The features that distinguish lichenases from other polysaccharide-hydrolyzing enzymes and the relevance of lichenases for biotechnological applications

Goldenkova-Pavlova, I. V.; Tyurin, A. A.; Mustafaev, O. N.

doi:10.1007/s00253-018-8904-x

Cited by 21 publications

(17 citation statements)

References 89 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Thus, our data demonstrate a higher sensitivity of the fluorometric assay for lichenase quantification (15 ng in the preparation over 180-min incubation of lichenase with the substrate) as compared with the Somogyi-Nelson assay (to 2 µg in the preparation). As has been earlier demonstrated, thermostable lichenase is rather resistant to various chemical reagents, retaining a high level of enzyme activity in the presence of EDTA, SDS, Triton X-100, and several others [9]. In addition, we compared the effects of several components contained in the buffers for extraction of soluble plant proteins on the modulation of lichenase quantification in samples using fluorometric and Somogyi-Nelson assays, namely, EDTA (50-100 mM), NaCl (10-100 mM), and SDS (0.1-0.5%).…”

Section: Comparative Analysis Of Thermostable Lichenase Quantification With Somogyi-nelson and Fluorometric Assaysmentioning

confidence: 74%

“…The ability to refold in vitro after heat treatment at 70 • Cor ethanol denaturation can be used for rapid and cost-efficient purification of plant protein lysates, in particular, when utilizing lichenase in plant biotechnology. For example, it has been shown that the heat treatment at 70 • Cremoves up to 50% of contaminating plant proteins, while lichenase and the proteins fused to lichenase remain intact [9,28]. The C. thermocellum thermostable lichenase is active in a wide range of temperatures and pH [29], while the thermostable lichenase preparations isolated from biological samples, in particular, from plants, retain their high specific activity during a long-term storage in a container of a closed system under changing temperature or during a thawing-freezing procedure.…”

Section: Discussionmentioning

confidence: 99%

“…Note that each reporter system has its own limitations with respect to the quantification of the protein product of a reporter gene and, in particular, for the use of high-throughput approaches. Earlier, the thermostable lichenase-β-1,3-1,4-glucanase (lichenase) (endo-β-1,3;1,4-glucan-D-glycosyl hydrolase) EC 3.2.1.73 (P29716) of Clostridium thermocellum-was proposed as an efficient reporter for plant systems [8], with a number of advantages over other reporters [9]. Lichenases strictly catalyze the endohydrolysis of the β-1,4-glycoside bond adjacent to 3-Osubstituted glucose residue in the β-glucans containing β-1,3 and β-1,4 bonds, for example, β-1,3-1,4-glucans of cereals and lichenan, which are as a rule used as substrates for lichenase quantification.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

A High Throughput Assay of Lichenase Activity with Congo Red Dye in Plants

Tyurin

Suhorukova

Deineko

et al. 2021

Preprint

Self Cite

View full text Add to dashboard Cite

Background : To elucidate the functional role of regulatory sequences and contexts identified and predicted during omics studies in the complex mechanisms of gene expression regulation, experimental verification methods in a plant cell are required. For this, the method of transient expression of reporter genes fused with the tested sequences is widely used. Several reporter systems are available that have shown good performance in the studies including the thermostable lichenase Clostridium thermocellum . However, each reporter system has its own limitations with respect to the quantification of the protein product of a reporter gene and, in particular, for the use of high-throughput approaches. Results: In this study, we report the design a high throughput fluorometric method for quantification of thermostable lichenase C. thermocellum using Congo red and further experimental verification of its relevance and efficiency in assessment of the functional role of regulatory sequences in the plant cell. Conclusion: The specific interaction between the dye Congo red and β -D-glucans formed the background for designing a high-throughput fluorometric assay for quantification of C. thermocellum thermostable lichenase as a reporter protein for plants. This assay (i) makes it possible to precisely measure the amount of reporter protein in a plant sample; (ii) has shown a high sensitivity for quantification of thermostable lichenase; (iii) is more time- and cost-efficient as compared with the Somogyi–Nelson assay; and (iv) is to the least degree dependent on the presence of the tested buffer components as compared with the Somogyi–Nelson assay.

show abstract

Section: Comparative Analysis Of Thermostable Lichenase Quantification With Somogyi-nelson and Fluorometric Assaysmentioning

confidence: 74%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

A High Throughput Assay of Lichenase Activity with Congo Red Dye in Plants

Tyurin

Suhorukova

Deineko

et al. 2021

Preprint

Self Cite

View full text Add to dashboard Cite

show abstract

“…The product of this gene, Cel12A, belongs to the glycosyl hydrolase family 12 (GH12) and was found to be a lichenase-like or non-typical cellulase showing low activity on cellulose but high activity on lichenan (β-1,3-1,4-glucan) and barley mixed glucans ((1 → 3, 1 → 4)-β-D-glucans). These properties show the potential application of Cel12A in the brewing and wine industries to facilitate filtration processes; in animal foodstuffs to improve β-glucans digestibility and nutritive quality; to produce valuable oligosaccharides; and in the processing of agricultural and industrial wastes for producing bioethanol and biodiesel (Thomas 1956;Goldenkova-Pavlova et al 2018;Chaari and Ellouz Chaabouni 2019). The aim of the present work was to study (real-time RT-qPCR) the effect of different carbon sources and initial pH values on the expression of cel12A.…”

Section: Introductionmentioning

confidence: 99%

Transcriptional analysis of the lichenase-like gene cel12A of the filamentous fungus Stachybotrys atra BP-A and its relevance for lignocellulose depolymerization

2021

View full text Add to dashboard Cite

To rationally optimize the production of industrial enzymes by molecular means requires previous knowledge of the regulatory circuits controlling the expression of the corresponding genes. The genus Stachybotrys is an outstanding producer of cellulosedegrading enzymes. Previous studies isolated and characterized the lichenase-like/non-typical cellulase Cel12A of S. atra (AKA S. chartarum) belonging to glycosyl hydrolase family 12 (GH12). In this study, we used RT-qPCR to determine the pattern of expression of cel12A under different carbon sources and initial ambient pH. Among the carbon sources examined, rice straw triggered a greater increase in the expression of cel12A than 1% lactose or 0.1% glucose, indicating specific induction by rice straw. In contrast, cel12A was repressed in the presence of glucose even when combined with this inducer. The proximity of 2 adjacent 5′-CTGGGGTCTGGGG-3′ CreA consensus target sites to the translational start site of cel12A strongly suggests that the carbon catabolite repression observed is directly mediated by CreA. Ambient pH did not have a significant effect on cel12A expression. These findings present new knowledge on transcriptional regulatory networks in Stachybotrys associated with cellulose/hemicellulose depolymerization. Rational engineering of CreA to remove CCR could constitute a novel strategy for improving the production of Cel12A.

show abstract

“…These enzymes act synergistically: endo-acting enzymes generate new reducing and non-reducing chain ends for the exo-acting enzymes, which release cellobiose that is further converted to glucose by β-glucosidases [ 15 ]. The above-mentioned enzymes involved in cellulose hydrolysis are also active on mixed-linked β-glucans along with lichenases (β-1,3−1,4-glucanase, EC 3.2.1.73), which specifically cleave β-1,4 glycoside bonds in 3-O substituted glucosyl residues, and β-1,3(4)-glucanases (EC 3.2.1.6), which act on β-1,3 or β-1,4 linkages when the glucose residues are substituted at C3 [ 16 ]. The enzymes that break down carbohydrates are grouped, based on their structural similarity, into several glycoside hydrolase (GH) families in the CAZy database [ 17 ].…”

Section: Introductionmentioning

confidence: 99%

Synergic activity of Cel8Pa β-1,4 endoglucanase and Bg1Pa β-glucosidase from Paenibacillus xylanivorans A59 in beta-glucan conversion

Ghio

Bradanini

Garrido

et al. 2020

Biotechnology Reports

View full text Add to dashboard Cite

Highlights Cel8Pa is an extracellular, halotolerant, broad substrate endoglucanase. Bg1Pa is an intracellular β-glucosidase, with activity on cello oligosaccharides and high resistance to ethanol. The concerted action of Cel8Pa and Bg1Pa has a synergistic effect on saccharification of β-glucans. Cel8Pa and Bg1Pa are cold-stable and candidates for SSF ethanol 2 G processes.

show abstract

The features that distinguish lichenases from other polysaccharide-hydrolyzing enzymes and the relevance of lichenases for biotechnological applications

Cited by 21 publications

References 89 publications

A High Throughput Assay of Lichenase Activity with Congo Red Dye in Plants

A High Throughput Assay of Lichenase Activity with Congo Red Dye in Plants

Transcriptional analysis of the lichenase-like gene cel12A of the filamentous fungus Stachybotrys atra BP-A and its relevance for lignocellulose depolymerization

Synergic activity of Cel8Pa β-1,4 endoglucanase and Bg1Pa β-glucosidase from Paenibacillus xylanivorans A59 in beta-glucan conversion

Contact Info

Product

Resources

About