Receptor Biology Section, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892, USA.
J Neurosci. 2011 Apr 20;31(16):5921-30. doi: 10.1523/JNEUROSCI.6253-10.2011.
Metabotropic glutamate receptors (mGluRs) are G-protein-coupled receptors that modulate excitatory neurotransmission and synaptic plasticity. The group I mGluRs (mGluR1 and mGluR5) have long intracellular C-terminal domains, which interact with many proteins. Our previous studies identified calmodulin (CaM) as a strong regulator of mGluR5 trafficking and mGluR5-induced calcium signaling. Although it has been accepted that both mGluR1 and mGluR5 interact with CaM, we now show that CaM specifically binds mGluR5 and not mGluR1. We have identified a single critical residue in mGluR5 (L896) that is required for CaM binding. In mGluR1, mutation of the corresponding residue, V909, to leucine is sufficient to confer CaM binding to mGluR1. To investigate the functional effects of CaM binding, we examined the surface expression of mGluR1 and mGluR5 in hippocampal neurons. The mutation in mGluR1 (V909L) that confers CaM binding dramatically increases mGluR1 surface expression, whereas the analogous mutation in mGluR5 that disrupts CaM binding (L896V) decreases mGluR5 surface expression. In addition, the critical residue that alters CaM binding regulates mGluR internalization. Furthermore, we find that mGluR-mediated AMPA receptor endocytosis is enhanced by CaM binding to group I mGluRs. Finally, we show that calcium responses evoked by group I mGluRs are modulated by these mutations, which regulate CaM binding. Our findings elucidate a critical mechanism that specifically affects mGluR5 trafficking and signaling, and distinguishes mGluR1 and mGluR5 regulation.
代谢型谷氨酸受体(mGluRs)是 G 蛋白偶联受体,可调节兴奋性神经传递和突触可塑性。I 组 mGluRs(mGluR1 和 mGluR5)具有长的细胞内 C 端结构域,与许多蛋白质相互作用。我们之前的研究确定钙调蛋白(CaM)是 mGluR5 运输和 mGluR5 诱导的钙信号的强调节剂。尽管已经接受 mGluR1 和 mGluR5 都与 CaM 相互作用,但我们现在表明 CaM 特异性结合 mGluR5 而不是 mGluR1。我们已经确定了 mGluR5 中一个单一的关键残基(L896),该残基是 CaM 结合所必需的。在 mGluR1 中,将相应残基 V909 突变为亮氨酸足以使 CaM 结合到 mGluR1 上。为了研究 CaM 结合的功能影响,我们在海马神经元中检查了 mGluR1 和 mGluR5 的表面表达。赋予 CaM 结合的 mGluR1 突变(V909L)极大地增加了 mGluR1 的表面表达,而在 mGluR5 中破坏 CaM 结合的类似突变(L896V)则降低了 mGluR5 的表面表达。此外,改变 CaM 结合的关键残基调节 mGluR 内化。此外,我们发现 CaM 结合到 I 组 mGluRs 增强了 mGluR 介导的 AMPA 受体内吞作用。最后,我们发现这些突变调节了 I 组 mGluR 引发的钙反应,从而调节了 CaM 结合。我们的发现阐明了一个关键机制,该机制特异性地影响 mGluR5 的运输和信号转导,并区分了 mGluR1 和 mGluR5 的调节。