Abstract
Paecilomyces variotii xylanase was, produced in stirred tank bioreactor with yield of 760 U/mL and purified using 70% ammonium sulfate precipitation and ultra-filtration causing 3.29-fold purification with 34.47% activity recovery. The enzyme purity was analyzed on sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS-PAGE) confirming its monomeric nature as single band at 32 KDa. Zymography showed xylan hydrolysis activity at the same band. The purified enzyme had optimum activity at 60 °C and pH 5.0. The pH stability range was 5–9 and the temperature stability was up 70 °C. Fe2+and Fe3+ exhibited inhibition of xylanase enzyme while Cu2+, Ca2+, Mg2+ and Mn2+ stimulated its activity. Mercaptoethanol stimulated its activity; however, Na2-EDTA and SDS inhibited its activity. The purified xylanase could hydrolyze beechwood xylan but not carboxymethyl cellulose (CMC), avicel or soluble starch. Paecilomyces variotii xylanase Km and Vmax for beechwood were determined to be 3.33 mg/mL and 5555 U/mg, respectively. The produced xylanase enzyme applied on beech xylan resulted in different types of XOS. The antioxidant activity of xylo-oligosaccharides increased from 15.22 to 70.57% when the extract concentration was increased from 0.1 to 1.5 mg/mL. The enzyme characteristics and kinetic parameters indicated its high efficiency in the hydrolysis of xylan and its potential effectiveness in lignocellulosic hydrolysis and other industrial application. It also suggests the potential of xylanase enzyme for production of XOS from biomass which are useful in food and pharmaceutical industries.
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Discover the latest articles, news and stories from top researchers in related subjects.Introduction
Endo-1,4-β-D-xylanases (EC 3.2.1.8) hydrolyze the β-1,4-xylosidic bonds of the hemicellulose xylan backbone to produce xylo-oligosaccharides (XOS), while β-D-xylosidases hydrolyze the non-reducing ends of XOS to produce xylose1,2,3. According to amino acid sequence and catalytic domain analysis, endoxylanase belong to the glycoside hydrolase (GH) families 10 and 11, however, they also have been mentioned in GH families (5, 7, 8, 16, 26, 30, 43, 52 and 62)4,5. Xylanases have been reported to be potentially applicable in industry. They can be used in food industry such as manufacture of bread, dough, juice and beer6,7. They can be used in pharmaceutical production as well2. Kumar and Satyanarayana8 reported the application of xylanases in the paper and pulp industry. Biorefineries also involve xylanases in ethanol production9.
Enzymatic hydrolysis of xylan to generate XOS is one important application of xylanase. XOS has a branched structure comprising b-(1,4) bonded 2–7 xylose units and a number of substituent’s such as acetyl groups, uronic acids and arabinose units. The enzymatic production of XOS is beneficial because it does not contain significant amounts of harmful by-products or monosaccharides10. XOS has a broad diversity of biological functions, such as promoting the production of beneficial bacteria (bifidobacteria and lactobacilli)11, enhancing calcium absorption, reducing colon cancer risk, immune-modulatory and anti-infective properties, blood and skin effects, and antimicrobial actions12. XOS aren’t hydrolyzed in the upper part of the gastrointestinal tract and they selectively stimulate the growth or activity of one or a limited number of bacteria in the colon and thus improve health13. They also have many essential medicinal uses, such as dermatological applications, antioxidant activity, anti-histaminic and anti-inflammatory properties, immune-modulatory effects, cosmetic applications, cytotoxic activity14.
Filamentous fungi were reported to be potential source of enzyme production15. Paecilomyces variotii is the asexual state of Byssochlamys spectabilis, a member of the Phylum Ascomycota (Family Trichocomaceae)16. Paecilomyces has high growth sporulation rates and grows over a wide range of temperatures andsubstrates. As a result, its rapid multiplication ensures viable and affordable development of commercial formulations17. Thermophilic fungi are apotential source of thermotolerant enzyme18.
There are very few studies on xylanase production by Paecilomyces variotti19. The present study represents production, purification and characterization of xylanase enzyme produced from Paecilomyces variotii. The purified xylanase enzyme was observed to be thermophilic, alkalophilic enzyme which has high specific activity, efficiency, and affinity to xylan substrate compared to other xylanases reported in literature. It also aimed to use the produced xylanase enzyme to produce XOS from beechwood xylan and evaluate its antioxidant properties to be applied in nutraceutical industries.
Materials and methods
Microbial strain
This study used Paecilomyces variotii NRRL 1115, collected from the Culture Collection of the Agricultural Research Service (ARS) (Peoria, Illinois, USA).
Preparation of inoculum
Spores reserved in fungal stock solution (20% glycerol, 10% lactose) at − 80 °C were thawed and 150 μL were spread in a Petri dish containing potato dextrose agar (PDA) medium. The plates were incubated at 30 °C for 7 days. The spores were scraped with distilled water, giving a final concentration of approximately 3 × 107 spores/mL.
Preparation of cell pellets
Cell pellets for seeding submerged fermentation in stirred tanks were prepared by inoculating spores (3 × 108) in a shake-flask containing 150 mL of the preculture medium, which contained only glucose (10 g/L) as the carbon source (no glycerol and wheat bran) and all other medium components as the fermentation medium. After inoculation, the flask was incubated at 30 °C on a rotatory shaker at 200 rpm for 48 h.
Xylanase production in stirred tank bioreactor
A 3-L stirred-tank reactor (STR) containing 1.5 L of the fermentation medium (g/L) was studied for batch fermentation: 5 glycerol, 3.5 wheat bran, 7.5 corn steep liquor, 1 NaNO3, 0.3 K2HPO4, 0.1 KCl, MgSO4·7H2O, and 0.01 FeSO4·7H2O. The bioreactor was inoculated with 150 mL of preformed cell pellets after autoclaving at 121 °C for 30 min and operated at 30 °C with aeration at 2 vvm and agitation at 450 rpm. During the fermentation, the medium pH was not controlled. To control foaming, silicone antifoam 204 (Sigma-Aldrich) was added as required. Broth samples were taken on 8th days and assayed for their β-glucosidase activities after removing the mycelia by centrifugation.
Purification of xylanase
Ammonium sulphate was added slowly with stirring to the crude enzyme togive 60% saturation at 4 °C, allowed to stir for 60 min, and then allowed to stand for 24 h at 4 °C. After centrifugation at 10,000 rpm for 20 min, supernatant was decanted, and the precipitate was discarded. Ammonium sulfate was added to bring supernatant to 70% saturation under the same conditions. After centrifugation at 10,000 rpm for 20 min, supernatant was decanted, and the precipitate was dissolved in 10 mL, 0.05 M citrate buffer (pH 5), and then dialyzed against the same buffer for 48 h. Then the clear supernatant was concentrated by ultrafiltration using Amicon Ultra centrifugal filters MWCO 10 kDa. The purity was checked using SDS-PAGE.
SDS-PAGE and zymogram analysis
After ultra-filtration, sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) zymography was applied20. SDS-PAGE was carried out using 10% polyacrylamide in the gel, β-mercaptoethanolwas not added to the samples21. On completion of electrophoresis, the gel was cut in two parts. One part was used for Coomassie brilliant blue staining and the other was used for zymography.
Zymography was done according to Kumar et al.22. The gel was soaked inside 50 mM sodium phosphate buffer (pH 7.0) containing 25% isopropanol 25% for 30 min at 4 °C. Then, the gel was removed and placed in the same buffer containing 1.0% beechwood xylan substrate at 37 °C for 30 min. 0.1% Congo red and 1 M NaCl were used for staining and de-staining of the gel, respectively. Decolorized bands of the red background indicated xylanase activity.
Measurement of xylanase and protein activity
Xylanase activity was assayed using xylan from beech wood (Sigma-Aldrich, Egypt) as substrate. 0.95 mL of 1% (xylan) in 0.05 M citrate buffer, (pH 5) was incubated with 0.05 mL of diluted crude enzyme extract at 50 °C for 15 min. Then the reaction was stopped using 0.5 mL of 3,5-dinitrosalicylic acid (DNS) reagent. The contents are boiled on water bath for 5 min. The absorbance was measured at 575 nm after cooling. The absorbance was compared to that of a substrate control123. One international unit (IU) of xylanase activity is defined as the amount of enzyme catalyzing the release of 1 μmol/min of reducing sugar equivalent to xylose under the specified assay condition24. Using a protein assay kit (BioRad Laboratories, USA) with bovine serum albumin as the standard, the total protein concentration was evaluated25.
Characterization of xylanase
The molecular weight of xylanase was confirmed by comparison with standard protein markers (Blue stain protein ladder, (20–245) KDa, Gold Biotechnology, USA) separated by SDS-PAGE. To determine optimum temperature, xylanase activity was measured attemperatures ranging from 30 °C to 80 °C in 0.05 M citrate buffer at pH 5. To determine the optimum pH, xylanase activity was measured at 50 °C citrate buffer at pH 3 to 6 and phosphate buffer at pH 7 and 8. Temperature stability was determined by measuring the residual activity after incubating the enzyme in 0.05 M citrate buffer pH 5 at various temperatures (30–80 °C) for 30 min. The pH stability was determined by measuring the remaining activity after incubating the enzyme in series of buffer at pH range of 3 to 9 at 4 °C for 24 h. Effect of metals on the activity of purified xylanase was measured by incubating the enzyme with 5 mM of various metal ions (Zn2+, Ca2+, K+, Mg2+, Mn2+, Cu2+, Na+, Co2+) in 0.05 M pH 5 citrate buffer for 60 min at 30 °C. Then, the residual enzymatic activity was measured. Effect of other chemicals on the activity of purified xylanase was measured by incubating the enzyme with 5 mM of the following compounds (Na2-EDTA, SDS, urea, dimethylsulfoxide (DMSO), mercaptoethanol and citric acid) in the 0.05 M citrate buffer (pH 5) for 60 min at (30 °C). Then, the residual enzymatic activity was measured.
Substrate specificity for purified xylanase was investigated by incubating the enzyme with a 1% (w/v) of the following polysaccharides (beechwood xylan, CM-cellulose, Avicel, pectin and starch) in 0.05 M pH 5 citrate buffer for 60 min at 30 °C. The initial hydrolysis rate of beechwood xylan at different substrate concentrations (1, 2, 5, 10 and 20 mg/mL) prepared in 0.05 M citrate buffer, pH 5.0 at 50 °C was used to study the enzyme kinetics. The Michaelis constant (Km) and maximum velocity (Vmax) values were calculated according to Lineweaver and Burk by linear regression from double-reciprocal plots26.
Analysis of xylo-oligosaccharides produced by xylanase enzyme hydrolysis of xylan
Fifty µL of xylanase was incubated with 1% w/v beechwood xylan in 0.05 M citrate buffer (pH 5) at 55 °C. Aliquots were withdrawn at intervals and boiled for 5 min. Control without enzyme was performed in parallel. Samples were analyzed by HPLC (HPLC, Shimadzu Class-VPV 5.03 (Kyoto, Japan) on an HPX-87H column (300 mm × 7.8 mm). The eluent was HPLC grade DI-water with a flow rate of 0.5 mL/min at 70 °C. Sugars were detected by a refractive index detector (Shodex, RI-101). Xylo-oligosaccharides (xylobiose, X2; xylotriose, X3; xylotetraose, X4; xylopentaose, X5; xylohexaose, X6) and xylose were used as standards for the analysis of the reaction products27.
Antioxidant activity of xylo-oligosaccharides
Using the scavenging effect of radicals on DPPH, antioxidant activity can be monitored. 1 mL of the beechwood hydrolysis products (xylo-oligosaccharides) was mixed with 1 mL of 0.04 mg/mL DPPH solution. The reaction was monitored after 15 min. Absorbance at 517 nm was used to calculate radical scavenging activity (% of inhibition) with the formula.
Inhibition (%) = 1 – Absample − Abblank/Abcontrol − Abblank × 100.
where Ab sample was the absorbance of the reaction in presence of sample (sample + DPPH solution), Ab blank was the absorbance of the blank for each sample dilution (sample + DPPH solvent) and Ab control was the absorbance of control reaction (sample solvent + DPPH solution). Then, this value obtained for every concentration was plotted to obtain IC50 values in each time point28.
Statistical analysis
All data were subjected to analysis of variance (ANOVA). Three samples of each item were analyzed and the main values as well as the SD were given. Significance of the variable mean differences was determined using Duncan’s multiple range tests (p ≤ 0.05). All analyses were carried out using SPSS 16 software.
Ethical statements
The manuscript does not contain experiments using human study.
Results and discussion
Production and purification of xylanase enzyme
Table 1 shows that the activity of xylanase enzyme produced in stirred tank bioreactor was 760 U/mL. The enzyme was purified by precipitation using 70% saturated ammonium sulfate solution. The precipitated enzyme was concentrated by ultra-filtration (Amicon Ultra-3 kDa, Millipore). The purification protocol led to a 3.29-fold increase in purity with 34.47% xylanase yield (recovery). The specific enzyme activity of the purified enzyme fraction was 3968 U/mg protein. It is one of the highest specific activities ever reported for xylanase29,30,31,32.
Characterization of xylanase
Determination of the molecular weight
Purified xylanase migrated as a single band on SDS-PAGE suggesting that the purified xylanase was a monomer consisting of a single polypeptide chain. The molecular weight of the xylanase was 32 kDa. The activity of purified xylanase was confirmed through zymography, which showed decolorization of the red background at 32 kDa, which confirmed the enzyme activity at that band (Fig. 1).
According to (Wang et al.,)33, who reported that low molecular weight xylanase is at the range of 21–34 kDa, this xylanase is considered to low molecular weight for xylanases. The low molecular weight of our purified xylanase was identical to the enzyme reported from an Aspergillus mutant strain34, Bacillus subtilis35, and Trichoderma inhamatum9. A higher molecular weight xylanase was reported for Bacillus pumilus36, for Bacillus sp. GRE737 and for Paenibacillus campinasensis BL1138. For the pulp and paper industry, low molecular weight xylanases are favored as they can penetrate pulp fibers more easily than higher molecular weight39.
Effect of temperature on xylanase activity and stability
The enzyme activity increased as temperature increased reaching a maximum activity at 60 °C, then activity declined at 70 and 80 °C, reaching 57% of its maximum activity at 80 °C (Fig. 2). The observed optimum temperature lies in the same range (50–60 °C) of most reported xylanases35.
Regarding thermal stability, 80% of enzyme activity was retained after incubation for 30 min at 60 °C. Only 68% and 55% of activity was retained after incubation for 30 min at 70 and 80 °C, respectively (Fig. 3). Our strain is relatively stable compared to xylanases from other Aspergillus species. Xylanase purified from A. phoenicis40 and A. giganteus41 exhibited half-lifes of only 25 and 13 min at 50 °C, respectively. Thermal stability is correlated to intermolecular bonds such as hydrogen and disulfide bonds and molecular interactions such as electrostatic and hydrophobic interactions. Studying these stabilizing factors is beneficial in re-engineering of mesophilic enzymes to more stable a enzymes42. Temperature stability is required in industrial applications, especially in biomass hydrolysis, which is carried out under high temperature43.
Effect of pH on xylanase activity and stability
The pH range of 5 to 6 was suitable for enzyme activity with optimum at pH 5 (Fig. 4) nearly similar to A. kawachii (pH 5.5)44, A. nidulans (pH 6.0)45 and A. foetidus (pH 5.3)3. This result confirmed the suitability of P. variotii xylanase for use in juice manufacture in which acidic pH is favorable46.
Xylanase enzyme retained 100% activity at pH 5–6, while 87%, 75% and 62% of activity was retained when assayed at pH 7, 8 and 9 respectively, after 24 h incubation (Fig. 5). The pH stability of xylanase from Aspergillus were different it ranged from pH (2 to 7) in case of A. ochraceus47, (4.5 to 6) in case of A. niveus, pH (6.0 to 8.0) in case of A. fumigatus48 and pH (7 to 9) in case of A. carneus M3449. The pulp bleaching process is usually carried out in a high temperature (60–80 °C) and high pH (8–10) atmosphere50, therefore, the xylanases for this application are required to be thermophilic, thermostable, alkaliphilic, and alkali-stable51.
Effect of metals on xylanase activity
Solution of different metal ions at 5 mM concentration was added to purified xylanase and their effects on xylanase activity are summarized in Table 2. Xylanase activity increased by 32% with Cu2+, 20% with Mn2+, 15% with Mg2+, and 13% with Ca2+; similar increases in activity in the presence of Cu2+ have been reported for xylanase purified from A. niger30 and A. ficuum52. In contrast, xylanases from A. giganteus53, Sorangium cellulosum32 and Geobacillus thermoleovorans54 were inhibited by copper. Enhancement of activity by Mn2+ was also reported for PXII-1 xylanase purified from A. awamori PXII-155 and for Xyn11NX xylanase purified from Nesterenkonia xinjiangensis56. (Hmida-Sayari et al.,57) also reported that Mg2+ improved the xylanase activity purified from A. niger by 12%. This may be due to structural stability induced by Mg2+58. Increases in activity in the presence of Ca2+ was also reported for xylanase purified from A. niger30 (Elgharbi et al., 2015). These metals may serve as a cofactor in the enzyme–substrate reaction6,59,60. Calcium also protects xylanase from proteinase inactivation and thermal unfolding61.
The metal ions Co2+, Zn2+, K+, Fe2+, Fe3+ reduced xylanase activity by 8%, 11%, 7%, 37%, and 48%, respectively, at concentrations of 5 mM. The inactivation of xylanase enzyme by the addition of salts of heavy metals such as Fe2+ and Fe3+ is well known. Yi et al.62 reported that Fe2+ inhibited activity of xylanases of Aspergillus sp. This inhibition may be due to nonspecific salt formation with the enzyme36,63. Metal ion interaction with SH or carboxyl groups will alter protein configuration64.
Effect of chemicals on xylanase activity
Table 3 shows the effects of 5 mM solutions of different chemicals on the enzyme activity. β-mercaptoethanol, due to its reducing activity, enhanced enzyme activity by 55%. Moreira et al.65 also reported enhancement of activity by β-mercaptoethanol for xylanase from A. terrus. This could be attributed to the prevention of oxidation of the thiol group in the enzyme66,67. Vieira Cardoso and Ferreira Filho68, also related the protection of cysteine residues from oxidation by mercaptoethanol and this maintain tertiary structure of the active site in Penicillium citrinum and Acrophialophor anainiana xylanases, respectively.
EDTA decreased P. variotii xylanase activity by 25% similar to A. giganteus xylanase53. This may be explained by the enhancement of xylanase activity by some metal ions for xylanase activity, as was observed in this study. Since EDTA is a metal chelator, decreased xylanase activity would be expected in the presence of EDTA66. SDS reduced activity by 77%. This large decrease in activity by SDS, which is an anionic surfactant, confirms the importance of hydrophobic interactions for stabilization of enzyme structure69. Hmida-Sayari et al.57 also reported that SDS decreased activity of xylanase enzyme purified from A. niger by 80%.
Substrate specificity
The greatest activity (5230 U/ml) was observed with beechwood xylan, which contains β-1,4 linkages between D-xylose residues70. The residual activity was 7.2% for pectin. This may be due to presence of xylan residues in pectin71. The enzyme was completely inactive with starch, avicel and carboxy-methyl cellulose sodium salt as substrates (Table 4). The same results were obtained by Chen et al.,72 who also observed that a xylanase enzyme produced from A. niger had no activity towards starch, Avicel and carboxy-methyl cellulose. Bai et al.,73 also reported that xylanase from Bacillus was inactive towards CMC, pectin, and starch.It has been suggested that shape recognition of the polysaccharide chain conformation plays a role in polysaccharidase speci¢city. Xylanase recognize the threefold helical structure of xylan as substrate and didn’t recognize the flat ribbon like conformation of cellulose74.
Determination of kinetic parameters of xylanase
The hydrolytic activity of the purified xylanase was measured using beechwood xylan as a substrate at concentrations of 1, 2, 5, 10 and 20 mg/mL. The xylanase was observed to exhibit Michaelis–Menten Kinetics. The Km and Vmax values obtained from the Lineweaver–Burk plot for beechwood xylan were 3.33 mg/mL and 5555 U/mg respectively (Fig. 6). Xylanase produced in our study was shown to have low Km 3.33 mg/mL and very high Vmax 5555 U/mg compared to A. terrus, A. fumigatus, A. kawachii, Penicillium glabrum, Sorangium cellulosum and Saccharopolyspora pathumthaniensis which have Km (2.09, 3.12, 10, 3.1, 26.5 and 3.92) and Vmax (640, 2587, 1250, 194,7.89 and 256) respectively29,30,31,32,75. Table 5 A low Km indicated high affinity to substrate while high Vmax indicate high enzyme activity. Km and Vmax values were in the range of reported literature (0.09 to 40.9 mg/L for Km) and (0.106 to 10,000 U/mg for Vmax), respectively.
Analysis of xylooligosaccharides produced by xylanase enzyme hydrolysis of xylan
The hydrolytic constituents of insoluble beechwood xylan incubated with xylanase were identified to give better understanding of the mode of action of purified xylanase. The concentrations of XOS from hydrolysis for different times are depicted in Fig. 7. The XOS produced with xylan hydrolysis by xylanase secreted by P. variotti mainly were composed of xylobiose (X2), xylotriose (X3), and xylotetrose(X4), together with a small amount of xylopentaose (X5) and xylohexose (X6) and xylose (X1).
The accumulation of XOS in the hydrolysate was about 0.8% X1, 14% X2, 27% X3, 23% X4, 18% X5 and 13% X6 after incubation for 0.5 h.The fast accumulation of X3 and X4 during the initial 0.5 h was possibly due to the preferential action of xylanase enzyme on xylan chain termini. The finding was consistent with Lin et al.,76 who stated that higher levels of X3 and X4 were found at the initial stage of hydrolysis reactions. After 3 h, X1 (9%), X2 (45%) and X3 (39%) contents had increased and the content of X4 (5%) decreased. While X5 and X6 disappeared. The disappearance of X5 and X6 was due to rapid hydrolysis of X5 and X6 into smaller oligosaccharides immediately after release. The same findings were obtained by Akpinar et al.,77 who stated that by increasing time of hydrolysis, concentration of XOS with a higher degree of polymerization (DP > 5) decreased. After 6 h, X1 (18%), X2 (56%) had increased, while X3 (30%) and X4 (2%) contents decreased. Since xylose concentration was less than the concentrations of XOS, especially xylotriose and xylobiose, it can be concluding that the purified xylanase was an endo-xylanase that randomly cleaves the internal glycosidic linkages in xylan as a substrate78.
In the present study, the XOS obtained were principally composed of xylobiose, xylotriose, and xylotetraose. Therefore, in biotechnological applications, xylanase may have potential applications, because these applications rely on its ability to solubilize hemicellulose rather than complete hydrolysis to xylose.
Antioxidant activity ofXylooligosaccharides
The DPPH radical-scavenging ability of XOS mixtures obtained from enzymatic hydrolysis of xylan using xylanase enzyme after 6 h of enzymatic hydrolysis was shown in Table 6. Xylo-oligosaccharides have a dose dependent antioxidant activity. The antioxidant activity increased with increasing concentration of XOS mixtures. Based on statistical analysis; the maximum scavenging percentage (70.57%) was observed using the concentration of 2 mg/mL (p < 0.05). moreover, the concentration of 0. 1 mg/mL gave the lowest scavenging potency with an average of 15.22% (P < 0.05).The same results were obtained by Bian et al.,79 who stated that increasing XOS concentration, increased antioxidant activity. IC50, of XOS mixture obtained after 6 h enzymatic hydrolysis using xylanase enzymes was 0.7154 mg/mL.
XOS has a branched structure comprising b-(1,4) bonded 2–7 xylose units and a number of substituents such as acetyl groups, uronic acids and arabinose units80. Structure of XOS vary in degree of polymerization (DP), monomeric units, and types of linkages depending on the source of xylan used for XOS production81. In addition to xylose residues, xylan is usually found in combination with other side groups such as α-D-glucopyranosyl uronic acid or its 4-O-methyl derivative, acetyl groups, or arabinofuranosyl residues82. Rao and Muralikrishna83 demonstrated that the existence of uronyl or acetyl sugars imparts strong antioxidant activity to polysaccharides. Carboxyl groups have also been reported to enhance the antioxidant function of polysaccharides84. The antioxidant mechanism may be also due to the supply of hydrogen by polysaccharides, which combines with radicals and forms a stable radical to terminate the radical chain reaction. The other possibility is that polysaccharides can combine with the radical ions which are necessary for radical chain reaction; then the reaction is terminated85. These findings showed that beech xylan XOS has outstanding radical-scavenging activity of DPPH and can be useful against oxidative damage.
Conclusion
Overall, Paecilomyces variotii strain produced low molecular weight thermophilic alkalophilic endoxylanase enzyme. It exhibited high stability at relatively high temperature and alkaline pH. It has a high affinity for xylan, very high Vmax and one of the highest specific activities ever reported for xylanase. The properties of the purified xylanase make it an ideal candidate in hydrolysis of lignocellulosic materials and other industries. It also suggests the potential of xylanase enzyme for production of XOS with potent antioxidant activities which are useful in food and pharmaceutical industries.
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A.A. initiated the laboratory experiments. A.A., M.A.A. and R.A.H. conducted the microbial assays and production of enzyme. A.A., S.R., M.A.A. and N.M.A. carried out the enzyme purification and zymogram analysis. A.A., M.A.A. and A.A.S. conducted xylo-oligosaccharides analysis and antioxidant activity assay. A.A. and R.A.H. carried out the statistical analyses. N.M.A. and A.A.S. prepared tables and figures. A.A and M.A.A. wrote and edited the main manuscript text. All authors commented on the manuscript and gave final approval for its publication.
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Abdella, A., Ramadan, S., Hamouda, R.A. et al. Paecilomyces variotii xylanase production, purification and characterization with antioxidant xylo-oligosaccharides production. Sci Rep 11, 16468 (2021). https://doi.org/10.1038/s41598-021-95965-w
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DOI: https://doi.org/10.1038/s41598-021-95965-w
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