A Method for Rapid, Quantitative Evaluation of Particle Sorting in Microfluidics Using Basic Cytometry Equipment.

Salomon, R; Razavi Bazaz, S; Li, W; Gallego-Ortega, D; Jin, D; Warkiani, ME

A Method for Rapid, Quantitative Evaluation of Particle Sorting in Microfluidics Using Basic Cytometry Equipment.

Salomon, R

Razavi Bazaz, S

Li, W Gallego-Ortega, D Jin, D

Warkiani, ME

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Publisher:: MDPI
Publication Type:: Journal Article
Citation:: Micromachines (Basel), 2023, 14, (4), pp. 751
Issue Date:: 2023-03-29

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Field	Value	Language
dc.contributor.author	Salomon, R https://orcid.org/0000-0003-4504-2901
dc.contributor.author	Razavi Bazaz, S https://orcid.org/0000-0002-6419-3361
dc.contributor.author	Li, W
dc.contributor.author	Gallego-Ortega, D
dc.contributor.author	Jin, D https://orcid.org/0000-0003-1046-2666
dc.contributor.author	Warkiani, ME
dc.date.accessioned	2024-02-06T02:01:49Z
dc.date.available	2023-03-27
dc.date.available	2024-02-06T02:01:49Z
dc.date.issued	2023-03-29
dc.identifier.citation	Micromachines (Basel), 2023, 14, (4), pp. 751
dc.identifier.issn	2072-666X
dc.identifier.issn	2072-666X
dc.identifier.uri	http://hdl.handle.net/10453/175349
dc.description.abstract	This paper describes, in detail, a method that uses flow cytometry to quantitatively characterise the performance of continuous-flow microfluidic devices designed to separate particles. Whilst simple, this approach overcomes many of the issues with the current commonly utilised methods (high-speed fluorescent imaging, or cell counting via either a hemocytometer or a cell counter), as it can accurately assess device performance even in complex, high concentration mixtures in a way that was previously not possible. Uniquely, this approach takes advantage of pulse processing in flow cytometry to allow quantitation of cell separation efficiencies and resulting sample purities on both single cells as well as cell clusters (such as circulating tumour cell (CTC) clusters). Furthermore, it can readily be combined with cell surface phenotyping to measure separation efficiencies and purities in complex cell mixtures. This method will facilitate the rapid development of a raft of continuous flow microfluidic devices, will be helpful in testing novel separation devices for biologically relevant clusters of cells such as CTC clusters, and will provide a quantitative assessment of device performance in complex samples, which was previously impossible.
dc.format	Electronic
dc.language	eng
dc.publisher	MDPI
dc.relation.ispartof	Micromachines (Basel)
dc.relation.isbasedon	10.3390/mi14040751
dc.rights	info:eu-repo/semantics/openAccess
dc.subject	1007 Nanotechnology
dc.subject.classification	4018 Nanotechnology
dc.title	A Method for Rapid, Quantitative Evaluation of Particle Sorting in Microfluidics Using Basic Cytometry Equipment.
dc.type	Journal Article
utslib.citation.volume	14
utslib.location.activity	Switzerland
utslib.for	1007 Nanotechnology
pubs.organisational-group	University of Technology Sydney
pubs.organisational-group	University of Technology Sydney/Faculty of Engineering and Information Technology
pubs.organisational-group	University of Technology Sydney/Faculty of Science
pubs.organisational-group	University of Technology Sydney/Strength - CHT - Health Technologies
pubs.organisational-group	University of Technology Sydney/Faculty of Science/School of Mathematical and Physical Sciences
pubs.organisational-group	University of Technology Sydney/Faculty of Engineering and Information Technology/School of Biomedical Engineering
pubs.organisational-group	University of Technology Sydney/Strength - IBMD - Initiative for Biomedical Devices
pubs.organisational-group	University of Technology Sydney/Centre for Health Technologies (CHT)
utslib.copyright.status	open_access	*
dc.date.updated	2024-02-06T02:01:47Z
pubs.issue	4
pubs.publication-status	Published online
pubs.volume	14
utslib.citation.issue	4

Abstract:

This paper describes, in detail, a method that uses flow cytometry to quantitatively characterise the performance of continuous-flow microfluidic devices designed to separate particles. Whilst simple, this approach overcomes many of the issues with the current commonly utilised methods (high-speed fluorescent imaging, or cell counting via either a hemocytometer or a cell counter), as it can accurately assess device performance even in complex, high concentration mixtures in a way that was previously not possible. Uniquely, this approach takes advantage of pulse processing in flow cytometry to allow quantitation of cell separation efficiencies and resulting sample purities on both single cells as well as cell clusters (such as circulating tumour cell (CTC) clusters). Furthermore, it can readily be combined with cell surface phenotyping to measure separation efficiencies and purities in complex cell mixtures. This method will facilitate the rapid development of a raft of continuous flow microfluidic devices, will be helpful in testing novel separation devices for biologically relevant clusters of cells such as CTC clusters, and will provide a quantitative assessment of device performance in complex samples, which was previously impossible.

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http://hdl.handle.net/10453/175349