Literature DB >> 21704835

Parallel imaging microfluidic cytometer.

Daniel J Ehrlich1, Brian K McKenna, James G Evans, Anna C Belkina, Gerald V Denis, David H Sherr, Man Ching Cheung.   

Abstract

By adding an additional degree of freedom from multichannel flow, the parallel microfluidic cytometer (PMC) combines some of the best features of fluorescence-activated flow cytometry (FCM) and microscope-based high-content screening (HCS). The PMC (i) lends itself to fast processing of large numbers of samples, (ii) adds a 1D imaging capability for intracellular localization assays (HCS), (iii) has a high rare-cell sensitivity, and (iv) has an unusual capability for time-synchronized sampling. An inability to practically handle large sample numbers has restricted applications of conventional flow cytometers and microscopes in combinatorial cell assays, network biology, and drug discovery. The PMC promises to relieve a bottleneck in these previously constrained applications. The PMC may also be a powerful tool for finding rare primary cells in the clinic. The multichannel architecture of current PMC prototypes allows 384 unique samples for a cell-based screen to be read out in ∼6-10 min, about 30 times the speed of most current FCM systems. In 1D intracellular imaging, the PMC can obtain protein localization using HCS marker strategies at many times for the sample throughput of charge-coupled device (CCD)-based microscopes or CCD-based single-channel flow cytometers. The PMC also permits the signal integration time to be varied over a larger range than is practical in conventional flow cytometers. The signal-to-noise advantages are useful, for example, in counting rare positive cells in the most difficult early stages of genome-wide screening. We review the status of parallel microfluidic cytometry and discuss some of the directions the new technology may take.
Copyright © 2011 Elsevier Inc. All rights reserved.

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Year:  2011        PMID: 21704835      PMCID: PMC3139515          DOI: 10.1016/B978-0-12-374912-3.00003-1

Source DB:  PubMed          Journal:  Methods Cell Biol        ISSN: 0091-679X            Impact factor:   1.441


  28 in total

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Journal:  Methods Enzymol       Date:  2006       Impact factor: 1.600

Review 4.  Microscopic imaging techniques for drug discovery.

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Journal:  Nat Rev Drug Discov       Date:  2008-01       Impact factor: 84.694

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7.  Flow cytometry of Escherichia coli on microfluidic devices.

Authors:  M A McClain; C T Culbertson; S C Jacobson; J M Ramsey
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Authors:  Jurjen Emmelkamp; Floor Wolbers; Helene Andersson; Ralph S Dacosta; Brian C Wilson; Istvan Vermes; Albert van den Berg
Journal:  Electrophoresis       Date:  2004-11       Impact factor: 3.535

9.  E mu-BRD2 transgenic mice develop B-cell lymphoma and leukemia.

Authors:  Rebecca J Greenwald; Joseph R Tumang; Anupama Sinha; Nicolas Currier; Robert D Cardiff; Thomas L Rothstein; Douglas V Faller; Gerald V Denis
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Authors:  Anne E Carpenter; Thouis R Jones; Michael R Lamprecht; Colin Clarke; In Han Kang; Ola Friman; David A Guertin; Joo Han Chang; Robert A Lindquist; Jason Moffat; Polina Golland; David M Sabatini
Journal:  Genome Biol       Date:  2006-10-31       Impact factor: 13.583

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  1 in total

1.  Microfluidic flow cytometry: The role of microfabrication methodologies, performance and functional specification.

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Journal:  Technology (Singap World Sci)       Date:  2018-03-16
  1 in total

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