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培养细胞中乙酰胆碱酯酶的超微结构定位。III. 经二异丙基氟磷酸处理的胚胎肌肉

Ultrastructural localization of acetylcholinesterase in cultured cells. III. DFP treated embryo muscle.

作者信息

Golder T K, Nieberg P S, Wilson B W

出版信息

J Histochem Cytochem. 1978 Sep;26(9):719-28. doi: 10.1177/26.9.568640.

Abstract

Brief treatment with 10(-4)M diisopropylfluorophosphate (DEP) irreversibly inactivates acetylcholinesterase (E.C.3.1.1.7; acetylcholine hydrolase) (AChE) activity in 10 day old chick embryonic muscle cultures. Electron microscopic cytochemistry was employed to follow the distribution of new AChE during recovery from DEP treatment. In normal 10 day cultures of embryo pectoralis muscles AChE is localized in the nuclear envelope, perinuclear sarcoplasm, sarcotubular system, subsurface vesicles and bound outside the cells. Immediately after DFP treatment AChE activity is absent in large myotubes. Within 15 min, activity is randomly present in small amounts in the sarcotubular system and nuclear envelope. There is a dramatic increase in activitv in the nuclear envelope during the 1st hr of recovery, and connections between the nuclear envelope and sarcotubular system are often seen. The next few hr of recovery show increased AChE activity. By 4 hr activity approaches that of controls. Six to 8 hr after treatment, AChE activity can be detected spectrophotometrically in the medium and can be seen bound outside the cells with the electron microscope. The spatial and temporal patterns of AChE activity demonstrate that the recovery of AChE and its mobilization and release from DFP-treated cells are not governed solely by the levels attained by the enzyme in the cultured embryo muscle.

摘要

用10⁻⁴M二异丙基氟磷酸酯(DEP)进行短暂处理可使10日龄鸡胚肌肉培养物中的乙酰胆碱酯酶(E.C.3.1.1.7;乙酰胆碱水解酶)(AChE)活性不可逆地失活。采用电子显微镜细胞化学方法追踪DEP处理后恢复过程中新AChE的分布情况。在正常的10日龄胚胎胸肌培养物中,AChE定位于核膜、核周肌浆、肌管系统、表面下囊泡以及细胞外结合部位。DFP处理后即刻,大型肌管中不存在AChE活性。在15分钟内,活性随机少量出现在肌管系统和核膜中。在恢复的第1小时内,核膜中的活性急剧增加,并且经常可见核膜与肌管系统之间的连接。恢复的接下来几个小时显示AChE活性增加。到4小时时,活性接近对照水平。处理后6至8小时,可通过分光光度法在培养基中检测到AChE活性,并且用电子显微镜可以看到其结合在细胞外。AChE活性的空间和时间模式表明,AChE的恢复及其从DFP处理的细胞中的动员和释放并非仅由培养的胚胎肌肉中该酶所达到的水平所决定。

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