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Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells

The role of circulating plasma cells (CPCs) and circulating leukemic cells (CLCs) as biomarkers for several blood cancers, such as multiple myeloma and leukemia, respectively, have recently been reported. These markers can be attractive due to the minimally invasive nature of their acquisition throu...

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Autores principales: M. Weerakoon-Ratnayake, Kumuditha, Vaidyanathan, Swarnagowri, Larkey, Nicholas, Dathathreya, Kavya, Hu, Mengjia, Jose, Jilsha, Mog, Shalee, August, Keith, K. Godwin, Andrew, L. Hupert, Mateusz, A. Witek, Malgorzata, A. Soper, Steven
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7072755/
https://www.ncbi.nlm.nih.gov/pubmed/32102446
http://dx.doi.org/10.3390/cells9020519
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author M. Weerakoon-Ratnayake, Kumuditha
Vaidyanathan, Swarnagowri
Larkey, Nicholas
Dathathreya, Kavya
Hu, Mengjia
Jose, Jilsha
Mog, Shalee
August, Keith
K. Godwin, Andrew
L. Hupert, Mateusz
A. Witek, Malgorzata
A. Soper, Steven
author_facet M. Weerakoon-Ratnayake, Kumuditha
Vaidyanathan, Swarnagowri
Larkey, Nicholas
Dathathreya, Kavya
Hu, Mengjia
Jose, Jilsha
Mog, Shalee
August, Keith
K. Godwin, Andrew
L. Hupert, Mateusz
A. Witek, Malgorzata
A. Soper, Steven
author_sort M. Weerakoon-Ratnayake, Kumuditha
collection PubMed
description The role of circulating plasma cells (CPCs) and circulating leukemic cells (CLCs) as biomarkers for several blood cancers, such as multiple myeloma and leukemia, respectively, have recently been reported. These markers can be attractive due to the minimally invasive nature of their acquisition through a blood draw (i.e., liquid biopsy), negating the need for painful bone marrow biopsies. CPCs or CLCs can be used for cellular/molecular analyses as well, such as immunophenotyping or fluorescence in situ hybridization (FISH). FISH, which is typically carried out on slides involving complex workflows, becomes problematic when operating on CLCs or CPCs due to their relatively modest numbers. Here, we present a microfluidic device for characterizing CPCs and CLCs using immunofluorescence or FISH that have been enriched from peripheral blood using a different microfluidic device. The microfluidic possessed an array of cross-channels (2–4 µm in depth and width) that interconnected a series of input and output fluidic channels. Placing a cover plate over the device formed microtraps, the size of which was defined by the width and depth of the cross-channels. This microfluidic chip allowed for automation of immunofluorescence and FISH, requiring the use of small volumes of reagents, such as antibodies and probes, as compared to slide-based immunophenotyping and FISH. In addition, the device could secure FISH results in <4 h compared to 2–3 days for conventional FISH.
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spelling pubmed-70727552020-03-19 Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells M. Weerakoon-Ratnayake, Kumuditha Vaidyanathan, Swarnagowri Larkey, Nicholas Dathathreya, Kavya Hu, Mengjia Jose, Jilsha Mog, Shalee August, Keith K. Godwin, Andrew L. Hupert, Mateusz A. Witek, Malgorzata A. Soper, Steven Cells Article The role of circulating plasma cells (CPCs) and circulating leukemic cells (CLCs) as biomarkers for several blood cancers, such as multiple myeloma and leukemia, respectively, have recently been reported. These markers can be attractive due to the minimally invasive nature of their acquisition through a blood draw (i.e., liquid biopsy), negating the need for painful bone marrow biopsies. CPCs or CLCs can be used for cellular/molecular analyses as well, such as immunophenotyping or fluorescence in situ hybridization (FISH). FISH, which is typically carried out on slides involving complex workflows, becomes problematic when operating on CLCs or CPCs due to their relatively modest numbers. Here, we present a microfluidic device for characterizing CPCs and CLCs using immunofluorescence or FISH that have been enriched from peripheral blood using a different microfluidic device. The microfluidic possessed an array of cross-channels (2–4 µm in depth and width) that interconnected a series of input and output fluidic channels. Placing a cover plate over the device formed microtraps, the size of which was defined by the width and depth of the cross-channels. This microfluidic chip allowed for automation of immunofluorescence and FISH, requiring the use of small volumes of reagents, such as antibodies and probes, as compared to slide-based immunophenotyping and FISH. In addition, the device could secure FISH results in <4 h compared to 2–3 days for conventional FISH. MDPI 2020-02-24 /pmc/articles/PMC7072755/ /pubmed/32102446 http://dx.doi.org/10.3390/cells9020519 Text en © 2020 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
M. Weerakoon-Ratnayake, Kumuditha
Vaidyanathan, Swarnagowri
Larkey, Nicholas
Dathathreya, Kavya
Hu, Mengjia
Jose, Jilsha
Mog, Shalee
August, Keith
K. Godwin, Andrew
L. Hupert, Mateusz
A. Witek, Malgorzata
A. Soper, Steven
Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title_full Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title_fullStr Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title_full_unstemmed Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title_short Microfluidic Device for On-Chip Immunophenotyping and Cytogenetic Analysis of Rare Biological Cells
title_sort microfluidic device for on-chip immunophenotyping and cytogenetic analysis of rare biological cells
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7072755/
https://www.ncbi.nlm.nih.gov/pubmed/32102446
http://dx.doi.org/10.3390/cells9020519
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