Single Cell In Situ Detection and Quantification of Metal Oxide Nanoparticles Using Multimodal Correlative Microscopy

Assessing in situ nanoparticles (NPs) internalization at the level of a single cell is a difficult but critical task due to their potential use in nanomedicine. One of the main actual challenges is to control the number of internalized NPs per cell. To in situ detect, track, and above all quantify N...

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Veröffentlicht in:	Analytical chemistry (Washington) 2014-08, Vol.86 (15), p.7311-7319
Hauptverfasser:	Le Trequesser, Quentin, Devès, Guillaume, Saez, Gladys, Daudin, Laurent, Barberet, Philippe, Michelet, Claire, Delville, Marie-Hélène, Seznec, Hervé
Format:	Artikel
Sprache:	eng
Schlagworte:	Analytical chemistry Analytical techniques Biochemistry Cells Chemical Sciences Correlation Dyes Fluorescence Material chemistry Metal Nanoparticles Microscopy Microscopy - methods Nanoparticles Nanostructure Oxides - chemistry Scanning electron microscopy Single-Cell Analysis Toxicology
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container_title	Analytical chemistry (Washington)
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creator	Le Trequesser, Quentin Devès, Guillaume Saez, Gladys Daudin, Laurent Barberet, Philippe Michelet, Claire Delville, Marie-Hélène Seznec, Hervé
description	Assessing in situ nanoparticles (NPs) internalization at the level of a single cell is a difficult but critical task due to their potential use in nanomedicine. One of the main actual challenges is to control the number of internalized NPs per cell. To in situ detect, track, and above all quantify NPs in a single cell, we propose an approach based on a multimodal correlative microscopy (MCM), via the complementarity of three imaging techniques: fluorescence microscopy (FM), scanning electron microscopy (SEM), and ion beam analysis (IBA). This MCM was performed on single targeted individual primary human foreskin keratinocytes (PHFK) cells cultured and maintained on a specifically designed sample holder, to probe either dye-modified or bare NPs. The data obtained by both FM and IBA on dye-modified NPs were strongly correlated in terms of detection, tracking, and colocalization of fluorescence and metal detection. IBA techniques should therefore open a new field concerning specific studies on bare NPs and their toxicological impact on cells. Complementarity of SEM and IBA analyses provides surface (SEM) and in depth (IBA) information on the cell morphology as well as on the exact localization of the NPs. Finally, IBA not only provides in a single cell the in situ quantification of exogenous elements (NPs) but also that all the other endogenous elements and the subsequent variation of their homeostasis. This unique feature opens further insights in dose-dependent response analyses and adds the perspective of a better understanding of NPs behavior in biological specimens for toxicology or nanomedicine purposes.
doi_str_mv	10.1021/ac501318c
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Chem</addtitle><description>Assessing in situ nanoparticles (NPs) internalization at the level of a single cell is a difficult but critical task due to their potential use in nanomedicine. One of the main actual challenges is to control the number of internalized NPs per cell. To in situ detect, track, and above all quantify NPs in a single cell, we propose an approach based on a multimodal correlative microscopy (MCM), via the complementarity of three imaging techniques: fluorescence microscopy (FM), scanning electron microscopy (SEM), and ion beam analysis (IBA). This MCM was performed on single targeted individual primary human foreskin keratinocytes (PHFK) cells cultured and maintained on a specifically designed sample holder, to probe either dye-modified or bare NPs. The data obtained by both FM and IBA on dye-modified NPs were strongly correlated in terms of detection, tracking, and colocalization of fluorescence and metal detection. IBA techniques should therefore open a new field concerning specific studies on bare NPs and their toxicological impact on cells. Complementarity of SEM and IBA analyses provides surface (SEM) and in depth (IBA) information on the cell morphology as well as on the exact localization of the NPs. Finally, IBA not only provides in a single cell the in situ quantification of exogenous elements (NPs) but also that all the other endogenous elements and the subsequent variation of their homeostasis. 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Chem</addtitle><date>2014-08-05</date><risdate>2014</risdate><volume>86</volume><issue>15</issue><spage>7311</spage><epage>7319</epage><pages>7311-7319</pages><issn>0003-2700</issn><eissn>1520-6882</eissn><coden>ANCHAM</coden><abstract>Assessing in situ nanoparticles (NPs) internalization at the level of a single cell is a difficult but critical task due to their potential use in nanomedicine. One of the main actual challenges is to control the number of internalized NPs per cell. To in situ detect, track, and above all quantify NPs in a single cell, we propose an approach based on a multimodal correlative microscopy (MCM), via the complementarity of three imaging techniques: fluorescence microscopy (FM), scanning electron microscopy (SEM), and ion beam analysis (IBA). This MCM was performed on single targeted individual primary human foreskin keratinocytes (PHFK) cells cultured and maintained on a specifically designed sample holder, to probe either dye-modified or bare NPs. The data obtained by both FM and IBA on dye-modified NPs were strongly correlated in terms of detection, tracking, and colocalization of fluorescence and metal detection. IBA techniques should therefore open a new field concerning specific studies on bare NPs and their toxicological impact on cells. Complementarity of SEM and IBA analyses provides surface (SEM) and in depth (IBA) information on the cell morphology as well as on the exact localization of the NPs. Finally, IBA not only provides in a single cell the in situ quantification of exogenous elements (NPs) but also that all the other endogenous elements and the subsequent variation of their homeostasis. 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subjects	Analytical chemistry Analytical techniques Biochemistry Cells Chemical Sciences Correlation Dyes Fluorescence Material chemistry Metal Nanoparticles Microscopy Microscopy - methods Nanoparticles Nanostructure Oxides - chemistry Scanning electron microscopy Single-Cell Analysis Toxicology
title	Single Cell In Situ Detection and Quantification of Metal Oxide Nanoparticles Using Multimodal Correlative Microscopy
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