The MEK inhibitor, U0126, alters fertilization-induced [Ca2+]i oscillation parameters and secretion: Differential effects associated with in vivo and in vitro meiotic maturation

2007 
Abstract Although mitogen-activated protein kinase (MAPK) is a well-known cell cycle regulator, emerging studies have also implicated its activity in the regulation of intracellular calcium concentration ([Ca 2+ ] i ) and secretion. Those studies raise the hypothesis that MAPK activity during oocyte maturation and early fertilization is required for normal egg Ca 2+ oscillations and cortical granule (CG) secretion. We extend the findings of [Lee, B., Vermassen, E., Yoon, S.-Y., Vanderheyden, V., Ito, J., Alfandari, D., De Smedt, H., Parys, J.B., Fissore, R.A., 2006. Phosphorylation of IP 3 R1 and the regulation of [Ca 2+ ] i responses at fertilization: a role for the MAP kinase pathway. Development 133, 4355–4365] by demonstrating acute effects on Ca 2+ oscillation frequency, amplitude, and duration in fertilized mouse eggs matured in vitro with the MAPK inhibitor, U0126. Frequency was increased, whereas amplitude and duration were greatly decreased. These effects were significantly reduced in eggs matured in vivo and fertilized in the presence of the inhibitor. Ionomycin studies indicated that intracellular Ca 2+ stores were differentially affected in eggs matured in vitro with U0126. Consistent with these effects on [Ca 2+ ] i elevation, fertilization-induced CG exocytosis and metaphase II exit were also reduced in in vitro-matured eggs with U0126, but not in those similarly treated after in vivo maturation. These results indicate that MAPK targets Ca 2+ regulatory proteins during both maturation and fertilization, as well as provide a new hypothesis for MAPK function, which is to indirectly regulate events of early development by controlling Ca 2+ oscillation parameters.
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