hemicellulose is another major weakness of fungal pretreatment, although remarkable enhancement of cellulose digestibility has been obtained from lignocellulosic biomass pretreated by white-rot fungi (Wu et al., 2005;Lee et al., 2007).
A number of bacteria are able to produce various lignocellulolytic enzymes like endoglucanase (CMCase), xylanase and laccase (Bugg et al., 2011;Guo et al., 2017a). Of these bacteria, Bacillus sp., Pseudomonas sp., Streptomyces sp. and Aeromonas sp. strains have been reported to break down lignin (Bugg et al., 2011;Chang et al., 2014). Bacillus sp. CS-1 isolated from forest soils was used to degrade up to 20% lignin in rice straw with remarkable laccase production (Chang et al., 2014). The laccase from Bacillus licheniformis showed strong oxidation capacity towards substrates 2,2-azinobis (3-ethylbenzothiazoline-6-sulphonic acid) (ABTS), syringaldazine, 2,6-dimethoxyphenol and phenolic acids (Koschorreck et al., 2008). A soil bacterium, Pseudomonas putida, known as aromatic degrader, was capable of removing lignin from various lignocellulose biomasses accompanied by producing monocyclic phenolic products (Ahmad et al., 2010). However, the laccase production yields of bacteria are much lower than those of fungi and thus impeding their application in industry. In our previous study, it was found that the laccase production of bacteria can be significantly induced by lignocellulosic biomass, such as algae and Miscanthus. The high activity of laccase induced by Miscanthus may be due to the high components of total ester-bound phenolics, which can stimulate the secretion of laccase (Guo et al., 2017b). In addition, the delignification efficiency of laccase can be largely improved by the laccase mediators, which can increase the oxidation of polymeric lignin by transferring hydrogen atoms (Baiocco et al., 2003;Yao and Ji, 2014).
Therefore, a two-step pretreatment procedure was developed in this study. A low concentration Miscanthus biomass (0.5%, w/v) was first used to induce the production of laccase, and then, the crude enzymes of these bacteria induced by 0.5% Miscanthus biomass were directly mixed with equal volumes of citrate buffer and Miscanthus at solid concentration of 4% (w/v) to debilitate the lignin. The effects of two laccase mediators, 2,2azino-bis(3-ethylbenzothiazoline-6-sulphonic acid) (ABTS) and 1-hydroxybenzotriazole (HBT), on the degradation of lignin were also determined in the process of pretreatment. Then, the pretreatment effect was evaluated by measuring the sugar released after enzymatic hydrolysis.

Screening the Miscanthus-degrading bacteria
Twelve bacterial strains isolated previously by Guo and colleagues (2017a,b), Maki and colleagues (2012) and Paudel and Qin (2015), including 7 Bacillus, 2 Pseudomonas, 1 Exiguobacterium, 1 Aeromonas and 1 Raoultella species (Table 1), were tested for the hydrolysis of biomass using Miscanthus as carbon source. All tested strains and positive strain C. xylanilytica showed a halo region in the plate after Gram's iodine staining, and nine strains (A0, A4, AS1, AS2B, GH2OS1, K1, X1, X4 and X8) showed bigger halo regions than that of C. xylanilytica (Fig 1). The hydrolytic potential of Miscanthus of each bacterial colony was further evaluated by calculating the square of the halo diameter: colony diameter ratio. The hydrolytic potential values of these strains ranged from 2.8 to 18.1, while only strains A4, AS1, AS2B, K1, X4 and X8 had higher hydrolytic potential than that of positive strain (hydrolytic potential value: 9.8) (Table 1). Therefore, these strains were selected for the next experiments.

Activities of laccase secreted by selected bacteria
The laccase production abilities were different among the six bacterial strains when Miscanthus was used as the sole carbon source (Fig. 2). Peak laccase activity was detected on the first day in strains AS1 (8091 U l À1 ) and K1 (1049 U l À1 ). Maximum activity occurred on the third day in strains AS2B (2365 U l À1 ) and X8 (103 U l À1 ), on the fourth day in stain X4 (646 U l À1 ), and on the fifth day in strain A4 (1122 U l À1 ) (Fig. 2).

Effects of bacteria pretreatment on delignification
The crude enzymes (Lac) produced by bacteria and two laccase mediators (Lac + ABTS and Lac + HBT) were tested in the enzymatic pretreatment of Miscanthus biomass. The crude enzymes autoclaved at 121°C for 25 min were used as a control (Inact). The native M. sacchariflorus used in this study mainly consisted of 32.9% cellulose, 22.5% hemicellulose and 27.9% lignin.
After pretreatment of crude enzymes produced by the six bacteria, the cell wall composition of Miscanthus significantly differed with selective degradation of lignin, especially in the presence of two laccase meditators. Without laccase mediators, the lignin contents were 22.0, 19.5, 21.2, 16.1, 22.5 and 22.7% for Lac pretreatment of A4, AS1, AS2B, K1, X4 and X8 respectively. The most lignin was removed by Lac + HBT for all strains, and the lignin removal percentages were 47, 59.5, 42.7, 47.7, 52.7 and 41.2% for strains A4, AS1, AS2B, K1, X4 and X8 respectively. For Lac + ABTS pretreatment, strain AS1 degraded the most lignin of Miscanthus, with a lignin removal percentage of 50.9%, while the least lignin remove was found by X8 with the lignin removal percentage of 29.7%, compared with that of untreated Miscanthus (Table 2). Interestingly, the cellulose (Calculated as glucan) and hemicellulose (Calculated as xylan) contents were all significantly increased  after pretreatment, compared with that of untreated and Inact-treated Miscanthus ( Table 2). The maximum cellulose content was obtained by Lac + HBT pretreatment of strain AS1, being 49.4% and 46.7% higher than those of untreated biomass and biomass treated by Inact respectively. The biomass pretreated by Lac + ABTS of X4 strain showed the highest hemicellulose content (30.1%) compared with that of untreated (22.5%) and Inact of X4 strain (23.5%). The almost no cellulose and hemicellulose loss were proved by the little sugar increase in the liquor after bacteria pretreatment (Table 2). Moreover, the addition of laccase mediators in all bacterial strains significantly changed the cellulose and lignin contents, while there were no significant effects to hemicellulose content compared with Lac pretreatment alone (

Effects of bacteria pretreatment on enzymatic hydrolysis
To evaluate the effects of bacteria pretreatment on biomass digestibility, the sugar yield (hexoses and pentoses) released from pretreated Miscanthus after hydrolysing with a mixed cellulase cocktail (Celluclast 1.5L and Novozyme 188) was determined (Fig. 4). The hexoses released (% of cellulose), pentoses released (% of hemicellulose) and total sugar released (including hexoses and pentoses, % of dry weight) from untreated Miscanthus were 43.2, 40.3 and 25.4% respectively ( Fig. 4). After enzymatic hydrolysis, the hexoses and total sugar released from pretreated Miscanthus by Lac, Lac + ABTS and Lac + HBT were all significantly increased (P < 0.05) in all strains, compared with that of untreated and corresponding pretreated Miscanthus by Inact. For each strain, the total sugar released from Lac + HBT was higher than that from Lac + ABTS and Lac. The highest total sugar yield was obtained by Lac + HBT of strain AS1 (54.2%), followed by Lac + HBT of strain X4 (53.1%) (Fig. 4).The hexose released from Lac + ABTS pretreated Miscanthus was higher than that of Lac + HBT and Lac in all strains except the strain A4, which obtained the peak hexoses yield by Lac + HBT (Fig. 4). The maximum hexoses were released by the Lac + ABTS of strain AS1 (87.0%; Fig. 4). For the release of pentoses, the maximum yields were harvested by Lac of strain X4 (59.5%), by Lac + ABTS of strain A4 (53.8%), by Lac + HBT of strains AS1 (48.8%), AS2B (78.7%), K1 (66.9%) and X8 (54.6%) respectively (Fig. 4).

Correlation of lignin removal and sugars release and mass balance
We analysed the correlation between lignin removal and sugar released from six bacteria strains with or without mediators pretreated Miscanthus (Fig. 5). Significantly, a positive linear correlation was observed with correlation coefficient (R 2 ) values of 0.9044 (P < 0.01) and 0.6286 (P < 0.01) for the lignin removal and total sugar and hexoses yield released after bacteria pretreatment ( Fig. 5A and B). However, there was no positive correlation between lignin removal and pentoses released by bacteria pretreated Miscanthus (R 2 = 0.2581; P = 0.14; Fig. 5C).
To further evaluate the effects of bacteria pretreatment and track carbohydrate degradation during the pretreatment process, the results obtained from laccase production, delignification and enzymatic hydrolysis were used to make a detailed mass balance using Lac + ABTS of strain AS1 (Fig. 6). The maximum laccase production in AS1 strain was 1618 U g À1 dry biomass. After Lac + ABTS pretreatment of strain AS1, the solid recovery was 72.6%, and the glucan content was unchanged (P > 0.05) compared with that of raw material, while the xylan and lignin content decreased from 2.25 g to 1.96 g and 2.79 g to 1.10 g per 10 g dry biomass compared with that of raw material respectively. After enzymatic hydrolysis, the glucose released from Lac + ABTS pretreated Miscanthus was 2.2-fold higher than that of untreated Miscanthus (Fig. 6). The total monosaccharide yield was 4.34 g per 10 g dry biomass, which was a 1.7fold increase compared with that of untreated Miscanthus after enzymatic hydrolysis (Fig. 6).

Miscanthus biomass is a good candidate for laccase production
Twelve biomass-degrading bacteria (seven Bacillus, two Pseudomonas, one Exiguobacterium, one Aeromonas and one Raoultella species) were isolated on plates using carboxymethyl cellulose as the sole carbon source by our previously laboratory members (Bugg et al., 2011;Maki et al., 2012;Paudel and Qin, 2015). It has been reported that the degradation ability was extremely different using different carbon sources in both fungi (Olsson et al., 2003;Sipos et al., 2010) and bacteria (Waghmare et al., 2014;Mohammadkazemi et al.,  Values represent mean AE SDs (n = 4). Different letters indicate a significant difference at P < 0.05. . In this study, the degradation abilities of the twelve bacteria to Miscanthus biomass were determined using the Gram's iodine method, while only six bacteria strains (A4, AS1, AS2B, K1, X4 and X8) showed higher hydrolytic potential than that of the industrial strain C. xylanilytica when Miscanthus was used as the sole carbon source. To further evaluate the characteristics of these six strains, laccase activities were monitored in the mineral salt medium containing 0.5% (w/v) Miscanthus.
The results showed the strains A4, AS1, AS2B, K1, X4 and X8 can efficiently secrete laccase into the medium, with the significantly different among the bacteria strains. Previous studies have shown the production of bacterial lignocellulolytic enzymes differed markedly using  , and they were 501, 1149, 586 and 378 U l À1 in the presence of Miscanthus respectively. The lignocellulolytic enzyme activity produced by Klebsiella sp. PRW-1 was higher when grass power and sugarcane were used as carbon source compared with that of other agricultural wastes like sorghum husks, corn straw and paddy straw (Waghmare et al., 2014). The biodegradation and enzyme production of lignocellulosic biomass by fungi and bacteria mainly depended on the porosity of biomass materials and crystallinity of cellulosic fibre (Zhang et al., 2006;Kumar et al., 2009). A series of lignocellulosic enzymes were produced by microorganisms using lignocellulosic biomass as carbon source, and certain lignocellulosic biomasses possess abundant soluble carbohydrates and enzyme synthesis-related inducers, which can efficiently increase the production of lignocellulosic enzymes (Rosales et al., 2005;Singhania et al., 2010). Moreover, our results showed that in the presence of Miscanthus, the Pseudomonas strain AS1 specifically produced a large amount of laccase, which has been regarded as the main lignin-degrading enzymes in the process of delignification of biomass (Martinez et al., 2009;Pollegioni et al., 2015).

Delignification of Miscanthus and improved saccharification by bacterial pretreatment and laccase mediators
The polymers of lignin closely overlay the other polymers (mainly including cellulose and hemicellulose) in various ways in the lignocellulosics biomass. Lignin is very impervious and hard to degrade by enzymes or chemicals, and this is the main barrier to make cellulose and hemicellulose more susceptible to enzymatic hydrolysis in industrial processes (Brebu and Vasile, 2010). The degradation of lignin by using fungi has been well-studied, especially by using white-rot and brown-rot fungi (Leonowicz et al., 1999;Guill en et al., 2005). But research about the degradation of lignin by using bacteria is scarce. In this study, six Miscanthus-degrading bacteria were screened to degrade the lignin of Miscanthus biomass. The results showed that the crude enzymes produced by all the tested bacteria efficiently decreased the lignin content of Miscanthus, especially in the presence of two laccase mediators. The maximum lignin removal percentage (59.5%) was observed by the Pseudomonas sp. AS1 strain with the addition of 0.5% HBT (g g À1 dry biomass). Our previous study reported that the Pseudomonas sp. AS1 isolated from municipal waste showed good potential for black liquor decolourization and industrial degradation of lignocellulosic biomass (Maki et al., 2012). Moreover, the other four Bacillus sp. strains and one Exiguobacterium similarly reduced the content of lignin even if only their crude enzymes were used, which obtained the lignin removal percentage range from 18.6% to 42.3%. It has been reported that some of bacterial stains were able to degrade lignin via producing laccase and other lignin peroxidase (Bugg et al., 2011;Chang et al., 2014). The Bacillus sp. CS-1 strain isolated from forest soils can degrade at least 61% alkali lignin within 48 h, and pretreatment using this strain followed by lactic acid bacteria removed 61.9% lignin of rice straw and enhanced cellulase performance (Chang et al., 2014). The Pseudomonas sp. LD002 and Bacillus sp. LD003 were isolated from beneath decomposing wood logs and exhibited good growth on lignin fractions and excellent dye-decolourizing abilities (Bandounas et al., 2011). The chemicals of ABTS and HBT have been regarded as the most efficient laccase mediators, which play as an electron carrier between laccase and oxidized substrate (Munk et al., 2015). In the current study, the average lignin contents of Miscanthus pretreated by six bacteria strains with two laccase mediators (ABTS and HBT) were 20.2% and 30.1% lower than that without laccase mediator. This was consistent with the higher lignin removal percentage obtained by laccase pretreatment in the presence of various laccase mediators (Rico et al., 2014;Rencoret et al., 2016). Furthermore, all bacteria pretreatment in the citrate buffer (pH 3.0) selectively degraded the lignin and improved the cellulose and hemicellulose contents of Miscanthus. The results were similar to that of pretreatment of feedstock with commercial laccase, which removed up to 50% of lignin and significantly increased the content of glucose and xylose in the presence of laccase mediators (Rico et al., 2014;Rencoret et al., 2016).
A previous study showed Miscanthus biomass saccharification largely depends on the effective lignin removal rather than the hemicellulose extraction under various alkali and acid pretreatments (Si et al., 2015). In this study, total sugar and hexoses released after enzymatic hydrolysis were significantly improved by all pretreatments and showed a positive correlation with the lignin removal percentage, which indicated that lignin ratio was the key factor that positively influenced Miscanthus digestibility after bacterial pretreatments. In addition, the maximum enzymatic digestibility (calculated as glucose released) from bacterial pretreatment was up to 87%, which was comparable with that of most fungal pretreatments, such as Trameteshirsute yj9 (73.99%; Sun et al., 2011) and Pycnoporus sp. SYBC-13 (90%; Liu et al., 2013). Therefore, the bacterial pretreatment in this study might be more promising in the removal of lignin on Miscanthus compared with that of direct incubation biomass with fungi from the following three aspects: first, the laccase secreted by most of the tested bacteria in this study can rapidly reach the maximum after 1-3 days of incubation, which was easier to obtain crude laccases than most of fungi (Wesenberg et al., 2003;Liu et al., 2013). Second, even though the lower redox potential was found in most bacterial laccases (Bugg et al., 2011), the lignolytic enzyme activities induced by biomass in these bacteria were much higher than that in fungi. For example, the highest laccase activity of AS1 strain in this study was 1618 U g À1 dry biomass, while the maximum of it in reported fungi was 935.4 U g À1 dry biomass (Chang et al., 2012;Yang et al., 2012). Third, the process of lignin removal by fungal pretreatment was accompanied by large losses of cellulose and hemicellulose, which may be utilized as a carbon source to support fungal growth and metabolism (Wan and Li, 2010;Bugg et al., 2011).

Conclusions
This study showed that the enzymatic digestibility of Miscanthus can be improved by laccase-secreted bacteria. Six efficient Miscanthus-degrading bacteria secreted abundant laccase when Miscanthus was used as sole carbon source. The crude enzymes induced by Miscanthus markedly decreased the content of lignin, especially in the presence of two laccase mediators, with the lignin removal percentage of 29.7-59.5%. After enzymatic hydrolysis, the glucose released from bacterial pretreated Miscanthus was 1.3-2.2-fold higher than that from untreated biomass. These results will provide a two-step pretreatment method to further studies on the use of laccase-producing bacteria for bioenergy production.

Strains and culture conditions
The following twelve lignocellulose-degrading bacteria, which were isolated and identified previously by our laboratory members, were used in this study (Table 1). The detailed information of Bacillus sp. A0 and K1 was described by Paudel and Qin (2015), Bacillus sp. A4, Raoultella sp. X1 and Bacillus subtilis X4 by Guo and colleagues (2017a) and Pseudomonas sp. AS1, Exiguobacterium sp. AS2B, Aeromonas sp. CDS1B, Bacillus sp. CTS1A, Pseudomonas sp. GH2OS1 and Bacillus sp. 6S1 by Maki and colleagues (2012). The strain Bacillus sp. X8 was isolated from forest soil (Thunder Bay, Ontario, Canada) and identified as Bacillus sp. X8 in this study. Cellumonas xylanilytica and Escherichia coli BL21 were used as positive and negative controls respectively. The strains and their corresponding accession number and source are shown in Table 1. All the strains were stored at À70°C. Prior to the experiments, all the strains were activated in Luria-Bertani (LB) medium at 37°C, with agitation at 200 rpm for 12 h. The bacteria were then cultured on a large scale in mineral salt medium (0.1% NaNO 3 , 0.1% K 2 HPO 4 , 0.1% KCl, 0.05% MgSO 4 , 0.05% yeast extract and 0.3% peptone) containing 0.5% (w/v) Miscanthus sacchariflorus (M. sacchariflorus) biomass for 7 days at 37°C, with agitation at 200 rpm. The production of laccase was monitored every day, and the culture medium from different strains with the highest laccase activity was directly used for M. sacchariflorus pretreatment.

Screening and evaluation of Miscanthus-degrading bacteria
To measure the hydrolysis activity of M. sacchariflorus by these bacteria strains, the strains were cultured on an agar plate using M. sacchariflorus as the sole carbon source according to our previous study (Guo et al., 2017a). Briefly, 5 ll of overnight-grown each bacterial culture was dropped in an agar plate containing 0.1% NaNO 3 , 0.1% K 2 HPO 4 , 0.1% KCl, 0.05% MgSO 4 , 0.05% yeast extract, 0.3% peptone, 1.5% agar and 0.5% M. sacchariflorus biomass. All of the plates were incubated at 37°C for 48 h and flooded with Gram's iodine solution for 3-5 min. The diameters of the halo region (D) and bacterial colony (d) were then measured on a centimetre scale. The hydrolysis activity was calculated as (D/d) 2 , as described previously by Guo et al., 2017a.

Determination of enzyme activities
For determination of laccase activities, 1 ml of cultures of each strain was collected after 1, 2, 3, 4, 5, 6 and 7 days of incubation and centrifuged at 12 000 g for 3 min. The supernatants were used as crude enzymes for enzyme activities analysis. The activities of laccase were measured according to the description of Guo and colleagues (2017a). Briefly, 200 ll of reaction solution including 20 ll diluted crude enzyme and 20 ll of 20 mM ABTS in a 0.1 M citrate buffer (pH 3.0) was incubated at 40°C for 3 min. Then, the optical density (OD) was measured at 420 nm (e 420 = 36 000 M À1 cm À1 ) using a Microplate Spectrophotometer (Epoch; Bio Tek Instruments, Winooski, VT, USA). One unit of laccase activity was defined as the amount of enzyme required to oxidize 1 lmol of substrate per min.

Inoculum preparation and pretreatment
The screened six Miscanthus-degrading bacteria (A4, AS1, AS2B, K1, X4 and X8) were firstly cultured in 125 ml mineral salt medium containing 0.625 g (0.5%, w/v) M. sacchariflorus biomass to produce laccase at 37°C, with agitation at 200 rpm. At the day with the highest laccase activity in the culture medium, equal volumes of citrate buffer (pH 3.0) and another 9.375 g M. sacchariflorus biomass were added to the culture medium to make the final biomass ratio at 4.0% (w/v). The final pH was adjusted to 3.0 using 1M hydrochloric acid. Then, the mixture was saturated with oxygen by bubbling air for 20 min. Tetracycline (40 mg l À1 ) was added into the mixture to control the growth of bacteria. For the effects of laccase mediators (HBT and ABTS) on the delignification of Miscanthus biomass, 0.1 mM ABTS and 5% HBT (g g À1 dry weight biomass) were added to the culture. Bacterial culture autoclaved at 121°C for 25 min was used as a control. The pretreatment was performed at 37°C, with agitation at 200 rpm. After 96 h of pretreatment, the samples were washed with distilled water five times to remove the bacterial cells through a double-layered muslin cloth with the meshes of 300. Then, solid residues were oven dried at 50°C until constant weight and used for cell wall composition analysis and subsequent enzymatic hydrolysis.

Plant cell wall composition analysis
The cellulose and hemicellulose contents were measured according to the method of Guo and colleagues (2017c). Briefly, the sample (0.1 g) was extracted twice with 1.5 ml hot water, once with 1.5 ml absolute ethanol and once with 1.5 ml acetone at 65°C for 30 min. Then, the sediment was air-dried in a chemical hood for 2 days, and the dry samples were hydrolysed with 1 ml of 72% (w/w) sulphuric acid (H 2 SO 4 ) at 30°C for 1 h. The hydrolysates were diluted to 3% sulphuric acid by adding deionized water and autoclaved at 121°C for 1 h. After cooling down, the mixture was filtered through a pre-weighted glass microfilter. The solutions were used to determine the contents of hexose and pentose using the anthrone-sulphuric acid method and orcinol-hydrochloric acid method respectively. The filter and solids were dried at 105°C until constant weight and weighed, and then, the solids were ashed at 575°C for 3 h and weighted again. The Klason lignin contents were calculated as the weight of the dry solids minus that of the ash as a percentage of the weight of the initial dry weight of sample.

Determination of total hexoses and pentoses
The total hexose and pentose contents were determined according to the method of Xu and colleagues (2012), with minor modifications. For determination of total hexoses, 80 ll diluted sample was added to 160 ll of 0.2% (w/v) anthrone in concentrated H 2 SO 4 , mixed well and incubated in boiling water for 5 min. After cooling down, 200 ll of the mixture was removed to the 96-well microtiter plate and the absorbance was determined at 620 nm using a microplate spectrophotometer (Epoch; Bio Tek Instruments). For determination of total pentoses, 75 ll diluted sample and 10 ll of 6% orcinol (0.6 g orcinol dissolved in 10 ml ethanol) were mixed with 150 ll of 0.1% (w/v) ferric chloride in concentrated HCl, mixed well and incubated in the boiling water for 20 min. After cooling down, 200 ll of the mixture was transferred to the 96well microtiter plate and the absorbance was determined at 660 nm using a microplate spectrophotometer (Epoch; Bio Tek Instruments). A range of D-glucose (0-100 lg ml À1 ) and D-xylose (0-40 lg ml À1 ) concentrations were used to plot the standard curves for hexoses and pentoses respectively.

Enzymatic hydrolysis
Enzymatic hydrolysis was performed according to NREL Laboratory Analytical Procedure LAP 009. The solid residues of pretreatment and untreated Miscanthus biomass were loaded at a solid concentration of 2.0% (w/v) in a 50 mM citrate buffer (pH 4.8) containing 0.005% (w/v) sodium azide. Cellulase (Celluclast 1.5L; Novozymes, Franklinton, NC, USA) from Trichoderma reesei and beta-glucosidase (Novozyme 188; Novozymes, Bagsvaerd, Denmark) from Aspergillus niger were used for hydrolysis experiments. The enzyme loadings of Celluclast 1.5L and Novozyme 188 were 20 FPU g À1 glucan and 30 CBU g À1 glucan respectively. The hydrolysis experiment was conducted at 50°C and 150 rpm in a shaking incubator for 72 h. After enzymatic hydrolysis, the mixture was centrifuged at 12 000 g for 3 min and the supernatants were collected for measurement of hexose and pentose content. The sugars released were calculated using the following equation: Hexoses related ð% of celluoseÞ ¼ g of hexoses g of glucan added to hydrolysis Â 1:11 Â 100% Pentoses released ð% of hemicelluloseÞ ¼ g of pentoses g of xylan added to hydrolysis Â 1:14 Â 100% Total sugars released ð% of dry biomassÞ ¼ g of hexoses þ g of pentoses g of biomass added to hydrolysis Â 100% The value of 1.11 is the conversion factor of glucan to equivalent glucose. The value of 1.14 is the conversion factor of xylan to equivalent xylose. The total sugars were calculated as the total mass of glucose and xylose released treated and untreated dry biomass.

Statistical analysis
Correlation coefficients were calculated by performing spearman rank correlation analysis. All the experiments were repeated at least three times, and the results were shown as mean AE SDs. Differences between treatments were evaluated, and statistical significance was accepted at P < 0.05.