One of the first events that occurs at fertilization is a
transient modification of the electrical properties of the
oocyte plasma membrane. The whole-cell voltage clamp
technique was used to demonstrate an outward ion current
and a hyperpolarization of the plasma membrane after
fertilization in bovine oocytes. These electrical events,
together with measurement of internal calcium concentrations,
were also recorded after injection with sperm
factor and exposure to parthenogenetic activators, such as
Ca2+ ionophore, ethanol and thapsigargin. Experiments
were carried out simultaneously in immature and in vitro
matured oocytes. Significant differences were recorded
in the activation current and hyperpolarization among
oocyte activators and between immature and matured
oocytes. However, outward ion current and Ca2+ release
showed similar dynamics. The injection of the calcium
chelator EGTA completely abolished both ion current and
hyperpolarization, indicating that these electrical events
are calcium dependent. Addition of specific calcium
releasers, such as 1,4,5-inositol trisphosphate (IP3) and
caffeine, triggered ion activation current and hyperpolarization
indicating that IP3 and ryanodine receptors are
active in both immature and matured oocytes. Different
ion channel inhibitors were used to characterize the
channels underlying outward currents. Only addition of
rIberiotoxin caused a complete inhibition of the current,
indicating the involvement of high conductance Ca2+-
activated K+ channels in generating activation current. In
conclusion, these findings provide evidence that bovine
oocyte activation is associated with Ca2+-dependent
electrical events. Oocytes have the potential to react to
different activators even when immature; however, oocyte
maturation seems to increase sensitivity to physiological
activators, such as spermatozoa and sperm factor, and
chemicals, such as ethanol
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