Juan-José Escuder-Rodríguez, María González-Suarez, María-Eugenia deCastro, Almudena Saavedra-Bouza, Manuel Becerra, María-Isabel González-Siso
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Predictions on protein structure and conserved amino acid sequences were conducted, as well as expression in heterologous systems with Escherichia coli and Saccharomyces cerevisiae as the host. Cel776Ec was correctly expressed and purified by taking advantage of the His-Tag system, with a yield of 0.346 U/mL in the eluted fraction. Cel776Sc was expressed extracellulary and was easily recovered from the supernatant without the need of further purification, requiring only a concentration step by ultrafiltration, with a significantly higher yield of 531.95 U/mL, revealing a much more suitable system for production of large amounts of the enzyme. Their biochemical characterization revealed biotechnologically interesting enzymes. Both Cel776Ec and Cel776Sc had an optimal temperature of 80 °C and optimal pH of 5. Cel776Ec exhibited high thermostability maintaining its activity for 24 h at 60 °C and maintained its activity longer than Cel776Sc at increasing incubation temperatures. Moreover, its substrate specificity allowed the degradation of both cellulose and xylan. Whereas Cel776Ec was more active in the presence of calcium and magnesium, manganese was found to increase Cel776Sc activity. A stronger inhibitory effect was found for Cel776Ec than Cel776Sc adding detergent SDS to the reaction mix, whereas EDTA only significantly affected Cel776Sc activity.</p><p><strong>Conclusions: </strong>Our study reports the discovery of a new promising biocatalyst for its application in processes, such as the production of biofuel and the saccharification of plant biomass, due to its bifunctional enzymatic activity as an endoglucanase and as a xylanase, as well as highlights the advantages of a yeast expression system over bacteria.</p>","PeriodicalId":9125,"journal":{"name":"Biotechnology for Biofuels and Bioproducts","volume":" ","pages":"76"},"PeriodicalIF":0.0000,"publicationDate":"2022-07-07","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9264688/pdf/","citationCount":"4","resultStr":"{\"title\":\"Characterization of a novel thermophilic metagenomic GH5 endoglucanase heterologously expressed in Escherichia coli and Saccharomyces cerevisiae.\",\"authors\":\"Juan-José Escuder-Rodríguez, María González-Suarez, María-Eugenia deCastro, Almudena Saavedra-Bouza, Manuel Becerra, María-Isabel González-Siso\",\"doi\":\"10.1186/s13068-022-02172-4\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><strong>Background: </strong>Endoglucanases from thermophilic microorganisms are a valuable resource as they can be used in a wide variety of biotechnological applications including the valorisation of biomass and the production of biofuels. In the present work we analysed the metagenome from the hot spring Muiño da Veiga, located in the northwest of Spain (in the Galicia region), in search for novel thermostable endoglucanases.</p><p><strong>Results: </strong>Sequence analysis of the metagenome revealed a promising enzyme (Cel776). Predictions on protein structure and conserved amino acid sequences were conducted, as well as expression in heterologous systems with Escherichia coli and Saccharomyces cerevisiae as the host. Cel776Ec was correctly expressed and purified by taking advantage of the His-Tag system, with a yield of 0.346 U/mL in the eluted fraction. Cel776Sc was expressed extracellulary and was easily recovered from the supernatant without the need of further purification, requiring only a concentration step by ultrafiltration, with a significantly higher yield of 531.95 U/mL, revealing a much more suitable system for production of large amounts of the enzyme. Their biochemical characterization revealed biotechnologically interesting enzymes. Both Cel776Ec and Cel776Sc had an optimal temperature of 80 °C and optimal pH of 5. Cel776Ec exhibited high thermostability maintaining its activity for 24 h at 60 °C and maintained its activity longer than Cel776Sc at increasing incubation temperatures. Moreover, its substrate specificity allowed the degradation of both cellulose and xylan. Whereas Cel776Ec was more active in the presence of calcium and magnesium, manganese was found to increase Cel776Sc activity. 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引用次数: 4
摘要
背景:来自嗜热微生物的内切葡聚糖酶是一种有价值的资源,因为它们可以广泛用于各种生物技术应用,包括生物质的增值和生物燃料的生产。在目前的工作中,我们分析了位于西班牙西北部(加利西亚地区)的Muiño da Veiga温泉的宏基因组,以寻找新的耐热内切葡聚糖酶。结果:宏基因组序列分析发现了一种有前景的酶(Cel776)。对其蛋白结构和保守氨基酸序列进行预测,并在大肠杆菌和酿酒酵母为宿主的异源系统中进行表达。利用His-Tag系统对Cel776Ec进行了正确的表达和纯化,洗脱部分的产率为0.346 U/mL。Cel776Sc在细胞外表达,无需进一步纯化即可从上清中回收,只需要超滤浓缩一步,产率高达531.95 U/mL,这表明Cel776Sc是一种更适合大量生产酶的体系。它们的生化特性揭示了生物技术上有趣的酶。Cel776Ec和Cel776Sc的最适温度为80℃,最适pH为5。Cel776Ec表现出较高的热稳定性,在60℃下可维持24 h的活性,在提高孵育温度下比Cel776Sc保持更长的活性。此外,它的底物特异性允许降解纤维素和木聚糖。而Cel776Ec在钙和镁的存在下更活跃,锰被发现可以增加Cel776Sc的活性。添加SDS对Cel776Ec的抑制作用强于添加SDS对Cel776Sc的抑制作用,而EDTA仅对Cel776Sc的活性有显著影响。结论:我们的研究报告了一种新的生物催化剂的发现,由于其作为内切葡聚糖酶和木聚糖酶的双功能酶活性,它在生物燃料生产和植物生物质糖化等过程中具有应用前景,并且突出了酵母表达系统相对于细菌的优势。
Characterization of a novel thermophilic metagenomic GH5 endoglucanase heterologously expressed in Escherichia coli and Saccharomyces cerevisiae.
Background: Endoglucanases from thermophilic microorganisms are a valuable resource as they can be used in a wide variety of biotechnological applications including the valorisation of biomass and the production of biofuels. In the present work we analysed the metagenome from the hot spring Muiño da Veiga, located in the northwest of Spain (in the Galicia region), in search for novel thermostable endoglucanases.
Results: Sequence analysis of the metagenome revealed a promising enzyme (Cel776). Predictions on protein structure and conserved amino acid sequences were conducted, as well as expression in heterologous systems with Escherichia coli and Saccharomyces cerevisiae as the host. Cel776Ec was correctly expressed and purified by taking advantage of the His-Tag system, with a yield of 0.346 U/mL in the eluted fraction. Cel776Sc was expressed extracellulary and was easily recovered from the supernatant without the need of further purification, requiring only a concentration step by ultrafiltration, with a significantly higher yield of 531.95 U/mL, revealing a much more suitable system for production of large amounts of the enzyme. Their biochemical characterization revealed biotechnologically interesting enzymes. Both Cel776Ec and Cel776Sc had an optimal temperature of 80 °C and optimal pH of 5. Cel776Ec exhibited high thermostability maintaining its activity for 24 h at 60 °C and maintained its activity longer than Cel776Sc at increasing incubation temperatures. Moreover, its substrate specificity allowed the degradation of both cellulose and xylan. Whereas Cel776Ec was more active in the presence of calcium and magnesium, manganese was found to increase Cel776Sc activity. A stronger inhibitory effect was found for Cel776Ec than Cel776Sc adding detergent SDS to the reaction mix, whereas EDTA only significantly affected Cel776Sc activity.
Conclusions: Our study reports the discovery of a new promising biocatalyst for its application in processes, such as the production of biofuel and the saccharification of plant biomass, due to its bifunctional enzymatic activity as an endoglucanase and as a xylanase, as well as highlights the advantages of a yeast expression system over bacteria.
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