Surface Density of Cellobiohydrolase on Crystalline Celluloses. A Critical Parameter to Evaluate Enzymatic Kinetics at a Solid-liquid Interface

Overview

Journal FEBS J

Specialty Biochemistry

Date 2006 Jun 9

PMID 16759230

Citations 16

Authors

Kiyohiko Igarashi

Masahisa Wada

Ritsuko Hori

Masahiro Samejima

Affiliations

Soon will be listed here.

Abstract

The enzymatic kinetics of glycoside hydrolase family 7 cellobiohydrolase (Cel7A) towards highly crystalline celluloses at the solid-liquid interface was evaluated by applying the novel concept of surface density (rho) of the enzyme, which is defined as the amount of adsorbed enzyme divided by the maximum amount of adsorbed enzyme. When the adsorption levels of Trichoderma viride Cel7A on cellulose I(alpha) from Cladophora and cellulose I(beta) from Halocynthia were compared, the maximum adsorption of the enzyme on cellulose I(beta) was approximately 1.5 times higher than that on cellulose I(alpha), although the rate of cellobiose production from cellulose I(beta) was lower than that from cellulose I(alpha). This indicates that the specific activity (k) of Cel7A adsorbed on cellulose I(alpha) is higher than that of Cel7A adsorbed on cellulose I(beta). When k was plotted versus rho, a dramatic decrease of the specific activity was observed with the increase of surface density (rho-value), suggesting that overcrowding of enzyme molecules on a cellulose surface lowers their activity. An apparent difference of the specific activity was observed between crystalline polymorphs, i.e. the specific activity for cellulose I(alpha) was almost twice that for cellulose I(beta). When cellulose I(alpha) was converted to cellulose I(beta) by hydrothermal treatment, the specific activity of Cel7A decreased and became similar to that of native cellulose I(beta) at the same rho-value. These results indicate that the hydrolytic activity (rate) of bound Cel7A depends on the nature of the crystalline cellulose polymorph, and an analysis that takes surface density into account is an effective means to evaluate cellulase kinetics at a solid-liquid interface.

Citing Articles

Mechanism-based Modelling for Fitting the Double-exponential Progress Curves of Cellulase Reaction.

Igarashi K, Ezaki T, Samejima M J Appl Glycosci (1999). 2024; 71(4):103-110.

PMID: 39720779 PMC: 11664118. DOI: 10.5458/jag.jag.JAG-2024_0007.

Alanine substitution in cellobiohydrolase provides new insights into substrate threading.

Mitsuzawa S, Fukuura M, Shinkawa S, Kimura K, Furuta T Sci Rep. 2017; 7(1):16320.

PMID: 29176588 PMC: 5701224. DOI: 10.1038/s41598-017-16434-x.

Free Energy Diagram for the Heterogeneous Enzymatic Hydrolysis of Glycosidic Bonds in Cellulose.

Sorensen T, Cruys-Bagger N, Borch K, Westh P J Biol Chem. 2015; 290(36):22203-11.

PMID: 26183776 PMC: 4571971. DOI: 10.1074/jbc.M115.659656.

Kinetics of cellobiohydrolase (Cel7A) variants with lowered substrate affinity.

Kari J, Olsen J, Borch K, Cruys-Bagger N, Jensen K, Westh P J Biol Chem. 2014; 289(47):32459-68.

PMID: 25271162 PMC: 4239601. DOI: 10.1074/jbc.M114.604264.

Multi-mode binding of Cellobiohydrolase Cel7A from Trichoderma reesei to cellulose.

Jalak J, Valjamae P PLoS One. 2014; 9(9):e108181.

PMID: 25265511 PMC: 4180464. DOI: 10.1371/journal.pone.0108181.