2017
Fluorescence microscopy as a tool for visualization of metal-induced oxidative stress in plants
KOVACIK, Jozef a Petr BABULAZákladní údaje
Originální název
Fluorescence microscopy as a tool for visualization of metal-induced oxidative stress in plants
Autoři
KOVACIK, Jozef (703 Slovensko) a Petr BABULA (203 Česká republika, garant, domácí)
Vydání
Acta Physiologiae Plantarum, Cracow, Polish Academy of Sciences, 2017, 0137-5881
Další údaje
Jazyk
angličtina
Typ výsledku
Článek v odborném periodiku
Obor
10700 1.7 Other natural sciences
Stát vydavatele
Polsko
Utajení
není předmětem státního či obchodního tajemství
Impakt faktor
Impact factor: 1.438
Kód RIV
RIV/00216224:14110/17:00097480
Organizační jednotka
Lékařská fakulta
UT WoS
000405471300002
Klíčová slova anglicky
Bioaccumulation; Heavy metals; Maize; Reactive oxygen species; Root anatomy
Štítky
Příznaky
Mezinárodní význam, Recenzováno
Změněno: 7. 3. 2018 16:20, Soňa Böhmová
Anotace
V originále
Various fluorescence reagents are often used for the detection of oxidative stress, but more extensive comparison in the same study is rather rare. We tested five ROS-related and two non-ROS-related reagents in the roots of Zea mays germinated and growing in 1 or 100 mu M cadmium-enriched solution. Namely, "general'' ROS (CellROX Deep Red reagent and 20,70-dichlorodihydrofluorescein diacetate), hydrogen peroxide (Amplex UltraRed), superoxide radical (dihydroethidium), hydroxyl radical/peroxynitrite (aminophenyl fluorescein), nitric oxide (1,2-diaminoanthraquinone), and glutathione/-SH (monochlorobimane) indicators were tested. Both Cd doses stimulated signal of various ROS often extensively compared to control and mainly H2O2 differed between 1 and 100 mu M Cd. Signal of ROS was clearly visible in exodermis and vascular tissue through which cadmium is transported via transpiration stream. CellROX Deep Red reagent gives bright and clear signal on the root cross sections. The standard spectrophotometry (detection of H2O2 and superoxide) did not reveal differences between control and 1 mu M Cd, indicating that fluorescence microscopy is more sensitive to detect low change in oxidative balance. Nitric oxide and glutathione/SH signal was less different between control and Cd treatments, indicating their contribution to metal tolerance. Cd accumulation and translocation and the use of reagents under the excess of other metals are also discussed.