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黑曲霉、里氏木霉和乳白耙齿菌产生的四种外切型纤维素酶对(1→3),(1→4)-β-D-葡聚糖和木葡聚糖的精细底物特异性。

Fine substrate specificities of four exo-type cellulases produced by Aspergillus niger, Trichoderma reesei, and Irpex lacteus on (1-->3), (1-->4)-beta-D-glucans and xyloglucan.

作者信息

Amano Y, Shiroishi M, Nisizawa K, Hoshino E, Kanda T

机构信息

Department of Chemistry and Material Engineering, Faculty of Engineering, Shinshu University, Nagano.

出版信息

J Biochem. 1996 Dec;120(6):1123-9. doi: 10.1093/oxfordjournals.jbchem.a021531.

Abstract

To investigate the fine substrate specificities of four highly purified exo-type cellulases (Exo-A from Aspergillus niger, CBHI and CBHII from Trichoderma reesei, and Ex-1 from Irpex lacteus), water-soluble substrates such as barley glucan, xyloglucan from tamarind (Tamarindus indica L.), and their oligosaccharides were employed. Four exo-type cellulases immediately hydrolyzed 3-O-beta-D-cellotriosylglucose to produce cellobiose and laminaribiose. In contrast, CBHII showed no hydrolytic activity towards 3(2)-O-beta-D-cello-biosylcellobiose, which was hydrolyzed to cellobiose by the other exo-type cellulases. These cellulases hydrolyzed the internal linkages of barley glucan and lichenan in an endo-type fashion to produce cellobiose and mix-linked oligosaccharides as main products. The DP-lowering activities of the four exo-type cellulases on barley glucan were in the order of Ex-1, CBHII, Exo-A, and CBHI. Based on gel permeation chromatography analysis of the hydrolysates, Ex-1 seemed to attack the internal cellobiosyl unit adjacent to beta-1,3-glucosidic linkages in barley glucan molecule more frequently than did the other cellulases. Xyloglucan was hydrolyzed only by CBHI and CBHII, and produced hepta-, octa-, and nona-saccharides. In addition, a xyloglucan tetradecasaccharide (XG14) was split only to heptasaccharide (XG7) by CBHI and CBHII.

摘要

为研究四种高度纯化的外切型纤维素酶(黑曲霉的外切 -A、里氏木霉的 CBHI 和 CBHII 以及乳白耙齿菌的 Ex-1)的精细底物特异性,使用了水溶性底物,如大麦葡聚糖、罗望子(罗望子属)的木葡聚糖及其寡糖。四种外切型纤维素酶能立即水解 3 -O-β-D-纤维三糖基葡萄糖以产生纤维二糖和层叠二糖。相比之下,CBHII 对 3(2)-O-β-D-纤维二糖基纤维二糖没有水解活性,而其他外切型纤维素酶能将其水解为纤维二糖。这些纤维素酶以内切型方式水解大麦葡聚糖和地衣多糖的内部连接,以产生纤维二糖和混合连接的寡糖作为主要产物。四种外切型纤维素酶对大麦葡聚糖的降低聚合度活性顺序为 Ex-1、CBHII、外切 -A 和 CBHI。基于水解产物的凝胶渗透色谱分析,Ex-1 似乎比其他纤维素酶更频繁地攻击大麦葡聚糖分子中与β-1,3-糖苷键相邻的内部纤维二糖基单元。木葡聚糖仅被 CBHI 和 CBHII 水解,并产生七糖、八糖和九糖。此外,木葡聚糖十四糖(XG14)仅被 CBHI 和 CBHII 裂解为七糖(XG7)。

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