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The dynamics of MAPK inactivation at fertilization in mouse eggs

机译:小鼠卵受精过程中MAPK失活的动力学

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Egg activation at fertilization in mammals is initiated by prolonged Ca2+ oscillations that trigger the completion of meiosis and formation of pronuclei. A fall in mitogen-activated protein kinase (MAPK) activity is essential for pronuclear formation, but the precise timing and mechanism of decline are unknown. Here, we have measured the dynamics of MAPK pathway inactivation during fertilization of mouse eggs using novel chemiluminescent MAPK activity reporters. This reveals that the MAPK activity decrease begins during the Ca2+ oscillations, but MAPK does not completely inactivate until after pronuclear formation. The MAPKs present in eggs are Mos, MAP2K1 and MAP2K2 (MEK1 and MEK2, respectively) and MAPK3 and MAPK1 (ERK1 and ERK2, respectively). Notably, the MAPK activity decline at fertilization is not explained by upstream destruction of Mos, because a decrease in the signal from a Mos-luciferase reporter is not associated with egg activation. Furthermore, Mos overexpression does not affect the timing ofMAPK inactivation or pronuclear formation. However, the late decrease in MAPK could be rapidly reversed by the protein phosphatase inhibitor, okadaic acid. These data suggest that the completion of meiosis in mouse zygotes is driven by an increased phosphatase activity and not by a decline in Mos levels or MEK activity.
机译:哺乳动物受精过程中卵的活化是由延长的Ca2 +振荡引发的,Ca2 +振荡触发了减数分裂的完成和原核的形成。有丝分裂原激活的蛋白激酶(MAPK)活性的下降对于原核形成至关重要,但是下降的确切时间和机制尚不清楚。在这里,我们已经使用新型化学发光MAPK活性报道基因测量了小鼠卵子受精过程中MAPK途径失活的动力学。这表明,MAPK活性下降是在Ca2 +振荡期间开始的,但是直到原核形成后MAPK才完全失活。卵中存在的MAPK为Mos,MAP2K1和MAP2K2(分别为MEK1和MEK2)以及MAPK3和MAPK1(分别为ERK1和ERK2)。值得注意的是,受精过程中MAPK活性的下降不能用Mos的上游破坏来解释,因为来自Mos-萤光素酶报告基因的信号下降与卵的活化无关。此外,Mos过表达不会影响MAPK失活或前核形成的时间。但是,蛋白磷酸酶抑制剂冈田酸可以迅速逆转MAPK的后期减少。这些数据表明,小鼠受精卵减数分裂的完成是由增加的磷酸酶活性而不是由Mos水平或MEK活性的下降驱动的。

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