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Neutrophil leukocyte motility requires directed water influx
Author(s) -
Loitto VesaMatti,
Forslund Tony,
Sundqvist Tommy,
Magnusson KarlEric,
Gustafsson Mikael
Publication year - 2002
Publication title -
journal of leukocyte biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.819
H-Index - 191
eISSN - 1938-3673
pISSN - 0741-5400
DOI - 10.1189/jlb.71.2.212
Subject(s) - motility , lamellipodium , biology , microbiology and biotechnology , aquaporin , fluorescence microscope , biophysics , video microscopy , cell migration , cell , biochemistry , fluorescence , physics , quantum mechanics
The ability of neutrophils to sense and move to sites of infection is essential for our defense against pathogens. For motility, lamellipodium extension and stabilization are prerequisites, but how cells form such membrane protrusions is still obscure. Using contrast‐enhanced video microscopy and Transwell® assays, we show that water‐selective aquaporin channels regulate lamellipodium formation and neutrophil motility. Addition of anti‐aquaporin‐9 antibodies, HgCl 2 , or tetraethyl ammonium inhibited the function(s) of the channels and blocked motility‐related shape changes. On human neutrophils, aquaporin‐9 preferentially localized to the cell edges, where N ‐formyl peptide receptors also accumulated, as assessed with fluorescence microscopy. To directly visualize water fluxes at cell edges, cells were loaded with high dilution‐sensitive, self‐quenching concentrations of fluorophore. In these cells, motile regions always displayed increased fluorescence compared with perinuclear regions. Our observations provide the first experimental support for motility models where water fluxes play a pivotal role in cell‐volume increases accompanying membrane extensions.