Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter

Biomaterials-associated infections are primarily initiated by the adhesion of microorganisms on the biomaterial surfaces and subsequent biofilm formation. Understanding the fundamental microbial adhesion mechanisms and biofilm development is crucial for developing strategies to prevent such infectio...

Descripción completa

Detalles Bibliográficos
Autores principales: Lüdecke, Claudia, Jandt, Klaus D., Siegismund, Daniel, Kujau, Marian J., Zang, Emerson, Rettenmayr, Markus, Bossert, Jörg, Roth, Martin
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2014
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3880331/
https://www.ncbi.nlm.nih.gov/pubmed/24404192
http://dx.doi.org/10.1371/journal.pone.0084837
_version_ 1782298072818122752
author Lüdecke, Claudia
Jandt, Klaus D.
Siegismund, Daniel
Kujau, Marian J.
Zang, Emerson
Rettenmayr, Markus
Bossert, Jörg
Roth, Martin
author_facet Lüdecke, Claudia
Jandt, Klaus D.
Siegismund, Daniel
Kujau, Marian J.
Zang, Emerson
Rettenmayr, Markus
Bossert, Jörg
Roth, Martin
author_sort Lüdecke, Claudia
collection PubMed
description Biomaterials-associated infections are primarily initiated by the adhesion of microorganisms on the biomaterial surfaces and subsequent biofilm formation. Understanding the fundamental microbial adhesion mechanisms and biofilm development is crucial for developing strategies to prevent such infections. Suitable in vitro systems for biofilm cultivation and bacterial adhesion at controllable, constant and reproducible conditions are indispensable. This study aimed (i) to modify the previously described constant-depth film fermenter for the reproducible cultivation of biofilms at non-depth-restricted, constant and low shear conditions and (ii) to use this system to elucidate bacterial adhesion kinetics on different biomaterials, focusing on biomaterials surface nanoroughness and hydrophobicity. Chemostat-grown Escherichia coli were used for biofilm cultivation on titanium oxide and investigating bacterial adhesion over time on titanium oxide, poly(styrene), poly(tetrafluoroethylene) and glass. Using chemostat-grown microbial cells (single-species continuous culture) minimized variations between the biofilms cultivated during different experimental runs. Bacterial adhesion on biomaterials comprised an initial lag-phase I followed by a fast adhesion phase II and a phase of saturation III. With increasing biomaterials surface nanoroughness and increasing hydrophobicity, adhesion rates increased during phases I and II. The influence of materials surface hydrophobicity seemed to exceed that of nanoroughness during the lag-phase I, whereas it was vice versa during adhesion phase II. This study introduces the non-constant-depth film fermenter in combination with a chemostat culture to allow for a controlled approach to reproducibly cultivate biofilms and to investigate bacterial adhesion kinetics at constant and low shear conditions. The findings will support developing and adequate testing of biomaterials surface modifications eventually preventing biomaterial-associated infections.
format Online
Article
Text
id pubmed-3880331
institution National Center for Biotechnology Information
language English
publishDate 2014
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-38803312014-01-08 Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter Lüdecke, Claudia Jandt, Klaus D. Siegismund, Daniel Kujau, Marian J. Zang, Emerson Rettenmayr, Markus Bossert, Jörg Roth, Martin PLoS One Research Article Biomaterials-associated infections are primarily initiated by the adhesion of microorganisms on the biomaterial surfaces and subsequent biofilm formation. Understanding the fundamental microbial adhesion mechanisms and biofilm development is crucial for developing strategies to prevent such infections. Suitable in vitro systems for biofilm cultivation and bacterial adhesion at controllable, constant and reproducible conditions are indispensable. This study aimed (i) to modify the previously described constant-depth film fermenter for the reproducible cultivation of biofilms at non-depth-restricted, constant and low shear conditions and (ii) to use this system to elucidate bacterial adhesion kinetics on different biomaterials, focusing on biomaterials surface nanoroughness and hydrophobicity. Chemostat-grown Escherichia coli were used for biofilm cultivation on titanium oxide and investigating bacterial adhesion over time on titanium oxide, poly(styrene), poly(tetrafluoroethylene) and glass. Using chemostat-grown microbial cells (single-species continuous culture) minimized variations between the biofilms cultivated during different experimental runs. Bacterial adhesion on biomaterials comprised an initial lag-phase I followed by a fast adhesion phase II and a phase of saturation III. With increasing biomaterials surface nanoroughness and increasing hydrophobicity, adhesion rates increased during phases I and II. The influence of materials surface hydrophobicity seemed to exceed that of nanoroughness during the lag-phase I, whereas it was vice versa during adhesion phase II. This study introduces the non-constant-depth film fermenter in combination with a chemostat culture to allow for a controlled approach to reproducibly cultivate biofilms and to investigate bacterial adhesion kinetics at constant and low shear conditions. The findings will support developing and adequate testing of biomaterials surface modifications eventually preventing biomaterial-associated infections. Public Library of Science 2014-01-03 /pmc/articles/PMC3880331/ /pubmed/24404192 http://dx.doi.org/10.1371/journal.pone.0084837 Text en © 2014 Lüdecke et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Lüdecke, Claudia
Jandt, Klaus D.
Siegismund, Daniel
Kujau, Marian J.
Zang, Emerson
Rettenmayr, Markus
Bossert, Jörg
Roth, Martin
Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title_full Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title_fullStr Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title_full_unstemmed Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title_short Reproducible Biofilm Cultivation of Chemostat-Grown Escherichia coli and Investigation of Bacterial Adhesion on Biomaterials Using a Non-Constant-Depth Film Fermenter
title_sort reproducible biofilm cultivation of chemostat-grown escherichia coli and investigation of bacterial adhesion on biomaterials using a non-constant-depth film fermenter
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3880331/
https://www.ncbi.nlm.nih.gov/pubmed/24404192
http://dx.doi.org/10.1371/journal.pone.0084837
work_keys_str_mv AT ludeckeclaudia reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT jandtklausd reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT siegismunddaniel reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT kujaumarianj reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT zangemerson reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT rettenmayrmarkus reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT bossertjorg reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter
AT rothmartin reproduciblebiofilmcultivationofchemostatgrownescherichiacoliandinvestigationofbacterialadhesiononbiomaterialsusinganonconstantdepthfilmfermenter

Ejemplares similares