Literature DB >> 18813394

Microfluidic platform for real-time signaling analysis of multiple single T cells in parallel.

Shannon Faley1, Kevin Seale, Jacob Hughey, David K Schaffer, Scott VanCompernolle, Brett McKinney, Franz Baudenbacher, Derya Unutmaz, John P Wikswo.   

Abstract

Deciphering the signaling pathways that govern stimulation of naïve CD4+ T helper cells by antigen-presenting cells via formation of the immunological synapse is key to a fundamental understanding of the progression of successful adaptive immune response. The study of T cell-APC interactions in vitro is challenging, however, due to the difficulty of tracking individual, non-adherent cell pairs over time. Studying single cell dynamics over time reveals rare, but critical, signaling events that might be averaged out in bulk experiments, but these less common events are undoubtedly important for an integrated understanding of a cellular response to its microenvironment. We describe a novel application of microfluidic technology that overcomes many limitations of conventional cell culture and enables the study of hundreds of passively sequestered hematopoietic cells for extended periods of time. This microfluidic cell trap device consists of 440 18 micromx18 micromx10 microm PDMS, bucket-like structures opposing the direction of flow which serve as corrals for cells as they pass through the cell trap region. Cell viability analysis revealed that more than 70% of naïve CD4+ T cells (TN), held in place using only hydrodynamic forces, subsequently remain viable for 24 hours. Cytosolic calcium transients were successfully induced in TN cells following introduction of chemical, antibody, or cellular forms of stimulation. Statistical analysis of TN cells from a single stimulation experiment reveals the power of this platform to distinguish different calcium response patterns, an ability that might be utilized to characterize T cell signaling states in a given population. Finally, we investigate in real time contact- and non-contact-based interactions between primary T cells and dendritic cells, two main participants in the formation of the immunological synapse. Utilizing the microfluidic traps in a daisy-chain configuration allowed us to observe calcium transients in TN cells exposed only to media conditioned by secretions of lipopolysaccharide-matured dendritic cells, an event which is easily missed in conventional cell culture where large media-to-cell ratios dilute cellular products. Further investigation into this intercellular signaling event indicated that LPS-matured dendritic cells, in the absence of antigenic stimulation, secrete chemical signals that induce calcium transients in T(N) cells. While the stimulating factor(s) produced by the mature dendritic cells remains to be identified, this report illustrates the utility of these microfluidic cell traps for analyzing arrays of individual suspension cells over time and probing both contact-based and intercellular signaling events between one or more cell populations.

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Year:  2008        PMID: 18813394      PMCID: PMC4160168          DOI: 10.1039/b719799c

Source DB:  PubMed          Journal:  Lab Chip        ISSN: 1473-0189            Impact factor:   6.799


  48 in total

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3.  A practical guide to microfluidic perfusion culture of adherent mammalian cells.

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4.  Mechanisms for segregating T cell receptor and adhesion molecules during immunological synapse formation in Jurkat T cells.

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5.  Differential activation requirements associated with stimulation of T cells via different epitopes of CD3.

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7.  Rapid identification of antigenic T-cell epitopes by extracellular acidification rate signals.

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8.  A microfluidic device to confine a single cardiac myocyte in a sub-nanoliter volume on planar microelectrodes for extracellular potential recordings.

Authors:  Andreas A Werdich; Eduardo A Lima; Borislav Ivanov; Igor Ges; Mark E Anderson; John P Wikswo; Franz J Baudenbacher
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Review 9.  Interleukin-2: inception, impact, and implications.

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10.  Imaging the single cell dynamics of CD4+ T cell activation by dendritic cells in lymph nodes.

Authors:  Mark J Miller; Olga Safrina; Ian Parker; Michael D Cahalan
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  49 in total

1.  Variability in G-protein-coupled signaling studied with microfluidic devices.

Authors:  Xiaoyan Robert Bao; Iain D C Fraser; Estelle A Wall; Stephen R Quake; Melvin I Simon
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2.  Towards monitoring real-time cellular response using an integrated microfluidics-matrix assisted laser desorption ionisation/nanoelectrospray ionisation-ion mobility-mass spectrometry platform.

Authors:  J R Enders; C C Marasco; A Kole; B Nguyen; S Sevugarajan; K T Seale; J P Wikswo; J A McLean
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3.  Mechanistic analysis of challenge-response experiments.

Authors:  M S Shotwell; K J Drake; V Y Sidorov; J P Wikswo
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4.  A microfluidic chip for the versatile chemical analysis of single cells.

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5.  Single-cell attachment and culture method using a photochemical reaction in a closed microfluidic system.

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6.  Microfluidic confinement of single cells of bacteria in small volumes initiates high-density behavior of quorum sensing and growth and reveals its variability.

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7.  Engineering challenges for instrumenting and controlling integrated organ-on-chip systems.

Authors:  John P Wikswo; Frank E Block; David E Cliffel; Cody R Goodwin; Christina C Marasco; Dmitry A Markov; David L McLean; John A McLean; Jennifer R McKenzie; Ronald S Reiserer; Philip C Samson; David K Schaffer; Kevin T Seale; Stacy D Sherrod
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8.  On-chip activation and subsequent detection of individual antigen-specific T cells.

Authors:  Qing Song; Qing Han; Elizabeth M Bradshaw; Sally C Kent; Khadir Raddassi; Björn Nilsson; Gerald T Nepom; David A Hafler; J Christopher Love
Journal:  Anal Chem       Date:  2010-01-15       Impact factor: 6.986

9.  Microfluidic platform for real-time signaling analysis of multiple single T cells in parallel.

Authors:  Shannon Faley; Kevin Seale; Jacob Hughey; David K Schaffer; Scott VanCompernolle; Brett McKinney; Franz Baudenbacher; Derya Unutmaz; John P Wikswo
Journal:  Lab Chip       Date:  2008-08-19       Impact factor: 6.799

10.  Microfluidic single-cell array cytometry for the analysis of tumor apoptosis.

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Journal:  Anal Chem       Date:  2009-07-01       Impact factor: 6.986

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