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Difference between revisions of "Glycoside Hydrolase Family 16"

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* [[Author]]: [[User:JensEklof|Jens Eklöf]]
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* [[Author]]: [[User:JensEklof|Jens Eklöf]] and [[User:Jan-Hendrik Hehemann|Jan-Hendrik Hehemann]]
* [[Responsible Curator]]:  ^^^Harry Brumer^^^
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* [[Responsible Curator]]:  [[User:Harry Brumer|Harry Brumer]]
 
----
 
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|{{Hl2}} colspan="2" align="center" |'''CAZy DB link'''
 
|{{Hl2}} colspan="2" align="center" |'''CAZy DB link'''
 
|-
 
|-
| colspan="2" |http://www.cazy.org/fam/GH16.html
+
| colspan="2" |{{CAZyDBlink}}GH16.html
 
|}
 
|}
 
</div>
 
</div>
  
 
== Substrate specificities ==
 
== Substrate specificities ==
[[Glycoside hydrolases]] of family 16 enzymes cleave &beta;-1,4 or &beta;-1,3 glycosidic bonds in various glucans and galactans. Some members of this family operating on xyloglucan exhibit predominant ''[[endo]]''-transglycosylase activity <cite>NXG</cite>.
+
The members of family 16 are active on &beta;-1,4 or &beta;-1,3 glycosidic bonds in various glucans and galactans. A wide diversity of [[glycoside hydrolases]] active on plant and marine polysaccharides are found in GH16, including:
The substrate specificities found in GH16 are: xyloglucan:xyloglucosyltransferases (EC [{{EClink}}2.4.1.207 2.4.1.207]),  
+
* keratan-sulfate ''[[endo]]''-1,4-&beta;-galactosidases (EC [{{EClink}}3.2.1.103 3.2.1.103]),
keratan-sulfate ''[[endo]]''-1,4-&beta;-galactosidases (EC [{{EClink}}3.2.1.103 3.2.1.103]), ''[[endo]]''-1,3-&beta;-glucanases (EC [{{EClink}}3.2.1.39 3.2.1.39]), ''[[endo]]''-1,3(4)-&beta;-glucanases (EC [{{EClink}}3.2.1.6 3.2.1.6]), lichenases (EC [{{EClink}}3.2.1.73 3.2.1.73]), &beta;-agarases (EC [{{EClink}}3.2.1.81 3.2.1.81]), &kappa;-carrageenases (EC [{{EClink}}3.2.1.83 3.2.1.83]) and xyloglucanases (EC [{{EClink}}3.2.1.151 3.2.1.151]).
+
* ''[[endo]]''-1,3-&beta;-galactanases (EC [{{EClink}}3.2.1.* 3.2.1.-]),
 +
* ''[[endo]]''-1,3-&beta;-glucanases (EC [{{EClink}}3.2.1.39 3.2.1.39]),
 +
* ''[[endo]]''-1,3(4)-&beta;-glucanases (EC [{{EClink}}3.2.1.6 3.2.1.6]),
 +
* licheninases (EC [{{EClink}}3.2.1.73 3.2.1.73]),
 +
* &beta;-agarases (EC [{{EClink}}3.2.1.81 3.2.1.81]),
 +
* &beta;-porphyranases (EC [{{EClink}}3.2.1.178 3.2.1.178]) <cite>Hehemann2010</cite>,
 +
* &kappa;-carrageenases (EC [{{EClink}}3.2.1.83 3.2.1.83]), and
 +
* endo-xyloglucanases (EC [{{EClink}}3.2.1.151 3.2.1.151], a.k.a. xyloglucan endo-hydrolases, XEHs, in plants <cite>Eklof2010</cite>).
 +
 
 +
Notably, some members of GH16 are predominant [[transglycosylases]].  These include the plant xyloglucan:xyloglucosyltransferases (EC [{{EClink}}2.4.1.207 2.4.1.207], a.k.a. xyloglucan endo-transglycosylases, XETs) <cite>Eklof2010</cite> and yeast chitin/beta-glucan crosslinking enzymes Crh1 and Crh2 <cite>Cabib2008 Mazan2013 Blanco2015</cite>. Some invertebrate GH16 proteins have lost their catalytic amino acids and are involved in immune response activation through the Toll pathway upon binding of &beta;-1,3 glucan. The role of the GH16 domain in this immune response has not been fully elucidated <cite>Lee2009</cite>.
 +
 
 +
Several of the activities observed for GH16 members are delineated into individual sequence-based subfamilies, while other polyspecific subfamilies capture a range of activities <cite>Viborg2019</cite>.
 +
 
 +
<gallery widths=270px perrow=3 caption="Diverse polysaccharides cleaved by GH16 enzymes">
 +
 
 +
File:AgarIII.png|'''Agar''' <br> &beta;-D-Gal''p''-(1,4)-&alpha;-L-3,6-anhydro-Gal''p''-1,3-&beta;-D-Gal''p''-(1,4)-&alpha;-L-3,6-anhydro-Gal''p''
 +
 
 +
File:Kappa_carrageenan.png|'''&kappa;-carrageenan''' <br> &beta;-D-Gal''p''-(1,4)-&alpha;-D-3,6-anhydro-Gal''p''-1,3-&beta;-D-Gal''p''-(1,4)-&alpha;-D-3,6-anhydro-Gal''p''
 +
 
 +
File:porphyran.png|'''Porphyran''' <br>
 +
 
 +
File:laminaritetraose.png|'''&beta;-1,3-glucan''' <br> &beta;-D-Glc''p''-(1,3)- &beta;-D-Glc''p''-(1,3)- &beta;-D-Glc''p''-(1,3)- &beta;-D-Glc''p''
 +
 
 +
File:keratan_sulphate.png|'''Keratan sulphate''' <br> &beta;-D-Gal''p''-(1,4)- &beta;-D-Glc''p''NAc 6-sulphate-(1,3)- &beta;-D-Gal''p''-(1,4)- &beta;-D-Glc''p''NAc 6-sulphate
 +
 
 +
File:beta_13_galactan.png|'''&beta;-1,3-galactan''' <br> &beta;-D-Gal''p''-(1,3)- &beta;-D-Gal''p''-(1,3)- &beta;-D-Gal''p''-(1,3)- &beta;-D-Gal''p''
 +
 
 +
File:MLG_pentaose.png|'''&beta;-1,4/1,3-glucan''' <br> &beta;-D-Glc''p''-(1,4)- &beta;-D-Glc''p''-(1,4)- &beta;-D-Glc''p''-(1,3)- &beta;-D-Glc''p''-(1,4)- &beta;-D-Glc''p''
 +
 
 +
 
 +
File:beta_14_galactan.png|'''&beta;-1,4-galactan''' <br> &beta;-D-Gal''p''-(1,4)- &beta;-D-Gal''p''-(1,4)- &beta;-D-Gal''p''-(1,4)- &beta;-D-Gal''p''
 +
 
 +
File:Xyloglucan.png|'''Xyloglucan''' <br>
 +
 
 +
</gallery>
  
 
== Kinetics and Mechanism ==
 
== Kinetics and Mechanism ==
Family 16 enzymes are [[retaining]] enzymes, as first shown by NMR <cite>REF3</cite> on an ''[[endo]]''-1,3-1,4-&beta;-D-glucan 4-glucanohydrolase from ''Bacillus licheniformis''.  
+
Members of GH16 enzymes are [[retaining]] enzymes, as first shown by NMR <cite>Malet1993</cite> on an ''[[endo]]''-1,3-1,4-&beta;-D-glucan 4-glucanohydrolase from ''Bacillus licheniformis''. As such, they utilize a covalent glycosyl-enzyme intermediate, which is broken-down by glycosyl transfer <cite>Sinnott1990 Bissaro2015</cite> to water or a carbohydrate acceptor substrate in [[glycoside hydrolases]] or [[transglycosylases]], respectively.
  
 
== Catalytic Residues ==
 
== Catalytic Residues ==
The [[catalytic nucleophile]] was first proposed using a non-specific epoxyalkyl &beta;-glycoside inhibitor and subsequent peptide identification by ESI-MS and Edman degradation on an ''[[endo]]''-1,3-1,4-&beta;-D-glucan 4-glucanohydrolase from ''Bacillus amyloliquefaciens'' <cite>REF4</cite>. This was subsequently verified by azide rescue of the E134A mutant of a ''Bacillus licheniformis''  1,3-1,4-&beta;-D-glucan 4-glucanohydrolase resulting in an &alpha;-glycosyl azide from the &beta;-glycosyl substrate <cite>7</cite>.
+
The [[catalytic nucleophile]] of GH16 enzymes was first proposed using a non-specific epoxyalkyl &beta;-glycoside inhibitor and identification of the site of covalent labelling using ESI-MS and Edman degradation on an ''[[endo]]''-1,3-1,4-&beta;-D-glucan 4-glucanohydrolase from ''Bacillus amyloliquefaciens'' <cite>Hoj1992</cite>. This was subsequently verified by azide rescue of the E134A mutant of a ''Bacillus licheniformis''  1,3-1,4-&beta;-D-glucan 4-glucanohydrolase resulting in an &alpha;-glycosyl azide from the &beta;-glycoside substrate <cite>Viladot1998</cite>. The [[general acid/base]] residue was identified by making the E138A site-directed mutant of the ''Bacillus licheniformis''  1,3-1,4-&beta;-D-glucan 4-glucanohydrolase together with kinetic analysis and azide rescue, which resulted in a &beta;-glycosyl azide product <cite>Viladot1998</cite>.  These structurally conserved catalytic residues have been confirmed in a number of other GH16 members, including plant XETs and XEHs <cite>Gullfot2009 Piens2007</cite>, and yeast Crh1 and Crh2 <cite>Blanco2015</cite>.
The [[general acid/base]] residue was found by making the E138A mutant from the ''Bacillus licheniformis''  1,3-1,4-&beta;-D-glucan 4-glucanohydrolase and subsequent azide rescue resulting in a &beta;-glycosyl azide product <cite>7</cite>.
+
 
 +
The mechanistic analysis of bacterial mixed-linkage [[endo]]-glucanases has been expertly reviewed in the broader context of GH16 <cite>Planas2000</cite>.
  
 
== Three-dimensional structures ==
 
== Three-dimensional structures ==
Several three-dimensional structures have been solved of family 16 members of archeal, bacterial, and eukaryotic origin. The first solved 3-D structure was a hybrid protein of lichenase M from ''Paenibacillus macerans'' and BglA from ''Bacillus amyloliquefaciens'' ([{{PDBlink}}1byh PDB 1byh]) in 1992 <cite>5</cite>.  
+
Proteins in GH16 share a β-jelly-roll fold in which two β-sheets align in a curved, sandwich-like manner and present a cleft-shaped active-site bounded by loops extending from the β-strands. The first solved 3D structure was a hybrid protein of licheninase M from ''Paenibacillus macerans'' and BglA from ''Bacillus amyloliquefaciens'' ([{{PDBlink}}1byh PDB 1byh]) in 1992 <cite>Keitel1993</cite>. Many three-dimensional structures have been solved of family 16 members of archeal, bacterial, and eukaryotic origin (see http://www.cazy.org/GH16_structure.html for an updated list).  Of these, the first eukaryotic 3D structure was the xyloglucan ''endo''-transglycosylase ''Ptt''XET16-34 from ''Populus tremula&times;tremuloides'' ([{{PDBlink}}1umz PDB 1umz]) <cite>Johansson2004</cite> and the first archeal 3D structure was a ''[[endo]]''-1,3-&beta;-glucanase Lam16 from ''Pyrococcus furiosus'' ([{{PDBlink}}2vy0 PDB 2vy0]) <cite>Ilari2009</cite>.
The first eukaryotic 3-D structure was the xyloglucan ''endo''-transglycosylase ''Ptt''XET16-34 from ''Populus tremula&times;tremuloides'' ([{{PDBlink}}1umz PDB 1umz]) <cite>REF1</cite>. The first archeal 3-D structure was a ''endo''-1,3-&beta;-glucanase Lam16 from ''Pyrococcus furiosus'' ([{{PDBlink}}2vy0 PDB 2vy0]) <cite>8</cite>.
 
  
 +
The structural diversity of GH16 members across sequence-related subfamilies has been reviewed in detail <cite>Viborg2019</cite>.
 
== Evolution of GH16 ==
 
== Evolution of GH16 ==
Family 16 is a member of clan GH-B together with family 7 with whom they share their &beta;-jellyroll fold. The different specificities of family 16 has been proposed to have evoloved from an ancestral &beta;-1,3-glucanase <cite>10</cite>. The first branching in family 16 lead to the evolution of the &kappa;-carrageenases and the &beta;-agarases and a later branching event lead to the arisal of the lichenases and the XETs <cite>9</cite> (see figure).
+
[[Image:TreeGH16new.png|thumb|right|450px|'''Figure 1. Proposed evolution of GH16 (''click to enlarge'').''']]
[[Image:TreeGH16.png|thumb|Evolution of family 16]]
+
GH16 is a member of [[clans|clan]] GH-B together with [[GH7]]; both families share the &beta;-jellyroll fold. The different specificities of GH16 are proposed to have evolved from an ancestral &beta;-1,3-glucanase <cite>Barbeyron1998</cite>. This proposal was first elaborated using a structure-based phylogeny approach, which suggested that an early branching event lead to the evolution of the bacterial &kappa;-carrageenases and the &beta;-agarases, while a later branching event lead to the bacterial licheninases and the plant XETs <cite>Michel2001</cite> (Figure 1). GH16 has more recently been divided into subfamilies within CAZy, the corresponding phylogenetic analysis of which supports this overall evolutionary trajectory <cite>Viborg2019</cite>.
 +
 
 +
Particularly notable, the GH16 active-site residues are located in-train on one beta-strand at the center of the substrate binding cleft. Depending upon the phylogenetic clade, this beta-strand features one of two topologies.  The beta-bulge motif, which has the consensus sequence EXDXXE, is more frequent in GH16 compared to the regular beta-strand with the consensus sequence EXDXE (the [[catalytic nucleophile]] is the first glutamate and the [[catalytic acid/base]] is the second, with a proposed "helper" asparate in-between <cite>Planas2000</cite>). Due to the predominance of the beta-bulge motif and its presence as the only motif in [[GH7]], Michel et al. proposed that the beta-bulge is the ancestral motif, which subsequently gave rise to the regular beta-strand of extant plant XETs and bacterial licheninases <cite>Michel2001</cite>.
 +
 
 +
Within plant lineages, similar structure-based phylogenetic approaches have suggested that XEHs evolved subsequently to XEHs within the ''xyloglucan endo-transglycosylase/hydrolase (XTH)'' gene family <cite>Baumann2007 Eklof2010</cite>.  The identification of a group of bifunctional GH16 [[glycoside hydrolases]], which is active on both mixed-linkage beta-glucan and xyloglucan, provides additional support for the close evolutionary relationship of XETs and licheninases <cite>Eklof2013 McGregor2016 Behar2018</cite>.
  
 
== Family firsts ==
 
== Family firsts ==
; First stereochemistry determination : ''Bacillus licheniformis'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase by NMR <cite>REF3</cite>.
+
; First stereochemistry determination : ''Bacillus licheniformis'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase by NMR <cite>Malet1993</cite>.
; First [[catalytic nucleophile]] identification : Suggested in  ''Bacillus amyloliquefaciens'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase via non-specific epoxyalkyl β-glycoside labelling<cite>REF4</cite>. Later verified in by azide rescue of inactivated mutants <cite>7</cite>.
+
; First [[catalytic nucleophile]] identification : Suggested in  ''Bacillus amyloliquefaciens'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase via non-specific epoxyalkyl β-glycoside labeling <cite>Hoj1992</cite>. Later verified by azide rescue of inactivated mutants <cite>Viladot1998</cite>.
; First [[general acid/base]] residue identification : ''Bacillus licheniformis'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase, first suggested by sequence homology and mutational studies <cite>6</cite>. This was later verified by azide rescue of inactivated mutants <cite>7</cite>.
+
; First [[general acid/base]] residue identification : ''Bacillus licheniformis'' 1,3-1,4-&beta;-D-glucan 4-glucanohydrolase, first suggested by sequence homology and mutational studies <cite>Juncosa1994</cite>. This was later verified by azide rescue of inactivated mutants <cite>Viladot1998</cite>.
; First 3-D structure : A hybrid lichenase (''Bacillus amyloliquefaciens'' and ''Paenibacillus macerans'')  by X-ray crystallography ([{{PDBlink}}1byh PDB 1byh]) <cite>5</cite>.
+
; First 3-D structure : A hybrid licheninase (''Bacillus amyloliquefaciens'' and ''Paenibacillus macerans'')  by X-ray crystallography ([{{PDBlink}}1byh PDB 1byh]) <cite>Keitel1993</cite>.
  
 
== Reference list ==
 
== Reference list ==
 
<biblio>
 
<biblio>
#REF1 pmid=15020748
+
#Johansson2004 pmid=15020748
#REF4 pmid=1360982
+
#Hoj1992 pmid=1360982
#REF3 pmid=8280073
+
#Malet1993 pmid=8280073
#5 pmid=8099449
+
#Keitel1993 pmid=8099449
#6 pmid=8182059
+
#Juncosa1994 pmid=8182059
#7 pmid=9698381
+
#Viladot1998 pmid=9698381
#8 pmid=19154353
+
#Ilari2009 pmid=19154353
#9 pmid=11435116 tree GH16
+
#Michel2001 pmid=11435116 tree GH16
#10 pmid=9580981 first GH16 paper
+
#Barbeyron1998 pmid=9580981 first GH16 paper
#NXG pmid=17557806  
+
#Baumann2007 pmid=17557806
</biblio>
+
#Planas2000 pmid=11150614
 +
#Hehemann2010 pmid=20376150
 +
#Kotake2011 pmid=21653698
 +
#Lee2009 pmid=19712587
 +
#Eklof2010 pmid=20421457
 +
#Sinnott1990 Sinnott, M.L. (1990) Catalytic mechanisms of enzymic glycosyl transfer. Chem. Rev. 90, 1171-1202. [http://dx.doi.org/10.1021/cr00105a006 DOI: 10.1021/cr00105a006]
 +
#Cabib2008 pmid=18694928
 +
#Mazan2013 pmid=23919454
 +
#Blanco2015 pmid=25495733
 +
#Gullfot2009 pmid=19419143
 +
#Piens2007 pmid=18043802
 +
#Eklof2013 pmid=23572521
 +
#Bissaro2015 pmid=25793417
 +
#McGregor2016 pmid=27859885
  
 +
#Viborg2019 pmid=31501245
 +
#Behar2018 pmid=29932263</biblio>
 
<!-- DO NOT REMOVE THIS CATEGORY TAG! -->
 
<!-- DO NOT REMOVE THIS CATEGORY TAG! -->
 
[[Category:Glycoside Hydrolase Families|GH016]]
 
[[Category:Glycoside Hydrolase Families|GH016]]

Latest revision as of 13:18, 18 December 2021

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Glycoside Hydrolase Family 16
Clan GH-B
Mechanism retaining
Active site residues known
CAZy DB link
https://www.cazy.org/GH16.html

Substrate specificities

The members of family 16 are active on β-1,4 or β-1,3 glycosidic bonds in various glucans and galactans. A wide diversity of glycoside hydrolases active on plant and marine polysaccharides are found in GH16, including:

Notably, some members of GH16 are predominant transglycosylases. These include the plant xyloglucan:xyloglucosyltransferases (EC 2.4.1.207, a.k.a. xyloglucan endo-transglycosylases, XETs) [2] and yeast chitin/beta-glucan crosslinking enzymes Crh1 and Crh2 [3, 4, 5]. Some invertebrate GH16 proteins have lost their catalytic amino acids and are involved in immune response activation through the Toll pathway upon binding of β-1,3 glucan. The role of the GH16 domain in this immune response has not been fully elucidated [6].

Several of the activities observed for GH16 members are delineated into individual sequence-based subfamilies, while other polyspecific subfamilies capture a range of activities [7].

Kinetics and Mechanism

Members of GH16 enzymes are retaining enzymes, as first shown by NMR [8] on an endo-1,3-1,4-β-D-glucan 4-glucanohydrolase from Bacillus licheniformis. As such, they utilize a covalent glycosyl-enzyme intermediate, which is broken-down by glycosyl transfer [9, 10] to water or a carbohydrate acceptor substrate in glycoside hydrolases or transglycosylases, respectively.

Catalytic Residues

The catalytic nucleophile of GH16 enzymes was first proposed using a non-specific epoxyalkyl β-glycoside inhibitor and identification of the site of covalent labelling using ESI-MS and Edman degradation on an endo-1,3-1,4-β-D-glucan 4-glucanohydrolase from Bacillus amyloliquefaciens [11]. This was subsequently verified by azide rescue of the E134A mutant of a Bacillus licheniformis 1,3-1,4-β-D-glucan 4-glucanohydrolase resulting in an α-glycosyl azide from the β-glycoside substrate [12]. The general acid/base residue was identified by making the E138A site-directed mutant of the Bacillus licheniformis 1,3-1,4-β-D-glucan 4-glucanohydrolase together with kinetic analysis and azide rescue, which resulted in a β-glycosyl azide product [12]. These structurally conserved catalytic residues have been confirmed in a number of other GH16 members, including plant XETs and XEHs [13, 14], and yeast Crh1 and Crh2 [5].

The mechanistic analysis of bacterial mixed-linkage endo-glucanases has been expertly reviewed in the broader context of GH16 [15].

Three-dimensional structures

Proteins in GH16 share a β-jelly-roll fold in which two β-sheets align in a curved, sandwich-like manner and present a cleft-shaped active-site bounded by loops extending from the β-strands. The first solved 3D structure was a hybrid protein of licheninase M from Paenibacillus macerans and BglA from Bacillus amyloliquefaciens (PDB 1byh) in 1992 [16]. Many three-dimensional structures have been solved of family 16 members of archeal, bacterial, and eukaryotic origin (see http://www.cazy.org/GH16_structure.html for an updated list). Of these, the first eukaryotic 3D structure was the xyloglucan endo-transglycosylase PttXET16-34 from Populus tremula×tremuloides (PDB 1umz) [17] and the first archeal 3D structure was a endo-1,3-β-glucanase Lam16 from Pyrococcus furiosus (PDB 2vy0) [18].

The structural diversity of GH16 members across sequence-related subfamilies has been reviewed in detail [7].

Evolution of GH16

Figure 1. Proposed evolution of GH16 (click to enlarge).

GH16 is a member of clan GH-B together with GH7; both families share the β-jellyroll fold. The different specificities of GH16 are proposed to have evolved from an ancestral β-1,3-glucanase [19]. This proposal was first elaborated using a structure-based phylogeny approach, which suggested that an early branching event lead to the evolution of the bacterial κ-carrageenases and the β-agarases, while a later branching event lead to the bacterial licheninases and the plant XETs [20] (Figure 1). GH16 has more recently been divided into subfamilies within CAZy, the corresponding phylogenetic analysis of which supports this overall evolutionary trajectory [7].

Particularly notable, the GH16 active-site residues are located in-train on one beta-strand at the center of the substrate binding cleft. Depending upon the phylogenetic clade, this beta-strand features one of two topologies. The beta-bulge motif, which has the consensus sequence EXDXXE, is more frequent in GH16 compared to the regular beta-strand with the consensus sequence EXDXE (the catalytic nucleophile is the first glutamate and the catalytic acid/base is the second, with a proposed "helper" asparate in-between [15]). Due to the predominance of the beta-bulge motif and its presence as the only motif in GH7, Michel et al. proposed that the beta-bulge is the ancestral motif, which subsequently gave rise to the regular beta-strand of extant plant XETs and bacterial licheninases [20].

Within plant lineages, similar structure-based phylogenetic approaches have suggested that XEHs evolved subsequently to XEHs within the xyloglucan endo-transglycosylase/hydrolase (XTH) gene family [2, 21]. The identification of a group of bifunctional GH16 glycoside hydrolases, which is active on both mixed-linkage beta-glucan and xyloglucan, provides additional support for the close evolutionary relationship of XETs and licheninases [22, 23, 24].

Family firsts

First stereochemistry determination
Bacillus licheniformis 1,3-1,4-β-D-glucan 4-glucanohydrolase by NMR [8].
First catalytic nucleophile identification
Suggested in Bacillus amyloliquefaciens 1,3-1,4-β-D-glucan 4-glucanohydrolase via non-specific epoxyalkyl β-glycoside labeling [11]. Later verified by azide rescue of inactivated mutants [12].
First general acid/base residue identification
Bacillus licheniformis 1,3-1,4-β-D-glucan 4-glucanohydrolase, first suggested by sequence homology and mutational studies [25]. This was later verified by azide rescue of inactivated mutants [12].
First 3-D structure
A hybrid licheninase (Bacillus amyloliquefaciens and Paenibacillus macerans) by X-ray crystallography (PDB 1byh) [16].

Reference list

  1. Hehemann JH, Correc G, Barbeyron T, Helbert W, Czjzek M, and Michel G. (2010). Transfer of carbohydrate-active enzymes from marine bacteria to Japanese gut microbiota. Nature. 2010;464(7290):908-12. DOI:10.1038/nature08937 | PubMed ID:20376150 [Hehemann2010]
  2. Eklöf JM and Brumer H. (2010). The XTH gene family: an update on enzyme structure, function, and phylogeny in xyloglucan remodeling. Plant Physiol. 2010;153(2):456-66. DOI:10.1104/pp.110.156844 | PubMed ID:20421457 [Eklof2010]
  3. Cabib E, Farkas V, Kosík O, Blanco N, Arroyo J, and McPhie P. (2008). Assembly of the yeast cell wall. Crh1p and Crh2p act as transglycosylases in vivo and in vitro. J Biol Chem. 2008;283(44):29859-72. DOI:10.1074/jbc.M804274200 | PubMed ID:18694928 [Cabib2008]
  4. Mazáň M, Blanco N, Kováčová K, Firáková Z, Rehulka P, Farkaš V, and Arroyo J. (2013). A novel fluorescence assay and catalytic properties of Crh1 and Crh2 yeast cell wall transglycosylases. Biochem J. 2013;455(3):307-18. DOI:10.1042/BJ20130354 | PubMed ID:23919454 [Mazan2013]
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