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Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery

Droplet microfluidics has made large impacts in diverse areas such as enzyme evolution, chemical product screening, polymer engineering, and single-cell analysis. However, while droplet reactions have become increasingly sophisticated, phenotyping droplets by a fluorescent signal and sorting them to...

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Autores principales: Brower, Kara K., Carswell-Crumpton, Catherine, Klemm, Sandy, Cruz, Bianca, Kim, Gaeun, Calhoun, Suzanne G. K., Nichols, Lisa, Fordyce, Polly M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7670282/
https://www.ncbi.nlm.nih.gov/pubmed/32417874
http://dx.doi.org/10.1039/d0lc00261e
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author Brower, Kara K.
Carswell-Crumpton, Catherine
Klemm, Sandy
Cruz, Bianca
Kim, Gaeun
Calhoun, Suzanne G. K.
Nichols, Lisa
Fordyce, Polly M.
author_facet Brower, Kara K.
Carswell-Crumpton, Catherine
Klemm, Sandy
Cruz, Bianca
Kim, Gaeun
Calhoun, Suzanne G. K.
Nichols, Lisa
Fordyce, Polly M.
author_sort Brower, Kara K.
collection PubMed
description Droplet microfluidics has made large impacts in diverse areas such as enzyme evolution, chemical product screening, polymer engineering, and single-cell analysis. However, while droplet reactions have become increasingly sophisticated, phenotyping droplets by a fluorescent signal and sorting them to isolate individual variants-of-interest at high-throughput remains challenging. Here, we present sdDE-FACS (single droplet Double Emulsion-FACS), a new method that uses a standard flow cytometer to phenotype, select, and isolate individual double emulsion droplets of interest. Using a 130 μm nozzle at high sort frequency (12–14 kHz), we demonstrate detection of droplet fluorescence signals with a dynamic range spanning 5 orders of magnitude and robust post-sort recovery of intact double emulsion (DE) droplets using 2 commercially-available FACS instruments. We report the first demonstration of single double emulsion droplet isolation with post-sort recovery efficiencies >70%, equivalent to the capabilities of single-cell FACS. Finally, we establish complete downstream recovery of nucleic acids from single, sorted double emulsion droplets via qPCR with little to no cross-contamination. sdDE-FACS marries the full power of droplet microfluidics with flow cytometry to enable a variety of new droplet assays, including rare variant isolation and multiparameter single-cell analysis.
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spelling pubmed-76702822020-11-17 Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery Brower, Kara K. Carswell-Crumpton, Catherine Klemm, Sandy Cruz, Bianca Kim, Gaeun Calhoun, Suzanne G. K. Nichols, Lisa Fordyce, Polly M. Lab Chip Article Droplet microfluidics has made large impacts in diverse areas such as enzyme evolution, chemical product screening, polymer engineering, and single-cell analysis. However, while droplet reactions have become increasingly sophisticated, phenotyping droplets by a fluorescent signal and sorting them to isolate individual variants-of-interest at high-throughput remains challenging. Here, we present sdDE-FACS (single droplet Double Emulsion-FACS), a new method that uses a standard flow cytometer to phenotype, select, and isolate individual double emulsion droplets of interest. Using a 130 μm nozzle at high sort frequency (12–14 kHz), we demonstrate detection of droplet fluorescence signals with a dynamic range spanning 5 orders of magnitude and robust post-sort recovery of intact double emulsion (DE) droplets using 2 commercially-available FACS instruments. We report the first demonstration of single double emulsion droplet isolation with post-sort recovery efficiencies >70%, equivalent to the capabilities of single-cell FACS. Finally, we establish complete downstream recovery of nucleic acids from single, sorted double emulsion droplets via qPCR with little to no cross-contamination. sdDE-FACS marries the full power of droplet microfluidics with flow cytometry to enable a variety of new droplet assays, including rare variant isolation and multiparameter single-cell analysis. 2020-05-17 2020-06-21 /pmc/articles/PMC7670282/ /pubmed/32417874 http://dx.doi.org/10.1039/d0lc00261e Text en This article is licensed under a Creative Commons Attribution-NonCommercial 3.0 Unported Licence (https://creativecommons.org/licenses/by-nc/3.0/) .
spellingShingle Article
Brower, Kara K.
Carswell-Crumpton, Catherine
Klemm, Sandy
Cruz, Bianca
Kim, Gaeun
Calhoun, Suzanne G. K.
Nichols, Lisa
Fordyce, Polly M.
Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title_full Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title_fullStr Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title_full_unstemmed Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title_short Double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
title_sort double emulsion flow cytometry with high-throughput single droplet isolation and nucleic acid recovery
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7670282/
https://www.ncbi.nlm.nih.gov/pubmed/32417874
http://dx.doi.org/10.1039/d0lc00261e
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