Jasplakinolide (JAS), which induces microfilament polymerization and stabilization, inhibits microfilament-mediated events in murine oocyte maturation and fertilization in a fashion unlike the effects of cytochalasin B (CCB) and latranculin A (LAT A). JAS prevents egg polar body emission at a much lower concentration than either CCB or LAT A. Microfilament bundles were detected on the entire egg cortex after JAS exposure. Conversely, microfilament patterns did not change after exposure to CCB, and few microfilaments were observed after exposure to LAT A. Eggs that were allowed to recover from JAS were unable to recover normal microfilament organization. During oocyte maturation, JAS prevented both spindle migration to the oocyte cortex and first polar body emission. During in vitro fertilization, sperm head entered the eggs and formed pronuclei, but sperm tail entry, pronuclear centration, and second polar body emission were not detected. DNA synthesis occurs in these JAS-treated zygotes. JAS inhibited not only the formation, but also the disassembly, of incorporation cones. JAS was also found to prevent cortical granule exocytosis following artificial activation, and cortical granules were still beneath the plasma membrane even after activation. Finally, incorporation of microinjected nonmuscle actin into the microfilament network of mice eggs was delayed by JAS. We conclude that JAS acts as a microfilament inhibitor during maturation and fertilization and is more powerful than other inhibitors. Its mechanism differs in that it promotes assembly and stabilization of microfilaments. JAS is a novel cell permeable tool for the investigation of microfilament-dependent events in early mammalian development.

译文

:Jasplakinolide(JAS)诱导微丝聚合和稳定,抑制微丝介导的鼠卵母细胞成熟和受精中的事件,其方式不同于细胞松弛素B(CCB)和Latranculin A(LATA)的作用。 JAS可以防止鸡蛋极体发射,其浓度远低于CCB或LATA。在JAS暴露后,整个鸡蛋皮层均检测到微丝束。相反,暴露于CCB后微丝形态没有变化,暴露于LAT A后观察到很少的微丝。被允许从JAS中恢复的卵无法恢复正常的微丝组织。在卵母细胞成熟过程中,JAS既阻止了纺锤体向卵母细胞皮层的迁移,又阻止了第一极体的发射。在体外受精过程中,精子头进入卵内并形成原核,但未检测到精子尾部进入,原核集中和第二极体发射。这些JAS处理的受精卵发生DNA合成。 JAS不仅抑制了结合锥的形成,而且抑制了其分解。还发现JAS可以防止人工激活后皮质颗粒的胞吐作用,即使激活后皮质颗粒仍位于质膜下方。最终,通过JAS延迟了将微注射的非肌动蛋白掺入小鼠卵的微丝网络中。我们得出的结论是,JAS在成熟和受精过程中起微丝抑制剂的作用,并且比其他抑制剂更有效。其机制的不同之处在于,它促进了微丝的组装和稳定。 JAS是一种新型的细胞可渗透工具,用于研究哺乳动物早期发育中依赖于微丝的事件。

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