Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1

Leuconostoc lactis AV1 strain isolated from a Tunisian avocado was characterized as a dextran producer. The promoter P(dsrLL) and the dsrLL gene encoding the DsrLL dextransucrase responsible for the dextran synthesis were transcriptionally fused to the mCherry coding gene generating the pRCR20 plasm...

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Autores principales: Besrour-Aouam, Norhane, Mohedano, Maria Luz, Fhoula, Imene, Zarour, Kenza, Najjari, Afef, Aznar, Rosa, Prieto, Alicia, Ouzari, Hadda-Imene, López, Paloma
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2019
Materias:
Microbiology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6513889/
https://www.ncbi.nlm.nih.gov/pubmed/31134012
http://dx.doi.org/10.3389/fmicb.2019.00959
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author Besrour-Aouam, Norhane
Mohedano, Maria Luz
Fhoula, Imene
Zarour, Kenza
Najjari, Afef
Aznar, Rosa
Prieto, Alicia
Ouzari, Hadda-Imene
López, Paloma
author_facet Besrour-Aouam, Norhane
Mohedano, Maria Luz
Fhoula, Imene
Zarour, Kenza
Najjari, Afef
Aznar, Rosa
Prieto, Alicia
Ouzari, Hadda-Imene
López, Paloma
author_sort Besrour-Aouam, Norhane
collection PubMed
description Leuconostoc lactis AV1 strain isolated from a Tunisian avocado was characterized as a dextran producer. The promoter P(dsrLL) and the dsrLL gene encoding the DsrLL dextransucrase responsible for the dextran synthesis were transcriptionally fused to the mCherry coding gene generating the pRCR20 plasmid. Upon plasmid transfer, both AV1n and the dextran non-producing Leuconostoc mesenteroides CM70 became red due to expression of the mCherry from the P(dsrLL)-dsr-mrfp transcriptional fusion. Characterization of the polymers present in cultures supernatants revealed that the DsrLL encoded from pRCR20 in the recombinant bacteria was able to synthesize dextran. The production of dextran by the DsrLL in AV1n increased in response to low temperature, reaching 10-fold higher levels at 20°C than at 37°C (4.15 g/L versus 0.41 g/L). To analyze if this stress response includes activation at the transcriptional level and if it was only restricted to Leuconostoc, AV1n was transformed with plasmids carrying either the P(dsrLL)-mrfp fusion or the P(dsrLS) of Lactobacillus sakei MN1 fused to the mrfp gene, and the influence of temperature and carbon source on expression from the Dsr promoters was monitored by measurement of the mCherry levels. The overall expression analysis confirmed an induction of expression from P(dsrLL) upon growth at low temperature (20°C versus 30°C and 37°C) in the presence of sugars tested (sucrose, glucose, maltose, and fructose). In addition, the presence of sucrose, the substrate of Dsr, also resulted in activation of expression from P(dsrLL). A different behavior was detected, when expression from P(dsrLS) was evaluated. Similar levels of fluorescence were observed irrespectively of the carbon source or temperature, besides a sequential decrease at 30°C and 20°C, when sucrose was present in the growth medium. In conclusion, the two types of regulation of expression of Dsr presented here revealed two different mechanisms for environmental adaptation of Leuconostoc and Lactobacillus that could be exploited for industrial applications.
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spelling pubmed-65138892019-05-27 Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1 Besrour-Aouam, Norhane Mohedano, Maria Luz Fhoula, Imene Zarour, Kenza Najjari, Afef Aznar, Rosa Prieto, Alicia Ouzari, Hadda-Imene López, Paloma Front Microbiol Microbiology Leuconostoc lactis AV1 strain isolated from a Tunisian avocado was characterized as a dextran producer. The promoter P(dsrLL) and the dsrLL gene encoding the DsrLL dextransucrase responsible for the dextran synthesis were transcriptionally fused to the mCherry coding gene generating the pRCR20 plasmid. Upon plasmid transfer, both AV1n and the dextran non-producing Leuconostoc mesenteroides CM70 became red due to expression of the mCherry from the P(dsrLL)-dsr-mrfp transcriptional fusion. Characterization of the polymers present in cultures supernatants revealed that the DsrLL encoded from pRCR20 in the recombinant bacteria was able to synthesize dextran. The production of dextran by the DsrLL in AV1n increased in response to low temperature, reaching 10-fold higher levels at 20°C than at 37°C (4.15 g/L versus 0.41 g/L). To analyze if this stress response includes activation at the transcriptional level and if it was only restricted to Leuconostoc, AV1n was transformed with plasmids carrying either the P(dsrLL)-mrfp fusion or the P(dsrLS) of Lactobacillus sakei MN1 fused to the mrfp gene, and the influence of temperature and carbon source on expression from the Dsr promoters was monitored by measurement of the mCherry levels. The overall expression analysis confirmed an induction of expression from P(dsrLL) upon growth at low temperature (20°C versus 30°C and 37°C) in the presence of sugars tested (sucrose, glucose, maltose, and fructose). In addition, the presence of sucrose, the substrate of Dsr, also resulted in activation of expression from P(dsrLL). A different behavior was detected, when expression from P(dsrLS) was evaluated. Similar levels of fluorescence were observed irrespectively of the carbon source or temperature, besides a sequential decrease at 30°C and 20°C, when sucrose was present in the growth medium. In conclusion, the two types of regulation of expression of Dsr presented here revealed two different mechanisms for environmental adaptation of Leuconostoc and Lactobacillus that could be exploited for industrial applications. Frontiers Media S.A. 2019-05-07 /pmc/articles/PMC6513889/ /pubmed/31134012 http://dx.doi.org/10.3389/fmicb.2019.00959 Text en Copyright © 2019 Besrour-Aouam, Mohedano, Fhoula, Zarour, Najjari, Aznar, Prieto, Ouzari and López. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Microbiology
Besrour-Aouam, Norhane
Mohedano, Maria Luz
Fhoula, Imene
Zarour, Kenza
Najjari, Afef
Aznar, Rosa
Prieto, Alicia
Ouzari, Hadda-Imene
López, Paloma
Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title_full Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title_fullStr Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title_full_unstemmed Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title_short Different Modes of Regulation of the Expression of Dextransucrase in Leuconostoc lactis AV1n and Lactobacillus sakei MN1
title_sort different modes of regulation of the expression of dextransucrase in leuconostoc lactis av1n and lactobacillus sakei mn1
topic Microbiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6513889/
https://www.ncbi.nlm.nih.gov/pubmed/31134012
http://dx.doi.org/10.3389/fmicb.2019.00959
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