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Pharmacological and anatomical separation of calcium currents in rat dentate granule neurones in vitro.

机译:大鼠齿状颗粒神经元中钙电流的药理和解剖学分离。

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摘要

1. Rat dentate granule neurones in hippocampal slices were voltage-clamped at 21-23 degrees C using CsCl-filled microelectrodes. The perfusate contained TTX and K+ channel blockers to isolate pharmacologically inward Ca2+ currents. 2. From hyperpolarized holding potentials of -65 to -85 mV, depolarizing test potentials to between -50 and -40 mV elicited a transient (100-200 ms) low-threshold (TLT) current which was also elicited from more depolarized holding potentials following hyperpolarizing voltage steps of -40 mV or greater. 3. Larger depolarizing steps from a hyperpolarized holding potential triggered a large (2-6 nA), transient high-threshold (THT) inward current, rapidly peaking and decaying over 500 ms, followed by a sustained inward current component. 4. At depolarized holding potentials (-50 to -20 mV), the THT current was apparently inactivated and a sustained high-threshold (SHT) inward current was evident during depolarizing voltage steps of 10 mV or more. 5. From hyperpolarized holding potentials with depolarizing voltage steps of 10-30 mV, most neurones demonstrated a small-amplitude, sustained low-threshold (SLT) inward current with similar characteristics to the SHT current. 6. Zero-Ca2+ perfusate or high concentrations of Ca2+ channel blockers (Cd2+, Mn2+ or Ni2+) diminished or abolished all inward currents. 7. Repetitive voltage step activation of each current at 0.5 Hz reduced the large THT current to less than 25% of an unconditioned control current, reduced the SHT current by 50%, but had little effect on the TLT current. 8. A low concentration of Cd2+ (50 microM) blocked the THT and SHT currents with little effect on the TLT current. Nimodipine (1 microM) attenuated the SHT current. Ni2+ (100 microM) selectively attenuated the TLT current. 9. In low-Ca2+ perfusate, high concentrations of Ca2+ (10-15 mM), focally applied to different parts of the neurone, increased the THT current when applied to the dendrites, the SHT current when applied to the soma and the TLT current at all locations. Conversely, in regular perfusate, Cd2+ (1-5 mM), focally applied to the dendrites decreased the THT current and somatic applications decreased the SHT current. The TLT current was diminished regardless of the site of Cd2+ application. 10. These results suggest the existence of three different Ca2+ currents in dentate granule cells separable by their activation and inactivation characteristics, pharmacology and site of initiation.
机译:1.使用充满CsCl的微电极将海马切片中的大鼠齿状颗粒神经元电压钳制在21-23摄氏度。灌注液包含TTX和K +通道阻滞剂,以隔离药理学上的Ca2 +电流。 2.从-65至-85 mV的超极化保持电势,去极化测试电势至-50至-40 mV之间会引起瞬态(100-200 ms)低阈值(TLT)电流,这也由更多的去极化保持电势引起遵循-40 mV或更高的超极化电压阶跃。 3.从超极化保持电势开始的较大去极化步骤触发了大的(2-6 nA)瞬态高阈值(THT)内向电流,在500 ms内迅速达到峰值并衰减,随后是持续的内向电流分量。 4.在去极化的保持电势(-50至-20 mV)下,THT电流明显失活,并且在10 mV或更高的去极化电压阶跃期间,明显存在持续的高阈值(SHT)内向电流。 5.从具有10-30 mV的去极化电压阶跃的超极化保持电势,大多数神经元表现出小幅度,持续的低阈值(SLT)内向电流,其特性与SHT电流相似。 6.零Ca2 +灌注液或高浓度的Ca2 +通道阻滞剂(Cd2 +,Mn2 +或Ni2 +)减小或消除了所有内向电流。 7.每个电流以0.5 Hz的重复电压阶跃激活将大的THT电流减小到小于未调节控制电流的25%,将SHT电流减小50%,但对TLT电流影响很小。 8.低浓度的Cd2 +(50 microM)阻止了THT和SHT电流,而对TLT电流的影响很小。尼莫地平(1 microM)减弱了SHT电流。 Ni2 +(100 microM)有选择地衰减了TLT电流。 9.在低Ca2 +灌流液中,高浓度的Ca2 +(10-15 mM)集中应用于神经元的不同部位,当应用于树突时会增加THT电流,应用于体细胞时会增加SHT电流,而TLT电流会增加在所有地点。相反,在常规灌注液中,集中施用于树突的Cd2 +(1-5 mM)降低了THT电流,体细胞施用降低了SHT电流。无论使用Cd2 +的位置如何,TLT电流均减小。 10.这些结果表明,在齿状颗粒细胞中存在三种不同的Ca2 +电流,这些电流可以通过其激活和失活特性,药理作用和起始位点来分离。

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