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Single-channel activations and concentration jumps: comparison of recombinant NR1a/NR2A and NR1a/NR2D NMDA receptors

机译:单通道激活和浓度跳跃:重组NR1a / NR2A和NR1a / NR2D NMDA受体的比较

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摘要

We have expressed recombinant NR1a/NR2A and NR1a/NR2D N-methyl-D-aspartate (NMDA) receptor channels in Xenopus oocytes and made recordings of single-channel and macroscopic currents in outside-out membrane patches. For each receptor type we measured (a) the individual single-channel activations evoked by low glutamate concentrations in steady-state recordings, and (b) the macroscopic responses elicited by brief concentration jumps with high agonist concentrations, and we explore the relationship between these two sorts of observation.Low concentration (5–100 nM) steady-state recordings of NR1a/NR2A and NR1a/NR2D single-channel activity generated shut-time distributions that were best fitted with a mixture of five and six exponential components, respectively. Individual activations of either receptor type were resolved as bursts of openings, which we refer to as ‘super-clusters’.During a single activation, NR1a/NR2A receptors were open for 36 % of the time, but NR1a/NR2D receptors were open for only 4 % of the time. For both, distributions of super-cluster durations were best fitted with a mixture of six exponential components. Their overall mean durations were 35.8 and 1602 ms, respectively.Steady-state super-clusters were aligned on their first openings and averaged. The average was well fitted by a sum of exponentials with time constants taken from fits to super-cluster length distributions. It is shown that this is what would be expected for a channel that shows simple Markovian behaviour.The current through NR1a/NR2A channels following a concentration jump from zero to 1 mM glutamate for 1 ms was well fitted by three exponential components with time constants of 13 ms (rising phase), 70 ms and 350 ms (decaying phase). Similar concentration jumps on NR1a/NR2D channels were well fitted by two exponentials with means of 45 ms (rising phase) and 4408 ms (decaying phase) components. During prolonged exposure to glutamate, NR1a/NR2A channels desensitized with a time constant of 649 ms, while NR1a/NR2D channels exhibited no apparent desensitization.We show that under certain conditions, the time constants for the macroscopic jump response should be the same as those for the distribution of super-cluster lengths, though the resolution of the latter is so much greater that it cannot be expected that all the components will be resolvable in a macroscopic current. Good agreement was found for jumps on NR1a/NR2D receptors, and for some jump experiments on NR1a/NR2A. However, the latter were rather variable and some were slower than predicted. Slow decays were associated with patches that had large currents.
机译:我们已经在非洲爪蟾卵母细胞中表达了重组NR1a / NR2A和NR1a / NR2D N-甲基-D-天冬氨酸(NMDA)受体通道,并在外而外的膜片中记录了单通道和宏观电流。对于每种受体类型,我们测量(a)稳态记录中低谷氨酸浓度引起的单个单通道激活,以及(b)高激动剂浓度引起的短暂浓度跃变引起的宏观响应,并探讨这些之间的关系。两种观察。低浓度(5–100 nM)NR1a / NR2A和NR1a / NR2D单通道活性的稳态记录产生的关闭时间分布最好分别与5个和6个指数成分的混合物拟合。任一受体类型的单个激活都被解决为一连串的开口,我们称之为“超级簇”。在一次激活中,NR1a / NR2A受体打开的时间为36%,而NR1a / NR2D受体打开的时间为只有4%的时间。对于这两种情况,超级集群持续时间的分布最好与六个指数成分的混合物拟合。它们的平均平均持续时间分别为35.8和1602 ms.Steady-state超级群集在其第一个开口处对齐并取平均值。该平均值由指数总和很好地拟合,其中时间常数从拟合到超集群长度分布取。结果表明,这是显示简单马尔可夫行为的通道所期望的。浓度从0到1 mM谷氨酸的浓度跃变1毫秒后,流经NR1a / NR2A通道的电流与时间常数为13毫秒(上升阶段),70毫秒和350毫秒(衰减阶段)。 NR1a / NR2D通道上类似的浓度跃变通过两个指数分别为45 ms(上升阶段)和4408 ms(衰减阶段)很好地拟合。在长时间暴露于谷氨酸的过程中,NR1a / NR2A通道的脱敏时间常数为649毫秒,而NR1a / NR2D通道则没有明显的脱敏作用。我们表明,在某些条件下,宏观跳跃响应的时间常数应与那些相同对于超级集群长度的分布,尽管后者的分辨率非常大,以至于无法期望所有组件都可以在宏观电流下解析。对于NR1a / NR2D受体的跳跃和在NR1a / NR2A上的一些跳跃实验,发现了很好的一致性。但是,后者变化很大,并且有些速度比预期的要慢。衰减缓慢与大电流斑块有关。

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