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Difference between revisions of "Carbohydrate Binding Module Family 1"

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== Ligand specificities ==
 
== Ligand specificities ==
Mention here all major natural ligand specificities that are found within a given family (also plant or mammalian origin). Certain linkages and promiscuity would also be mentioned here if biologically relevant.
+
The family 1 CBMs are found mainly in fungal enzymes <cite>Varnai2014,Martinez2015</cite>. Early work showed that family 1 CBMs bind to cellulose <cite>Johansson1989</cite> and that some, but not all, family 1 CBMs bind to chitin as well <cite>Linder1996</cite>. There is also a contribution of CBMs in binding to lignin, but this binding was shown to be non-specific as it was easily blocked by surfactants <cite>Palonen2004</cite>. The site of binding of a CBM1 to crystalline cellulose was determined by transmission electron microscopy of gold labelled CBM1 fused to modified Protein A. The data showed that the CBM1 bound to the 110 face of Valonia cellulose <cite>Lehtio2003</cite> Based on NMR measurements it was shown that family 1 CBMs could bind to cellohexaose, but not to shorter cellotriose and cellobiose <cite>Mattinen1997</cite>.
 
 
''Note: Here is an example of how to insert references in the text, together with the "biblio" section below:'' Please see these references for an essential introduction to the CAZy classification system: <cite>DaviesSinnott2008 Cantarel2009</cite>. CBMs, in particular, have been extensively reviewed <cite>Boraston2004 Hashimoto2006 Shoseyov2006 Guillen2010</cite>.
 
  
 
== Structural Features ==
 
== Structural Features ==
''Content in this section should include, in paragraph form, a description of:''
+
[[File:CBM 1.png|thumb|300px|right|'''Figure 1.''' ''Top.'' A backbone trace of the ''T.reesei'' Cel7A CBM showing residues that have been identified as important for the interaction with cellulose. ''Below.'' The structure flipped 90 degrees to show how the aromatic residues align with pyronose rings in a cellulose molecule.]]
* '''Fold:''' Structural fold (beta trefoil, beta sandwich, etc.)
+
Structurally the family 1 CBMs are distinct from other families. They are relatively small, only about 35 amino acids and have two or three disulphide bridges that stabilize their fold <cite>Kraulis1989</cite>. This type of fold is called a cystine knot and is also found in a family of toxins, called conotoxins produced by cone shells <cite>Norton1989</cite>. This structure is rigid and on the CBM there are three aromatic residues (tyrosines or tryptophans) that align so that their spacing is the same as every second pyranose ring on cellulose. Together with some hydrogen bond forming side chains this triad of aromatic residues form a binding face that docks onto the cellulose surface. It has also been shown using synthesised peptides that carbohydrates added to the CBMs affect their binding properties <cite>Happs2015</cite>.
* '''Type:''' Include here Type A, B, or C and properties
 
* '''Features of ligand binding:''' Describe CBM binding pocket location (Side or apex) important residues for binding (W, Y, F, subsites), interact with reducing end, non-reducing end, planar surface or within polysaccharide chains. Include examples pdb codes. Metal ion dependent. Etc.
 
  
 
== Functionalities ==  
 
== Functionalities ==  
''Content in this section should include, in paragraph form, a description of:''
+
The CBMs affect enzyme activity by bringing the enzymes close to the cellulose surface <cite>Igarashi2009</cite>, but there are reports that family 1 CBMs can disrupt the crystalline structure of cellulose as well <cite>Hall2011</cite>. Family 1 CBMs are found widely in fungal cellulases, also in several enzymes that are not active on cellulose such as mannanase <cite>Hagglund2003</cite> and acetyl xylan esterase <cite>Margolles1996</cite>. Also swollenins have been found to contain family 1 CBMs <cite>Saloheimo2002</cite>.
* '''Functional role of CBM:''' Describe common functional roles such as targeting, disruptive, anchoring, proximity/position on substrate.
+
 
* '''Most Common Associated Modules:''' 1. Glycoside Hydrolase Activity; 2. Additional Associated Modules (other CBM, FNIII, cohesin, dockerins, expansins, etc.)
+
Family 1 CBMs have been used in different types of applications such stabilizing colloid dispersions of drugs by mediating binding to nanocellulose <cite>Varjonen2011</cite>.
* '''Novel Applications:'''  Include here if CBM has been used to modify another enzyme, or if a CBM was used to label plant/mammalian tissues? Etc.
 
  
 
== Family Firsts ==
 
== Family Firsts ==
;First Identified
+
 
:Insert archetype here, possibly including ''very brief'' synopsis.
+
;First Identified: Family 1 CBMs were found first in studies on the ''Trichoderma reesei'' Cel7A enzyme (then called cellobiohydrolase I, CBHI) using papain for fragmentation. These studies revealed that Cel7A had a “bifunctional” organization with one part binding strongly to cellulose and the other part containing the catalytic machinery <cite>vantilbeurgh1986</cite>. It was noted that sequences homologous to the smaller cellulose binding polypeptide sequence was found in many fungal cellulases and that a synthetic analogue functioned identically to the native fragments produced by proteolysis <cite>Johansson1989</cite>.  
;First Structural Characterization
+
 
:Insert archetype here, possibly including ''very brief'' synopsis.
+
;First Structural Characterization: The synthetic version of the ''Trichoderma reesei'' Cel7A cellulose binding domain was analysed by NMR and it was the first CBM1 structure determined <cite>#Kraulis1989</cite>. With the structure determined the research then led to a number of structure-function studies identifying the amino acids responsible for binding <cite>Linder1995</cite> and changing of binding properties by protein engineering <cite>Linder1999</cite>.
  
 
== References ==
 
== References ==
 
<biblio>
 
<biblio>
#Cantarel2009 pmid=18838391
+
#Varnai2014 pmid=24767427
#DaviesSinnott2008 Davies, G.J. and Sinnott, M.L. (2008) Sorting the diverse: the sequence-based classifications of carbohydrate-active enzymes. ''The Biochemist'', vol. 30, no. 4., pp. 26-32. [http://www.biochemist.org/bio/03004/0026/030040026.pdf Download PDF version].
+
#Martinez2015 pmid=26390127
#Boraston2004 pmid=15214846
+
#Johansson1989 Johansson, G., Ståhlberg, J., Lindeberg, G., Engström, Å., Pettersson, G. Isolated Fungal Cellulose Terminal Domains and a Synthetic Minimum Analogue Bind to Cellulose. FEBS Lett. 1989; 243, 389–393. [https://doi.org/10.1016/0014-5793(89)80168-1 DOI:10.1016/0014-5793(89)80168-1]
#Hashimoto2006 pmid=17131061
+
#Linder1996 pmid=8702902
#Shoseyov2006 pmid=16760304
+
#Palonen2004 pmid=14687972
#Guillen2010 pmid=19908036
+
 
 +
#Lehtio2003 pmid=12522267
 +
#Mattinen1997 pmid=9175871
 +
#Kraulis1989 pmid=2554967
 +
#Igarashi2009 pmid=19858200
 +
#Hall2011 pmid=21111611
 +
#Saloheimo2002 pmid=12199698
 +
#Varjonen2011 Varjonen, S.; Laaksonen, P.; Paananen, A.; Valo, H.; Hähl, H.; Laaksonen, T.; Linder, M. Ben. Self-Assembly of Cellulose Nanofibrils by Genetically Engineered Fusion Proteins. Soft Matter 2011, 7, 2402–2411. [https://doi.org/10.1039/C0SM01114B DOI:10.1039/C0SM01114B]
 +
#Norton1989 pmid=9792173
 +
#vantilbeurgh1986 van Tilbeurgh, H.; Tomme, P.; Claeyssens, M.; Bhikhabhai, R.; Pettersson, G. Limited Proteolysis of the cellobiohydrolase I from Trichoderma Reesei Separation of Functional Domains. FEBS Lett. 1986; 204, 223–227. [https://doi.org/10.1016/0014-5793(86)80816-X DOI:10.1016/0014-5793(86)80816-X]
 +
#Linder1995 pmid=7549870
 +
#Linder1999 pmid=10218572
 +
#Happs2015 pmid=26307003
 
</biblio>
 
</biblio>
  
 
[[Category:Carbohydrate Binding Module Families|CBM001]]
 
[[Category:Carbohydrate Binding Module Families|CBM001]]

Latest revision as of 13:14, 18 December 2021

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CAZy DB link
https://www.cazy.org/CBM1.html

Ligand specificities

The family 1 CBMs are found mainly in fungal enzymes [1, 2]. Early work showed that family 1 CBMs bind to cellulose [3] and that some, but not all, family 1 CBMs bind to chitin as well [4]. There is also a contribution of CBMs in binding to lignin, but this binding was shown to be non-specific as it was easily blocked by surfactants [5]. The site of binding of a CBM1 to crystalline cellulose was determined by transmission electron microscopy of gold labelled CBM1 fused to modified Protein A. The data showed that the CBM1 bound to the 110 face of Valonia cellulose [6] Based on NMR measurements it was shown that family 1 CBMs could bind to cellohexaose, but not to shorter cellotriose and cellobiose [7].

Structural Features

Figure 1. Top. A backbone trace of the T.reesei Cel7A CBM showing residues that have been identified as important for the interaction with cellulose. Below. The structure flipped 90 degrees to show how the aromatic residues align with pyronose rings in a cellulose molecule.

Structurally the family 1 CBMs are distinct from other families. They are relatively small, only about 35 amino acids and have two or three disulphide bridges that stabilize their fold [8]. This type of fold is called a cystine knot and is also found in a family of toxins, called conotoxins produced by cone shells [9]. This structure is rigid and on the CBM there are three aromatic residues (tyrosines or tryptophans) that align so that their spacing is the same as every second pyranose ring on cellulose. Together with some hydrogen bond forming side chains this triad of aromatic residues form a binding face that docks onto the cellulose surface. It has also been shown using synthesised peptides that carbohydrates added to the CBMs affect their binding properties [10].

Functionalities

The CBMs affect enzyme activity by bringing the enzymes close to the cellulose surface [11], but there are reports that family 1 CBMs can disrupt the crystalline structure of cellulose as well [12]. Family 1 CBMs are found widely in fungal cellulases, also in several enzymes that are not active on cellulose such as mannanase [13] and acetyl xylan esterase [14]. Also swollenins have been found to contain family 1 CBMs [15].

Family 1 CBMs have been used in different types of applications such stabilizing colloid dispersions of drugs by mediating binding to nanocellulose [16].

Family Firsts

First Identified
Family 1 CBMs were found first in studies on the Trichoderma reesei Cel7A enzyme (then called cellobiohydrolase I, CBHI) using papain for fragmentation. These studies revealed that Cel7A had a “bifunctional” organization with one part binding strongly to cellulose and the other part containing the catalytic machinery [17]. It was noted that sequences homologous to the smaller cellulose binding polypeptide sequence was found in many fungal cellulases and that a synthetic analogue functioned identically to the native fragments produced by proteolysis [3].
First Structural Characterization
The synthetic version of the Trichoderma reesei Cel7A cellulose binding domain was analysed by NMR and it was the first CBM1 structure determined [8]. With the structure determined the research then led to a number of structure-function studies identifying the amino acids responsible for binding [18] and changing of binding properties by protein engineering [19].

References

  1. Várnai A, Mäkelä MR, Djajadi DT, Rahikainen J, Hatakka A, and Viikari L. (2014). Carbohydrate-binding modules of fungal cellulases: occurrence in nature, function, and relevance in industrial biomass conversion. Adv Appl Microbiol. 2014;88:103-65. DOI:10.1016/B978-0-12-800260-5.00004-8 | PubMed ID:24767427 [Varnai2014]
  2. Martinez T, Texier H, Nahoum V, Lafitte C, Cioci G, Heux L, Dumas B, O'Donohue M, Gaulin E, and Dumon C. (2015). Probing the Functions of Carbohydrate Binding Modules in the CBEL Protein from the Oomycete Phytophthora parasitica. PLoS One. 2015;10(9):e0137481. DOI:10.1371/journal.pone.0137481 | PubMed ID:26390127 [Martinez2015]
  3. Johansson, G., Ståhlberg, J., Lindeberg, G., Engström, Å., Pettersson, G. Isolated Fungal Cellulose Terminal Domains and a Synthetic Minimum Analogue Bind to Cellulose. FEBS Lett. 1989; 243, 389–393. DOI:10.1016/0014-5793(89)80168-1

    [Johansson1989]
  4. Linder M, Salovuori I, Ruohonen L, and Teeri TT. (1996). Characterization of a double cellulose-binding domain. Synergistic high affinity binding to crystalline cellulose. J Biol Chem. 1996;271(35):21268-72. DOI:10.1074/jbc.271.35.21268 | PubMed ID:8702902 [Linder1996]
  5. Palonen H, Tjerneld F, Zacchi G, and Tenkanen M. (2004). Adsorption of Trichoderma reesei CBH I and EG II and their catalytic domains on steam pretreated softwood and isolated lignin. J Biotechnol. 2004;107(1):65-72. DOI:10.1016/j.jbiotec.2003.09.011 | PubMed ID:14687972 [Palonen2004]
  6. Lehtiö J, Sugiyama J, Gustavsson M, Fransson L, Linder M, and Teeri TT. (2003). The binding specificity and affinity determinants of family 1 and family 3 cellulose binding modules. Proc Natl Acad Sci U S A. 2003;100(2):484-9. DOI:10.1073/pnas.212651999 | PubMed ID:12522267 [Lehtio2003]
  7. Mattinen ML, Linder M, Teleman A, and Annila A. (1997). Interaction between cellohexaose and cellulose binding domains from Trichoderma reesei cellulases. FEBS Lett. 1997;407(3):291-6. DOI:10.1016/s0014-5793(97)00356-6 | PubMed ID:9175871 [Mattinen1997]
  8. Kraulis J, Clore GM, Nilges M, Jones TA, Pettersson G, Knowles J, and Gronenborn AM. (1989). Determination of the three-dimensional solution structure of the C-terminal domain of cellobiohydrolase I from Trichoderma reesei. A study using nuclear magnetic resonance and hybrid distance geometry-dynamical simulated annealing. Biochemistry. 1989;28(18):7241-57. DOI:10.1021/bi00444a016 | PubMed ID:2554967 [Kraulis1989]
  9. Norton RS and Pallaghy PK. (1998). The cystine knot structure of ion channel toxins and related polypeptides. Toxicon. 1998;36(11):1573-83. DOI:10.1016/s0041-0101(98)00149-4 | PubMed ID:9792173 [Norton1989]
  10. Happs RM, Guan X, Resch MG, Davis MF, Beckham GT, Tan Z, and Crowley MF. (2015). O-glycosylation effects on family 1 carbohydrate-binding module solution structures. FEBS J. 2015;282(22):4341-56. DOI:10.1111/febs.13500 | PubMed ID:26307003 [Happs2015]
  11. Igarashi K, Koivula A, Wada M, Kimura S, Penttilä M, and Samejima M. (2009). High speed atomic force microscopy visualizes processive movement of Trichoderma reesei cellobiohydrolase I on crystalline cellulose. J Biol Chem. 2009;284(52):36186-36190. DOI:10.1074/jbc.M109.034611 | PubMed ID:19858200 [Igarashi2009]
  12. Hall M, Bansal P, Lee JH, Realff MJ, and Bommarius AS. (2011). Biological pretreatment of cellulose: enhancing enzymatic hydrolysis rate using cellulose-binding domains from cellulases. Bioresour Technol. 2011;102(3):2910-5. DOI:10.1016/j.biortech.2010.11.010 | PubMed ID:21111611 [Hall2011]
  13. Saloheimo M, Paloheimo M, Hakola S, Pere J, Swanson B, Nyyssönen E, Bhatia A, Ward M, and Penttilä M. (2002). Swollenin, a Trichoderma reesei protein with sequence similarity to the plant expansins, exhibits disruption activity on cellulosic materials. Eur J Biochem. 2002;269(17):4202-11. DOI:10.1046/j.1432-1033.2002.03095.x | PubMed ID:12199698 [Saloheimo2002]
  14. Varjonen, S.; Laaksonen, P.; Paananen, A.; Valo, H.; Hähl, H.; Laaksonen, T.; Linder, M. Ben. Self-Assembly of Cellulose Nanofibrils by Genetically Engineered Fusion Proteins. Soft Matter 2011, 7, 2402–2411. DOI:10.1039/C0SM01114B

    [Varjonen2011]
  15. van Tilbeurgh, H.; Tomme, P.; Claeyssens, M.; Bhikhabhai, R.; Pettersson, G. Limited Proteolysis of the cellobiohydrolase I from Trichoderma Reesei Separation of Functional Domains. FEBS Lett. 1986; 204, 223–227. DOI:10.1016/0014-5793(86)80816-X

    [vantilbeurgh1986]
  16. Linder M, Mattinen ML, Kontteli M, Lindeberg G, Ståhlberg J, Drakenberg T, Reinikainen T, Pettersson G, and Annila A. (1995). Identification of functionally important amino acids in the cellulose-binding domain of Trichoderma reesei cellobiohydrolase I. Protein Sci. 1995;4(6):1056-64. DOI:10.1002/pro.5560040604 | PubMed ID:7549870 [Linder1995]
  17. Linder M, Nevanen T, and Teeri TT. (1999). Design of a pH-dependent cellulose-binding domain. FEBS Lett. 1999;447(1):13-6. DOI:10.1016/s0014-5793(99)00253-7 | PubMed ID:10218572 [Linder1999]

All Medline abstracts: PubMed