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Título
Dynamics of mitochondrial [Ca2+] measured with the low-Ca2+-affinity dye rhod-5N
Autor
Año del Documento
2012
Editorial
Elsevier Ltd.
Descripción
Producción Científica
Documento Fuente
Cell Calcium, 2012, vol. 51, p. 65-71
Abstract
Available methods to measure mitochondrial [Ca2+] ([Ca2+]M) include both targeted proteins and fluorescent
dyes. Targeted proteins usually report much higher [Ca2+]M values than fluorescent dyes, up to two
orders of magnitude. However, we show here that the low-Ca2+-affinity dye rhod-5N provides [Ca2+]M
values similar to those reported by targeted aequorin, suggesting that the discrepancies are mainly due
to the higher Ca2+-affinity of the fluorescent dyes used. We find rhod-5N has an apparent in situ intramitochondrial
Kd around 0.5 mM. Addition of Ca2+ buffers containing between 4.5 and 10 M [Ca2+] to
permeabilized cells loaded with rhod-5N induced increases in calibrated [Ca2+]M up to the 100 M–1 mM
range, which were dependent on mitochondrial membrane potential. Ca2+ release from mitochondria was
largely dependent on [Na+]. We have then used rhod-5N loaded cells to investigate the [Ca2+]M response
to agonist stimulation at the single-cell and subcellular level.The [Ca2+]M peaks induced by histamine
varied by nearly 10-fold among different cells, with a mean about 25 M. In the presence of the Ca2+
uniporter stimulator kaempferol, the [Ca2+]M peaks induced by histamine were also highly variable, and
the mean [Ca2+]M peak was 3-fold higher. Simultaneous measurement of cytosolic and mitochondrial
[Ca2+] peaks showed little correlation among the heights of the peaks in both compartments. Studying
the [Ca2+]M peaks at the subcellular level, we found significant heterogeneities among regions in the
same cell. In particular, the [Ca2+]M increase in mitochondrial regions close to the nucleus was more than
double that of mitochondrial regions far from the nucleus.
Materias (normalizadas)
Mitocondria
ISSN
0143-4160
Revisión por pares
SI
Idioma
eng
Derechos
openAccess
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