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Visualizing Cell-to-cell Transfer of HIV using Fluorescent Clones of HIV and Live Confocal Microscopy
Author(s) -
Benjamin M. Dale,
Gregory P. McNerney,
Deanna L. Thompson,
Wolfgang Hübner,
Thomas Huser,
Benjamin K. Chen
Publication year - 2010
Publication title -
journal of visualized experiments
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.596
H-Index - 91
ISSN - 1940-087X
DOI - 10.3791/2061
Subject(s) - confocal microscopy , fluorescence microscope , green fluorescent protein , clone (java method) , microbiology and biotechnology , transfection , live cell imaging , biology , context (archaeology) , confocal , cell culture , intracellular , microscopy , virus , cell , human immunodeficiency virus (hiv) , fluorescence lifetime imaging microscopy , virology , fluorescence , pathology , genetics , gene , medicine , paleontology , physics , geometry , mathematics , quantum mechanics
By fusing the green fluorescent protein to their favorite proteins, biologists now have the ability to study living complex cellular processes using fluorescence video microscopy. To track the movements of the human immunodeficiency virus core protein during cell-to-cell transmission of human immunodeficiency virus, we have GFP-tagged the Gag protein in the context of an infectious molecular clone of HIV, called HIV Gag-iGFP. We study this viral clone using video confocal microscopy. In the following visualized experiment, we transfect a human T cell line with HIV Gag-iGFP, and we use fluorescently labeled uninfected CD4+ T cells to serve as target cells for the virus. Using the different fluorescent labels we can readily follow viral production and transport across intercellular structures called virological synapses. Simple gas permeable imaging chambers allow us to observe synapses with live confocal microscopy from minutes to days. These approaches can be used to track viral proteins as they move in from one cell to the next.

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