Skip to main content

Comparative study of sulfite pretreatments for robust enzymatic saccharification of corn cob residue

Abstract

Background

Corn cob residue (CCR) is a kind of waste lignocellulosic material with enormous potential for bioethanol production. The moderated sulphite processes were used to enhance the hydrophily of the material by sulfonation and hydrolysis. The composition, FT-IR spectra, and conductometric titrations of the pretreated materials were measured to characterize variations of the CCR in different sulfite pretreated environments. And the objective of this study is to compare the saccharification rate and yield of the samples caused by these variations.

Results

It was found that the lignin in the CCR (43.2%) had reduced to 37.8%, 38.0%, 35.9%, and 35.5% after the sulfite pretreatment in neutral, acidic, alkaline, and ethanol environments, respectively. The sulfite pretreatments enhanced the glucose yield of the CCR. Moreover, the ethanol sulfite sample had the highest glucose yield (81.2%, based on the cellulose in the treated sample) among the saccharification samples, which was over 10% higher than that of the raw material (70.6%). More sulfonic groups and weak acid groups were produced during the sulfite pretreatments. Meanwhile, the ethanol sulfite treated sample had the highest sulfonic group (0.103 mmol/g) and weak acid groups (1.85 mmol/g) in all sulfite treated samples. In FT-IR spectra, the variation of bands at 1168 and 1190 cm-1 confirmed lignin sulfonation during sulfite pretreatment. The disappearance of the band at 1458 cm-1 implied the methoxyl on lignin had been removed during the sulfite pretreatments.

Conclusions

It can be concluded that the lignin in the CCR can be degraded and sulfonated during the sulfite pretreatments. The pretreatments improve the hydrophility of the samples because of the increase in sulfonic group and weak acid groups, which enhances the glucose yield of the material. The ethanol sulfite pretreatment is the best method for lignin removal and with the highest glucose yield.

Background

Waste lignocellulosic material, which is easily available, inexpensive, and renewable, represents a kind of significant cellulosic biomass as raw material to produce fuel ethanol with many advantages in bioethanol conversion[1]. Corn cob residue (CCR) is a kind of waste lignocellulosic material. During the production of furfural from the lignocellulosic materials with abundant pentose sugars, such as corncob, the hemicelluloses have been hydrolyzed to furfural in a dilute acid environment at high temperature, leaving the lignin and cellulose in the CCR[2]. It has been estimated that about 12–15 tons of CCR can be obtained after 1 ton of furfural is produced, and an average of 23 million tons of CCR were available annually for alternative use in China[3]. However, the residue, considered as waste, are widely utilized for burning at present, far away form resource utilization. It would be a better choice to produce bioethanol with such abundant lignocellulosic waste.

Among the available technologies for lignocelluloses-to-ethanol production, a conversion process based on enzymatic hydrolysis is considered the most promising for large-scale operation[4, 5]. However, one of the key factors to construct the recalcitrance of lignocellulosic biomass is the presence of lignin, which plays the “glue” to bind cellulose and hemicellulose. Besides playing a physical barrier, lignin has also been found to irreversibly adsorb enzymes, which causes enzyme loss and decrease in the saccharification rate[6]. Therefore, delignification is always adopted to overcome the recalcitrance of lignocellulosic biomass and increase the enzymatic digestibility of cellulose.

The effect of lignin content on enzymatic hydrolysis of CCR has been evaluated, and it is found that the glucose yield was improved by increasing the lignin removal. However, the maximum glucose yield of CCR was obtained when the residue with a lignin content of about 21.0%[3]. The results further prove that the chemical and physical structure of lignin plays a significant role in determining the magnitude of inhibition of lignin to hydrolysis. There has been strong evidence[7] supporting the role of hydrophilic interactions in the non-productive binding of cellulases to lignin. Multiple studies[7, 8] have shown that the addition of the surfactant to cellulolytic hydrolysis improved hydrolysis yields. It reported that increasing the carboxylic acid content of the lignin seemed to significantly decrease the non-productive binding of cellulase and consequently increased the enzymatic hydrolysis of the cellulose[9]. So the hydrolysis yields of CCR may be benefited from the enhanced hydrophily of lignin after a temperate pretreatment.

The sulfite process has been used for pretreating wood chips for ethanol production. Sulfonation of lignin increases its hydrophilicity, which will promote the enzymatic hydrolysis process[10, 11]. And the lignosulfonate has been used as pesticide emulsifier, oil field chemicals, dyeing and finishing auxiliaries for textile, which can been obtained from the concentrated sulfite pretreated solution. Traditional sulfite pulping has been in industry practice for more than a century and can be operated over a wide range of pH and temperature. And the active reagents in sulfite pretreatment liquor are also depended on the pH of the pretreatment temperature[12]. Sulfonation is always enhanced because of the acid or alkaline catalysis. The acid sulfite and neutral sulfite pretreatment has been well documented as the SPORL pretreatment[12] with numerous publications to variety of feed stocks. And sulfite pretreated in alkaline environments also can increase the sulfonation and dissolubility of lignin. It has reported that during fraction of spruce by SO2-ethanol-water treatment, lignin is effectively dissolved, whereas cellulose is preserved in the solid (fiber) phase[13]. And the organophilic sulfite pretreatment is also a good choice for lignin separation and sulfonation because of the addition of ethanol, which caused a reduction of the surface tension and a benefit of solution penetration. Moreover, the hydrolysed lignin can be dissolved and recovered in the organophilic phase to obtained high purity lignin.

Our previous study has found that the glucan in CCR was easily degraded in severe pretreated processes. So in this study, the CCR were pretreated with sodium sulfite under moderate condition in acidic, alkaline, neutral, and ethanol environments to enhance the hydrophily of lignin by sulfonation reaction. And the objective is to compare the composition and characteristic variation of CCR during these sulfite pretreatments, and to compare the differences of saccharification rate and yield caused by these variations of the samples.

Results and discussion

Chemical composition of substrates

The variation of the chemical composition in CCR is given in Table1. Glucan (48.1%) and lignin (43.2%) accounted for more than 90% of the CCR, implying that they are the main chemical compositions of the CCR and the hemicelluloses have been mostly removed during furfural production. After the pretreatments, lignin in the CCR had been removed partly, resulting in an increase in glucan proportion. Comparatively speaking, the amount of removed lignin after alkaline and ethanol sulfite pretreatment was higher than that after acidic and neutral sulfite pretreatment. The proportion of lignin in samples after alkaline and ethanol sulfite pretreatment decreased to 35.9% and 35.5%, respectively, which were lower than that in the samples after acidic pretreatment (38.0%) and neutral sulfite pretreatment (37.8%). Moreover, the residual lignin in the treated samples, based on the quality of the untreated CCR, was in according with the results of lignin proportion in pretreated samples. The lowest residual lignin sample was from the alkaline sulfite pretreated sample, only 28.08%.

Table 1 Variation of corn cob residue chemical composition after sulfite pretreatments

The variation of glucan proportion after sulfite pretreatments was not the same as the decrease in lignin proportion. The sample treated with ethanol sulfite had the highest glucan proportion (55.5%), while the values of the neutral and alkaline sulfite pretreated sample were 51.6% and 51.8%, respectively. The sample of acidic sulfite sample had the lowest glucan proportion (49.3%) of all the pretreated samples. However, the residual glucan in all the treated samples had endured a decline, especially the alkaline sulfite pretreated sample (40.47%). The ethanol sulfite pretreated sample had the highest residual glucan (47.01%), a little lower than the glucan proportion in raw material (48.10%).

The ratio of ash increased as the degradation of organic matter (including glucan and lignin) during sulfite pretreatments. The fact that acid soluble lignin in the CCR decreased after sulfite pretreatments was attributed to the solvable lignin with low molecular weight during pretreated process.

Undoubtedly, during sulfite processes, the delignification was realized by the formation of soluble fragments after lignin sulfonation and degradation. The considerable distinctive composition of pretreated samples was attributed to the different active reagents in the sulfite liquor, which depended on its pH and temperature[12, 14]. The nucleophilic reaction of these active reagents resulted in the sulfonation and degradation of lignin in the raw materials[15]. The lignin solubility is connected with the pH value of the pretreated solution. The alkaline solution has better lignin solubility at a higher pH value than the acidic solution with a lower pH value[16]. So, the amount of lignin removal after alkaline pretreatment was more than that after treatment with acidic and neutral sulfite. During the ethanol sulfite pretreatment, the surface tension reduced because of the addition of ethanol, which was a benefit of solution penetration and lignin sulfonation, resulting in more lignin removal[1719]. Moreover, the boiling point of ethanol is lower than that of water; hence, the pressure in the ethanol sulfite pretreated bottle was the highest. These advantages of ethanol sulfite pretreatment enhanced the sulfonation and degradation of lignin. The dissolved lignin can be directly used in various industrial fields as the surfactant after the concentration. It paved a new path for the utilization of the lignin in CCR.

It cannot be neglected that the cellulose can be degraded at acidic or alkaline solution[20, 21]. Because of the acid hydrolysis of cellulose during acidic sulfite pretreatment, the increase in the glucan proportion was the lowest in all sulfite pretreatments. However, the lowest yield and the highest ash amount in the CCR after alkaline sulfite pretreatment was attributed to degradation of organic polymer, not only the removal of lignin, but also the damage of cellulose. The results of residual glucan also supposed these conclusions. However, it can not be neglected that the ethanol sulfite pretreatment had the weakest glucan degradation among these pretreatments. Moreover, the strong vitality of this organic pretreatment is also reflected in the cyclic utilization of ethanol and high purity lignin obtained from the pretreated solution.

Enzymatic saccharification

The glucose concentration of the pretreated CCR was higher than that of the raw CCR (Figure1). The glucose released from the substrates was increased rapidly in the initial stage, while the rate of hydrolysis progressively reduced as the reaction proceeded. The glucose concentration in the raw material saccharification solution reached 6.76 g/L in the first 24 h, which was over 50% of the concentration at 96 h (9.43 g/L). The sulfite pretreated samples shared the same tendency with the CCR without pretreatment, but the glucose concentration in the saccharification solution of these samples was higher than that in the CCR at corresponding hours. After 96 h of enzymatic hydrolysis, the glucose concentration in the ethanol sulfite pretreated sample was the highest (12.56 g/L), and the glucose concentration in the other three samples had approximate values (11.23 g/L, Neutral; 11.02 g/L, Acidic; 11.42 g/L, Alkaline), which were higher than that of the untreated sample.

Figure 1
figure 1

Glucose concentration variation of corn cob residue after sulfite pretreatments. RM represents the raw material of corn cob residue, while Neutral, Acidic, Alkaline and Ethanol represent corn cob residue treated with sulfite in neutral, acidic, alkaline and ethanol environment, respectively.

Similarly, the glucose yield (based on the cellulose in the treated sample) of all the samples experienced a rapid growth in the first 24 h, and the growth moderated from then on (Figure2). And, the glucose yield of the samples after sulfite pretreated was higher than that of untreated CCR. However, as the glucan proportion of the samples was not the same, the difference in glucose yield from the samples was not in accordance with that of glucose concentration. The glucose yield of the CCR without pretreatment was 70.6% after 96 h of enzymatic hydrolysis, which just a littler lower than that of the sample treated with neutral sulfite (74.5%). The ethanol sulfite sample had the highest glucose yield (81.2%) in the saccharification samples, which was over 10% higher than that of the raw material. The acidic sulfite pretreated sample shared a similar glucose yield (78.2%) with the CCR treated with alkaline sulfite (79.4%).

Figure 2
figure 2

Glucose yield variation of corn cob residue after sulfite pretreatments. RM represents the raw material of corn cob residue, while Neutral, Acidic, Alkaline and Ethanol represent corn cob residue treated with sulfite in neutral, acidic, alkaline and ethanol environment, respectively.

It is well known that the physical barrier and non-productive binding to enzyme of lignin is the main problem in CCR enzymatic hydrolysis[22, 23]. After the sulfite pretreatment, part of the lignin had been removed and reduced the barrier of lignin to cellulose enzymatic hydrolysis[24, 25]. More importantly, the sulfonation and degradation of the lignin increased its hydrophilism, which may be favorable to reduce the non-productive binding between lignin and cellulase[7]. Among the four kinds of sulfite pretreatment, the ethanol and alkaline sulfite pretreatment had similar amounts of lignin removal, but the glucose yield of the ethanol sulfite sample was higher than that of the alkaline sulfite treated sample. It may be attributed to the fact that more hydrophilic groups had been introduced in the CCR after ethanol sulfite pretreatment[26]. Moreover, the glucose yield from the acidic sulfite sample was higher than that from neutral when they shared similar lignin proportion. This phenomenon was closely related to the enhanced hydrophily of lignin during the sulfite pretreatment.

The glucose yield of the pretreated samples based on the cellulose in raw material (GPR) can be obtained from the saccharification efficiency together with solid yield in pretreated progresses. All pretreated samples had higher GPR than the raw material expect the alkaline sulfite sample. It should be attributed to the serve degradation of cellulose during the alkaline sulfite pretreatment. The sample treated with ethanol sulfite had the highest GPR (79.34% after 96 h of enzymatic hydrolysis). However, if the soluble lignin had been rationally used, it would be a good choice to adopt these pretreatment, especially the ethanol sulfite pretreatment, which not only can increase the glucose yield of CCR, but also results in a certain amount of lignin solution. Furthermore, the residual of cellulosic hydrolysis may have a good application prospect, as the lignin had been sulfonated during the sulfite pretreatments.

The sulfites pretreatments had enhanced the lignin sulfonation which can not only be benefited to the cellulosic hydrolysis but also bring a good application prospect for lignin (both degraded and residual). So from the whole processes of the biorefineries, the sulfite pretreatment may be a good choice. Moreover, the ethanol sulfite pretreatment presented an appealing effect.

Conductometric titrations

The hydrophility of lignin is intimate connection with its hydrophilic groups. So, in this study, the sulfonic group and weak acid groups of the samples had been measured by conductometric titration. The conductivity titration curves of the raw material and the ethanol sulfite pretreated sample were shown in Figure3a and Figure3b, respectively.

Figure 3
figure 3

Conductivity titration curve of raw material (a) and the ethanol sulfite pretreated sample (b). “A” represents the equivalent point of strong acid, while “B” represents the equivalent point of weak acid groups.

The conductometric titration is based on changes in conductance of the suspension. The resultant conductivity of the suspension was plotted against the volume of alkali added. So, before the equivalent point “A,” the alkali was used to neutralize the hydrogen from HCl added before the titration as well as the sulfonic group in the sample. The content of sulfonic group was the difference between the alkali required to reach the inflection point “A” and the HCl added before the titration. The weak acid groups were calculated using the volume of alkali required to reach the second inflection point “B” from the first inflection point “A” of the plot[27, 28]. And, the total amount of hydrophilic groups was the sum of the sulfonic group and the weak acid groups.

The conductivity titration curves of other samples were similar with that of the ethanol sulfite pretreated sample, but the volumes of alkali required to reach the two inflection points “A” and “B” were different, which implied that the amount of sulfonic group and weak acid groups in these samples was different (Figure4). In the raw material, there was little sulfonic group that may have been introduced during the furfural production with dilute sulphuric acid hydrolysis. And, the amount of weak acid groups was 0.196 mmol/g. The sulfite pretreatments increased the amount of both the sulfonic group and the weak acid groups. The nucleophilic performance of the active agents determines the degree of lignin sulfonation and degradation. During the neutral sulfite pretreatment, the nucleophilic reagents were SO32- and HSO3-, which attracted the ether linkage in lignin resulting in its break and the introduction of the sulfonic acid group. So, the sulfonic group as well as the weak acid groups increased to 0.022 mmol/g and 0.637 mmol/g, repectively, after neutral sulfite treated. Compared with the neutral sulfite pretreatment, the nucleophilic reaction during sulfite treatment in the acidic and alkaline environments was catalyzed by the hydrogen or hydroxyl ions, which was beneficial to the lignin sulfonation and degradation, and their weak acid groups were similar (1.01 mmol/g, acidic; 1.02 mmol/g, alkaline). However, the dissolubility of lignin in the alkaline environment was higher than that in the acidic environment, so the lignin after sulfonate was much easier to dissolve in aqueous alkali, causing lower sulfonic acid group in the alkaline sulfite treated sample (0.039 mmol/g) than in the acidic sample (0.094 mmol/g). The ethanol sulfite treated sample showed the highest sulfonic group (0.103 mmol/g) and weak acid groups (1.85 mmol/g) in all sulfite treated samples. As explained above, the ethanol sulfite pretreatment was beneficial to solution penetration and its reaction with lignin. And, the ethanol may not only provide an alcohol solution environment but also take part in the reaction with lignin. The hydroxyl may have grafted to lignin and increased its hydrophilicity. The increased hydroxyl provided convenience for sulfonation reaction[29], which improved the solubility and amount of removed lignin. The increase in these hydrophilic groups reduced the non-productive binding between lignin and cellulase and enhanced the glucose yield of the ethanol sulfite pretreated sample.

Figure 4
figure 4

Variation of sulfonic group and weak acid groups after sulfite pretreatments. RM represents the raw material of corn cob residue, while Neutral, Acidic, Alkaline and Ethanol represent corn cob residue treated with sulfite in neutral, acidic, alkaline and ethanol environment, respectively.

FT-IR spectra

FT-IR spectroscopy provides information about chemical composition, molecular conformation, and hydrogen bonding patterns of cellulose allomorphs[30]. The FT-IR spectra of the CCR samples are shown in Figure5.

Figure 5
figure 5

FT-IR spectra of samples. ‘a’ represents the raw material of the corn cob residue, while ‘b’, ‘c’, ‘d’, and ‘e’ represent the corn cob residue treated with sulfite in neutral, acidic, alkaline, and ethanol environments, respectively.

The analyses of the recorded spectra of the lignin samples used in this study were all based upon the assignments given by previous investigations[31, 32]. As can be seen from the spectra, all the samples showed broad bands at 3410–3460 and 2897–2905 cm-1, attributed to the stretching of –OH groups and to C–H stretching, respectively, corresponding to the aliphatic moieties in cellulose, and survived lignin. The band around 1715 cm-1 in the spectra, assigned to carbonyl/carboxyl stretching, indicates the existence of the hydrophilic groups in the samples. The bands at 1605 and 1512 cm-1, which are attributed to the skeletal and stretching vibration of benzene rings, became weak in spectra of the sulfite treated samples because of lignin removal during the sulfite pretreatments. The disappearance of the band at 1458 cm-1 (bending vibration of the methoxyl on benzene rings) in the spectra of the samples after pretreatments implied the methoxyl in the lignin had been removed during the sulfite pretreatments. Moreover, this conclusion was confirmed by the variation of the bands at 1270 and 1230 cm-1, which are attributed to the aromatic core of guaiacyl and syringyl, respectively. C–H bending occurs at 1370 (1368) cm -1, and the C–C (C–O) vibration absorption appears at 1328 cm-1. The main differences in the spectra after sulfite pretreatment were the bands at 1168 and 1190 cm-1 (attributed to the absorption of sulfonic group), which were not obvious in the spectrum of the raw material. Furthermore, the fact that the bands were stronger in the spectrum of the ethanol sulfite pretreated sample than the other treated samples indicates that the sulfonation degree of the ethanol sulfite treated sample was the highest, which was according with the result of conductivity titration.

Two absorption bands around 1119 and 899 cm-1 arise from C–O–C stretching at the β-(1–4)-glycosidic linkages[33]. Strong peaks at 1056 (1058) and 1038 cm-1 are indicative of C–O stretching at C-3 and C–C stretching and C–O stretching at C-6[34]. The most important bands that helped to identify the cellulose component are at 1042 cm-1, attributed to amorphous cellulose and crystallized cellulose II, and at 1430 cm-1, attributed to crystallized cellulose I. The band around 1427 cm-1 in the spectra of sulfite treated samples indicated a mixed structure of crystallized cellulose I and amorphous cellulose in all the samples[35]. However, the band of the untreated sample appearing at 1423 cm-1 may imply that the crystallized areas of cellulose in the CCR increased after the sulfite pretreatments. The FT-IR spectra analysis further confirmed that the lignin of the CCR had been removed partly and the lignin had been sulfonated after the sulfite pretreatments. These variations were beneficial to its enzymatic hydrolysis.

Conclusion

The lignin in the CCR (43.2%) reduced to 37.8%, 38.0%, 35.9%, and 35.5% after the sulfite pretreatment in neutral, acidic, alkaline, and ethanol environments, respectively. Meanwhile, the glucan of the CCR increased from 48.1% to 51.6%, 51.8%, 49.3%, and 55.5%, respectively after the corresponding sulfite pretreatment. These results indicate that the ethanol sulfite pretreatment is the best method for lignin removal and has the least cellulose degradation among the selected sulfite methods. The glucose yield (based on the cellulose in the treated sample) of the ethanol sulfite sample was the highest (81.2%) among the saccharification samples, which was over 10% higher than that of the raw material (70.6%). In the raw material, there was a little sulfonic group and weak acid groups, which increased after sulfite pretreatments. Meanwhile, the ethanol sulfite treated sample had the highest sulfonic group (0.103 mmol/g) and weak acid groups (1.85 mmol/g) in all the sulfite treated samples. These variations enhance the hydrophilicity of the samples, which may improve the glucose yield of the samples. In the FT-IR spectra, the variation of bands at 1168 and 1190 cm-1 (attributed to the absorption of the sulfonic group) confirmed lignin sulfonation during sulfite pretreatment. The disappearance of the band 1458 cm-1 in the spectra of the samples after pretreatments implied that the methoxyl in the lignin had been removed during the sulfite pretreatments. So, during the sulfite pretreatments, the lignin in the CCR can be degraded and sulfonated, and the pretreatments improve the hydrophility and enhance the glucose yield of the material. Moreover, the ethanol sulfite pretreatment with higher lignin removal and glucose yield is slightly better than the other sulfite pretreatments.

Methods

Corn cob residue

The corn cob residue (CCR) produced from corn cob was kindly supplied by the Chunlei Furfural Corporation (Hebei, China). The residues, which had a pH of 2 to 3 initially, were immersed in the fresh water for 24 h and then washed with distilled water until neutral to remove acid, furfural and other toxic products to enzyme and yeast. Before milled to a size under 40 meshes, CCR should be dry at 50°C for 12 h. And then the dried materials were stored in sealed bags at room temperature until further processing.

Sulfite pretreatments

The pretreatments were performed in the pressure bottles with screw cap (Synthware Co., Ltd). During neutral sulfite pretreatment, the sodium sulfite (1%, w/v) were added in the bottles with CCR slurry in water (10%, w/v); additionally no other more chemicals was used, and the final pH was 7.5 at normal temperature. When the CCR (10%, w/v) was dispersible in dilute acidic solution (0.5% H2SO4, w/v) before the sodium sulfite (1%, w/v) added, this process was defined as acidic sulfite pretreatment (pH 2.3). The alkaline sulfite pretreatment (pH 12.4) was operated similarly as the acidic sulfite pretreatment, but the dilute acidic solution had been replaced by dilute alkali solution (0.5% NaOH, w/v) to provide alkaline environment. The ethanol sulfite pretreatment was slightly different, and 1% sodium sulfite (w/v) was added in the bottle with CCR (10%, w/v) dispersed in alcohol solution (80%, v/v), with pH 7.9.

The screw caps of the bottles were tightened after the sodium sulfite had been added. Then the bottles were placed in the water bath shaker with 100 rpm at 80°C for 3 h. The mixture in the bottles after pretreatment was filtered to separate the solid residues and the filtrate fraction. The solid residues were thoroughly washed with tap water to neutral pH, then vacuum dried at 50°C, and finally weighed. The pretreated samples after vacuum dry were ground into powder with mortar before analysis. The lignin and glucan contents of CCR as well as pretreated samples were analyzed according to the National Renewable Energy Laboratory (NREL) methods[36].

Enzymatic saccharification

The solid residues obtained from the pretreatment were further submitted to enzymatic hydrolysis. Each enzymatic hydrolysis treatment was preformed at 47°C, pH 4.8 with a substrate concentration of 2.5% (w/v). Cellulase (Celluclast 1.5L, 74FPU/ml, Sigma Co., St. Louis, MO) loading for the CCR was 12 FPU/g-cellulose and the β-glucosidase (Novozyme 188, 175 CBU/ml, Sigma Co., St. Louis, MO) loading was 15 CBU/g-cellulose. The hydrolysis of CCR without pretreatment was performed as control. The saccharification was cultivated on a rotary shaker at 180 rpm for 96 h. Samples were withdrawn and centrifuged at 10000×g for 5 min. The hydrolysates were filtered through 0.2 um filters and diluted properly for further neutral sugar analysis.

Analysis

The neutral sugars during saccharification process were analyzed by HPLC (Waters 2695e, USA) with Aminex HPX-87P (300×7.8 mm, Bio-Rad, USA) at 85°C and refractive index detection detector at 35°C. The injection volume of the sample was 10 μL, and distilled water was used as the eluent, at a flow rate of 0.6 ml/min. The glucose yield was calculated assuming that 1 g cellulose present in the liquid theoretically gave 1.11 g of glucose. Assays were performed in 3 repeated experiments, and the mean values are calculated.

The conductometric titrations were used to detect the content of weak acid groups and sulfonic group in the samples. Before the conductometric titrations, the ground CCR samples were converted to their fully protonated form by soaking the samples at 1% consistency in 0.01 M hydrochloric acid for 16 h. The samples with pH close to 2.2 after 16 h of soaking were then vacuum-filtered using a Buchner funnel and washed several times with deionized water until the pH of the water filtrate was close to 6.0. The vacuum was maintained until no more water could be extracted from the CCR samples. Approximately 0.5 g of the protonated CCR sample was dispersed in 1 mM sodium chloride (100 ml) and addition of 0.5 ml of 0.05M HCl was made before the start of titration. The titration was performed with 5 mM NaOH in a constant temperature water bath set at 25°C. The conductivity meter (DDSJ-308A, Shanghai Precision & Scientific Instrument Co. Ltd.) was exploited to detect the variation of the conductance during the titration[27]. The content of sulfonic groups (SG) and weak acid groups (WAG) were calculated according to the following formulas:

S G = c 2 * V 2 c 1 * V 1 / m m mol / g ; W A G = c 2 * V 3 c 2 * V 2 / m m mol / g .

In which, c 1 is the concentration of HCl solution (mol/L); V 1 is the volume of HCl solution addition (ml); c 2 is the concentration of NaOH solution (mol/L); V 2 is the consumed volume of NaOH solution before first equivalent point (ml); V 3 is the consumed volume of NaOH solution before second equivalent point (ml); m is quality of the tested sample.

The FT-IR spectra of ground samples the lignin fractions were obtained on a Nicolet-750 FT-IR spectrophotometer using KBr discs containing 1% finely ground samples in the range of 4000–400 cm-1.

Abbreviations

CCR:

Corn cob residue

GPR:

Glucose yield of the pretreated samples based on the cellulose in raw material

NREL:

National Renewable Energy Laboratory

SG:

Sulfonic groups

WAG:

Weak acid groups.

References

  1. Draude KM, Kurniawan CB, Duff SJ: Effect oxygen delignification on the rate and extent of enzymatic hydrolysis of lignocellulosic material. Bioresour Technol 2001, 79: 113-120. 10.1016/S0960-8524(01)00055-4

    Article  CAS  Google Scholar 

  2. Bu LX, Tang Y, Gao YX, Jian HL, Sun RC, Jiang JX: Comparative characterization of milled wood lignin from furfural residues and corncob. Chem Eng J 2011,175(15):176-184.

    Article  CAS  Google Scholar 

  3. Sun R, Song XL, Sun RC, Jiang JX: Effect of lignin content on enzymatic hydrolysis of furfural residues. Bioresources 2011,6(1):317-328.

    CAS  Google Scholar 

  4. Hahn-Hägerdal B, Galbe M, Gorwa-Grauslund MF, Liden G, Zacchi G: Bio-ethanol—the fuel of tomorrow from the residues of today. Trends Biotechnol 2006, 24: 549-556. 10.1016/j.tibtech.2006.10.004

    Article  Google Scholar 

  5. Qi BK, Chen XR, Wan YH: Pretreatment of wheat straw by nonionic surfactant-assisted dilute acid for enhancing enzymatic hydrolysis and ethanol production. Bioresour Technol 2010, 101: 4875-4883. 10.1016/j.biortech.2010.01.063

    Article  CAS  Google Scholar 

  6. Zhao XB, Song YQ, Liu DH: Enzymatic hydrolysis and simultaneous saccharification and fermentation of alkali/peracetic acid-pretreated sugarcane bagasse for ethanol and 2, 3-bultanediol production. Enzyme Microb Tech 2011, 49: 413-419. 10.1016/j.enzmictec.2011.07.003

    Article  CAS  Google Scholar 

  7. Eriksson T, Börjesson J, Tjerneld F: Mechanism of surfactant effect in enzymatic hydrolysis of lignocellulose. Enzyme Microb Technol 2002, 31: 353-364. 10.1016/S0141-0229(02)00134-5

    Article  CAS  Google Scholar 

  8. Yang B, Wyman CE: BSA treatment to enhance enzymatic hydrolysis of cellulose in lignin containing substrates. Biotechnol Bioeng 2006, 94: 611-617. 10.1002/bit.20750

    Article  CAS  Google Scholar 

  9. Nakagame S, Chandra RP, Kadla JF, Saddler JN: Enhancing the enzymatic hydrolysis of lignocellulosic biomass by increasing the carboxylic acid content of the associated lignin. Biotechnol Bioeng 2011, 108: 538-548. 10.1002/bit.22981

    Article  CAS  Google Scholar 

  10. Cheng KK, Wang W, Zhang JA, Zhao Q, Li JP, Xue JW: Statistical optimization of sulfite pretreatment of corncob residues for high concentration ethanol production. Bioresour Technol 2011, 102: 3014-3019. 10.1016/j.biortech.2010.09.117

    Article  CAS  Google Scholar 

  11. Shuai L, Yang Q, Zhu JY, Lu FC, Weimer PJ, Palph J, Pan XJ: Comparative study of SPORL and dilute-acid pretreatments of spruce for cellulosic ethanol production. Bioresour Technol 2010, 101: 3106-3114. 10.1016/j.biortech.2009.12.044

    Article  CAS  Google Scholar 

  12. Zhu JY, Pan XJ, Wang GS, Gleisner R: Sulfite pretreatment (SPORL) for robust enzymatic saccharification of spruce and red pine. Bioresour Technol 2009, 100: 2411-2418. 10.1016/j.biortech.2008.10.057

    Article  CAS  Google Scholar 

  13. Mikhail L, Adriaan VH: Efficient fractionation ofspruceby SO2-ethanol-water treatment: closed mass balances for carbohydrates and sulfur. ChemSusChem 2012, 5: 1625-1637. 10.1002/cssc.201100600

    Article  Google Scholar 

  14. Mendonca R, Ferraz A, Kordsachia O, Patt R: Alkaline sulfite/anthraquinone pulping of pine wood chips biotreated with ceriporiopsis subvermispora. J Chem Technol Biot 2004, 79: 584-589. 10.1002/jctb.1024

    Article  CAS  Google Scholar 

  15. James P: Casey: Pulp and paper science and technology. I edition. New York: Pulp. Interscience; 1960.

    Google Scholar 

  16. Ghatak HR, Kundu PP, Kumar S: Thermochemical comparison of lignin separated by electrolysis and acid precipitation from soda black liquor of agricultural residues. Thermochim Acta 2010, 502: 85-89. 10.1016/j.tca.2010.02.012

    Article  CAS  Google Scholar 

  17. Yawalata D, Paszner L: Characteristics of NAEM salt-catalyzed alcohol organosolv pulping as a biorefinery. Holzforschung 2006, 60: 230-244.

    Article  Google Scholar 

  18. Wei H, Ulkem N, Berk D, Kubes GJ: Neutral sulphite pulping with surfactants. J Pulp Pap Sci 2005, 31: 188-192.

    CAS  Google Scholar 

  19. Lakovlev M: Va Heiningen A: Kinetics of fractionation by SO2-ethanol-water (SEW) treatment: understanding the deconstruction of spruce wood chips. RSC Advances 2012, 7: 3057-3068.

    Article  Google Scholar 

  20. Cara C, Ruiz E, Oliva JM, Saez F, Castro E: Conversion of olive tree biomass intofermentable sugars by dilute acid pretreatment and enzymatic saccharification. Bioresource Technol 2007, 99: 1869-1876.

    Article  Google Scholar 

  21. Kassim EA, El-Shahed AS: Enzymatic and chemical hydrolysis of certain cellulosic materials. Agr Wastes 1986, 17: 229-233. 10.1016/0141-4607(86)90097-1

    Article  CAS  Google Scholar 

  22. Rabinobich ML, Melnick MS, Bolobova AV: The structure and mechanism of action of cellulolytic enzymes. Biochem 2002, 67: 850-871.

    Google Scholar 

  23. Seiji N, Richard PC, Jack NS: The influence of lignin on the enzymatic hydrolysis of pretreated biomass substrates. Washington, DC: American Chemical Society; 2011:145-167.

    Google Scholar 

  24. Bansal P, Hall M, Realff MJ, Lee JH, Bommarius AS: Modeling Cellulase kinetics on lignocellulosic substrates. Biotechnol Adv 2009, 27: 833-848. 10.1016/j.biotechadv.2009.06.005

    Article  CAS  Google Scholar 

  25. Kumar L, Chandra R, Saddler J: Influence of steam pretreatment severity on post-treatments used to enhance the enzymatic hydrolysis of pretreated softwoods at low enzyme loadings. Biotechnol Bioeng 2011, 108: 2300-2311. 10.1002/bit.23185

    Article  CAS  Google Scholar 

  26. Norde W: Adsorption of proteins from solution at the solid–liquid interface. Adv Colloid Interfac 1986,25(C):267-340.

    Article  CAS  Google Scholar 

  27. Bhardwai NK, Duong TD, Hoang V, Nguyen KL: Determination of fiber charge components of Lo-Solids unbleached kraft pulps. J Colloid Interf Sci 2004, 274: 543-549. 10.1016/j.jcis.2003.12.062

    Article  Google Scholar 

  28. Stark NM, Matuana LM: Characterization of weathered wood-plastic composite surfaces using FTIR spectroscopy, contact angle, and XPS. Polymer Degrad Stabil 2007, 92: 2677-2687.

    Article  Google Scholar 

  29. Ouyang XP, Ke LX, Qiu XQ, Guo YX, Pang YX: Sulfonation of alkali lignin and its potential use in dispersant for cement. J Disper Sci Technol 2009, 30: 1-6. 10.1080/01932690802473560

    Article  CAS  Google Scholar 

  30. Wang K, Jiang JX, Xu F, Sun RC: Influence of steaming pressure on steam explosion pretreatment of Lespedeza stalks (Lespedeza crytobotrya): part 1. Characteristics of degraded cellulose. Polym Degrad Stabil 2009, 94: 1379-1388. 10.1016/j.polymdegradstab.2009.05.019

    Article  CAS  Google Scholar 

  31. Kaparaju P, Felby C: Characterization of lignin during oxidative and hydrothermal pre-treatment processes of wheat straw and corn stover. Bioresource Technol 2010, 101: 3175-3181. 10.1016/j.biortech.2009.12.008

    Article  CAS  Google Scholar 

  32. Nadji H, Diouf PN, Benaboura A, Bedard Y, Riedl B, Stevanovic T: Comparative study of lignins isolated from Alfa grass (Stipa tenacissima L.). Bioresource Technol 2009, 100: 3585-3592. 10.1016/j.biortech.2009.01.074

    Article  CAS  Google Scholar 

  33. Oh SY, Yoo DI, Shin Y, Kim HC, Kim HY, Chung YS, Park WH, Youk JH: Crystalline structure analysis of cellulose treated with sodium hydroxide and carbon dioxide by means of X-ray diffraction and FTIR spectroscopy. Carbohydr Res 2005, 340: 2376-2391. 10.1016/j.carres.2005.08.007

    Article  CAS  Google Scholar 

  34. Liu CF, Xu F, Sun JX, Ren JL, Curling S, Sun RC, Fowler P, Baird MS: Physicochemical characterization of cellulose from perennial ryegrass leaves (Lolium perenne). Carbohydr Res 2006, 341: 2677-2687. 10.1016/j.carres.2006.07.008

    Article  CAS  Google Scholar 

  35. Jiang JX, Tang Y, Wang K, Bu LX: Influence of Steam Pretreatment Time on Chemical Composition and Simultaneous Saccharification and Fermentation for Ethanol From pruning Shrub Stalks. J Biobased Marer Bio 2011, 5: 258-264. 10.1166/jbmb.2011.1133

    Article  CAS  Google Scholar 

  36. Sluiter A, Hames B, Ruiz R: National Renewable Energy Laboratory (NREL): Determination of Structural Carbohydrates and Lignin in Biomass. USA; 2008. http://www.nrel.gov/biomass/analytical_procedures.html#lap-002

    Google Scholar 

Download references

Acknowledgement

The authors are grateful for the financial support of this research from the Fundamental Research Funds for the Central Universities (200–1242331), National Science Foundation of China (31070510) and Major State Basic Research Projects of China (973-2010CB732204).

Author information

Authors and Affiliations

Authors

Corresponding author

Correspondence to Jianxin Jiang.

Additional information

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

BL and JJ designed and coordinated the study; BL, XY and GY carried out the experiments; BL and YH analyzed the results; BL and XY wrote the paper; JJ and YH reviewed the paper. All authors read and approved the final manuscript.

Authors’ original submitted files for images

Rights and permissions

Open Access This article is published under license to BioMed Central Ltd. This is an Open Access article is distributed under the terms of the Creative Commons Attribution License ( https://creativecommons.org/licenses/by/2.0 ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Reprints and permissions

About this article

Cite this article

Bu, L., Xing, Y., Yu, H. et al. Comparative study of sulfite pretreatments for robust enzymatic saccharification of corn cob residue. Biotechnol Biofuels 5, 87 (2012). https://doi.org/10.1186/1754-6834-5-87

Download citation

  • Received:

  • Accepted:

  • Published:

  • DOI: https://doi.org/10.1186/1754-6834-5-87

Keywords