A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level

Escherichia coli K–12 and B strains are among the most frequently used bacterial hosts for production of recombinant proteins on an industrial scale. To improve existing processes and to accelerate bioprocess development, we performed a detailed host analysis. We investigated the different behaviors...

Descripción completa

Detalles Bibliográficos
Autores principales: Marisch, Karoline, Bayer, Karl, Scharl, Theresa, Mairhofer, Juergen, Krempl, Peter M., Hummel, Karin, Razzazi-Fazeli, Ebrahim, Striedner, Gerald
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3738542/
https://www.ncbi.nlm.nih.gov/pubmed/23950949
http://dx.doi.org/10.1371/journal.pone.0070516
_version_ 1782476857835257856
author Marisch, Karoline
Bayer, Karl
Scharl, Theresa
Mairhofer, Juergen
Krempl, Peter M.
Hummel, Karin
Razzazi-Fazeli, Ebrahim
Striedner, Gerald
author_facet Marisch, Karoline
Bayer, Karl
Scharl, Theresa
Mairhofer, Juergen
Krempl, Peter M.
Hummel, Karin
Razzazi-Fazeli, Ebrahim
Striedner, Gerald
author_sort Marisch, Karoline
collection PubMed
description Escherichia coli K–12 and B strains are among the most frequently used bacterial hosts for production of recombinant proteins on an industrial scale. To improve existing processes and to accelerate bioprocess development, we performed a detailed host analysis. We investigated the different behaviors of the E. coli production strains BL21, RV308, and HMS174 in response to high-glucose concentrations. Tightly controlled cultivations were conducted under defined environmental conditions for the in-depth analysis of physiological behavior. In addition to acquisition of standard process parameters, we also used DNA microarray analysis and differential gel electrophoresis (Ettan(TM) DIGE). Batch cultivations showed different yields of the distinct strains for cell dry mass and growth rate, which were highest for BL21. In addition, production of acetate, triggered by excess glucose supply, was much higher for the K–12 strains compared to the B strain. Analysis of transcriptome data showed significant alteration in 347 of 3882 genes common among all three hosts. These differentially expressed genes included, for example, those involved in transport, iron acquisition, and motility. The investigation of proteome patterns additionally revealed a high number of differentially expressed proteins among the investigated hosts. The subsequently selected 38 spots included proteins involved in transport and motility. The results of this comprehensive analysis delivered a full genomic picture of the three investigated strains. Differentially expressed groups for targeted host modification were identified like glucose transport or iron acquisition, enabling potential optimization of strains to improve yield and process quality. Dissimilar growth profiles of the strains confirm different genotypes. Furthermore, distinct transcriptome patterns support differential regulation at the genome level. The identified proteins showed high agreement with the transcriptome data and suggest similar regulation within a host at both levels for the identified groups. Such host attributes need to be considered in future process design and operation.
format Online
Article
Text
id pubmed-3738542
institution National Center for Biotechnology Information
language English
publishDate 2013
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-37385422013-08-15 A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level Marisch, Karoline Bayer, Karl Scharl, Theresa Mairhofer, Juergen Krempl, Peter M. Hummel, Karin Razzazi-Fazeli, Ebrahim Striedner, Gerald PLoS One Research Article Escherichia coli K–12 and B strains are among the most frequently used bacterial hosts for production of recombinant proteins on an industrial scale. To improve existing processes and to accelerate bioprocess development, we performed a detailed host analysis. We investigated the different behaviors of the E. coli production strains BL21, RV308, and HMS174 in response to high-glucose concentrations. Tightly controlled cultivations were conducted under defined environmental conditions for the in-depth analysis of physiological behavior. In addition to acquisition of standard process parameters, we also used DNA microarray analysis and differential gel electrophoresis (Ettan(TM) DIGE). Batch cultivations showed different yields of the distinct strains for cell dry mass and growth rate, which were highest for BL21. In addition, production of acetate, triggered by excess glucose supply, was much higher for the K–12 strains compared to the B strain. Analysis of transcriptome data showed significant alteration in 347 of 3882 genes common among all three hosts. These differentially expressed genes included, for example, those involved in transport, iron acquisition, and motility. The investigation of proteome patterns additionally revealed a high number of differentially expressed proteins among the investigated hosts. The subsequently selected 38 spots included proteins involved in transport and motility. The results of this comprehensive analysis delivered a full genomic picture of the three investigated strains. Differentially expressed groups for targeted host modification were identified like glucose transport or iron acquisition, enabling potential optimization of strains to improve yield and process quality. Dissimilar growth profiles of the strains confirm different genotypes. Furthermore, distinct transcriptome patterns support differential regulation at the genome level. The identified proteins showed high agreement with the transcriptome data and suggest similar regulation within a host at both levels for the identified groups. Such host attributes need to be considered in future process design and operation. Public Library of Science 2013-08-08 /pmc/articles/PMC3738542/ /pubmed/23950949 http://dx.doi.org/10.1371/journal.pone.0070516 Text en © 2013 Marisch 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
Marisch, Karoline
Bayer, Karl
Scharl, Theresa
Mairhofer, Juergen
Krempl, Peter M.
Hummel, Karin
Razzazi-Fazeli, Ebrahim
Striedner, Gerald
A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title_full A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title_fullStr A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title_full_unstemmed A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title_short A Comparative Analysis of Industrial Escherichia coli K–12 and B Strains in High-Glucose Batch Cultivations on Process-, Transcriptome- and Proteome Level
title_sort comparative analysis of industrial escherichia coli k–12 and b strains in high-glucose batch cultivations on process-, transcriptome- and proteome level
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3738542/
https://www.ncbi.nlm.nih.gov/pubmed/23950949
http://dx.doi.org/10.1371/journal.pone.0070516
work_keys_str_mv AT marischkaroline acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT bayerkarl acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT scharltheresa acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT mairhoferjuergen acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT kremplpeterm acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT hummelkarin acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT razzazifazeliebrahim acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT striednergerald acomparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT marischkaroline comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT bayerkarl comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT scharltheresa comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT mairhoferjuergen comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT kremplpeterm comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT hummelkarin comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT razzazifazeliebrahim comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel
AT striednergerald comparativeanalysisofindustrialescherichiacolik12andbstrainsinhighglucosebatchcultivationsonprocesstranscriptomeandproteomelevel

Ejemplares similares