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[乙醇或电刺激诱导小鼠卵母细胞激活及孤雌发育过程中的细胞内游离钙变化]

[Intracellular free calcium changes of mouse oocytes during activation induced by ethanol or electrical stimulations and parthenogenetic development].

作者信息

Deng M Q, Fan B Q

机构信息

Jiangsu Academy of Agricultural Science, Nanjing.

出版信息

Shi Yan Sheng Wu Xue Bao. 1994 Sep;27(3):289-97.

PMID:7801722
Abstract

Oocytes collected 18-19 h after HCG injection were stimulated with 7-8% ethanol or electrical pulses (1.7 KV/cm field strength, 80-100 microseconds duration, 3-4 times, 5-6 min interval). The parthenogenetic embryos derived from the above-mentioned methods developed to blastocyst stage just like those developed from fertilized eggs. Mouse oocytes were rather sensitive to ethanol stimulation. More than 95% of the treated oocytes were activated after stimulation of 7-8% ethanol for 5 min. Multiple electrical stimulations induced higher activation percentages of oocytes than only single electrical stimulation (71.5% vs. 63.6%). Intact oocytes were loaded with fluorescent Ca2+ indicator fura-2 and intracellular free calcium changes during artificial activation were measured by fluorescence detector. The results showed that ethanol could induce repetitive transient Ca2+ concentration increase in activated oocytes. Single electrical stimulation only induced single free calcium concentration elevation in oocyte while multiple electrical pulses could induce repetitive Ca2+ increase (each electrical pulse elicited the corresponding Ca2+ concentration peak). The pronuclei were not observed in the oocytes which had not exhibited calcium concentration rise during activation. Apart from electrical stimulation parameter, sufficient amount of Ca2+ in electric medium was crucial to mouse oocyte activation when stimulated with electrical pulses. The oocytes were hardly activated by electrical stimulations in a medium without Ca2+ even with longer pulse duration and the intracellular free calcium concentration in the oocytes showed no elevation. This indicates that the inflow of extracellular Ca2+ from tiny pores across the oocyte membrane caused by electrical stimulation is the main source of intracellular free calcium increase.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在注射人绒毛膜促性腺激素(HCG)18 - 19小时后采集的卵母细胞,用7 - 8%乙醇或电脉冲(场强1.7千伏/厘米,持续时间80 - 100微秒,3 - 4次,间隔5 - 6分钟)进行刺激。上述方法获得的孤雌生殖胚胎发育至囊胚阶段,与受精卵发育而来的胚胎相似。小鼠卵母细胞对乙醇刺激相当敏感。用7 - 8%乙醇刺激5分钟后,超过95%的处理卵母细胞被激活。多次电刺激诱导的卵母细胞激活率高于单次电刺激(71.5%对63.6%)。完整的卵母细胞加载荧光钙指示剂fura - 2,通过荧光检测器测量人工激活过程中细胞内游离钙的变化。结果表明,乙醇可诱导激活的卵母细胞中钙离子浓度反复短暂升高。单次电刺激仅诱导卵母细胞内游离钙浓度单次升高,而多次电脉冲可诱导钙离子反复升高(每个电脉冲引发相应的钙离子浓度峰值)。在激活过程中未出现钙浓度升高的卵母细胞中未观察到原核。除电刺激参数外,电刺激时电介质中足够量的钙离子对小鼠卵母细胞激活至关重要。即使脉冲持续时间更长,在无钙的介质中电刺激也很难激活卵母细胞,且卵母细胞内游离钙浓度无升高。这表明电刺激引起的细胞外钙离子通过卵母细胞膜微孔流入是细胞内游离钙增加的主要来源。(摘要截断于250字)

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