| Literature DB >> 26002145 |
Nana F Keinath1, Rainer Waadt2, Rik Brugman3, Julian I Schroeder4, Guido Grossmann3, Karin Schumacher1, Melanie Krebs5.
Abstract
Intracellular Ca(2+) transients are an integral part of the signaling cascade during pathogen-associated molecular pattern (PAMP)-triggered immunity in plants. Yet, our knowledge about the spatial distribution of PAMP-induced Ca(2+) signals is limited. Investigation of cell- and tissue-specific properties of Ca(2+)-dependent signaling processes requires versatile Ca(2+) reporters that are able to extract spatial information from cellular and subcellular structures, as well as from whole tissues over time periods from seconds to hours. Fluorescence-based reporters cover both a broad spatial and temporal range, which makes them ideally suited to study Ca(2+) signaling in living cells. In this study, we compared two fluorescence-based Ca(2+) sensors: the Förster resonance energy transfer (FRET)-based reporter yellow cameleon NES-YC3.6 and the intensity-based sensor R-GECO1. We demonstrate that R-GECO1 exhibits a significantly increased signal change compared with ratiometric NES-YC3.6 in response to several stimuli. Due to its superior sensitivity, R-GECO1 is able to report flg22- and chitin-induced Ca(2+) signals on a cellular scale, which allowed identification of defined [Ca(2+)]cyt oscillations in epidermal and guard cells in response to the fungal elicitor chitin. Moreover, we discovered that flg22- and chitin-induced Ca(2+) signals in the root initiate from the elongation zone.Entities:
Keywords: Arabidopsis; R-GECO1; calcium imaging; chitin; flg22; sensor
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Year: 2015 PMID: 26002145 PMCID: PMC5134422 DOI: 10.1016/j.molp.2015.05.006
Source DB: PubMed Journal: Mol Plant ISSN: 1674-2052 Impact factor: 13.164