Activity studies of eight purified cellulases: Specificity, synergism, and binding domain effects

Irwin, Diana C.; Spezio, M; Walker, Larry P.; Wilson, David B.

doi:10.1002/bit.260420811

Cited by 335 publications

(352 citation statements)

References 38 publications

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“…Furthermore, the addition of CBMs in trans to the cognate catalytic module has led to a modest potentiation (0.2-to 1.5-fold) in catalytic activity against insoluble substrates (Din et al, 1994;Moser et al, 2008). Cellulases, typically endoglucanases, however, are often 3 orders of magnitude more active against soluble forms of cellulose than the crystalline polysaccharide (Durrant et al, 1991;Irwin et al, 1993). Thus, CBMs acting in trans have only a minor influence on the access problem, although this might reflect the dissociation of the targeting and (possible) disrupting function of these modules.…”

Section: How Do Cbms Potentiate Catalysis?mentioning

confidence: 99%

The Biochemistry and Structural Biology of Plant Cell Wall Deconstruction

2010

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Section: How Do Cbms Potentiate Catalysis?mentioning

confidence: 99%

The Biochemistry and Structural Biology of Plant Cell Wall Deconstruction

2010

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“…Cellulase enzymes produced by T. reesei have been shown to act synergistically to depolymerize cellulose in biomass with Cel7A playing the primary role of de-crystallizing and hydrolyzing cellulose microfibrils to its monomeric unit, cellobiose (Henrissat et al, 1985). T. reesei Cel7A has been shown to be highly effective on recalcitrant cellulose when acting alone, while also significantly enhancing the overall activity of cellulase mixtures (Irwin et al, 1993). The importance of the Cel7A enzyme in the cellulase system suggests that improvements in overall cellulase activity can be achieved by improving its access to cellulose.…”

Section: Introductionmentioning

confidence: 99%

Cellulase digestibility of pretreated biomass is limited by cellulose accessibility

Jeoh¹,

Ishizawa²,

Davis³

et al. 2007

Biotech & Bioengineering

459

318

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Attempts to correlate the physical and chemical properties of biomass to its susceptibility to enzyme digestion are often inconclusive or contradictory depending on variables such as the type of substrate, the pretreatment conditions and measurement techniques. In this study, we present a direct method for measuring the key factors governing cellulose digestibility in a biomass sample by directly probing cellulase binding and activity using a purified cellobiohydrolase (Cel7A) from Trichoderma reesei. Fluorescence-labeled T. reesei Cel7A was used to assay pretreated corn stover samples and pure cellulosic substrates to identify barriers to accessibility by this important component of cellulase preparations. The results showed cellulose conversion improved when T. reesei Cel7A bound in higher concentrations, indicating that the enzyme had greater access to the substrate. Factors such as the pretreatment severity, drying after pretreatment, and cellulose crystallinity were found to directly impact enzyme accessibility. This study provides direct evidence to support the notion that the best pretreatment schemes for rendering biomass more digestible to cellobiohydrolase enzymes are those that improve access to the cellulose in biomass cell walls, as well as those able to reduce the crystallinity of cell wall cellulose.

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“…The most effective means of lignocellulosic hydrolysis uses a cocktail of different cellulolytic enzymes, but conversion is still not optimal (Berlin et al, 2007;Cherry and Fidantsef, 2003;Irwin et al, 1993;Jeoh et al, 2002;Kabel et al, 2006). There is a need to develop more effective cocktails with a range of properties complementary to current cellulase systems, at a significantly reduced cost.…”

Section: Introductionmentioning

confidence: 99%

An optimized microplate assay system for quantitative evaluation of plant cell wall–degrading enzyme activity of fungal culture extracts

King

Donnelly

Bergstrom

et al. 2008

Biotech & Bioengineering

Self Cite

135

102

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Developing enzyme cocktails for cellulosic biomass hydrolysis complementary to current cellulase systems is a critical step needed for economically viable biofuels production. Recent genomic analysis indicates that some plant pathogenic fungi are likely a largely untapped resource in which to prospect for novel hydrolytic enzymes for biomass conversion. In order to develop high throughput screening assays for enzyme bioprospecting, a standardized microplate assay was developed for rapid analysis of polysaccharide hydrolysis by fungal extracts, incorporating biomass substrates. Fungi were grown for 10 days on cellulose-or switchgrass-containing media to produce enzyme extracts for analysis. Reducing sugar released from filter paper, Avicel, corn stalk, switchgrass, carboxymethylcellulose, and arabinoxylan was quantified using a miniaturized colorimetric assay based on 3,5-dinitrosalicylic acid. Significant interactions were identified among fungal species, growth media composition, assay substrate, and temperature. Within a small sampling of plant pathogenic fungi, some extracts had crude activities comparable to or greater than T. reesei, particularly when assayed at lower temperatures and on biomass substrates. This microplate assay system should prove useful for high-throughput bioprospecting for new sources of novel enzymes for biofuel production.

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Activity studies of eight purified cellulases: Specificity, synergism, and binding domain effects

Cited by 335 publications

References 38 publications

The Biochemistry and Structural Biology of Plant Cell Wall Deconstruction

The Biochemistry and Structural Biology of Plant Cell Wall Deconstruction

Cellulase digestibility of pretreated biomass is limited by cellulose accessibility

An optimized microplate assay system for quantitative evaluation of plant cell wall–degrading enzyme activity of fungal culture extracts

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