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Effects of hypoxia on rat hippocampal neurones in vitro.

机译:缺氧对大鼠海马神经元的影响。

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1. The effects of hypoxia on the rat hippocampal CA1 neurones in tissue slices of the rat brain were studied in vitro by intracellular recording. 2. In response to superfusion of a hypoxic medium equilibrated with 95% N2-5% CO2, a majority of the neurones showed a hyperpolarization of 5-15 mV in amplitude and 4-12 min in duration. The hyperpolarization was, in turn, followed by a slow depolarization which within 20 min of hypoxic exposure reached a plateau level of about 25 mV above the pre-hypoxic resting potential. Both the initial hyperpolarization and subsequent depolarization were associated with a reduction in membrane resistance. 3. The hyperpolarization reversed in polarity at a membrane potential of -83 mV. There was an almost linear relationship between amplitude of the hyperpolarization and membrane potential. The hyperpolarization was markedly enhanced in potassium-free media and was depressed in high-potassium solutions. 4. The hyperpolarization was not significantly affected by low-chloride or low-sodium medium or by solution containing tetraethylammonium (10 mM), 4-aminopyridine (1.5 mM) or caesium (3 mM). Moreover, intracellular injection of ethyleneglycol-bis-(beta-aminoethylether)N,N-tetraacetic acid (EGTA) did not alter the hyperpolarization. On the other hand, barium (0.5 mM)-containing medium reduced the amplitude of the hyperpolarization by 20-40%. 5. Superfusion of ouabain (5-7 microM)-containing medium in normoxic conditions produced hyperpolarizing and depolarizing responses similar to those elicited by hypoxic exposure. The slow depolarization was also mimicked by elevation of the extracellular potassium concentration to 10-20 mM. 6. Evoked i.p.s.p.s were abolished within 4 min of hypoxic exposure while evoked e.p.s.p.s were maintained for about 20 min of hypoxic superfusion. Soma spikes of the neurones elicited by a depolarizing pulse were also well preserved. Their threshold was, however, raised, concomitant with a decrease in the peak amplitude. 7. When the slice was reoxygenated after 20-40 min of hypoxic exposure, the neurones immediately began to repolarize and showed a transient hyperpolarization of 5-10 mV in amplitude and 1-2 min in duration. The membrane potential, input resistance and action potential returned to the pre-hypoxic levels after 15-20 min of reoxygenation. The amplitude of the reoxygenation-induced hyperpolarization was not significantly changed when the membrane was hyperpolarized or depolarized. The hyperpolarization was eliminated by potassium-free medium or solution containing ouabain (1 microM).(ABSTRACT TRUNCATED AT 400 WORDS)
机译:1.通过细胞内记录体外研究了缺氧对大鼠脑组织切片中海马CA1神经元的影响。 2.响应于用95%N2-5%CO2平衡的低氧介质的灌注,大多数神经元显示出5-15 mV的超极化幅度和4-12分钟的持续时间。反过来,超极化之后是缓慢的去极化,低氧暴露在20分钟内达到了高于低氧前静息电位约25 mV的平稳水平。最初的超极化和随后的去极化都与膜电阻的降低有关。 3.超极化在-83 mV的膜电位下极性反转。超极化的幅度与膜电位之间几乎呈线性关系。在无钾培养基中,超极化显着增强,而在高钾溶液中则被抑制。 4.超极化不受低氯化物或低钠介质或含有四乙铵(10 mM),4-氨基吡啶(1.5 mM)或铯(3 mM)的溶液的显着影响。而且,细胞内注射乙二醇-双-(β-氨基乙基醚)N,N-四乙酸(EGTA)不会改变超极化。另一方面,含钡(0.5 mM)的介质可将超极化幅度降低20-40%。 5.在常氧条件下对含哇巴因(5-7 microM)的培养基进行过灌注,产生了与低氧暴露相似的超极化和去极化反应。缓慢的去极化也可以通过将细胞外钾浓度提高到10-20 mM来模拟。 6.在低氧暴露的4分钟内废除诱发的腹膜内注射,而诱发的e.p.s.p.s维持低氧超融合约20分钟。还可以很好地保存由去极化脉冲引起的神经元的索马峰。但是,它们的阈值却升高了,同时峰值幅度也随之降低了。 7.缺氧暴露20-40分钟后对切片进行复氧后,神经元立即开始重新极化,并显示幅度为5-10 mV,持续时间为1-2分钟的瞬时超极化。复氧15-20分钟后,膜电位,输入阻力和动作电位恢复到缺氧前的水平。当膜超极化或去极化时,复氧诱导的超极化的幅度没有明显改变。通过无钾培养基或含哇巴因(1 microM)的溶液消除了超极化现象。(以400字截短的抽象截断值)

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