Dynamic quantitative assays of phagosomal function

Maria Podinovskaia; Brian C. VanderVen; Robin M. Yates; Sarah Glennie; Duncan Fullerton; Henry Mwandumba; David G. Russell

doi:10.1002/0471142735.im1434s102

Dynamic quantitative assays of phagosomal function

Maria Podinovskaia, Brian C. VanderVen, Robin M. Yates, Sarah Glennie, Duncan Fullerton, Henry Mwandumba, David G. Russell

Liverpool School of Tropical Medicine

Research output: Contribution to journal › Article › peer-review

20 Citations (Scopus)

Abstract

Much of the activity of the macrophage as an effector cell is performed within its phagocytic compartment. This ranges from the degradation of tissue debris as part of its homeostatic function to the generation of the superoxide burst as part of its microbicidal response to infection. We have developed a range of real-time readouts of phagosomal function that enable these activities to be rigorously quantified. This unit contains descriptions of several of these assays assessed by different methods of quantitation, including a fluorescence resonance emission transfer (FRET) assay for phagosome/ lysosome fusion measured by spectrofluorometry, a fluorogenic assay for the superoxide burst measured by flow cytometry, and a fluorogenic assay for bulk proteolysis measured by confocal microscopy. These assays illustrate both the range of parameters that can be quantified and the flexibility of instrumentation that can be exploited for their quantitation.

Original language	English
Article number	14.34
Journal	Current Protocols in Immunology
Issue number	SUPPL.102
DOIs	https://doi.org/10.1002/0471142735.im1434s102
Publication status	Published - 1 Jan 2013

Keywords

Macrophage
Phagocytosis
Phagosome
Phagosome maturation

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10.1002/0471142735.im1434s102

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title = "Dynamic quantitative assays of phagosomal function",

abstract = "Much of the activity of the macrophage as an effector cell is performed within its phagocytic compartment. This ranges from the degradation of tissue debris as part of its homeostatic function to the generation of the superoxide burst as part of its microbicidal response to infection. We have developed a range of real-time readouts of phagosomal function that enable these activities to be rigorously quantified. This unit contains descriptions of several of these assays assessed by different methods of quantitation, including a fluorescence resonance emission transfer (FRET) assay for phagosome/ lysosome fusion measured by spectrofluorometry, a fluorogenic assay for the superoxide burst measured by flow cytometry, and a fluorogenic assay for bulk proteolysis measured by confocal microscopy. These assays illustrate both the range of parameters that can be quantified and the flexibility of instrumentation that can be exploited for their quantitation.",

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doi = "10.1002/0471142735.im1434s102",

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T1 - Dynamic quantitative assays of phagosomal function

AU - Podinovskaia, Maria

AU - VanderVen, Brian C.

AU - Yates, Robin M.

AU - Glennie, Sarah

AU - Fullerton, Duncan

AU - Mwandumba, Henry

AU - Russell, David G.

PY - 2013/1/1

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N2 - Much of the activity of the macrophage as an effector cell is performed within its phagocytic compartment. This ranges from the degradation of tissue debris as part of its homeostatic function to the generation of the superoxide burst as part of its microbicidal response to infection. We have developed a range of real-time readouts of phagosomal function that enable these activities to be rigorously quantified. This unit contains descriptions of several of these assays assessed by different methods of quantitation, including a fluorescence resonance emission transfer (FRET) assay for phagosome/ lysosome fusion measured by spectrofluorometry, a fluorogenic assay for the superoxide burst measured by flow cytometry, and a fluorogenic assay for bulk proteolysis measured by confocal microscopy. These assays illustrate both the range of parameters that can be quantified and the flexibility of instrumentation that can be exploited for their quantitation.

AB - Much of the activity of the macrophage as an effector cell is performed within its phagocytic compartment. This ranges from the degradation of tissue debris as part of its homeostatic function to the generation of the superoxide burst as part of its microbicidal response to infection. We have developed a range of real-time readouts of phagosomal function that enable these activities to be rigorously quantified. This unit contains descriptions of several of these assays assessed by different methods of quantitation, including a fluorescence resonance emission transfer (FRET) assay for phagosome/ lysosome fusion measured by spectrofluorometry, a fluorogenic assay for the superoxide burst measured by flow cytometry, and a fluorogenic assay for bulk proteolysis measured by confocal microscopy. These assays illustrate both the range of parameters that can be quantified and the flexibility of instrumentation that can be exploited for their quantitation.

KW - Macrophage

KW - Phagocytosis

KW - Phagosome

KW - Phagosome maturation

U2 - 10.1002/0471142735.im1434s102

DO - 10.1002/0471142735.im1434s102

M3 - Article

SN - 1934-3671

JO - Current Protocols in Immunology

JF - Current Protocols in Immunology

IS - SUPPL.102

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Dynamic quantitative assays of phagosomal function

Abstract

Keywords

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