Promoter knock-in: a novel rational method for the fine tuning of genes

BACKGROUND: Metabolic engineering aims at channeling the metabolic fluxes towards a desired compound. An important strategy to achieve this is the modification of the expression level of specific genes. Several methods for the modification or the replacement of promoters have been proposed, but most...

Descripción completa

Detalles Bibliográficos
Autores principales: De Mey, Marjan, Maertens, Jo, Boogmans, Sarah, Soetaert, Wim K, Vandamme, Erick J, Cunin, Raymond, Foulquié-Moreno, Maria R
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Methodology article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2858092/
https://www.ncbi.nlm.nih.gov/pubmed/20334648
http://dx.doi.org/10.1186/1472-6750-10-26
_version_ 1782180380146663424
author De Mey, Marjan
Maertens, Jo
Boogmans, Sarah
Soetaert, Wim K
Vandamme, Erick J
Cunin, Raymond
Foulquié-Moreno, Maria R
author_facet De Mey, Marjan
Maertens, Jo
Boogmans, Sarah
Soetaert, Wim K
Vandamme, Erick J
Cunin, Raymond
Foulquié-Moreno, Maria R
author_sort De Mey, Marjan
collection PubMed
description BACKGROUND: Metabolic engineering aims at channeling the metabolic fluxes towards a desired compound. An important strategy to achieve this is the modification of the expression level of specific genes. Several methods for the modification or the replacement of promoters have been proposed, but most of them involve time-consuming screening steps. We describe here a novel optimized method for the insertion of constitutive promoters (referred to as "promoter knock-in") whose strength can be compared with the native promoter by applying a promoter strength predictive (PSP) model. RESULTS: Our method was successfully applied to fine tune the ppc gene of Escherichia coli. While developing the promoter knock-in methodology, we showed the importance of conserving the natural leader region containing the ribosome binding site (RBS) of the gene of interest and of eliminating upstream regulatory elements (transcription factor binding sites). The gene expression was down regulated instead of up regulated when the natural RBS was not conserved and when the upstream regulatory elements were eliminated. Next, three different promoter knock-ins were created for the ppc gene selecting three different artificial promoters. The measured constitutive expression of the ppc gene in these knock-ins reflected the relative strength of the different promoters as predicted by the PSP model. The applicability of our PSP model and promoter knock-in methodology was further demonstrated by showing that the constitutivity and the relative levels of expression were independent of the genetic background (comparing wild-type and mutant E. coli strains). No differences were observed during scaling up from shake flask to bioreactor-scale, confirming that the obtained expression was independent of environmental conditions. CONCLUSION: We are proposing a novel methodology for obtaining appropriate levels of expression of genes of interest, based on the prediction of the relative strength of selected synthetic promoters combined with an optimized promoter knock-in strategy. The obtained expression levels are independent of the genetic background and scale conditions. The method constitutes therefore a valuable addition to the genetic toolbox for the metabolic engineering of E. coli.
format Text
id pubmed-2858092
institution National Center for Biotechnology Information
language English
publishDate 2010
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-28580922010-04-22 Promoter knock-in: a novel rational method for the fine tuning of genes De Mey, Marjan Maertens, Jo Boogmans, Sarah Soetaert, Wim K Vandamme, Erick J Cunin, Raymond Foulquié-Moreno, Maria R BMC Biotechnol Methodology article BACKGROUND: Metabolic engineering aims at channeling the metabolic fluxes towards a desired compound. An important strategy to achieve this is the modification of the expression level of specific genes. Several methods for the modification or the replacement of promoters have been proposed, but most of them involve time-consuming screening steps. We describe here a novel optimized method for the insertion of constitutive promoters (referred to as "promoter knock-in") whose strength can be compared with the native promoter by applying a promoter strength predictive (PSP) model. RESULTS: Our method was successfully applied to fine tune the ppc gene of Escherichia coli. While developing the promoter knock-in methodology, we showed the importance of conserving the natural leader region containing the ribosome binding site (RBS) of the gene of interest and of eliminating upstream regulatory elements (transcription factor binding sites). The gene expression was down regulated instead of up regulated when the natural RBS was not conserved and when the upstream regulatory elements were eliminated. Next, three different promoter knock-ins were created for the ppc gene selecting three different artificial promoters. The measured constitutive expression of the ppc gene in these knock-ins reflected the relative strength of the different promoters as predicted by the PSP model. The applicability of our PSP model and promoter knock-in methodology was further demonstrated by showing that the constitutivity and the relative levels of expression were independent of the genetic background (comparing wild-type and mutant E. coli strains). No differences were observed during scaling up from shake flask to bioreactor-scale, confirming that the obtained expression was independent of environmental conditions. CONCLUSION: We are proposing a novel methodology for obtaining appropriate levels of expression of genes of interest, based on the prediction of the relative strength of selected synthetic promoters combined with an optimized promoter knock-in strategy. The obtained expression levels are independent of the genetic background and scale conditions. The method constitutes therefore a valuable addition to the genetic toolbox for the metabolic engineering of E. coli. BioMed Central 2010-03-24 /pmc/articles/PMC2858092/ /pubmed/20334648 http://dx.doi.org/10.1186/1472-6750-10-26 Text en Copyright ©2010 De Mey et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology article
De Mey, Marjan
Maertens, Jo
Boogmans, Sarah
Soetaert, Wim K
Vandamme, Erick J
Cunin, Raymond
Foulquié-Moreno, Maria R
Promoter knock-in: a novel rational method for the fine tuning of genes
title Promoter knock-in: a novel rational method for the fine tuning of genes
title_full Promoter knock-in: a novel rational method for the fine tuning of genes
title_fullStr Promoter knock-in: a novel rational method for the fine tuning of genes
title_full_unstemmed Promoter knock-in: a novel rational method for the fine tuning of genes
title_short Promoter knock-in: a novel rational method for the fine tuning of genes
title_sort promoter knock-in: a novel rational method for the fine tuning of genes
topic Methodology article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2858092/
https://www.ncbi.nlm.nih.gov/pubmed/20334648
http://dx.doi.org/10.1186/1472-6750-10-26
work_keys_str_mv AT demeymarjan promoterknockinanovelrationalmethodforthefinetuningofgenes
AT maertensjo promoterknockinanovelrationalmethodforthefinetuningofgenes
AT boogmanssarah promoterknockinanovelrationalmethodforthefinetuningofgenes
AT soetaertwimk promoterknockinanovelrationalmethodforthefinetuningofgenes
AT vandammeerickj promoterknockinanovelrationalmethodforthefinetuningofgenes
AT cuninraymond promoterknockinanovelrationalmethodforthefinetuningofgenes
AT foulquiemorenomariar promoterknockinanovelrationalmethodforthefinetuningofgenes

Ejemplares similares