首页> 外文期刊>The Journal of Neuroscience: The Official Journal of the Society for Neuroscience >DRPEER: a motif in the extracellular vestibule conferring high Ca2+ flux rates in NMDA receptor channels.
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DRPEER: a motif in the extracellular vestibule conferring high Ca2+ flux rates in NMDA receptor channels.

机译:DRPEER:胞外前庭中的一个基序,可在NMDA受体通道中赋予较高的Ca2 +通量率。

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摘要

The high flux rate of Ca2+ through NMDA receptor (NMDAR) channels is critical for their biological function and may depend on a Ca2+ binding site in the extracellular vestibule. We screened substitutions of hydrophilic residues exposed in the vestibule and identified a cluster of charged residues and a proline, the DRPEER motif, positioned C terminal to M3, that is unique to the NR1 subunit. Charge neutralization or conversion of residues in DRPEER altered fractional Ca2+ currents in a manner consistent with its forming a binding site for Ca2+. Similarly, in a mutant channel in which all of the negative charges are neutralized (ARPAAR), the block by extracellular Ca2+ of single-channel current amplitudes is attenuated. In these same channels, the block by extracellular Mg2+ is unaffected. DRPEER is located extracellularly, and its contribution to Ca2+ influx is distinct from that of the narrow constriction. We conclude that key residues in DRPEER, acting as an external binding site for Ca2+, along witha conserved asparagine in the M3 segment proper, contribute to the high fractional Ca2+ currents in these channels under physiological conditions. Therefore, these domains represent critical molecular determinants of NMDAR function in synaptic physiology.
机译:Ca2 +通过NMDA受体(NMDAR)通道的高通量速率对其生物学功能至关重要,并且可能取决于细胞外前庭中的Ca2 +结合位点。我们筛选了暴露在前庭中的亲水性残基的取代基,并确定了一个带电残基簇和一个脯氨酸(DRPEER基序),该脯氨酸位于M3的C端,这对NR1亚基是唯一的。电荷中和或DRPEER中残基的转化以与其形成Ca2 +结合位点一致的方式改变了部分Ca2 +电流。类似地,在所有负电荷均被中和的突变通道中(ARPAAR),单通道电流幅度的细胞外Ca2 +阻滞被减弱。在这些相同的通道中,细胞外Mg2 +的阻滞作用不受影响。 DRPEER位于细胞外,其对Ca2 +内流的贡献不同于狭窄的颈缩。我们得出的结论是,在生理条件下,DRPEER中的关键残基充当Ca2 +的外部结合位点,以及M3区段中适当的保守的天冬酰胺,有助于这些通道中高比例的Ca2 +电流。因此,这些域代表在突触生理学中NMDAR功能的关键分子决定因素。

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