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Difference between revisions of "Glycoside Hydrolase Family 128"
Harry Brumer (talk | contribs) m (minor grammatical improvements) |
Harry Brumer (talk | contribs) (Made "Clustering" section a subsection of Substrate Specificites and shortened it.) |
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== Substrate specificities == | == Substrate specificities == | ||
− | The first GH128 enzyme, GLU1, was cloned from ''Lentinula edodes'' fruiting bodies (shiitake mushroom) <cite>Sakamoto2011</cite>. GLU1 cleaves β-1,3 linkages in various β-glucans such as endogenous 'L. edodes'' lentinan, laminarin from ''Laminaria digitata'', pachyman from ''Poria cocos'', and curdlan from ''Alcaligenes faecalis'', but does not degrade β-1,3-linkages within β-1,3-1,4-glucans such as barley glucan, indicating the enzyme is categorized into EC [{{EClink}}3.2.1.39 3.2.1.39] <cite>Sakamoto2011</cite>. Further work with several GH128 members corroborated that this family is specific for β-1,3-glucans <cite>Santos2020</cite>. In addition, it was demonstrated that bacterial members, such as those from ''Amycolatopsis mediterranei'' (subgroup I) and ''Pseudomonas viridiflava'' (subgroup II), are endo-β-1,3-glucanases that degrade these carbohydrates at higher rates <cite>Santos2020</cite>. Fungal GH128 members are more diverse in terms of activity: endo-β-1,3-glucanases, represented by the GLU1 from ''L. edodes'' (subgroup IV) <cite>Sakamoto2011 Santos2020</cite>; exo-β-1,3-glucanases that release trisaccharides (''Aureobsidium namibiae'') (subgroup VI) <cite>Santos2020</cite> and monosaccharides (''Cryptococcus neoformans'') (subgroup V) from the reducing ends; and exo-β-1,3-glucanases that release trisaccharides from the non-reducing ends of triple-helical β-1,3-glucans, represented by the enzyme from ''Blastomyces gilchristii'' (subgroup III) <cite>Santos2020</cite>. Some fungal members from this family, such as those from ''Trichoderma gamsii'' and ''C. neoformans'', are devoid of catalytic activity but conserve the capacity to bind short β-1,3-glucooligosaccharides (subgroup VII) <cite>Santos2020</cite>. | + | The first GH128 enzyme, GLU1, was cloned from ''Lentinula edodes'' fruiting bodies (shiitake mushroom) <cite>Sakamoto2011</cite>. GLU1 cleaves β-1,3 linkages in various β-glucans such as endogenous ''L. edodes'' lentinan, laminarin from ''Laminaria digitata'', pachyman from ''Poria cocos'', and curdlan from ''Alcaligenes faecalis'', but does not degrade β-1,3-linkages within β-1,3-1,4-glucans such as barley glucan, indicating the enzyme is categorized into EC [{{EClink}}3.2.1.39 3.2.1.39] <cite>Sakamoto2011</cite>. Further work with several GH128 members corroborated that this family is specific for β-1,3-glucans <cite>Santos2020</cite>. In addition, it was demonstrated that bacterial members, such as those from ''Amycolatopsis mediterranei'' (subgroup I) and ''Pseudomonas viridiflava'' (subgroup II), are endo-β-1,3-glucanases that degrade these carbohydrates at higher rates <cite>Santos2020</cite>. Fungal GH128 members are more diverse in terms of activity: endo-β-1,3-glucanases, represented by the GLU1 from ''L. edodes'' (subgroup IV) <cite>Sakamoto2011 Santos2020</cite>; exo-β-1,3-glucanases that release trisaccharides (''Aureobsidium namibiae'') (subgroup VI) <cite>Santos2020</cite> and monosaccharides (''Cryptococcus neoformans'') (subgroup V) from the reducing ends; and exo-β-1,3-glucanases that release trisaccharides from the non-reducing ends of triple-helical β-1,3-glucans, represented by the enzyme from ''Blastomyces gilchristii'' (subgroup III) <cite>Santos2020</cite>. Some fungal members from this family, such as those from ''Trichoderma gamsii'' and ''C. neoformans'', are devoid of catalytic activity but conserve the capacity to bind short β-1,3-glucooligosaccharides (subgroup VII) <cite>Santos2020</cite>. |
+ | |||
+ | === Clustering of GH128 === | ||
+ | [[Image:Santos_GH128_final.png|thumb|right|250px|Figure 1. Clustering of the GH128 family into seven subgroups. Adapted from <cite>Santos2020</cite>.]] | ||
+ | GH128 was created based on the study of ^^^Yuichi Sakamoto^^^ and colleagues <cite>Sakamoto2011</cite>. Years later, a group headed by ^^^Mario Murakami^^^ explored the functional and structural diversity of this family <cite>Santos2020</cite>. For this purpose, they employed phylogenetic and Sequence Similarity Network (SSN, <cite>Atkinson2009</cite>) analyses to segregate the family into putative isofunctional subgroups. The SSN analysis resulted in two discrete clusters (subgroups VI and VII) and a third cluster that was further subdivided into five subgroups (I to V) based on SSN alignment scores and evolutionary closeness (Fig. 1). At least one member of each subgroup was biochemically and structurally characterized: AmGH128_I, PvGH128_II, ScGH128_II, BgGH128_III, LeGH128_IV, CnGH128_V, AnGH128_VI, TgGH128_VII and CnGH128_VII. Subgroups I and II were found to be predominantly present in bacteria, and the subgroups III to VII are mostly found in fungi. Bacterial enzymes are faster, present a substrate-interacting "hydrophobic knuckle" (see [[#Three-dimensional structures]]) and attack the β-1,3-glucan in an endo mode of action, which is compatible with their biological function: nutrition and competition. Fungal β-1,3-glucanases are known to act on remodeling of their own cell walls. Therefore, these enzymes are slower, more diverse in terms of substrate recognition modes (flattening mechanism – subgroups IV and VI; hydrophobic knuckle – subgroups III, V and VII) and mode of action (exo-enzymes – subgroups III, V and VI; endo-enzymes – subgroup IV; oligosaccharide binding proteins – subgroup VII). | ||
== Kinetics and Mechanism == | == Kinetics and Mechanism == | ||
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Two distinct modes of substrate binding were observed in the GH128 family <cite>Santos2020</cite>. The most widespread mode, termed the "hydrophobic knuckle", involves a tryptophan residue that interacts with four glucoside moieties from –5 to –2 and is fully complementary to the typically curved conformation of β-1,3-glucan chains. The other mode, only observed in fungal members belonging to subgroups IV and VI, requires substrate conformational changes to allow the binding to the catalytic interface. In these fungal subgroups, the hydrophobic knuckle is absent and two aromatic residues, positioned at the -5 and -4 subsites, create a linearized cleft, which requires a 180° torsion in the glycosidic bond between the glycosyl moieties –2 and –3 in the β-1,3-glucan chain for binding. This mode of substrate recognition is referred to as the "flattening" mechanism, due to the unusual, but also stereochemically favorable, conformation adopted by the substrate. It is notable that the mode of substrate binding has not been observed in other CAZy families active on β-1,3-glucans. | Two distinct modes of substrate binding were observed in the GH128 family <cite>Santos2020</cite>. The most widespread mode, termed the "hydrophobic knuckle", involves a tryptophan residue that interacts with four glucoside moieties from –5 to –2 and is fully complementary to the typically curved conformation of β-1,3-glucan chains. The other mode, only observed in fungal members belonging to subgroups IV and VI, requires substrate conformational changes to allow the binding to the catalytic interface. In these fungal subgroups, the hydrophobic knuckle is absent and two aromatic residues, positioned at the -5 and -4 subsites, create a linearized cleft, which requires a 180° torsion in the glycosidic bond between the glycosyl moieties –2 and –3 in the β-1,3-glucan chain for binding. This mode of substrate recognition is referred to as the "flattening" mechanism, due to the unusual, but also stereochemically favorable, conformation adopted by the substrate. It is notable that the mode of substrate binding has not been observed in other CAZy families active on β-1,3-glucans. | ||
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== Family Firsts == | == Family Firsts == | ||
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#Sakamoto2011 pmid=21965406 | #Sakamoto2011 pmid=21965406 | ||
#Santos2020 pmid=32451508 | #Santos2020 pmid=32451508 | ||
− | # | + | #Atkinson2009 pmid=19190775 |
</biblio> | </biblio> |
Revision as of 07:37, 17 August 2020
This page is currently under construction. This means that the Responsible Curator has deemed that the page's content is not quite up to CAZypedia's standards for full public consumption. All information should be considered to be under revision and may be subject to major changes.
- Author: ^^^Yuichi Sakamoto^^^ and ^^^Camilla Santos^^^
- Responsible Curator: ^^^Mario Murakami^^^
Glycoside Hydrolase Family GH128 | |
Clan | GH-A |
Mechanism | retaining |
Active site residues | known |
CAZy DB link | |
https://www.cazy.org/GH128.html |
Substrate specificities
The first GH128 enzyme, GLU1, was cloned from Lentinula edodes fruiting bodies (shiitake mushroom) [1]. GLU1 cleaves β-1,3 linkages in various β-glucans such as endogenous L. edodes lentinan, laminarin from Laminaria digitata, pachyman from Poria cocos, and curdlan from Alcaligenes faecalis, but does not degrade β-1,3-linkages within β-1,3-1,4-glucans such as barley glucan, indicating the enzyme is categorized into EC 3.2.1.39 [1]. Further work with several GH128 members corroborated that this family is specific for β-1,3-glucans [2]. In addition, it was demonstrated that bacterial members, such as those from Amycolatopsis mediterranei (subgroup I) and Pseudomonas viridiflava (subgroup II), are endo-β-1,3-glucanases that degrade these carbohydrates at higher rates [2]. Fungal GH128 members are more diverse in terms of activity: endo-β-1,3-glucanases, represented by the GLU1 from L. edodes (subgroup IV) [1, 2]; exo-β-1,3-glucanases that release trisaccharides (Aureobsidium namibiae) (subgroup VI) [2] and monosaccharides (Cryptococcus neoformans) (subgroup V) from the reducing ends; and exo-β-1,3-glucanases that release trisaccharides from the non-reducing ends of triple-helical β-1,3-glucans, represented by the enzyme from Blastomyces gilchristii (subgroup III) [2]. Some fungal members from this family, such as those from Trichoderma gamsii and C. neoformans, are devoid of catalytic activity but conserve the capacity to bind short β-1,3-glucooligosaccharides (subgroup VII) [2].
Clustering of GH128
GH128 was created based on the study of ^^^Yuichi Sakamoto^^^ and colleagues [1]. Years later, a group headed by ^^^Mario Murakami^^^ explored the functional and structural diversity of this family [2]. For this purpose, they employed phylogenetic and Sequence Similarity Network (SSN, [3]) analyses to segregate the family into putative isofunctional subgroups. The SSN analysis resulted in two discrete clusters (subgroups VI and VII) and a third cluster that was further subdivided into five subgroups (I to V) based on SSN alignment scores and evolutionary closeness (Fig. 1). At least one member of each subgroup was biochemically and structurally characterized: AmGH128_I, PvGH128_II, ScGH128_II, BgGH128_III, LeGH128_IV, CnGH128_V, AnGH128_VI, TgGH128_VII and CnGH128_VII. Subgroups I and II were found to be predominantly present in bacteria, and the subgroups III to VII are mostly found in fungi. Bacterial enzymes are faster, present a substrate-interacting "hydrophobic knuckle" (see #Three-dimensional structures) and attack the β-1,3-glucan in an endo mode of action, which is compatible with their biological function: nutrition and competition. Fungal β-1,3-glucanases are known to act on remodeling of their own cell walls. Therefore, these enzymes are slower, more diverse in terms of substrate recognition modes (flattening mechanism – subgroups IV and VI; hydrophobic knuckle – subgroups III, V and VII) and mode of action (exo-enzymes – subgroups III, V and VI; endo-enzymes – subgroup IV; oligosaccharide binding proteins – subgroup VII).
Kinetics and Mechanism
As indicated by the first study of a GH128 enzyme [1], this family is part of Clan GH-A, thus suggesting that its members operate by a classical Koshland retaining mechanism. This prediction was confirmed through 1H-nuclear magnetic resonance spectroscopy of enzymatic products [2].
Catalytic Residues
From the sequence alignment of GH128 members, two glutamic acids, E103 and E195 in L. edodes GLU1, were predicted to be the catalytic residues [1]. They were further confirmed to be the general acid/base and the catalytic nucleophile, respectively, by site-directed mutagenesis of the bacterial GH128 member from A. mediterranei [2]. These residues are located at the C-terminal ends of the strands β7 and β4 [2], as observed for other clan GH-A families.
Three-dimensional structures
A three-dimensional homology model of L. edodes GLU1 indicated similarity with several (β/α)8-barrel (TIM-barrel) structures, including a GH39 β-xylosidase and a GH5 β-mannanase [1]. The fold resembling an (β/α)8-barrel was further confirmed with the crystal structure determination of 9 members of the family [2]. However, in all structures, the helix α2 and the strand β3 are strictly absent [2]. Moreover, some enzymes such as the endo-β-1,3-glucanase from L. edodes (GLU1) and the exo-β-1,3-glucanase from C. neoformans, also lack the helices α1 and α3, respectively [2].
Two distinct modes of substrate binding were observed in the GH128 family [2]. The most widespread mode, termed the "hydrophobic knuckle", involves a tryptophan residue that interacts with four glucoside moieties from –5 to –2 and is fully complementary to the typically curved conformation of β-1,3-glucan chains. The other mode, only observed in fungal members belonging to subgroups IV and VI, requires substrate conformational changes to allow the binding to the catalytic interface. In these fungal subgroups, the hydrophobic knuckle is absent and two aromatic residues, positioned at the -5 and -4 subsites, create a linearized cleft, which requires a 180° torsion in the glycosidic bond between the glycosyl moieties –2 and –3 in the β-1,3-glucan chain for binding. This mode of substrate recognition is referred to as the "flattening" mechanism, due to the unusual, but also stereochemically favorable, conformation adopted by the substrate. It is notable that the mode of substrate binding has not been observed in other CAZy families active on β-1,3-glucans.
Family Firsts
- First stereochemistry determination
- predicted to be retaining by membership in Clan GH-A [1] and further validated by 1H-NMR of products of the A. mediterranei endo-β-1,3-glucanase (AmGH128_I) [2].
- First catalytic nucleophile identification
- predicted by sequence alignment [1] and confirmed by site-directed mutagenesis of A. mediterranei endo-β-1,3-glucanase (AmGH128_I) [2].
- First general acid/base residue identification
- predicted by sequence alignment [1] and confirmed by site-directed mutagenesis of A. mediterranei endo-β-1,3-glucanase (AmGH128_I) [2].
- First 3-D structure
- predicted by modelling of L. edodes GLU1 [1] and experimentally determined for several GH128 members including endo-β-1,3-glucanases from A. mediterranei (AmGH128_I), P. viridiflava (PvGH128_II), Sorangium cellulosum (ScGH128_II) and L. edodes (LeGH128_IV); exo-β-1,3-glucanases from B. gilchristii (BgGH128_III), C. neoformans (CnGH128_V) and A. namibiae (AnGH128_VI); and β-1,3-glucooligosaccharide binding proteins from T. gamsii (TgGH128_VII) and C. neoformans (CnGH128_VII) [2].
References
- Sakamoto Y, Nakade K, and Konno N. (2011). Endo-β-1,3-glucanase GLU1, from the fruiting body of Lentinula edodes, belongs to a new glycoside hydrolase family. Appl Environ Microbiol. 2011;77(23):8350-4. DOI:10.1128/AEM.05581-11 |
- Santos CR, Costa PACR, Vieira PS, Gonzalez SET, Correa TLR, Lima EA, Mandelli F, Pirolla RAS, Domingues MN, Cabral L, Martins MP, Cordeiro RL, Junior AT, Souza BP, Prates ÉT, Gozzo FC, Persinoti GF, Skaf MS, and Murakami MT. (2020). Structural insights into β-1,3-glucan cleavage by a glycoside hydrolase family. Nat Chem Biol. 2020;16(8):920-929. DOI:10.1038/s41589-020-0554-5 |
- Atkinson HJ, Morris JH, Ferrin TE, and Babbitt PC. (2009). Using sequence similarity networks for visualization of relationships across diverse protein superfamilies. PLoS One. 2009;4(2):e4345. DOI:10.1371/journal.pone.0004345 |