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Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response

[Image: see text] An automated and straightforward detection and data treatment strategy for the determination of the protein relative concentration in individual human cells by single cell–inductively coupled plasma–time-of-flight mass spectrometry (sc-ICP-ToF-MS) is proposed. Metal nanocluster (NC...

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Autores principales: Menero-Valdés, Paula, Chronakis, Michail I., Fernández, Beatriz, Quarles, C. Derrick, González-Iglesias, Héctor, Meermann, Björn, Pereiro, Rosario
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2023
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10483461/
https://www.ncbi.nlm.nih.gov/pubmed/37566513
http://dx.doi.org/10.1021/acs.analchem.3c02558
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author Menero-Valdés, Paula
Chronakis, Michail I.
Fernández, Beatriz
Quarles, C. Derrick
González-Iglesias, Héctor
Meermann, Björn
Pereiro, Rosario
author_facet Menero-Valdés, Paula
Chronakis, Michail I.
Fernández, Beatriz
Quarles, C. Derrick
González-Iglesias, Héctor
Meermann, Björn
Pereiro, Rosario
author_sort Menero-Valdés, Paula
collection PubMed
description [Image: see text] An automated and straightforward detection and data treatment strategy for the determination of the protein relative concentration in individual human cells by single cell–inductively coupled plasma–time-of-flight mass spectrometry (sc-ICP-ToF-MS) is proposed. Metal nanocluster (NC)-labeled specific antibodies for the target proteins were employed, and ruthenium red (RR) staining, which binds to the cells surface, was used to determine the number of cell events as well as to evaluate the relative volume of the cells. As a proof of concept, the expression of hepcidin, metallothionein-2, and ferroportin employing specific antibodies labeled with IrNCs, PtNCs, and AuNCs, respectively, was investigated by sc-ICP-ToF-MS in human ARPE-19 cells. Taking into account that ARPE-19 cells are spherical in suspension and RR binds to the surface of the cells, the Ru intensity was related to the cell volume (i.e., the cell volume is directly proportional to (Ru intensity)(3/2)), making it possible to determine not only the mass of the target proteins in each individual cell but also the relative concentration. The proposed approach is of particular interest in comparing cell cultures subjected to different supplementations. ARPE-19 cell cultures under two stress conditions were compared: a hyperglycemic model and an oxidative stress model. The comparison of the control with treated cells shows not only the mass of analyzed species but also the relative changes in the cell volume and concentration of target proteins, clearly allowing the identification of subpopulations under the respective treatment.
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spelling pubmed-104834612023-09-08 Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response Menero-Valdés, Paula Chronakis, Michail I. Fernández, Beatriz Quarles, C. Derrick González-Iglesias, Héctor Meermann, Björn Pereiro, Rosario Anal Chem [Image: see text] An automated and straightforward detection and data treatment strategy for the determination of the protein relative concentration in individual human cells by single cell–inductively coupled plasma–time-of-flight mass spectrometry (sc-ICP-ToF-MS) is proposed. Metal nanocluster (NC)-labeled specific antibodies for the target proteins were employed, and ruthenium red (RR) staining, which binds to the cells surface, was used to determine the number of cell events as well as to evaluate the relative volume of the cells. As a proof of concept, the expression of hepcidin, metallothionein-2, and ferroportin employing specific antibodies labeled with IrNCs, PtNCs, and AuNCs, respectively, was investigated by sc-ICP-ToF-MS in human ARPE-19 cells. Taking into account that ARPE-19 cells are spherical in suspension and RR binds to the surface of the cells, the Ru intensity was related to the cell volume (i.e., the cell volume is directly proportional to (Ru intensity)(3/2)), making it possible to determine not only the mass of the target proteins in each individual cell but also the relative concentration. The proposed approach is of particular interest in comparing cell cultures subjected to different supplementations. ARPE-19 cell cultures under two stress conditions were compared: a hyperglycemic model and an oxidative stress model. The comparison of the control with treated cells shows not only the mass of analyzed species but also the relative changes in the cell volume and concentration of target proteins, clearly allowing the identification of subpopulations under the respective treatment. American Chemical Society 2023-08-11 /pmc/articles/PMC10483461/ /pubmed/37566513 http://dx.doi.org/10.1021/acs.analchem.3c02558 Text en © 2023 The Authors. Published by American Chemical Society https://creativecommons.org/licenses/by/4.0/Permits the broadest form of re-use including for commercial purposes, provided that author attribution and integrity are maintained (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Menero-Valdés, Paula
Chronakis, Michail I.
Fernández, Beatriz
Quarles, C. Derrick
González-Iglesias, Héctor
Meermann, Björn
Pereiro, Rosario
Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title_full Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title_fullStr Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title_full_unstemmed Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title_short Single Cell–ICP–ToF-MS for the Multiplexed Determination of Proteins: Evaluation of the Cellular Stress Response
title_sort single cell–icp–tof-ms for the multiplexed determination of proteins: evaluation of the cellular stress response
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10483461/
https://www.ncbi.nlm.nih.gov/pubmed/37566513
http://dx.doi.org/10.1021/acs.analchem.3c02558
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