Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes

ABSTRACT Marine algae produce a variety of glycans, which fulfill diverse biological functions and fuel the carbon and energy demands of heterotrophic microbes. A common approach to analysis of marine organic matter uses acid to hydrolyze the glycans into measurable monosaccharides. The monosacchari...

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Published in:Applied and Environmental Microbiology
Main Author: Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire
Language:unknown
Published: 2019
Subjects:
Arctic
Arctic Ocean
Online Access:http://www.osti.gov/servlets/purl/1536860
https://www.osti.gov/biblio/1536860
https://doi.org/10.1128/aem.03389-16
id ftosti:oai:osti.gov:1536860
record_format openpolar
spelling ftosti:oai:osti.gov:1536860 2023-05-15T15:19:24+02:00 Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire 2019-08-09 application/pdf http://www.osti.gov/servlets/purl/1536860 https://www.osti.gov/biblio/1536860 https://doi.org/10.1128/aem.03389-16 unknown http://www.osti.gov/servlets/purl/1536860 https://www.osti.gov/biblio/1536860 https://doi.org/10.1128/aem.03389-16 doi:10.1128/aem.03389-16 2019 ftosti https://doi.org/10.1128/aem.03389-16 2019-08-10T22:47:58Z ABSTRACT Marine algae produce a variety of glycans, which fulfill diverse biological functions and fuel the carbon and energy demands of heterotrophic microbes. A common approach to analysis of marine organic matter uses acid to hydrolyze the glycans into measurable monosaccharides. The monosaccharides may be derived from different glycans that are built with the same monosaccharides, however, and this approach does not distinguish between glycans in natural samples. Here we use enzymes to digest selectively and thereby quantify laminarin in particulate organic matter. Environmental metaproteome data revealed carbohydrate-active enzymes from marine flavobacteria as tools for selective hydrolysis of the algal β-glucan laminarin. The enzymes digested laminarin into glucose and oligosaccharides, which we measured with standard methods to establish the amounts of laminarin in the samples. We cloned, expressed, purified, and characterized three new glycoside hydrolases (GHs) of<named-content content-type='genus-species'>Formosa</named-content>bacteria: two are endo-β-1,3-glucanases, of the GH16 and GH17 families, and the other is a GH30 exo-β-1,6-glucanase.<named-content content-type='genus-species'>Formosa</named-content>sp. nov strain Hel1_33_131 GH30 (FbGH30) removed the β-1,6-glucose side chains, and<named-content content-type='genus-species'>Formosa agariphila</named-content>GH17A (FaGH17A) and FaGH16A hydrolyzed the β-1,3-glucose backbone of laminarin. Specificity profiling with a library of glucan oligosaccharides and polysaccharides revealed that FaGH17A and FbGH30 were highly specific enzymes, while FaGH16A also hydrolyzed mixed-linked glucans with β-1,4-glucose. Therefore, we chose the more specific FaGH17A and FbGH30 to quantify laminarin in two cultured diatoms, namely,<named-content content-type='genus-species'>Thalassiosira weissflogii</named-content>and<named-content content-type='genus-species'>Thalassiosira pseudonana</named-content>, and in seawater samples from the North Sea and the Arctic Ocean. Combined, these results demonstrate the potential of enzymes for faster, stereospecific, and sequence-specific analysis of select glycans in marine organic matter. IMPORTANCE Marine algae synthesize substantial amounts of the glucose polymer laminarin for energy and carbon storage. Its concentrations, rates of production by autotrophic organisms, and rates of digestion by heterotrophic organisms remain unknown. Here we present a method based on enzymes that hydrolyze laminarin and enable its quantification even in crude substrate mixtures, without purification. Compared to the commonly used acid hydrolysis, the enzymatic method presented here is faster and stereospecific and selectively cleaves laminarin in mixtures of glycans, releasing only glucose and oligosaccharides, which can be easily quantified with reducing sugar assays. Other/Unknown Material Arctic Arctic Ocean SciTec Connect (Office of Scientific and Technical Information - OSTI, U.S. Department of Energy) Arctic Arctic Ocean Applied and Environmental Microbiology 83 9
institution Open Polar
collection SciTec Connect (Office of Scientific and Technical Information - OSTI, U.S. Department of Energy)
op_collection_id ftosti
language unknown
description ABSTRACT Marine algae produce a variety of glycans, which fulfill diverse biological functions and fuel the carbon and energy demands of heterotrophic microbes. A common approach to analysis of marine organic matter uses acid to hydrolyze the glycans into measurable monosaccharides. The monosaccharides may be derived from different glycans that are built with the same monosaccharides, however, and this approach does not distinguish between glycans in natural samples. Here we use enzymes to digest selectively and thereby quantify laminarin in particulate organic matter. Environmental metaproteome data revealed carbohydrate-active enzymes from marine flavobacteria as tools for selective hydrolysis of the algal β-glucan laminarin. The enzymes digested laminarin into glucose and oligosaccharides, which we measured with standard methods to establish the amounts of laminarin in the samples. We cloned, expressed, purified, and characterized three new glycoside hydrolases (GHs) of<named-content content-type='genus-species'>Formosa</named-content>bacteria: two are endo-β-1,3-glucanases, of the GH16 and GH17 families, and the other is a GH30 exo-β-1,6-glucanase.<named-content content-type='genus-species'>Formosa</named-content>sp. nov strain Hel1_33_131 GH30 (FbGH30) removed the β-1,6-glucose side chains, and<named-content content-type='genus-species'>Formosa agariphila</named-content>GH17A (FaGH17A) and FaGH16A hydrolyzed the β-1,3-glucose backbone of laminarin. Specificity profiling with a library of glucan oligosaccharides and polysaccharides revealed that FaGH17A and FbGH30 were highly specific enzymes, while FaGH16A also hydrolyzed mixed-linked glucans with β-1,4-glucose. Therefore, we chose the more specific FaGH17A and FbGH30 to quantify laminarin in two cultured diatoms, namely,<named-content content-type='genus-species'>Thalassiosira weissflogii</named-content>and<named-content content-type='genus-species'>Thalassiosira pseudonana</named-content>, and in seawater samples from the North Sea and the Arctic Ocean. Combined, these results demonstrate the potential of enzymes for faster, stereospecific, and sequence-specific analysis of select glycans in marine organic matter. IMPORTANCE Marine algae synthesize substantial amounts of the glucose polymer laminarin for energy and carbon storage. Its concentrations, rates of production by autotrophic organisms, and rates of digestion by heterotrophic organisms remain unknown. Here we present a method based on enzymes that hydrolyze laminarin and enable its quantification even in crude substrate mixtures, without purification. Compared to the commonly used acid hydrolysis, the enzymatic method presented here is faster and stereospecific and selectively cleaves laminarin in mixtures of glycans, releasing only glucose and oligosaccharides, which can be easily quantified with reducing sugar assays.
author Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire
spellingShingle Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire
Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
author_facet Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire
author_sort Becker, Stefan; Scheffel, André; Polz, Martin F.; Hehemann, Jan-Hendrik; Vieille, Claire
title Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
title_short Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
title_full Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
title_fullStr Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
title_full_unstemmed Accurate Quantification of Laminarin in Marine Organic Matter with Enzymes from Marine Microbes
title_sort accurate quantification of laminarin in marine organic matter with enzymes from marine microbes
publishDate 2019
url http://www.osti.gov/servlets/purl/1536860
https://www.osti.gov/biblio/1536860
https://doi.org/10.1128/aem.03389-16
geographic Arctic
Arctic Ocean
geographic_facet Arctic
Arctic Ocean
genre Arctic
Arctic Ocean
genre_facet Arctic
Arctic Ocean
op_relation http://www.osti.gov/servlets/purl/1536860
https://www.osti.gov/biblio/1536860
https://doi.org/10.1128/aem.03389-16
doi:10.1128/aem.03389-16
op_doi https://doi.org/10.1128/aem.03389-16
container_title Applied and Environmental Microbiology
container_volume 83
container_issue 9
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