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Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations

Microbial cells experience physiological changes due to environmental change, such as pH and temperature, the release of bactericidal agents, or nutrient limitation. This has been shown to affect community assembly and physiological processes (e.g., stress tolerance, virulence, or cellular metabolic...

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Autores principales: García-Timermans, Cristina, Props, Ruben, Zacchetti, Boris, Sakarika, Myrsini, Delvigne, Frank, Boon, Nico
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Microbiology 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7593600/
https://www.ncbi.nlm.nih.gov/pubmed/33115836
http://dx.doi.org/10.1128/mSphere.00806-20
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author García-Timermans, Cristina
Props, Ruben
Zacchetti, Boris
Sakarika, Myrsini
Delvigne, Frank
Boon, Nico
author_facet García-Timermans, Cristina
Props, Ruben
Zacchetti, Boris
Sakarika, Myrsini
Delvigne, Frank
Boon, Nico
author_sort García-Timermans, Cristina
collection PubMed
description Microbial cells experience physiological changes due to environmental change, such as pH and temperature, the release of bactericidal agents, or nutrient limitation. This has been shown to affect community assembly and physiological processes (e.g., stress tolerance, virulence, or cellular metabolic activity). Metabolic stress is typically quantified by measuring community phenotypic properties such as biomass growth, reactive oxygen species, or cell permeability. However, bulk community measurements do not take into account single-cell phenotypic diversity, which is important for a better understanding and the subsequent management of microbial populations. Raman spectroscopy is a nondestructive alternative that provides detailed information on the biochemical makeup of each individual cell. Here, we introduce a method for describing single-cell phenotypic diversity using the Hill diversity framework of Raman spectra. Using the biomolecular profile of individual cells, we obtained a metric to compare cellular states and used it to study stress-induced changes. First, in two Escherichia coli populations either treated with ethanol or nontreated and then in two Saccharomyces cerevisiae subpopulations with either high or low expression of a stress reporter. In both cases, we were able to quantify single-cell phenotypic diversity and to discriminate metabolically stressed cells using a clustering algorithm. We also described how the lipid, protein, and nucleic acid compositions changed after the exposure to the stressor using information from the Raman spectra. Our results show that Raman spectroscopy delivers the necessary resolution to quantify phenotypic diversity within individual cells and that this information can be used to study stress-driven metabolic diversity in microbial populations. IMPORTANCE Microbial cells that live in the same community can exist in different physiological and morphological states that change as a function of spatiotemporal variations in environmental conditions. This phenomenon is commonly known as phenotypic heterogeneity and/or diversity. Measuring this plethora of cellular expressions is needed to better understand and manage microbial processes. However, most tools to study phenotypic diversity only average the behavior of the sampled community. In this work, we present a way to quantify the phenotypic diversity of microbial samples by inferring the (bio)molecular profile of its constituent cells using Raman spectroscopy. We demonstrate how this tool can be used to quantify the phenotypic diversity that arises after the exposure of microbes to stress. Raman spectroscopy holds potential for the detection of stressed cells in bioproduction.
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spelling pubmed-75936002020-11-06 Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations García-Timermans, Cristina Props, Ruben Zacchetti, Boris Sakarika, Myrsini Delvigne, Frank Boon, Nico mSphere Research Article Microbial cells experience physiological changes due to environmental change, such as pH and temperature, the release of bactericidal agents, or nutrient limitation. This has been shown to affect community assembly and physiological processes (e.g., stress tolerance, virulence, or cellular metabolic activity). Metabolic stress is typically quantified by measuring community phenotypic properties such as biomass growth, reactive oxygen species, or cell permeability. However, bulk community measurements do not take into account single-cell phenotypic diversity, which is important for a better understanding and the subsequent management of microbial populations. Raman spectroscopy is a nondestructive alternative that provides detailed information on the biochemical makeup of each individual cell. Here, we introduce a method for describing single-cell phenotypic diversity using the Hill diversity framework of Raman spectra. Using the biomolecular profile of individual cells, we obtained a metric to compare cellular states and used it to study stress-induced changes. First, in two Escherichia coli populations either treated with ethanol or nontreated and then in two Saccharomyces cerevisiae subpopulations with either high or low expression of a stress reporter. In both cases, we were able to quantify single-cell phenotypic diversity and to discriminate metabolically stressed cells using a clustering algorithm. We also described how the lipid, protein, and nucleic acid compositions changed after the exposure to the stressor using information from the Raman spectra. Our results show that Raman spectroscopy delivers the necessary resolution to quantify phenotypic diversity within individual cells and that this information can be used to study stress-driven metabolic diversity in microbial populations. IMPORTANCE Microbial cells that live in the same community can exist in different physiological and morphological states that change as a function of spatiotemporal variations in environmental conditions. This phenomenon is commonly known as phenotypic heterogeneity and/or diversity. Measuring this plethora of cellular expressions is needed to better understand and manage microbial processes. However, most tools to study phenotypic diversity only average the behavior of the sampled community. In this work, we present a way to quantify the phenotypic diversity of microbial samples by inferring the (bio)molecular profile of its constituent cells using Raman spectroscopy. We demonstrate how this tool can be used to quantify the phenotypic diversity that arises after the exposure of microbes to stress. Raman spectroscopy holds potential for the detection of stressed cells in bioproduction. American Society for Microbiology 2020-10-28 /pmc/articles/PMC7593600/ /pubmed/33115836 http://dx.doi.org/10.1128/mSphere.00806-20 Text en Copyright © 2020 García-Timermans et al. https://creativecommons.org/licenses/by/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Research Article
García-Timermans, Cristina
Props, Ruben
Zacchetti, Boris
Sakarika, Myrsini
Delvigne, Frank
Boon, Nico
Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title_full Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title_fullStr Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title_full_unstemmed Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title_short Raman Spectroscopy-Based Measurements of Single-Cell Phenotypic Diversity in Microbial Populations
title_sort raman spectroscopy-based measurements of single-cell phenotypic diversity in microbial populations
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7593600/
https://www.ncbi.nlm.nih.gov/pubmed/33115836
http://dx.doi.org/10.1128/mSphere.00806-20
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