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Difference between revisions of "Glycoside Hydrolase Family 113"

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* [[Author]]s: [[User:Rohan Williams|Rohan Williams]] and [[User:Spencer Williams|Spencer Williams]]
* [[Author]]s: ^^^Rohan Williams^^^ and ^^^Spencer Williams^^^
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* [[Responsible Curator]]: [[User:Spencer Williams|Spencer Williams]]
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== Substrate specificities ==
 
== Substrate specificities ==
Only a single [[glycoside hydrolase]] of family [[GH113]] has been characterized, intracellular ''Aa''ManA from ''Alicyclobacillus acidocaldarius'' Tc-12-31 <cite>Zhang2008</cite>. This thermoacidophilic organism was originally selected for its ability to hydrolyse konjac glucomannan <cite>Zhang2008</cite>. The recombinantly-expressed enzyme possessed activity against polysaccharides containing &beta;-1,4-mannosidic linkages, including significant activity against konjac glucomannan, and galactomannan from locust bean gum. Some activity was also observed against crystalline ivory nut mannan (an unsubstituted &beta;-1,4-mannan) and guar gum (a more highly-substituted galactomannan) <cite>Zhang2008</cite>. No activity was observed against the other polysaccharides and ''p''-nitrophenyl glycosides tested, including ''p''-nitrophenyl &beta;- and &alpha;-mannosides.
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Only a single [[glycoside hydrolase]] of family [[GH113]] has been characterized, intracellular ''Aa''ManA from ''Alicyclobacillus acidocaldarius'' Tc-12-31 <cite>Zhang2008</cite>. This thermoacidophilic organism was originally selected for its ability to hydrolyse konjac glucomannan <cite>Zhang2008</cite>. The recombinantly-expressed enzyme possesses activity against polysaccharides containing &beta;-1,4-mannosidic linkages, including significant activity against konjac glucomannan, and galactomannan from locust bean gum. Some activity was also observed against crystalline ivory nut mannan (an unsubstituted &beta;-1,4-mannan) and guar gum (a more highly-substituted galactomannan) <cite>Zhang2008</cite>. No activity was observed against the other polysaccharides and ''p''-nitrophenyl glycosides tested, including ''p''-nitrophenyl &beta;- and &alpha;-mannosides.
  
 
== Kinetics and Mechanism ==
 
== Kinetics and Mechanism ==
Thin layer chromatographic analysis of the hydrolysis products of ''Aa''ManA from ''A. acidocaldarius'' indicated ''[[endo]]''-type cleavage <cite>Zhang2008</cite>. The products also displayed obvious signs of [[transglycosylases|transglycosylation]], and thus ''Aa''ManA was assigned a [[retaining]] mechanism. The distance between the acid/base and nucleophile residues (assigned on the basis of structural comparison and mutagenesis, see below) is 4.75 Å <cite>Zhang2008</cite>. Together, these data support a [[classical Koshland retaining mechanism]]. Kinetic analysis of mannooligosaccharides reveals a preference for pentamannosides and higher; a tetramannoside was hydrolysed with ''k''<sub>cat</sub>/''K''<sub>M</sub> value approximately one quarter of that seen for the higher oligomers.
+
Thin layer chromatographic analysis of the hydrolysis products of ''Aa''ManA from ''A. acidocaldarius'' indicated ''[[endo]]''-type cleavage <cite>Zhang2008</cite>. The products also displayed obvious signs of [[transglycosylases|transglycosylation]], and thus ''Aa''ManA was assigned a [[retaining]] mechanism. The distance between the acid/base and nucleophile residues (assigned on the basis of structural comparison and mutagenesis, see below) is 4.75 Å <cite>Zhang2008</cite>. Together, these data support a [[classical Koshland retaining mechanism]]. Kinetic analysis of mannooligosaccharides reveals a preference for pentamannosides and higher; a tetramannoside was hydrolysed with ''k''<sub>cat</sub>/''K''<sub>M</sub> value approximately one quarter of that seen for the higher oligomers. Crystallographic evidence from a binary complexes of ''Aa''ManA with &beta;-mannosyl-1,4-mannoimidazole supports a <sup>1</sup>''S''<sub>5</sub>&rarr;''B''<sub>2,5</sub><sup>‡</sup>&rarr;<sup>O</sup>''S''<sub>2</sub> conformational reaction coordinate <cite>Williams2014</cite>.
  
 
== Catalytic Residues ==
 
== Catalytic Residues ==
Structural comparision of ''Aa''ManA with [[GH5]] endoglycosidases demonstrated conserved spatial arrangement of key active site amino acid residues <cite>Zhang2008</cite>. Structural comparison with Cel5G from ''Pseudoalteromonas haloplanktis'' suggested Glu151 to be the [[general acid/base]] and Glu231 to be the [[catalytic nucleophile]]. The Glu151Ala and Glu231Ala mutants did not affect overall fold but each resulted in a loss of approximately 1000-fold activity against mannan substrates, consistent with the proposed roles.  
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Structural comparision of ''Aa''ManA with [[GH5]] endoglycosidases demonstrated conserved spatial arrangement of key active site amino acid residues <cite>Zhang2008</cite>. Structural comparison with Cel5G from ''Pseudoalteromonas haloplanktis'' suggested Glu151 to be the [[general acid/base]] and Glu231 to be the [[catalytic nucleophile]]. The Glu151Ala and Glu231Ala mutants did not affect overall fold but each resulted in a loss of approximately 1000-fold activity against mannan substrates, consistent with the proposed roles. Crystallographic studies with ''Aa''ManA in complex with &beta;-mannosyl-1,4-mannoimidazole support the assignment of Glu151 as the acid/base <cite>Williams2014</cite>. A complex of ''Aa''ManA with &beta;-mannosyl-1,4-isofagomine supports the assignment of Glu231 as the nucleophile <cite>Williams2014</cite>.  
  
 
== Three-dimensional structures ==
 
== Three-dimensional structures ==
The three dimensional structure was first reported for ''Aa''ManA, which possesses a classical (&beta;/&alpha;)<sub>8</sub> TIM barrel fold that aligns well with enzymes of family [[GH5]] <cite>Zhang2008</cite>. Alignment of the ‘’Aa’’ManA structure with Cel5G from ''Pseudoalteromonas haloplanktis'' revealed eight equivalent residues around the proposed active site pocket: Lys93, Thr95, Cys150, Glu151, Ser201, Tyr203, Glu231, and Trp281 <cite>Zhang2008</cite>.  Binary complexes of ‘’Aa’’ManA with &beta;-mannosyl-1,4-mannoimidazole or &beta;-mannosyl-1,4-isofagomine support the identity of the active site residues originally proposed on the basis of structural comparisons of ‘’Aa’’ManA with Cel5G and mutagenesis <cite>Williams2014</cite>. An ''active-site spanning'' ternary complex of ‘’Aa’’ManA with &beta;-mannosyl-1,4-isofagomine and 1,4-&beta;-mannobiose has provided structural details of amino acids defining the -2 to +2 subsites <cite>Williams2014</cite>.     
+
The three dimensional structure was first reported for ''Aa''ManA, which possesses a classical (&beta;/&alpha;)<sub>8</sub> TIM barrel fold that aligns well with enzymes of family [[GH5]] <cite>Zhang2008</cite>. Alignment of the ''Aa''ManA structure with Cel5G from ''Pseudoalteromonas haloplanktis'' revealed eight equivalent residues around the proposed active site pocket: Lys93, Thr95, Cys150, Glu151, Ser201, Tyr203, Glu231, and Trp281 <cite>Zhang2008</cite>.  Binary complexes of ''Aa''ManA with &beta;-mannosyl-1,4-mannoimidazole or &beta;-mannosyl-1,4-isofagomine support the identity of the active site residues originally proposed on the basis of structural comparisons of ''Aa''ManA with Cel5G and mutagenesis <cite>Williams2014</cite>. An ''active-site spanning'' ternary complex of ''Aa''ManA with &beta;-mannosyl-1,4-isofagomine and 1,4-&beta;-mannobiose has provided structural details of amino acids defining the -2 to +2 subsites <cite>Williams2014</cite>.     
  
 
== Family Firsts ==
 
== Family Firsts ==
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<biblio>
 
<biblio>
 
#Zhang2008 pmid=18755688
 
#Zhang2008 pmid=18755688
#Williams2014 pmid=
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#Williams2014 pmid=24339341
 
</biblio>
 
</biblio>
  
  
 
[[Category:Glycoside Hydrolase Families|GH113]]
 
[[Category:Glycoside Hydrolase Families|GH113]]

Latest revision as of 13:16, 18 December 2021

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Glycoside Hydrolase Family GH113
Clan GH-A
Mechanism retaining
Active site residues known
CAZy DB link
https://www.cazy.org/GH113.html


Substrate specificities

Only a single glycoside hydrolase of family GH113 has been characterized, intracellular AaManA from Alicyclobacillus acidocaldarius Tc-12-31 [1]. This thermoacidophilic organism was originally selected for its ability to hydrolyse konjac glucomannan [1]. The recombinantly-expressed enzyme possesses activity against polysaccharides containing β-1,4-mannosidic linkages, including significant activity against konjac glucomannan, and galactomannan from locust bean gum. Some activity was also observed against crystalline ivory nut mannan (an unsubstituted β-1,4-mannan) and guar gum (a more highly-substituted galactomannan) [1]. No activity was observed against the other polysaccharides and p-nitrophenyl glycosides tested, including p-nitrophenyl β- and α-mannosides.

Kinetics and Mechanism

Thin layer chromatographic analysis of the hydrolysis products of AaManA from A. acidocaldarius indicated endo-type cleavage [1]. The products also displayed obvious signs of transglycosylation, and thus AaManA was assigned a retaining mechanism. The distance between the acid/base and nucleophile residues (assigned on the basis of structural comparison and mutagenesis, see below) is 4.75 Å [1]. Together, these data support a classical Koshland retaining mechanism. Kinetic analysis of mannooligosaccharides reveals a preference for pentamannosides and higher; a tetramannoside was hydrolysed with kcat/KM value approximately one quarter of that seen for the higher oligomers. Crystallographic evidence from a binary complexes of AaManA with β-mannosyl-1,4-mannoimidazole supports a 1S5B2,5OS2 conformational reaction coordinate [2].

Catalytic Residues

Structural comparision of AaManA with GH5 endoglycosidases demonstrated conserved spatial arrangement of key active site amino acid residues [1]. Structural comparison with Cel5G from Pseudoalteromonas haloplanktis suggested Glu151 to be the general acid/base and Glu231 to be the catalytic nucleophile. The Glu151Ala and Glu231Ala mutants did not affect overall fold but each resulted in a loss of approximately 1000-fold activity against mannan substrates, consistent with the proposed roles. Crystallographic studies with AaManA in complex with β-mannosyl-1,4-mannoimidazole support the assignment of Glu151 as the acid/base [2]. A complex of AaManA with β-mannosyl-1,4-isofagomine supports the assignment of Glu231 as the nucleophile [2].

Three-dimensional structures

The three dimensional structure was first reported for AaManA, which possesses a classical (β/α)8 TIM barrel fold that aligns well with enzymes of family GH5 [1]. Alignment of the AaManA structure with Cel5G from Pseudoalteromonas haloplanktis revealed eight equivalent residues around the proposed active site pocket: Lys93, Thr95, Cys150, Glu151, Ser201, Tyr203, Glu231, and Trp281 [1]. Binary complexes of AaManA with β-mannosyl-1,4-mannoimidazole or β-mannosyl-1,4-isofagomine support the identity of the active site residues originally proposed on the basis of structural comparisons of AaManA with Cel5G and mutagenesis [2]. An active-site spanning ternary complex of AaManA with β-mannosyl-1,4-isofagomine and 1,4-β-mannobiose has provided structural details of amino acids defining the -2 to +2 subsites [2].

Family Firsts

First stereochemistry determination
AaManA was shown to be retaining by evidence for transglycosylation as well as the spatial separation of the general acid/base and catalytic nucleophile [1].
First catalytic nucleophile identification
Glu231 in AaManA by structural study supported by mutagenesis [1].
First general acid/base residue identification
Glu151 in AaManA by structural study supported by mutagenesis [1].
First 3-D structure
AaManA from A. acidocaldarius, PDB code 3CIV [1] .

References

  1. Zhang Y, Ju J, Peng H, Gao F, Zhou C, Zeng Y, Xue Y, Li Y, Henrissat B, Gao GF, and Ma Y. (2008). Biochemical and structural characterization of the intracellular mannanase AaManA of Alicyclobacillus acidocaldarius reveals a novel glycoside hydrolase family belonging to clan GH-A. J Biol Chem. 2008;283(46):31551-8. DOI:10.1074/jbc.M803409200 | PubMed ID:18755688 [Zhang2008]
  2. Williams RJ, Iglesias-Fernández J, Stepper J, Jackson A, Thompson AJ, Lowe EC, White JM, Gilbert HJ, Rovira C, Davies GJ, and Williams SJ. (2014). Combined inhibitor free-energy landscape and structural analysis reports on the mannosidase conformational coordinate. Angew Chem Int Ed Engl. 2014;53(4):1087-91. DOI:10.1002/anie.201308334 | PubMed ID:24339341 [Williams2014]

All Medline abstracts: PubMed