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Difference between revisions of "Glycoside Hydrolase Family 25"

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|{{Hl2}} colspan="2" align="center" |'''Glycoside Hydrolase Family GH25'''
 
|{{Hl2}} colspan="2" align="center" |'''Glycoside Hydrolase Family GH25'''
 
|-
 
|-
|'''Clan'''  
+
|'''Clan'''  
 
|GH-K
 
|GH-K
 
|-
 
|-
 
|'''Mechanism'''
 
|'''Mechanism'''
|Retaining
+
|unknown, likely retaining<br>by analogy with<br>GH18,20,56,84,85 <cite>MartinezFleites2009</cite>
 
|-
 
|-
 
|'''Active site residues'''
 
|'''Active site residues'''
|Asp/Gul
+
|Asp/Glu
 
|-
 
|-
 
|{{Hl2}} colspan="2" align="center" |'''CAZy DB link'''
 
|{{Hl2}} colspan="2" align="center" |'''CAZy DB link'''
 
|-
 
|-
| colspan="2" |http://www.cazy.org/fam/GH25.html
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| colspan="2" |{{CAZyDBlink}}GH25.html
 
|}
 
|}
 
</div>
 
</div>
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== Substrate specificities ==
 
== Substrate specificities ==
Family GH25 lysozymes otherwise known as Chalaropsis (CH) type of lysozymes (from is initial characterisation from Chalaropsis species of fungus<cite>REF1</cite>) cleaves the β-1,4-glycosidic bond between N-acetylmuramic acid (NAM) and N-acetylglucosamine (NAG) in the carbohydrate backbone of bacterial peptidoglycan.  The characterized lysozymes from this family exhibit both β-1,4-N-acetyl- and β-1,4- N ,6-O-diacetylmuramidase activities and are able to degrade  O-acetylated peptidoglycan present in ''Staphylococcus aureus'' and other pathogens<cite>REF2</cite>. The activity of GH25 enzymes appears to fulfil two main biological roles in bacteria. These roles are the re-modelling of peptidoglycan in cellular process such as division and promoting the dissemination of phage progeny toward the end of the phage lytic cycle, which is achieved by bacterial cell lysis. For this reason many GH25 proteins are found to be either chromosomal, phage or prophage encoded. The majority of the GH25 family is comprised of bacterial or prokaryotic viral (phage) members. There are however a few eukaryotic representatives, but these are so far restricted to the fungal kingdom.  The roles of these fungal enzymes are less clear, many possess signal secretion peptides indicating a likely extracellular location, possibly for the purpose of obtaining or gaining assess to nutrients or even as a selective agent against bacteria.
+
[[Glycoside hydrolase]]s of family GH25 are lysozymes otherwise known as the Chalaropsis (CH) type of lysozymes (from their initial characterisation from Chalaropsis species of fungus <cite>Hash1967</cite>). They cleave the β-1,4-glycosidic bond between ''N''-acetylmuramic acid (NAM) and N-acetylglucosamine (NAG) in the carbohydrate backbone of bacterial peptidoglycan.  The characterized lysozymes from this family exhibit both β-1,4-''N''-acetyl- and β-1,4-''N'',6-O-diacetylmuramidase activities and are able to degrade  O-acetylated peptidoglycan present in ''Staphylococcus aureus'' and other pathogens <cite>Vollmer2008b</cite>. The activity of GH25 enzymes appears to fulfil two main biological roles in bacteria. These roles are the re-modelling of peptidoglycan in cellular process such as division and the dissemination of phage progeny toward the end of the phage lytic cycle, which is achieved by lysis of the bacterial cell. For this reason many GH25 proteins are found to be chromosomal, phage or prophage encoded. The majority of the GH25 family is comprised of bacterial or prokaryotic viral (phage) members. There are however a few eukaryotic representatives, but these are so far restricted to the fungal kingdom.  The roles of these fungal enzymes are less clear, many possess signal secretion peptides indicating a likely extracellular location, possibly for the purpose of obtaining or gaining assess to nutrients or even as a selective agent against bacteria.
 
   
 
   
 
== Kinetics and Mechanism ==
 
== Kinetics and Mechanism ==
The lack of activity on chitooligosaccharides and complexity in producing defined synthetic peptidoglycan substrates, has inevitably hampered the determination of kinetic parameters. Structural studies have shown the active-centre is extremely similar to those from GH18, 20, 56, 84 and 85 implying that, in the absence of evidence to the contrary, GH25 enzymes act with net retention of anomeric configuration using a neighboring-group catalytic mechanism common to this “super-family” of enzymes<cite>REF3</cite>.
+
The lack of activity on chitooligosaccharides and the difficulty of producing defined synthetic peptidoglycan substrates, has inevitably hampered the determination of kinetic parameters. Structural studies have shown the active-centre is closely similar to those from [[GH18]], [[GH20]], [[GH56]], [[GH84]] and [[GH85]] implying that, in the absence of evidence to the contrary, GH25 enzymes are [[retaining]] glycoside hydrolases that use a [[neighboring group participation]] mechanism common to this “super-family” of enzymes <cite>MartinezFleites2009</cite>.
  
 
== Catalytic Residues ==
 
== Catalytic Residues ==
This super-family has been shown to use an active site DE or DXE sequence motif ( or exceptionally in the case of GH85 a DXN moitif<cite>REF4< REF5</cite> ).  This carboxylate pair promotes a double displacement mechanism in which the nucleophile is not enzyme-derived but is provided by the substrate in an  intramolecular “neighboring group” attack of the N-acetyl carbonyl group<cite>REF6</cite>. Thus catalysis occurs via the formation, and subsequent breakdown of a covalent oxazoline intermediate.
+
The super-family comprised of families [[GH18]], [[GH20]], [[GH56]], [[GH84]] and [[GH85]] has been shown to use an active site DE or DXE sequence motif (or exceptionally in the case of GH85 a NXD motif <cite>Ling2009 Abbott2009</cite>).  This carboxylate pair promotes a double displacement mechanism in which the catalytic nucleophile is not enzyme-derived but is provided by the substrate in an  intramolecular “neighboring group” attack of the N-acetyl carbonyl group <cite>VocadloDavies2008</cite>. Thus catalysis occurs via the formation, and subsequent breakdown of a covalent oxazoline (or [[oxazolinium ion]]) [[intermediate]].
  
 
== Three-dimensional structures ==
 
== Three-dimensional structures ==
So far four members of this family of enzymes have been structural characterized, that of the ''Streptomyces coelicolor'' enzyme “cellosyl”<cite>REF7</cite>, the bacteriophage lysine PlyB<cite>REF8</cite>, and Clp-1lysozyme from a ''Streptococcus pneumoniae '' phage <cite>REF9 REF10</cite>, whose structure was also obtained in complex with fragments of peptidoglycan analogues 10 and  BaGh25c from ''Bacillus anthracis'' str. Ames<cite>REF3</cite>. The GH25 lysozymes,  are structurally unrelated to the [[GH22]], [[GH23]], [[GH24]], [[GH73]] and [[GH108]] lysozyme folds and instead these enzymes display a modified α -barrel-like fold that, like the classical “TIM-barrel” is composed of a eight-stranded β-barrel, but which is flanked by just three (as opposed to the normal eight) α-helices<cite>REF7</cite>.There is a prominent, long groove, very likely the substrate binding site, located on the C-terminal face. This groove culminates in a deep hole of a highly negative electrostatic potential forming the catalytic site<cite>REF11</cite>.
+
So far four members of this family of enzymes have been structural characterized, that of the ''Streptomyces coelicolor'' enzyme “cellosyl” <cite>Rau2001</cite>, the bacteriophage lysine PlyB <cite>Porter2007</cite>, and Clp-1lysozyme from a ''Streptococcus pneumoniae '' phage <cite>Hermoso2003 PerezDorado2007</cite>, whose structure was also obtained in complex with fragments of peptidoglycan analogues 10 and  BaGh25c from ''Bacillus anthracis'' str. Ames <cite>MartinezFleites2009</cite>. The GH25 lysozymes,  are structurally unrelated to the [[GH22]], [[GH23]], [[GH24]], [[GH73]] and [[GH108]] lysozyme folds and instead these enzymes display a modified α -barrel-like fold that, like the classical “TIM-barrel” is composed of a eight-stranded β-barrel, but which is flanked by just three (as opposed to the normal eight) α-helices <cite>Rau2001</cite>. There is a prominent, long groove, very likely the substrate binding site, located on the C-terminal face. This groove culminates in a deep hole of a highly negative electrostatic potential forming the catalytic site <cite>Vollmer2008a</cite>.
  
 
== Family Firsts ==
 
== Family Firsts ==
 
;First sterochemistry determination: Has yet to be experimentally determined.
 
;First sterochemistry determination: Has yet to be experimentally determined.
;First catalytic nucleophile identification: This remains to be experimentally proven, however it is likely that the nucleophile is not enzyme-derived, but is provided by the substrate in a “neighboring group" participation reaction<cite>REF3</cite>.  
+
;First catalytic nucleophile identification: This remains to be experimentally proven. Inverting mechanisms have been proposed <cite>Hermoso2003</cite>, but it is perhaps more likely that the enzyme is [[retaining]] and that the nucleophile is not enzyme-derived, but is provided by the substrate in a [[neighboring group participation]] mechanism <cite>MartinezFleites2009</cite>. This is based upon the considerable active centre structural similarity with other neighboring group enzymes in GH18, 20, 56, 84 and also 85.
;First general acid/base residue identification: Has yet to be fully experimentally determined.  
+
;First [[general acid/base]] residue identification: Has yet to be fully experimentally determined but again structural similarity strongly implicates the second carboxylate in the DXE motif described previously. In the case of the ''Bacillus anthracis'' enzyme this is Glu107 <cite>MartinezFleites2009</cite>.
;First 3-D structure:       The ''Streptomyces coelicolor'' enzyme "cellosyl" <cite>REF7</cite> was the first GH25 structure to be described in 2001.
+
;First 3-D structure: The ''Streptomyces coelicolor'' enzyme "cellosyl" <cite>Rau2001</cite> was the first GH25 structure to be described in 2001.
  
 
== References ==
 
== References ==
 
<biblio>
 
<biblio>
#REF1 pmid=12325376
+
#Hash1967 pmid=12325376
#REF2 pmid=18070068
+
#Vollmer2008a pmid=18266855
#REF3 pmid=19595298
+
#Vollmer2008b pmid=18070068
#REF4 pmid=19327363
+
#MartinezFleites2009 pmid=19595298
#REF5 pmid=19181667
+
#Ling2009 pmid=19327363
#REF6 pmid=18558099
+
#Abbott2009 pmid=19181667
#REF7 pmid=11427528
+
#VocadloDavies2008 pmid=18558099
#REF8 pmid=17182056
+
#Rau2001 pmid=11427528
#REF9 pmid=14527392
+
#Porter2007 pmid=17182056
#REF10 pmid=17581815
+
#Hermoso2003 pmid=14527392
#REF11 pmid=18266855
+
#PerezDorado2007 pmid=17581815
 
</biblio>
 
</biblio>
  
  
 
[[Category:Glycoside Hydrolase Families|GH025]]
 
[[Category:Glycoside Hydrolase Families|GH025]]

Latest revision as of 13:20, 18 December 2021

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Glycoside Hydrolase Family GH25
Clan GH-K
Mechanism unknown, likely retaining
by analogy with
GH18,20,56,84,85 [1]
Active site residues Asp/Glu
CAZy DB link
https://www.cazy.org/GH25.html


Substrate specificities

Glycoside hydrolases of family GH25 are lysozymes otherwise known as the Chalaropsis (CH) type of lysozymes (from their initial characterisation from Chalaropsis species of fungus [2]). They cleave the β-1,4-glycosidic bond between N-acetylmuramic acid (NAM) and N-acetylglucosamine (NAG) in the carbohydrate backbone of bacterial peptidoglycan. The characterized lysozymes from this family exhibit both β-1,4-N-acetyl- and β-1,4-N,6-O-diacetylmuramidase activities and are able to degrade O-acetylated peptidoglycan present in Staphylococcus aureus and other pathogens [3]. The activity of GH25 enzymes appears to fulfil two main biological roles in bacteria. These roles are the re-modelling of peptidoglycan in cellular process such as division and the dissemination of phage progeny toward the end of the phage lytic cycle, which is achieved by lysis of the bacterial cell. For this reason many GH25 proteins are found to be chromosomal, phage or prophage encoded. The majority of the GH25 family is comprised of bacterial or prokaryotic viral (phage) members. There are however a few eukaryotic representatives, but these are so far restricted to the fungal kingdom. The roles of these fungal enzymes are less clear, many possess signal secretion peptides indicating a likely extracellular location, possibly for the purpose of obtaining or gaining assess to nutrients or even as a selective agent against bacteria.

Kinetics and Mechanism

The lack of activity on chitooligosaccharides and the difficulty of producing defined synthetic peptidoglycan substrates, has inevitably hampered the determination of kinetic parameters. Structural studies have shown the active-centre is closely similar to those from GH18, GH20, GH56, GH84 and GH85 implying that, in the absence of evidence to the contrary, GH25 enzymes are retaining glycoside hydrolases that use a neighboring group participation mechanism common to this “super-family” of enzymes [1].

Catalytic Residues

The super-family comprised of families GH18, GH20, GH56, GH84 and GH85 has been shown to use an active site DE or DXE sequence motif (or exceptionally in the case of GH85 a NXD motif [4, 5]). This carboxylate pair promotes a double displacement mechanism in which the catalytic nucleophile is not enzyme-derived but is provided by the substrate in an intramolecular “neighboring group” attack of the N-acetyl carbonyl group [6]. Thus catalysis occurs via the formation, and subsequent breakdown of a covalent oxazoline (or oxazolinium ion) intermediate.

Three-dimensional structures

So far four members of this family of enzymes have been structural characterized, that of the Streptomyces coelicolor enzyme “cellosyl” [7], the bacteriophage lysine PlyB [8], and Clp-1lysozyme from a Streptococcus pneumoniae phage [9, 10], whose structure was also obtained in complex with fragments of peptidoglycan analogues 10 and BaGh25c from Bacillus anthracis str. Ames [1]. The GH25 lysozymes, are structurally unrelated to the GH22, GH23, GH24, GH73 and GH108 lysozyme folds and instead these enzymes display a modified α -barrel-like fold that, like the classical “TIM-barrel” is composed of a eight-stranded β-barrel, but which is flanked by just three (as opposed to the normal eight) α-helices [7]. There is a prominent, long groove, very likely the substrate binding site, located on the C-terminal face. This groove culminates in a deep hole of a highly negative electrostatic potential forming the catalytic site [11].

Family Firsts

First sterochemistry determination
Has yet to be experimentally determined.
First catalytic nucleophile identification
This remains to be experimentally proven. Inverting mechanisms have been proposed [9], but it is perhaps more likely that the enzyme is retaining and that the nucleophile is not enzyme-derived, but is provided by the substrate in a neighboring group participation mechanism [1]. This is based upon the considerable active centre structural similarity with other neighboring group enzymes in GH18, 20, 56, 84 and also 85.
First general acid/base residue identification
Has yet to be fully experimentally determined but again structural similarity strongly implicates the second carboxylate in the DXE motif described previously. In the case of the Bacillus anthracis enzyme this is Glu107 [1].
First 3-D structure
The Streptomyces coelicolor enzyme "cellosyl" [7] was the first GH25 structure to be described in 2001.

References

  1. Martinez-Fleites C, Korczynska JE, Davies GJ, Cope MJ, Turkenburg JP, and Taylor EJ. (2009). The crystal structure of a family GH25 lysozyme from Bacillus anthracis implies a neighboring-group catalytic mechanism with retention of anomeric configuration. Carbohydr Res. 2009;344(13):1753-7. DOI:10.1016/j.carres.2009.06.001 | PubMed ID:19595298 [MartinezFleites2009]
  2. Hash JH and Rothlauf MV. (1967). The N,O-diacetylmuramidase of Chalaropsis species. I. Purification and crystallization. J Biol Chem. 1967;242(23):5586-90. | Google Books | Open Library PubMed ID:12325376 [Hash1967]
  3. Vollmer W (2008). Structural variation in the glycan strands of bacterial peptidoglycan. FEMS Microbiol Rev. 2008;32(2):287-306. DOI:10.1111/j.1574-6976.2007.00088.x | PubMed ID:18070068 [Vollmer2008b]
  4. Ling Z, Suits MD, Bingham RJ, Bruce NC, Davies GJ, Fairbanks AJ, Moir JW, and Taylor EJ. (2009). The X-ray crystal structure of an Arthrobacter protophormiae endo-beta-N-acetylglucosaminidase reveals a (beta/alpha)(8) catalytic domain, two ancillary domains and active site residues key for transglycosylation activity. J Mol Biol. 2009;389(1):1-9. DOI:10.1016/j.jmb.2009.03.050 | PubMed ID:19327363 [Ling2009]
  5. Abbott DW, Macauley MS, Vocadlo DJ, and Boraston AB. (2009). Streptococcus pneumoniae endohexosaminidase D, structural and mechanistic insight into substrate-assisted catalysis in family 85 glycoside hydrolases. J Biol Chem. 2009;284(17):11676-89. DOI:10.1074/jbc.M809663200 | PubMed ID:19181667 [Abbott2009]
  6. Vocadlo DJ and Davies GJ. (2008). Mechanistic insights into glycosidase chemistry. Curr Opin Chem Biol. 2008;12(5):539-55. DOI:10.1016/j.cbpa.2008.05.010 | PubMed ID:18558099 [VocadloDavies2008]
  7. Rau A, Hogg T, Marquardt R, and Hilgenfeld R. (2001). A new lysozyme fold. Crystal structure of the muramidase from Streptomyces coelicolor at 1.65 A resolution. J Biol Chem. 2001;276(34):31994-9. DOI:10.1074/jbc.M102591200 | PubMed ID:11427528 [Rau2001]
  8. Porter CJ, Schuch R, Pelzek AJ, Buckle AM, McGowan S, Wilce MC, Rossjohn J, Russell R, Nelson D, Fischetti VA, and Whisstock JC. (2007). The 1.6 A crystal structure of the catalytic domain of PlyB, a bacteriophage lysin active against Bacillus anthracis. J Mol Biol. 2007;366(2):540-50. DOI:10.1016/j.jmb.2006.11.056 | PubMed ID:17182056 [Porter2007]
  9. Hermoso JA, Monterroso B, Albert A, Galán B, Ahrazem O, García P, Martínez-Ripoll M, García JL, and Menéndez M. (2003). Structural basis for selective recognition of pneumococcal cell wall by modular endolysin from phage Cp-1. Structure. 2003;11(10):1239-49. DOI:10.1016/j.str.2003.09.005 | PubMed ID:14527392 [Hermoso2003]
  10. Pérez-Dorado I, Campillo NE, Monterroso B, Hesek D, Lee M, Páez JA, García P, Martínez-Ripoll M, García JL, Mobashery S, Menéndez M, and Hermoso JA. (2007). Elucidation of the molecular recognition of bacterial cell wall by modular pneumococcal phage endolysin CPL-1. J Biol Chem. 2007;282(34):24990-9. DOI:10.1074/jbc.M704317200 | PubMed ID:17581815 [PerezDorado2007]
  11. Vollmer W, Joris B, Charlier P, and Foster S. (2008). Bacterial peptidoglycan (murein) hydrolases. FEMS Microbiol Rev. 2008;32(2):259-86. DOI:10.1111/j.1574-6976.2007.00099.x | PubMed ID:18266855 [Vollmer2008a]

All Medline abstracts: PubMed