| Literature DB >> 26462735 |
Insa M A Wolf1, Björn-Philipp Diercks1, Ellen Gattkowski1, Frederik Czarniak1, Jan Kempski1, René Werner2, Daniel Schetelig2, Hans-Willi Mittrücker3, Valéa Schumacher3, Manuel von Osten4, Dimitri Lodygin4, Alexander Flügel4, Ralf Fliegert1, Andreas H Guse5.
Abstract
The activation of T cells is the fundamental on switch for the adaptive immune system. Ca(2+) signaling is essential for T cell activation and starts as initial, short-lived, localized Ca(2+) signals. The second messenger nicotinic acid adenine dinucleotide phosphate (NAADP) forms rapidly upon T cell activation and stimulates early Ca(2+) signaling. We developed a high-resolution imaging technique using multiple fluorescent Ca(2+) indicator dyes to characterize these early signaling events and investigate the channels involved in NAADP-dependent Ca(2+) signals. In the first seconds of activation of either primary murine T cells or human Jurkat cells with beads coated with an antibody against CD3, we detected Ca(2+) signals with diameters close to the limit of detection and that were close to the activation site at the plasma membrane. In Jurkat cells in which the ryanodine receptor (RyR) was knocked down or in primary T cells from RyR1(-/-) mice, either these early Ca(2+) signals were not detected or the number of signals was markedly reduced. Local Ca(2+) signals observed within 20 ms upon microinjection of Jurkat cells with NAADP were also sensitive to RyR knockdown. In contrast, TRPM2 (transient receptor potential channel, subtype melastatin 2), a potential NAADP target channel, was not required for the formation of initial Ca(2+) signals in primary T cells. Thus, through our high-resolution imaging method, we characterized early Ca(2+) release events in T cells and obtained evidence for the involvement of RyR and NAADP in such signals.Entities:
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Year: 2015 PMID: 26462735 DOI: 10.1126/scisignal.aab0863
Source DB: PubMed Journal: Sci Signal ISSN: 1945-0877 Impact factor: 8.192