Two-way traffic of glycoside hydrolase family 18 processive chitinases on crystalline chitin

Background: Rate-limiting steps in the hydrolysis of recalcitrant polysaccharides by processive enzymes are not known. Results:The predominant molecular state of bound enzyme was revealed by the type and strength of product inhibition. Conclusion: Complexation with the polymer chain is rate-limiting for ChiA, whereas Cel7A is limited by dissociation. Significance: Knowledge of rate-limiting steps aids the engineering of better catalysts.

Section: C-cnw Hydrolysis (Equation 1)supporting

confidence: 48%

Section: Discussionmentioning

confidence: 99%

The Predominant Molecular State of Bound Enzyme Determines the Strength and Type of Product Inhibition in the Hydrolysis of Recalcitrant Polysaccharides by Processive Enzymes

Kuusk

Sørlie

Väljamaë

2015

“…Clearly these figures are far lower than P Intr values of 4000 and 560 measured on bacterial cellulose and amorphous cellulose, respectively (17). Experimentally measured P app values for ChiA range between 5 and 30, depending on the substrate and the method used for measuring (40,(57)(58)(59). Therefore, the large discrepancy between P app and P Intr seems to hold also for ChiA.…”

Section: Discussionmentioning

confidence: 57%

Slow Off-rates and Strong Product Binding Are Required for Processivity and Efficient Degradation of Recalcitrant Chitin by Family 18 Chitinases

Kurašin

Kuusk

et al. 2015

Background:The role of slow off-rates of processive enzymes acting on recalcitrant polysaccharides is poorly understood. Results: Chitinase variants with high off-rates and weak product binding were inefficient in degradation of recalcitrant chitin. Conclusion: Slow off-rates and strong product binding are required for high efficiency and processivity. Significance: Knowledge of determinants of processivity aids to design better enzymes.

“…The crystal structure of OfChtI gave structural evidence that ChtI has a long and open-ended substrate binding cleft with symmetrically distributed subsites that is believed to be a structural characteristic of an endo-acting chitinase (44). According to a structure-based sequence alignment, we found that Chi-h does not contain such a substrate binding cleft but contains a long substrate binding cleft with asymmetrically distributed subsites, a structural characteristic of the processive exo-acting chitinase SmChiA from Serratia marcescens (45). Thus, it is unlikely that Chi-h would be able to act through the same mode of action as ChtI.…”

mentioning

confidence: 98%

Structure, Catalysis, and Inhibition of OfChi-h, the Lepidoptera-exclusive Insect Chitinase

Liu

Chen

Zhou

et al. 2017

153

Edited by Gerald W. HartChitinase-h (Chi-h) is of special interest among insect chitinases due to its exclusive distribution in lepidopteran insects and high sequence identity with bacterial and baculovirus homologs. Here OfChi-h, a Chi-h from Ostrinia furnacalis, was investigated. Crystal structures of both OfChi-h and its complex with chitoheptaose ((GlcN) 7 ) reveal that OfChi-h possesses a long and asymmetric substrate binding cleft, which is a typical characteristics of a processive exo-chitinase. The structural comparison between OfChi-h and its bacterial homolog SmChiA uncovered two phenylalanine-to-tryptophan site variants in OfChi-h at subsites ؉2 and possibly ؊7. The F232W/ F396W double mutant endowed SmChiA with higher hydrolytic activities toward insoluble substrates, such as insect cuticle, ␣-chitin, and chitin nanowhisker. An enzymatic assay demonstrated that OfChi-h outperformed OfChtI, an insect endochitinase, toward the insoluble substrates, but showed lower activity toward the soluble substrate ethylene glycol chitin. Furthermore, OfChi-h was found to be inhibited by N,N,N؆-trimethylglucosamine-N,N,N؆,N؆-tetraacetylchitotetraose (TMG-(GlcNAc) 4 ), a substrate analog which can be degraded into TMG-(GlcNAc) 1-2 . Injection of TMG-(GlcNAc) 4 into 5th-instar O. furnacalis larvae led to severe defects in pupation. This work provides insights into a molting-indispensable insect chitinase that is phylogenetically closer to bacterial chitinases than insect chitinases.