首页> 美国卫生研究院文献>The Journal of Physiology >Effects of alcohols on responses evoked by inositol trisphosphate in Xenopus oocytes.
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Effects of alcohols on responses evoked by inositol trisphosphate in Xenopus oocytes.

机译:酒精对非洲爪蟾卵母细胞中三磷酸肌醇诱发的反应的影响。

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摘要

1. The effects of ethanol and other alcohols on inositol 1,4,5-trisphosphate (InsP3) signalling were studied in Xenopus oocytes by the use of flash photolysis of caged InsP3. Calcium liberation induced by InsP3 was monitored by voltage-clamp recording of Ca(2+)-activated membrane currents, and by fluorescence of the Ca2+ indicator Fluo-3. 2. Membrane current and fluorescence Ca2+ signals evoked by light flashes giving small responses were initially potentiated by bath application of ethanol (80-400 mM). However, the responses subsequently declined while ethanol was present and were strongly reduced or suppressed when it was removed. 3. These effects did not arise artifactually from changes in photolysis of caged InsP3, as similar results were seen with responses evoked by intracellular injections of InsP3. Also, the effects on the membrane current did not arise primarily through actions on the Ca(2+)-dependent Cl- channels, since currents evoked by intracellular injections of Ca2+ were little changed by ethanol. 4. Ethanol reduced the threshold level of InsP3 required to cause Ca2+ liberation. Thus, potentiation was most prominent with small responses evoked by brief light flashes, whereas the predominant effect on larger responses was inhibitory. 5. The facilitatory and inhibitory actions of ethanol persisted after removing extracellular Ca2+. 6. Intracellular injections of ethanol produced an initial inhibition of InsP3 responses, followed, in some oocytes, by a potentiation. 7. Methanol had little effect on InsP3 responses, whereas butanol and other long-chain alcohols produced strong inhibition, but little or no potentiation. 8. We conclude that extracellular application of ethanol produces a rapid potentiation of InsP3-mediated Ca2+ liberation, and a more slowly developing inhibition. The potentiation may arise through stimulation of InsP3 formation at the plasma membrane, whereas the inhibition occurs more deeply in the cell. Both actions were evident at relatively low concentrations (a few tens of millimoles per litre), and might thus be important in the behavioural effects of ethanol intoxication.
机译:1.在非洲爪蟾卵母细胞中,通过笼装InsP3的快速光解研究了乙醇和其他醇类对肌醇1,4,5-三磷酸(InsP3)信号传导的影响。通过电压钳记录Ca(2+)激活的膜电流和Ca2 +指示剂Fluo-3的荧光来监测InsP3诱导的钙释放。 2.首先通过浴液(80-400 mM)的乙醇增强由闪烁引起的膜电流和荧光Ca2 +信号的响应,从而产生较小的响应。然而,当存在乙醇时,响应随后下降,并且当去除乙醇时,响应被强烈降低或抑制。 3.这些影响不是由于笼中InsP3的光解变化而人为地产生的,因为通过细胞内注射InsP3引起的反应可以看到类似的结果。同样,对膜电流的影响主要不是通过对Ca(2+)依赖的Cl-通道的作用而引起的,因为乙醇胞内注射Ca2 +引起的电流几乎没有变化。 4.乙醇降低了导致Ca2 +释放所需的InsP3阈值水平。因此,增强作用在短暂的闪光引起的小反应中最为突出,而对大反应的主要作用是抑制作用。 5.去除细胞外Ca2 +后,乙醇的促进和抑制作用仍然存在。 6.胞内注射乙醇会最初抑制InsP3反应,然后在某些卵母细胞中产生增强作用。 7.甲醇对InsP3反应的影响很小,而丁醇和其他长链醇产生强烈的抑制作用,但几乎没有或没有增强作用。 8.我们得出的结论是,乙醇的细胞外应用产生InsP3介导的Ca2 +释放的快速增强,并产生更缓慢的抑制作用。增强作用可能是通过刺激质膜上InsP3的形成而产生的,而抑制作用则在细胞内更深处发生。在相对较低的浓度(每升几十毫摩尔)下,这两种作用都很明显,因此可能在乙醇中毒的行为效应中很重要。

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