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Difference between revisions of "Glycoside Hydrolase Family 9"

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* [[Author]]s: ^^^David Wilson^^^ and ^^^Breeanna Urbanowicz^^^
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* [[Author]]s: [[User:David Wilson|David Wilson]] and [[User:Breeanna Urbanowicz|Breeanna Urbanowicz]]
* [[Responsible Curator]]:  ^^^David Wilson^^^
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* [[Responsible Curator]]:  [[User:David Wilson|David Wilson]]
 
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|-
 
|-
 
|'''Clan'''     
 
|'''Clan'''     
|GH-G
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|not assigned
 
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|'''Mechanism'''
 
|'''Mechanism'''
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== Substrate specificities ==
 
== Substrate specificities ==
[[Glycoside hydrolases]] of family GH9 are mainly cellulases and GH9 is the second largest cellulase family. It contains mainly endoglucanases with a few processive endoglucanases. All of the processive endoglucanases contain a family 3c CBM rigidly attached to the C-terminus of the GH9 catalytic domain (cd) <cite>Sakon1997</cite>. This domain is part of the active site and is essential for processivity <cite>Sakon1997</cite>.  CBM3c domains bind weakly to cellulose as they lack several of the conserved aromatic residues that are important for cellulose binding in family 3a and family 3b members <cite>Tormo1996</cite>.  All known plant cellulases belong to GH9, and most of the other members are eubacterial although there are two archael members and some fungal, earthworm,  arthropod, chordate, echinoderma and molusk members. There are two subgroups in GH9, E1 which contains only cellulases from bacteria, including ones from both aerobes and anaeobes, and E2 which includes some bacterial and all nonbacterial cellulases <cite>Tomme1995</cite>. An evolutionary study shows that the eucaryote members contain two monophyletic groups that are amcient; one including all animal members and the other including all plant members <cite>Davison2005</cite>. All known processive endoglucanase genes are in subgroup E1.
+
Members of family GH9 are mainly cellulases ([{{EClink}}3.2.1.4 EC 3.2.1.4]), including primarily endo-glucanases and a few processive endo-glucanases. Indeed, as one of the first glycoside hydrolase families classified by hydrophobic cluster analysis, GH9 was previously known as "Cellulase Family E" <cite>Henrissat1989 Gilkes1991</cite>. More recently, certain GH9 members from ''Clostridia'' <cite>Ravachol2016</cite> and ''Bacteroides'' <cite>Larsbrink2014 Foley2019</cite> have been shown to be endo-xyloglucanases ([{{EClink}}3.2.1.151 EC 3.2.1.151]) or mixed-linkage endo-glucanases ([{{EClink}}3.2.1.73 EC 3.2.1.73])Exo-beta-glucosaminidases ([{{EClink}}3.2.1.165 EC 3.2.1.165]) are also found in this family <cite>Honda2016 Wu2018</cite>.
  
 +
All of the processive endoglucanases contain a family 3c CBM rigidly attached to the C-terminus of the GH9 catalytic domain (cd) <cite>Sakon1997</cite>. This domain is part of the active site and is essential for processivity <cite>Sakon1997</cite>.  [[CBM3]]c domains bind weakly to cellulose as they lack several of the conserved aromatic residues that are important for cellulose binding in family 3a and family 3b members <cite>Tormo1996</cite>.  All known plant cellulases belong to GH9, and most of the other members are eubacterial although there are two archael members and some fungal, earthworm,  arthropod, chordate, echinoderma and molusk members. There are two subgroups in GH9, E1 which contains only cellulases from bacteria, including ones from both aerobes and anaeobes, and E2 which includes some bacterial and all nonbacterial cellulases <cite>Tomme1995</cite>. An evolutionary study shows that the eucaryote members contain two monophyletic groups that are ancient; one including all animal members and the other including all plant members <cite>Davison2005</cite>. All known processive endoglucanase genes are in subgroup E1.
 
Most plant GH9 enzymes studied to date are endoglucanases ("cellulases", EC [{{EClink}}3.2.1.4 3.2.1.4]) with little or no activity on crystalline cellulose, but with discernible activity on soluble cellulose derivatives, including carboxymethyl cellulose (CMC), phosphoric acid swollen non-crystalline cellulose, and numerous plant polysaccharides including xylan, 1,3-1,4-ß-glucan, xyloglucan, and glucomannan <cite>Master2004 YoshidaKomae2006 Ohmiya2000 Woolley2001 Urbanowicz2007</cite>.  Due to their ubiquity and large numbers, the phylogeny of plant GH9 enzymes has been further sub-divided into three classes <cite>UrbanowiczBennett2007</cite>, which are described in detail on the [[Glycoside_Hydrolase_Family_9/Plant_endoglucanases|plant GH9 endoglucanase subpage]].
 
Most plant GH9 enzymes studied to date are endoglucanases ("cellulases", EC [{{EClink}}3.2.1.4 3.2.1.4]) with little or no activity on crystalline cellulose, but with discernible activity on soluble cellulose derivatives, including carboxymethyl cellulose (CMC), phosphoric acid swollen non-crystalline cellulose, and numerous plant polysaccharides including xylan, 1,3-1,4-ß-glucan, xyloglucan, and glucomannan <cite>Master2004 YoshidaKomae2006 Ohmiya2000 Woolley2001 Urbanowicz2007</cite>.  Due to their ubiquity and large numbers, the phylogeny of plant GH9 enzymes has been further sub-divided into three classes <cite>UrbanowiczBennett2007</cite>, which are described in detail on the [[Glycoside_Hydrolase_Family_9/Plant_endoglucanases|plant GH9 endoglucanase subpage]].
  
 
== Kinetics and Mechanism ==
 
== Kinetics and Mechanism ==
GH9 enzymes operate with [[inverting|inversion]] of anomeric stereochemistry. The processive endoglucanase, Cel9A from ''Thermobifda fusca'', has high activity on bacterial cellulose and is the only cellulase tested that can degrade crystalline regions in bacterial cellulose by itself although it prefers amorphous regions <cite>Chen2007</cite>.  A related cellulase in ''Clostridium phytofermentans'', which is the only family 9 cellulase encoded in its genome, has been shown to be essential for cellulose degradation by this organism. This is the only case where a single cellulase has been shown to be essential for growth on cellulose <cite>Tolonen2009</cite>.     
+
[[GH9]] enzymes operate with [[inverting|inversion]] of anomeric stereochemistry. The processive endoglucanase, Cel9A from ''Thermobifda fusca'', has high activity on bacterial cellulose and is the only cellulase tested that can degrade crystalline regions in bacterial cellulose by itself although it prefers amorphous regions <cite>Chen2007</cite>.  A related cellulase in ''Clostridium phytofermentans'', which is the only family 9 cellulase encoded in its genome, has been shown to be essential for cellulose degradation by this organism. This is the only case where a single cellulase has been shown to be essential for growth on cellulose <cite>Tolonen2009</cite>.     
  
 
== Catalytic Residues ==
 
== Catalytic Residues ==
There is a conserved Glu residue that functions as a catalytic [[general acid]] and two conserved Asp residues that bind the catalytic water, with one functioning as the catalytic [[general base]]; mutation of the other also greatly reduces activity on all substrates <cite>Zhou2004</cite>.
+
There is a conserved Glu residue that functions as a catalytic [[general acid]] and two conserved Asp residues that bind the catalytic water, with one functioning as the catalytic [[general base]]; mutation of the other also greatly reduces activity on all substrates <cite>Zhou2004</cite>. Mutation of the conserved Glu to Ala, Gly or Gln reduced activity to less than >0.5% of WT on all forms of cellulose but the Ala and Gly mutant enzymes had higher than WT activity on dinitrophenyl-cellobioside which has a good leaving group, proving that this residue functions as the catalytic acid <cite>Zhou2004</cite>. Mutation of either of two conserved Asp residues that bound the catalytic water to Ala or Asn reduced activity to less then 2% of WT on all cellulosic substrates. However, only one of the Ala mutant enzymes showed azide rescue proving that it was the actual catalytic base <cite>Li2007</cite>.
  
 
== Three-dimensional structures ==
 
== Three-dimensional structures ==
All known family 9 cd structures have an ( a / a ) 6 barrel fold that contains an open active site cleft that contains at least six sugar binding subsites -4 to +2 <cite>Sakon1997 Geurin2002</cite>. In processive endoglucanases the catalytic domain is joined to a family 3c CBM that is aligned with the active site cleft <cite>Sakon1997</cite>.
+
All reported GH9 catalytic domain structures have an (a/a)<sub>6</sub> barrel fold that contains an open active site cleft that contains at least six sugar binding subsites -4 to +2 <cite>Sakon1997 Geurin2002 Foley2019</cite>. In processive endoglucanases the catalytic domain is joined to a family 3c carbohydrate-binding module that is aligned with the active site cleft <cite>Sakon1997</cite>.
  
 
== Family Firsts ==
 
== Family Firsts ==
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;First [[general base]] identification: Asp 58 in ''T. fusca'' Cel9A was shown to be the [[general base]] by site directed mutagenesis and azide rescue <cite>Li2007</cite>.
 
;First [[general base]] identification: Asp 58 in ''T. fusca'' Cel9A was shown to be the [[general base]] by site directed mutagenesis and azide rescue <cite>Li2007</cite>.
  
;First [[general acid]] residue identification: Glu555 was shown to be the catalytic acid in ''C. thermocellum'' CelD by site directed mutagenesis <cite>Chavaux1962</cite>.
+
;First [[general acid]] residue identification: Glu555 was shown to be the catalytic acid in ''C. thermocellum'' CelD by site directed mutagenesis <cite>Chavaux1992</cite>.
  
 
;First 3-D structure: The structure of endocellulase CelD from ''Clostridium thermocellum'' was determined by X-ray crystallography (PDB ID [{{PDBlink}}1clc 1clc]) <cite>Lascombe1995</cite>.
 
;First 3-D structure: The structure of endocellulase CelD from ''Clostridium thermocellum'' was determined by X-ray crystallography (PDB ID [{{PDBlink}}1clc 1clc]) <cite>Lascombe1995</cite>.
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#Urbanowicz2007 pmid=17322304
 
#Urbanowicz2007 pmid=17322304
 
#UrbanowiczBennett2007 pmid=17687051
 
#UrbanowiczBennett2007 pmid=17687051
 +
#Henrissat1989 pmid=2806912
 +
#Gilkes1991 pmid=1886523
 +
#Chavaux1992 pmid=1537833
 +
#Foley2019 pmid=30668971
 +
#Larsbrink2014 pmid=24463512
 +
#Ravachol2016 pmid=26946939
 +
 +
#Wu2018 pmid=30084401
 +
 +
#Honda2016 pmid=26621872
 
</biblio>
 
</biblio>
  
 
[[Category:Glycoside Hydrolase Families|GH009]]
 
[[Category:Glycoside Hydrolase Families|GH009]]

Latest revision as of 13:18, 18 December 2021

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Glycoside Hydrolase Family GH9
Clan not assigned
Mechanism inverting
Active site residues known/known
CAZy DB link
https://www.cazy.org/GH9.html


Substrate specificities

Members of family GH9 are mainly cellulases (EC 3.2.1.4), including primarily endo-glucanases and a few processive endo-glucanases. Indeed, as one of the first glycoside hydrolase families classified by hydrophobic cluster analysis, GH9 was previously known as "Cellulase Family E" [1, 2]. More recently, certain GH9 members from Clostridia [3] and Bacteroides [4, 5] have been shown to be endo-xyloglucanases (EC 3.2.1.151) or mixed-linkage endo-glucanases (EC 3.2.1.73). Exo-beta-glucosaminidases (EC 3.2.1.165) are also found in this family [6, 7].

All of the processive endoglucanases contain a family 3c CBM rigidly attached to the C-terminus of the GH9 catalytic domain (cd) [8]. This domain is part of the active site and is essential for processivity [8]. CBM3c domains bind weakly to cellulose as they lack several of the conserved aromatic residues that are important for cellulose binding in family 3a and family 3b members [9]. All known plant cellulases belong to GH9, and most of the other members are eubacterial although there are two archael members and some fungal, earthworm, arthropod, chordate, echinoderma and molusk members. There are two subgroups in GH9, E1 which contains only cellulases from bacteria, including ones from both aerobes and anaeobes, and E2 which includes some bacterial and all nonbacterial cellulases [10]. An evolutionary study shows that the eucaryote members contain two monophyletic groups that are ancient; one including all animal members and the other including all plant members [11]. All known processive endoglucanase genes are in subgroup E1. Most plant GH9 enzymes studied to date are endoglucanases ("cellulases", EC 3.2.1.4) with little or no activity on crystalline cellulose, but with discernible activity on soluble cellulose derivatives, including carboxymethyl cellulose (CMC), phosphoric acid swollen non-crystalline cellulose, and numerous plant polysaccharides including xylan, 1,3-1,4-ß-glucan, xyloglucan, and glucomannan [12, 13, 14, 15, 16]. Due to their ubiquity and large numbers, the phylogeny of plant GH9 enzymes has been further sub-divided into three classes [17], which are described in detail on the plant GH9 endoglucanase subpage.

Kinetics and Mechanism

GH9 enzymes operate with inversion of anomeric stereochemistry. The processive endoglucanase, Cel9A from Thermobifda fusca, has high activity on bacterial cellulose and is the only cellulase tested that can degrade crystalline regions in bacterial cellulose by itself although it prefers amorphous regions [18]. A related cellulase in Clostridium phytofermentans, which is the only family 9 cellulase encoded in its genome, has been shown to be essential for cellulose degradation by this organism. This is the only case where a single cellulase has been shown to be essential for growth on cellulose [19].

Catalytic Residues

There is a conserved Glu residue that functions as a catalytic general acid and two conserved Asp residues that bind the catalytic water, with one functioning as the catalytic general base; mutation of the other also greatly reduces activity on all substrates [20]. Mutation of the conserved Glu to Ala, Gly or Gln reduced activity to less than >0.5% of WT on all forms of cellulose but the Ala and Gly mutant enzymes had higher than WT activity on dinitrophenyl-cellobioside which has a good leaving group, proving that this residue functions as the catalytic acid [20]. Mutation of either of two conserved Asp residues that bound the catalytic water to Ala or Asn reduced activity to less then 2% of WT on all cellulosic substrates. However, only one of the Ala mutant enzymes showed azide rescue proving that it was the actual catalytic base [21].

Three-dimensional structures

All reported GH9 catalytic domain structures have an (a/a)6 barrel fold that contains an open active site cleft that contains at least six sugar binding subsites -4 to +2 [5, 8, 22]. In processive endoglucanases the catalytic domain is joined to a family 3c carbohydrate-binding module that is aligned with the active site cleft [8].

Family Firsts

First stereochemistry determination
The stereospecificity of three family 9 cellulases were all determined to be inverting by NMR [23].
First general base identification
Asp 58 in T. fusca Cel9A was shown to be the general base by site directed mutagenesis and azide rescue [21].
First general acid residue identification
Glu555 was shown to be the catalytic acid in C. thermocellum CelD by site directed mutagenesis [24].
First 3-D structure
The structure of endocellulase CelD from Clostridium thermocellum was determined by X-ray crystallography (PDB ID 1clc) [25].

References

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Error fetching PMID 15703240:
Error fetching PMID 11884144:
Error fetching PMID 15274620:
Error fetching PMID 17369336:
Error fetching PMID 19775243:
Error fetching PMID 1618761:
Error fetching PMID 15287736:
Error fetching PMID 17056618:
Error fetching PMID 11069690:
Error fetching PMID 11762160:
Error fetching PMID 17322304:
Error fetching PMID 17687051:
Error fetching PMID 2806912:
Error fetching PMID 1886523:
Error fetching PMID 1537833:
Error fetching PMID 30668971:
Error fetching PMID 24463512:
Error fetching PMID 26946939:
Error fetching PMID 30084401:
Error fetching PMID 26621872:
  1. Error fetching PMID 2806912: [Henrissat1989]
  2. Error fetching PMID 1886523: [Gilkes1991]
  3. Error fetching PMID 26946939: [Ravachol2016]
  4. Error fetching PMID 24463512: [Larsbrink2014]
  5. Error fetching PMID 30668971: [Foley2019]
  6. Error fetching PMID 26621872: [Honda2016]
  7. Error fetching PMID 30084401: [Wu2018]
  8. Error fetching PMID 9334746: [Sakon1997]
  9. Error fetching PMID 8918451: [Tormo1996]
  10. Error fetching PMID 8540419: [Tomme1995]
  11. Error fetching PMID 15703240: [Davison2005]
  12. Error fetching PMID 15287736: [Master2004]
  13. Error fetching PMID 17056618: [YoshidaKomae2006]
  14. Error fetching PMID 11069690: [Ohmiya2000]
  15. Error fetching PMID 11762160: [Woolley2001]
  16. Error fetching PMID 17322304: [Urbanowicz2007]
  17. Error fetching PMID 17687051: [UrbanowiczBennett2007]

  18. Chen, Arthur J. Stipanovic, William T. Winter, David B. Wilson and Young-Jun Kim. Effect of digestion by pure cellulases on crystallinity and average chain length for bacterial and microcrystalline celluloses. Cellulose 2007: 14: 283-293.

    [Chen2007]
  19. Error fetching PMID 19775243: [Tolonen2009]
  20. Error fetching PMID 15274620: [Zhou2004]
  21. Error fetching PMID 17369336: [Li2007]
  22. Error fetching PMID 11884144: [Geurin2002]
  23. Error fetching PMID 1618761: [Gebler1992]
  24. Error fetching PMID 1537833: [Chavaux1992]

  25. Lascombe, M.B., Souchon, H., Juy, M., Alzari, P.M. Three-Dimensional Structure of Endoglucanase D at 1.9 Angstroms Resolution. Deposited 1995, unpublished. PDB ID 1clc

    [Lascombe1995]

All Medline abstracts: PubMed

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