首页> 美国卫生研究院文献>The Journal of Physiology >Latencies of membrane currents evoked in Xenopus oocytes by receptor activation inositol trisphosphate and calcium.
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Latencies of membrane currents evoked in Xenopus oocytes by receptor activation inositol trisphosphate and calcium.

机译:爪蟾卵母细胞通过受体激活三磷酸肌醇和钙引起的膜电流潜伏期。

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摘要

1. Application of serum to Xenopus oocytes elicits an oscillatory chloride membrane current, which begins after a latency of several seconds or minutes, and is mediated through a phosphoinositide-calcium signalling pathway. We studied the characteristics and origin of this latency in voltage-clamped oocytes. 2. Bath application of low doses of serum evoked responses beginning after latencies of 1 min or more. The latency decreased with increasing dose and reached a minimal value of several seconds that did not decrease with further increases in serum concentration. Experiments to study this minimal latency were done by applying brief 'puffs' of serum and other agonists at high concentrations from a local extracellular pipette. 3. The mean latency of the response evoked by local serum application was about 7 s (at 22-24 degrees C), but individual responses showed a wide variation, from 2 s to over 20 s. Diffusion of serum from the pipette tip to the membrane did not contribute appreciably to this delay, since short (less than 100 ms) delays were obtained when KCl was applied in the same way. 4. Currents evoked by acetylcholine and serotonin, in oocytes induced to acquire muscarinic and serotonergic receptors following injection of brain messenger RNA, began following latencies similar to that of the serum response. 5. The response latency was shorter when serum was applied to the vegetal rather than the animal hemisphere of the oocyte, even though smaller currents were obtained. 6. The latency showed a slight dependence upon membrane potential, becoming shorter with depolarization. 7. Cooling to temperatures below about 22 degrees C produced a striking lengthening of the delay, corresponding to a Q10 of about 5. In contrast, above 22 degrees C the temperature dependence was slight, with a Q10 of about 1.25. 8. Intracellular injections of calcium and inositol 1,4,5-trisphosphate (IP3) evoked chloride currents with short (a few tens of milliseconds) latency. Short (100 ms) latency responses were also evoked when intracellularly loaded caged IP3 was photolysed by strong illumination, but weak illumination gave responses with latencies of over 1 min. 9. Measurements of intracellular free calcium, made with Fura-2 and Indo-1, showed an increase following serum application beginning coincident with the onset of the membrane current response.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:1.将血清应用于非洲爪蟾卵母细胞会引起振荡的氯化​​物膜电流,该电流在几秒钟或几分钟的潜伏期后开始,并通过磷酸肌醇-钙信号通路介导。我们研究了电压钳型卵母细胞中这种潜伏期的特征和起源。 2.潜伏期为1分钟或更长时间后,开始使用低剂量血清引起的反应。潜伏期随剂量增加而降低,并达到几秒钟的最小值,该最小值并未随血清浓度的进一步升高而降低。通过从局部细胞外移液器中以高浓度应用简短的“抽吸”血清和其他激动剂来进行研究,以研究这种最小的潜伏期。 3.局部血清应用引起的反应的平均潜伏期约为7 s(在22-24摄氏度下),但单个反应的变化范围很广,从2 s到20 s以上。血清从移液器吸头到膜的扩散对这种延迟没有明显的影响,因为当以相同的方式使用KCl时,获得的延迟很短(少于100毫秒)。 4.注射脑信使RNA后,诱导被诱导获得毒蕈碱和血清素能受体的卵母细胞中,乙酰胆碱和5-羟色胺引起的电流开始于类似于血清反应的潜伏期。 5.当将血清应用于植物而非卵母细胞的动物半球时,即使获得的电流较小,响应潜伏期也较短。 6.潜伏期显示出对膜电位的轻微依赖性,随着去极化而变短。 7.冷却到大约22摄氏度以下的温度会显着延长延迟,相当于Q5约为5。相反,在22摄氏度以上,温度依赖性很小,Q10约为1.25。 8.钙和肌醇1,4,5-三磷酸(IP3)的细胞内注射引起氯化物电流,潜伏期短(几十毫秒)。当通过强光照射细胞内装载的笼状IP3时,也会引起短暂的(100 ms)潜伏期响应,但弱光会产生超过1分钟的潜伏期响应。图9.用Fura-2和Indo-1进行的细胞内游离钙的测量结果表明,血清施用后与膜电流反应的发生同时开始增加。(摘要截短为400字)

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