Materials Map

Discover the materials research landscape. Find experts, partners, networks.

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The Materials Map is an open tool for improving networking and interdisciplinary exchange within materials research. It enables cross-database search for cooperation and network partners and discovering of the research landscape.

The dashboard provides detailed information about the selected scientist, e.g. publications. The dashboard can be filtered and shows the relationship to co-authors in different diagrams. In addition, a link is provided to find contact information.

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The Materials Map is still under development. In its current state, it is only based on one single data source and, thus, incomplete and contains duplicates. We are working on incorporating new open data sources like ORCID to improve the quality and the timeliness of our data. We will update Materials Map as soon as possible and kindly ask for your patience.

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Technical University of Denmark

in Cooperation with on an Cooperation-Score of 37%

Topics

Publications (4/4 displayed)

  • 2023Molecular insights into alginate β-lactoglobulin A multivalencies—The foundation for their amorphous aggregates and coacervation2citations
  • 2023Molecular insights into alginate β‐lactoglobulin A multivalencies – the foundation for their amorphous aggregates and coacervation2citations
  • 2023Molecular insights into alginate β‐lactoglobulin A multivalencies – the foundation for their amorphous aggregates and coacervation2citations
  • 2022Structure-function analysis of two closely related cutinases from Thermobifida cellulosilytica21citations

Places of action

Chart of shared publication
Svensson, Birte
3 / 3 shared
Aachmann, Finn Lillelund
1 / 1 shared
Tøndervik, Anne
3 / 3 shared
Peters, Günther H. J.
3 / 4 shared
Kragelund, Birthe B.
3 / 3 shared
Prestel, Andreas
3 / 3 shared
Madsen, Mikkel
2 / 2 shared
Sletta, Håvard
3 / 3 shared
Madland, Eva
3 / 3 shared
Aachmann, Finn L.
2 / 2 shared
Bååth, Jenny Arnling
1 / 1 shared
Novy, Vera
1 / 1 shared
Ribitsch, Doris
1 / 2 shared
Olsson, Lisbeth
1 / 2 shared
Carneiro, Leonor Vieira
1 / 1 shared
Guebitz, Georg M.
1 / 5 shared
Chart of publication period
2023
2022

Co-Authors (by relevance)

  • Svensson, Birte
  • Aachmann, Finn Lillelund
  • Tøndervik, Anne
  • Peters, Günther H. J.
  • Kragelund, Birthe B.
  • Prestel, Andreas
  • Madsen, Mikkel
  • Sletta, Håvard
  • Madland, Eva
  • Aachmann, Finn L.
  • Bååth, Jenny Arnling
  • Novy, Vera
  • Ribitsch, Doris
  • Olsson, Lisbeth
  • Carneiro, Leonor Vieira
  • Guebitz, Georg M.
OrganizationsLocationPeople

article

Structure-function analysis of two closely related cutinases from Thermobifida cellulosilytica

  • Bååth, Jenny Arnling
  • Novy, Vera
  • Ribitsch, Doris
  • Olsson, Lisbeth
  • Westh, Peter
  • Carneiro, Leonor Vieira
  • Guebitz, Georg M.
Abstract

Cutinases can play a significant role in a biotechnology-based circular economy. However, relatively little is known about the structure-function relationship of these enzymes, knowledge that is vital to advance optimized, engineered enzyme candidates. Here, two almost identical cutinases from <i>Thermobifida cellulosilytica</i> DSM44535 (ThcCut1 and ThcCut2) with only 18 amino acids difference were used for a rigorous biochemical characterization of their ability to hydrolyze PET, PET-model substrates, and cutin-model substrates. Kinetic parameters were compared with detailed <i>in-silico</i> docking studies of enzyme-ligand interactions. The two enzymes interacted with, and hydrolyzed PET differently, with ThcCut1 generating smaller PET-degradation products. ThcCut1 also showed higher catalytic efficiency on long-chain aliphatic substrates, an effect likely caused by small changes in the binding architecture. ThcCut2, in contrast, showed improved binding and catalytic efficiency when approaching the glass transition temperature of PET, an effect likely caused by longer amino acid residues in one area at the enzyme’s surface. Finally, the position of the single residue Q93 close to the active site, rotated out in ThcCut2, influenced the ligand position of a trimeric PET-model substrate. In conclusion, we illustrate that even minor sequence differences in cutinases can affect their substrate binding, substrate specificity, and catalytic efficiency drastically.

Topics
  • impedance spectroscopy
  • surface
  • glass
  • glass
  • glass transition temperature