Glycoside hydrolases from Rhodothermus marinus Modular organisation and structure-function relationships
(2003)- Abstract
- The thermophilic bacterium <i>Rhodothermus marinus</i> produces several thermostable glycoside hydrolases. The studies presented in this thesis were performed on two enzymes, belonging to glycoside hydrolase families 10 and 12, produced by this microorganism. The family 10 xylanase, Xyn10A, is modular in architecture consisting of five domains or modules. The two isolated N-terminal modules were produced and characterised. These modules were proven to be carbohydrate-binding modules (CBMs) belonging to a novel subdivision of family 4 CBMs. Both modules display affinity for xylans, b-glucans, and to a less extent non-crystalline cellulose. The structure of the second of these binding modules (CBM4-2), solved by NMR, featured a... (More)
- The thermophilic bacterium <i>Rhodothermus marinus</i> produces several thermostable glycoside hydrolases. The studies presented in this thesis were performed on two enzymes, belonging to glycoside hydrolase families 10 and 12, produced by this microorganism. The family 10 xylanase, Xyn10A, is modular in architecture consisting of five domains or modules. The two isolated N-terminal modules were produced and characterised. These modules were proven to be carbohydrate-binding modules (CBMs) belonging to a novel subdivision of family 4 CBMs. Both modules display affinity for xylans, b-glucans, and to a less extent non-crystalline cellulose. The structure of the second of these binding modules (CBM4-2), solved by NMR, featured a b-sandwich with jelly roll-topology. Structural details and substrate titrations provided valuable insight on the determinants of specificity of the module. Both the Xyn10A CBMs and the third domain in the enzyme were shown to bind calcium ions, which had a pronounced effect on their thermostabilities. In addition, modular interactions seemed to enhance the stability of the enzyme, since deletion mutants were less stable than the full-length enzyme. No specific function could be ascribed the third domain of Xyn10A, while evidence suggested that the fifth domain is a novel module type that mediates cell-attachment. The primary structure of the family 12 endoglucanase Cel12A was analysed. These analyses showed that the catalytic module of this enzyme is preceded by a linker sequence and a putative signal peptide that destabilised the enzyme and impaired its expression in <i>Escherichia coli</i>. Designing mutants lacking this signal peptide readily solved the stability and production problems and these mutants retained their thermostability and activity. Finally, fusion proteins between the Xyn10A CBMs and the catalytic module of Cel12A were produced and some of their properties are reported. (Less)
Please use this url to cite or link to this publication:
https://lup.lub.lu.se/record/465573
- author
- Abou-Hachem, Maher LU
- supervisor
- opponent
-
- Professor Liebl, Wolfgang, Georg-August-Universität Göttingen, Germany
- organization
- publishing date
- 2003
- type
- Thesis
- publication status
- published
- subject
- keywords
- calcium-binding, modular, endoglucanase, thermostable, CBM, xylanase, Biotechnology, Bioteknik
- pages
- 160 pages
- publisher
- Maher Abou Hachem, Kämnärsvägen 13, E105, 226 46 Lund, Sweden,
- defense location
- lecture hall B, Center for Chemistry and Chemical Engineering, Sölvegatan 39, Lund
- defense date
- 2003-03-28 13:15:00
- external identifiers
-
- other:ISRN: LUTKDH/TKBT--03/1065--SE
- ISBN
- 91-7422-014-4
- language
- English
- LU publication?
- yes
- additional info
- Article: I. Abou Hachem, M., Nordberg Karlsson, E., Bartonek-Roxå, E., Raghothama, S., Simpson, P.J., Gilbert, H.J., Williamson, M.P. and Holst, O. (2000) Carbohydrate binding modules from a thermostable Rhodothermus marinus xylanase: Cloning, expression and binding studies. Biochemical Journal 345, 53-60A. Article: II. Abou Hachem, M., Nordberg Karlsson, E., Simpson, P.J., Williamson, M.P., Seller, P., Linse, S., Gilbert, H.J., Bolam D.N., and Holst, O. (2002) Calcium binding and thermodynamic studies on the thermostable carbohydrate binding modules of Xyn10A Rhodothermus marinus. Biochemistry 41, 5720-5729B. Article: III. Simpson, P.J, Jamieson, S.J., Abou-Hachem, M., Nordberg Karlsson, E., Gilbert, H.J., Holst, O., Williamson, M.P. (2002) The solution structure of the CBM4-2 carbohydrate binding module from a thermostable Rhodothermus marinus xylanase. Biochemistry 41, 5712-5719B. Article: IV. Abou Hachem, M., Olsson, F., and Nordberg Karlsson, E. Probing the stability of the modular family 10 xylanase from Rhodothermus marinus. (manuscript) Article: V. Wicher, K.B., Abou-Hachem M., Halldorsdottir, S., Thorbjarnadottir, S.H., Eggertsson, G., Hreggvidsson, G.O., Nordberg Karlsson E., Holst O. (2001) Deletion of a cytotoxic, N-terminal putative signal peptide results in a significant increase in production yields in Escherichia coli and improved specific activity of Cel12A from Rhodothermus marinus. Applied Microbiology and Biotechnology 55, 578-84C. Article: VI. Abou Hachem, M., Ramchuran, S.O., Oxhamre, C., Crennell, S.J., Holst, O. Nordberg Karlsson, E. Chimeric thermostable glycoside hydrolases: Fusion of family 4 carbohydrate binding modules to a family 12 endoglucanase catalytic module (manuscript).
- id
- 2bbc271d-1bc4-4dca-839e-214031c8aa65 (old id 465573)
- date added to LUP
- 2016-04-04 12:22:50
- date last changed
- 2018-11-21 21:10:37
@phdthesis{2bbc271d-1bc4-4dca-839e-214031c8aa65, abstract = {{The thermophilic bacterium <i>Rhodothermus marinus</i> produces several thermostable glycoside hydrolases. The studies presented in this thesis were performed on two enzymes, belonging to glycoside hydrolase families 10 and 12, produced by this microorganism. The family 10 xylanase, Xyn10A, is modular in architecture consisting of five domains or modules. The two isolated N-terminal modules were produced and characterised. These modules were proven to be carbohydrate-binding modules (CBMs) belonging to a novel subdivision of family 4 CBMs. Both modules display affinity for xylans, b-glucans, and to a less extent non-crystalline cellulose. The structure of the second of these binding modules (CBM4-2), solved by NMR, featured a b-sandwich with jelly roll-topology. Structural details and substrate titrations provided valuable insight on the determinants of specificity of the module. Both the Xyn10A CBMs and the third domain in the enzyme were shown to bind calcium ions, which had a pronounced effect on their thermostabilities. In addition, modular interactions seemed to enhance the stability of the enzyme, since deletion mutants were less stable than the full-length enzyme. No specific function could be ascribed the third domain of Xyn10A, while evidence suggested that the fifth domain is a novel module type that mediates cell-attachment. The primary structure of the family 12 endoglucanase Cel12A was analysed. These analyses showed that the catalytic module of this enzyme is preceded by a linker sequence and a putative signal peptide that destabilised the enzyme and impaired its expression in <i>Escherichia coli</i>. Designing mutants lacking this signal peptide readily solved the stability and production problems and these mutants retained their thermostability and activity. Finally, fusion proteins between the Xyn10A CBMs and the catalytic module of Cel12A were produced and some of their properties are reported.}}, author = {{Abou-Hachem, Maher}}, isbn = {{91-7422-014-4}}, keywords = {{calcium-binding; modular; endoglucanase; thermostable; CBM; xylanase; Biotechnology; Bioteknik}}, language = {{eng}}, publisher = {{Maher Abou Hachem, Kämnärsvägen 13, E105, 226 46 Lund, Sweden,}}, school = {{Lund University}}, title = {{Glycoside hydrolases from Rhodothermus marinus Modular organisation and structure-function relationships}}, year = {{2003}}, }