Novel β-glucanases along with xylanase identified in Thermomyces lanuginosus secretome for enhanced saccharification of different lignocellulosics

被引:6
作者
Brar, Kamalpreet Kaur [1 ,2 ]
Raheja, Yashika [1 ]
di Falco, Marcos [3 ]
Tsang, Adrian [3 ]
Chadha, Bhupinder Singh [1 ]
机构
[1] Guru Nanak Dev Univ, Dept Microbiol, Amritsar 143005, Punjab, India
[2] York Univ, Lassonde Sch Engn, Dept Civil Engn, Toronto, ON M3J 1P3, Canada
[3] Concordia Univ, Ctr Struct & Funct Genom, 7141 Sherbrooke St West, Montreal, PQ H4B 1R6, Canada
关键词
Thermomyces lanuginosus; Xylanase (GH11); Laminarinase (GH64); Lichenanase (GH81); LC/MS exo-proteome; Saccharification; GLYCOSIDE HYDROLASE FAMILY; ACCESSORY ENZYMES; ENZYMATIC-HYDROLYSIS; THERMOPHILIC FUNGI; CELLULASE; SUBSTRATE; OPTIMIZATION; PURIFICATION; RESIDUES; IMPROVE;
D O I
10.1007/s13399-020-01152-8
中图分类号
TE [石油、天然气工业]; TK [能源与动力工程];
学科分类号
0807 ; 0820 ;
摘要
The LC/MS-based exo-proteome analysis of thermophilic fungus Thermomyces lanuginosus showed 22.59% (40 proteins) of the total identified proteins (177) as CAZymes (carbohydrate-active enzymes). The CAZymes were primarily represented by glycosyl hydrolases (72.5%) belonging to 21 different GH families. Xylanase (GH11) was found to be the major protein (24.3%) in addition to the beta-glucanase and another complex polysaccharide-degrading (carbohydrate-active enzymes) CAZymes in the secretome. FPLC-based fractionation of secretome was employed to identify proteins responsible for enhancing the catalytic efficacy of Cellic Ctec2 during hydrolysis of acid pre-treated lignocellulosics and eventually xylanase (GH11) and beta-glucanases (GH64 and GH81) were identified and purified. The purified xylanase when supplemented with Cellic Ctec2 resulted in 2.05-, 1.79-, and 1.60-fold increase in the release of glucose from acid-treated bagasse at 10, 15, and 20% substrate loading rate, respectively when compared with the control. Similarly, enhanced hydrolysis of acid pre-treated corn residue and rice straw was observed upon supplementation with xylanase. Spiking benchmark cellulase with purified GH64 and GH81 also resulted in 1.18- and 1.23-fold enhanced hydrolysis of acid pre-treated sugarcane bagasse. The supplementation of xylanase (1000 units/g substrate) was found to reduce the Cellic Ctec2 loading rate from 36 mg/g substrate by 2.70-, 2.88-, and 2.57-fold required for hydrolysis of acid treated bagasse, corn residue, and rice straw, respectively, at high substrate loading rate (20%) and thus, it is an important candidate for economizing the 2G ethanol process.
引用
收藏
页码:273 / 286
页数:14
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