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Difference between revisions of "Carbohydrate Binding Module Family 16"
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* [[Author]]: [[User:Maria_Matard-Mann|Maria Matard-Mann]] | * [[Author]]: [[User:Maria_Matard-Mann|Maria Matard-Mann]] | ||
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== Ligand specificities == | == Ligand specificities == | ||
− | Family 16 CBMs | + | Family 16 CBMs are found essentially in bacteria (with the exception of some CBM16 members in archaea). They are also found associated with catalytic modules belonging mainly to 4 families of CAZymes: [[GH5]] mannanases <cite>Bae2008 Su2010</cite>, [[GH16]] kappa carrageenases <cite>Barbeyron1998 Matard-Mann2017 Salmean2018</cite>, [[GH18]] chitinases <cite>Barabote2009</cite> and [[PL18]] alginate lyases <cite>Dong2014 Sim2017</cite>. Binding to glucomannan and kappa-carrageenan has been demonstrated <cite>Bae2008 Su2010 Salmean2018</cite>. CBM16 binding to glucomannan (mixed β-1,4-linked polymer contains both glucose and mannose) has been studied by ITC (isothermal titration calorimetry) analyses and X-ray crystallography of complexes with pentomannan and pentoglucan <cite>Bae2008 Su2010</cite>. Conversely, binding to kappa-carrageenan has been shown by a double-blind approach using polysaccharide microarrays <cite>Salmean2018</cite>. |
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== Structural Features == | == Structural Features == | ||
+ | [[File:CBM16-1.png|thumb|300px|right|'''Figure 1.''' The structure of CBM16-1 of ''Caldanaerobius polysaccharolyticus'' ManA, in complex with cellopentaose, [{{PDBlink}}2zex PDB ID 2zex]. Four key residues of the binding cleft are highlighted. ]] | ||
+ | CBM16 is a [[Carbohydrate-binding_modules#Types|type B]] CBM family, with a characteristic concave cleft, allowing the binding of ligand longer than triose. The ligand binding cleft shows some promiscuity as it can accommodate pentoses containing glucose and mannose, but only in the context of planar polymers like β-1,4-glucans and not helical β-1,3-glucans <cite>Bae2008</cite>. The crystallographic structure determination of both CBMs from ''Caldanaerobius polysaccharolyticus'' (formerly ''Thermoanaerobacterium polysaccharolyticum'') ManA revealed the importance of two aromatic residues in the binding cleft as well as two stretches of polar residues on both sides of the cleft, [{{PDBlink}}2zew PDB ID 2zew] <cite>Bae2008</cite>. Affinity studies of targeted mutants for the predicted key residues confirmed the importance of two tryptophans (Trp-20 and Trp-125), and two glutamines (Gln-81 and Gln-93) <cite>Su2010</cite> (see Figure 1). | ||
− | + | Based on sequence similarity and conservation of secondary structure elements it has been proposed that, along with the [[CBM4]], [[CBM17]], [[CBM22]] and [[CBM27]] families, they form a superfamily <cite>Sunna2001</cite>. | |
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− | Based on sequence similarity and conservation of secondary structure | ||
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== Functionalities == | == Functionalities == | ||
− | In the Man5A of Caldanaerobius polysaccharolyticus, the deletion of its | + | In the Man5A of ''Caldanaerobius polysaccharolyticus'', the deletion of both its CBM16s severely impairs the ability of the catalytic module ([[GH5]]) to bind cellulose <cite>Cann1999</cite>. |
− | In the case of CgkA from Zobellia galactanivorans, the presence of the CBM16 is not required for the enzymatic activity on kappa-carrageenan, but has been shown to take part in the processive mechanism of the catalytic module (GH16) <cite>Matard-Mann2017</cite>. | + | In the case of CgkA from ''Zobellia galactanivorans'', the presence of the CBM16 is not required for the enzymatic activity on kappa-carrageenan, but has been shown to take part in the processive mechanism of the catalytic module ([[GH16]]) <cite>Matard-Mann2017</cite>. |
− | Even if frequently | + | Even if frequently encoded within the gene for alginate lyase from family [[PL18]], it is absent in the mature form of the enzyme, and no role in alginate degradation has been found up to now <cite>Sim2017</cite>. A chaperone function of this N-terminal module has been proposed after observation that its deletion hindered the correct folding and activity of the catalytic module <cite>Dong2014</cite>. |
− | + | == Family Firsts == | |
− | + | ;First Identified: Cloning of Man5A GH5 by Cann ''et al''. in 1999 reaveled the presence of two tandem CBM16s on the C-terminal end. Their deletion resulted in failure of the catalytic module to bind to a cellulose column, and significant loss of both mannanase and carboxy methylcellulase activities <cite>Cann1999</cite>. | |
− | |||
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− | + | ;First Structural Characterization: In 2008 Bae ''et al''. solved the first structures of the CBM16 family: both modules of ''Caldanaerobius polysaccharolyticus'' Man5A, [{{PDBlink}}2zew PDB ID 2zew], and two complexes of CBM16-1, one with cellopentaose [{{PDBlink}}2zex PDB ID 2zex] and one with mannopentaose [{{PDBlink}}2zey PDB ID 2zey]<cite>Bae2008</cite>. | |
− | ;First | ||
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− | <cite>Bae2008</cite> | ||
== References == | == References == | ||
<biblio> | <biblio> | ||
− | #Bae2008 pmid= | + | #Bae2008 pmid=18025086 |
− | #Su2010 pmid= | + | #Su2010 pmid=20739280 |
− | #Barbeyron1998 pmid= | + | #Barbeyron1998 pmid=9580981 |
− | #Matard-Mann2017 pmid= | + | #Matard-Mann2017 pmid=29030427 |
− | # | + | #Salmean2018 pmid=29410423 |
− | + | #Barabote2009 pmid=19270083 | |
− | #Barabote2009 pmid= | + | #Dong2014 pmid=25210041 |
− | + | #Sim2017 pmid=29057942 | |
− | #Dong2014 pmid= | + | #Sunna2001 pmid=11389686 |
− | #Sim2017 pmid= | + | #Cann1999 pmid=10049399 |
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− | # | ||
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</biblio> | </biblio> | ||
[[Category:Carbohydrate Binding Module Families|CBM016]] <!-- ATTENTION: Make sure to replace "nnn" with a three digit family number, e.g. "032" or "105" etc., for proper sorting of the page by family number. --> | [[Category:Carbohydrate Binding Module Families|CBM016]] <!-- ATTENTION: Make sure to replace "nnn" with a three digit family number, e.g. "032" or "105" etc., for proper sorting of the page by family number. --> |
Latest revision as of 13:16, 18 December 2021
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CAZy DB link | |
https://www.cazy.org/CBM16.html |
Ligand specificities
Family 16 CBMs are found essentially in bacteria (with the exception of some CBM16 members in archaea). They are also found associated with catalytic modules belonging mainly to 4 families of CAZymes: GH5 mannanases [1, 2], GH16 kappa carrageenases [3, 4, 5], GH18 chitinases [6] and PL18 alginate lyases [7, 8]. Binding to glucomannan and kappa-carrageenan has been demonstrated [1, 2, 5]. CBM16 binding to glucomannan (mixed β-1,4-linked polymer contains both glucose and mannose) has been studied by ITC (isothermal titration calorimetry) analyses and X-ray crystallography of complexes with pentomannan and pentoglucan [1, 2]. Conversely, binding to kappa-carrageenan has been shown by a double-blind approach using polysaccharide microarrays [5].
Structural Features
CBM16 is a type B CBM family, with a characteristic concave cleft, allowing the binding of ligand longer than triose. The ligand binding cleft shows some promiscuity as it can accommodate pentoses containing glucose and mannose, but only in the context of planar polymers like β-1,4-glucans and not helical β-1,3-glucans [1]. The crystallographic structure determination of both CBMs from Caldanaerobius polysaccharolyticus (formerly Thermoanaerobacterium polysaccharolyticum) ManA revealed the importance of two aromatic residues in the binding cleft as well as two stretches of polar residues on both sides of the cleft, PDB ID 2zew [1]. Affinity studies of targeted mutants for the predicted key residues confirmed the importance of two tryptophans (Trp-20 and Trp-125), and two glutamines (Gln-81 and Gln-93) [2] (see Figure 1).
Based on sequence similarity and conservation of secondary structure elements it has been proposed that, along with the CBM4, CBM17, CBM22 and CBM27 families, they form a superfamily [9].
Functionalities
In the Man5A of Caldanaerobius polysaccharolyticus, the deletion of both its CBM16s severely impairs the ability of the catalytic module (GH5) to bind cellulose [10].
In the case of CgkA from Zobellia galactanivorans, the presence of the CBM16 is not required for the enzymatic activity on kappa-carrageenan, but has been shown to take part in the processive mechanism of the catalytic module (GH16) [4].
Even if frequently encoded within the gene for alginate lyase from family PL18, it is absent in the mature form of the enzyme, and no role in alginate degradation has been found up to now [8]. A chaperone function of this N-terminal module has been proposed after observation that its deletion hindered the correct folding and activity of the catalytic module [7].
Family Firsts
- First Identified
- Cloning of Man5A GH5 by Cann et al. in 1999 reaveled the presence of two tandem CBM16s on the C-terminal end. Their deletion resulted in failure of the catalytic module to bind to a cellulose column, and significant loss of both mannanase and carboxy methylcellulase activities [10].
- First Structural Characterization
- In 2008 Bae et al. solved the first structures of the CBM16 family: both modules of Caldanaerobius polysaccharolyticus Man5A, PDB ID 2zew, and two complexes of CBM16-1, one with cellopentaose PDB ID 2zex and one with mannopentaose PDB ID 2zey[1].
References
- Bae B, Ohene-Adjei S, Kocherginskaya S, Mackie RI, Spies MA, Cann IK, and Nair SK. (2008). Molecular basis for the selectivity and specificity of ligand recognition by the family 16 carbohydrate-binding modules from Thermoanaerobacterium polysaccharolyticum ManA. J Biol Chem. 2008;283(18):12415-25. DOI:10.1074/jbc.M706513200 |
- Su X, Agarwal V, Dodd D, Bae B, Mackie RI, Nair SK, and Cann IK. (2010). Mutational insights into the roles of amino acid residues in ligand binding for two closely related family 16 carbohydrate binding modules. J Biol Chem. 2010;285(45):34665-76. DOI:10.1074/jbc.M110.168302 |
- Barbeyron T, Gerard A, Potin P, Henrissat B, and Kloareg B. (1998). The kappa-carrageenase of the marine bacterium Cytophaga drobachiensis. Structural and phylogenetic relationships within family-16 glycoside hydrolases. Mol Biol Evol. 1998;15(5):528-37. DOI:10.1093/oxfordjournals.molbev.a025952 |
- Matard-Mann M, Bernard T, Leroux C, Barbeyron T, Larocque R, Préchoux A, Jeudy A, Jam M, Nyvall Collén P, Michel G, and Czjzek M. (2017). Structural insights into marine carbohydrate degradation by family GH16 κ-carrageenases. J Biol Chem. 2017;292(48):19919-19934. DOI:10.1074/jbc.M117.808279 |
- Salmeán AA, Guillouzo A, Duffieux D, Jam M, Matard-Mann M, Larocque R, Pedersen HL, Michel G, Czjzek M, Willats WGT, and Hervé C. (2018). Double blind microarray-based polysaccharide profiling enables parallel identification of uncharacterized polysaccharides and carbohydrate-binding proteins with unknown specificities. Sci Rep. 2018;8(1):2500. DOI:10.1038/s41598-018-20605-9 |
- Barabote RD, Xie G, Leu DH, Normand P, Necsulea A, Daubin V, Médigue C, Adney WS, Xu XC, Lapidus A, Parales RE, Detter C, Pujic P, Bruce D, Lavire C, Challacombe JF, Brettin TS, and Berry AM. (2009). Complete genome of the cellulolytic thermophile Acidothermus cellulolyticus 11B provides insights into its ecophysiological and evolutionary adaptations. Genome Res. 2009;19(6):1033-43. DOI:10.1101/gr.084848.108 |
- Dong S, Wei TD, Chen XL, Li CY, Wang P, Xie BB, Qin QL, Zhang XY, Pang XH, Zhou BC, and Zhang YZ. (2014). Molecular insight into the role of the N-terminal extension in the maturation, substrate recognition, and catalysis of a bacterial alginate lyase from polysaccharide lyase family 18. J Biol Chem. 2014;289(43):29558-69. DOI:10.1074/jbc.M114.584573 |
- Sim PF, Furusawa G, and Teh AH. (2017). Functional and Structural Studies of a Multidomain Alginate Lyase from Persicobacter sp. CCB-QB2. Sci Rep. 2017;7(1):13656. DOI:10.1038/s41598-017-13288-1 |
- Sunna A, Gibbs MD, and Bergquist PL. (2001). Identification of novel beta-mannan- and beta-glucan-binding modules: evidence for a superfamily of carbohydrate-binding modules. Biochem J. 2001;356(Pt 3):791-8. DOI:10.1042/0264-6021:3560791 |
- Cann IK, Kocherginskaya S, King MR, White BA, and Mackie RI. (1999). Molecular cloning, sequencing, and expression of a novel multidomain mannanase gene from Thermoanaerobacterium polysaccharolyticum. J Bacteriol. 1999;181(5):1643-51. DOI:10.1128/JB.181.5.1643-1651.1999 |