Dual-Fluorescence Chromosome-Located Labeling System for Accurate In Vivo Single-Cell Gene Expression Analysis in Pseudomonas syringae.

dc.centroFacultad de Cienciases_ES
dc.contributor.authorLópez-Pagán, Nieves
dc.contributor.authorRufián, José S.
dc.contributor.authorRuiz-Albert, Francisco Javier
dc.contributor.authorBeuzón-López, Carmen del Rosario
dc.date.accessioned2025-01-30T12:28:13Z
dc.date.available2025-01-30T12:28:13Z
dc.date.issued2024-01-25
dc.departamentoBiología Celular, Genética y Fisiología
dc.descriptionhttps://www.springernature.com/gp/open-science/policies/book-policieses_ES
dc.description.abstractEpigenetic regulation as a means for bacterial adaptation is receiving increasing interest in the last decade. Significant efforts have been directed towards understanding the mechanisms giving raise to phenotypic heterogeneity within bacterial populations and its adaptive relevance. Phenotypic heterogeneity mostly refers to phenotypic variation not linked to genetic differences nor to environmental stimuli. Recent findings on the relevance of phenotypic heterogeneity on some bacterial complex traits are causing a shift from traditional assays where bacterial phenotypes are defined by averaging population-level data, to single-cell analysis that focus on bacterial individual behavior within the population. Fluorescent labeling is a key asset for single-cell gene expression analysis using flow cytometry, fluorescence microscopy, and/or microfluidics. We previously described the generation of chromosome-located transcriptional gene fusions to fluores-cent reporter genes using the model bacterial plant pathogen Pseudomonas syringae. These fusions allow researchers to follow variation in expression of the gene(s) of interest, without affecting gene function. In this report, we improve the analytic power of the method by combining such transcriptional fusions with constitutively expressed compatible fluorescent reporter genes integrated in a second, neutral locus of the bacterial chromosome. Constitutively expressed fluorescent reporters allow for the detection of all bacteria comprising a heterogeneous population, regardless of the level of expression of the concurrently monitored gene of interest, thus avoiding the traditional use of stains often incompatible with samples from complex contexts such as the leaf.es_ES
dc.description.sponsorshipGrants RTI2018-095069-B-I00 and PID2021-127245OB-100 funded by MCIN/AEI/10.13039/ 501100011033/ and by “ERDF A way of making Europe” Grant PY18-2398 funded by Plan Andaluz de Investigación, Desarrollo e Innovación (PAIDI 2020) Plan Andaluz de Investigación, Desarrollo e Innovación (PAIDI 2020)es_ES
dc.identifier.citationLópez-Pagán N, Rufián JS, Ruiz-Albert J, Beuzón CR. Dual-Fluorescence Chromosome-Located Labeling System for Accurate In Vivo Single-Cell Gene Expression Analysis in Pseudomonas syringae. Methods Mol Biol. 2024;2751:95-114es_ES
dc.identifier.doi10.1007/978-1-0716-3617-6_7
dc.identifier.urihttps://hdl.handle.net/10630/37408
dc.language.isoenges_ES
dc.publisherHumana Press (Springer Group)es_ES
dc.rights.accessRightsopen accesses_ES
dc.subjectGenéticaes_ES
dc.subjectMutación (Biología)es_ES
dc.subjectMicroscopía de fluorescenciaes_ES
dc.subjectCitometría de flujoes_ES
dc.subject.otherPhenotypic heterogeneityes_ES
dc.subject.otherGene expressiones_ES
dc.subject.otherFluorescent reporter geneses_ES
dc.subject.otherSingle-cell methodses_ES
dc.subject.otherFluorescence microscopyes_ES
dc.subject.otherNon-genetic variationes_ES
dc.subject.otherFlow cytometryes_ES
dc.titleDual-Fluorescence Chromosome-Located Labeling System for Accurate In Vivo Single-Cell Gene Expression Analysis in Pseudomonas syringae.es_ES
dc.typebook partes_ES
dc.type.hasVersionAMes_ES
dspace.entity.typePublication
relation.isAuthorOfPublication8e7d1c39-da6b-48be-9823-0767bf0215ec
relation.isAuthorOfPublication94562a8b-1a61-4c3e-88fc-ea3c8af99511
relation.isAuthorOfPublication.latestForDiscovery8e7d1c39-da6b-48be-9823-0767bf0215ec

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