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Título
Monitoring mitochondrial [Ca2+] dynamics with rhod-2, ratiometric pericam and aequorin
Autor
Año del Documento
2010
Editorial
Elsevier Ltd.
Descripción
Producción Científica
Documento Fuente
Cell Calcium, 2010, vol. 48, p. 61-69
Resumo
The dynamics of mitochondrial [Ca2+] ([Ca2+]M) plays a key role in a variety of cellular processes. The
most important methods available to monitor [Ca2+]M are fluorescent dyes such as rhod-2 and specifically
targeted proteins such as aequorin and pericam. However, significant discrepancies, both quantitative
and qualitative, exist in the literature between the results obtained with different methods. We have
made here a systematic comparison of the response of several fluorescent dyes, rhod-2 and rhod-FF,
and two Ca2+-sensitive proteins, aequorin and pericam. Our results show that measurements obtained
with aequorin and pericam are consistent in terms of dynamic Ca2+ changes. Instead, fluorescent dyes
failed to follow Ca2+ changes adequately, especially during repetitive stimulation. In particular, measures
obtained with rhod-2 or rhod-FF evidenced the previously reported Ca2+-dependent inhibition of
mitochondrial Ca2+ uptake, but data obtained with aequorin or pericam under the same conditions did
not. The reason for the loss of response of fluorescent dyes is unclear. Loading with these dyes produced
changes in mitochondrial morphology and membrane potential, which were small and reversible at low
concentrations (1–2 M), but produced large and prolonged damage at higher concentrations. In addition,
cells loaded with low concentrations of rhod-2 suffered large changes in mitochondrial morphology
after light excitation. Our results suggest that [Ca2+]M data obtained with these dyes should be taken with
care.
Materias (normalizadas)
Calcio - Metabolismo
ISSN
0143-4160
Revisión por pares
SI
Idioma
eng
Derechos
openAccess
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