Abstract:The NMDA receptor NR1 subunit has four splice variants that differ in their C-terminal, cytoplasmic domain. We investigated the contribution of the C-terminal cassettes, C0, C1, C2, and C2', to trafficking of NR1 in heterologous cells and neurons. We identified an ER retention signal (RRR) in the C1 cassette of NR1, which is similar to the RXR motif in ATP-sensitive K(+) channels (Zerangue et al., 1999). We found that surface expression of NR1-3, which contains C1, is due to a site on the C2' cassette, which i… Show more
“…Remarkably, although the K526N mutant did not diminish current, surface expression was reduced by 40% (Figure 3(a ) ). To confirm the impact of K526N in trafficking in mammalian cells, we fused the AB domain to the membrane protein Tac (interleukin-2 receptor α subunit) and monitored surface expression by flow cytometry in HEK293T cells as previously described [15,33,34]. The results confirmed that this mutation caused a reduction in surface expression (Figure 3(b)).10.1080/19336950.2018.1511512-F0003Figure 3.Surface expression is reduced in K526N and R333Q mutants.…”
Heteromers of Kv7.2/Kv7.3 subunits constitute the main substrate of the neuronal M-current that limits neuronal hyper-excitability and firing frequency. Calmodulin (CaM) binding is essential for surface expression of Kv7 channels, and disruption of this interaction leads to diseases ranging from mild epilepsy to early onset encephalopathy. In this study, we addressed the impact of a charge neutralizing mutation located at the periphery of helix B (K526N). We found that, CaM binding and surface expression was impaired, although current amplitude was not altered. Currents were reduced at a faster rate after activation of a voltage-dependent phosphatase, suggesting that phosphatidylinositol-4,5-bisphosphate (PIP2) binding was weaker. In contrast, a charge neutralizing mutation located at the periphery of helix A (R333Q) did not affect CaM binding, but impaired trafficking and led to a reduction in current amplitude. Taken together, these results suggest that disruption of CaM-dependent or CaM-independent trafficking of Kv7.2/Kv7.3 channels can lead to pathology regardless of the consequences on the macroscopic ionic flow through the channel.
“…Remarkably, although the K526N mutant did not diminish current, surface expression was reduced by 40% (Figure 3(a ) ). To confirm the impact of K526N in trafficking in mammalian cells, we fused the AB domain to the membrane protein Tac (interleukin-2 receptor α subunit) and monitored surface expression by flow cytometry in HEK293T cells as previously described [15,33,34]. The results confirmed that this mutation caused a reduction in surface expression (Figure 3(b)).10.1080/19336950.2018.1511512-F0003Figure 3.Surface expression is reduced in K526N and R333Q mutants.…”
Heteromers of Kv7.2/Kv7.3 subunits constitute the main substrate of the neuronal M-current that limits neuronal hyper-excitability and firing frequency. Calmodulin (CaM) binding is essential for surface expression of Kv7 channels, and disruption of this interaction leads to diseases ranging from mild epilepsy to early onset encephalopathy. In this study, we addressed the impact of a charge neutralizing mutation located at the periphery of helix B (K526N). We found that, CaM binding and surface expression was impaired, although current amplitude was not altered. Currents were reduced at a faster rate after activation of a voltage-dependent phosphatase, suggesting that phosphatidylinositol-4,5-bisphosphate (PIP2) binding was weaker. In contrast, a charge neutralizing mutation located at the periphery of helix A (R333Q) did not affect CaM binding, but impaired trafficking and led to a reduction in current amplitude. Taken together, these results suggest that disruption of CaM-dependent or CaM-independent trafficking of Kv7.2/Kv7.3 channels can lead to pathology regardless of the consequences on the macroscopic ionic flow through the channel.
“…terminus of NR1 influences intracellular distribution (Ehlers et al, 1995) and surface expression (Okabe et al, 1999;Standley et al, 2000) of NR1/NR2 heteromers. To identify the relevant trafficking signals in NR1 and to minimize effects of NR2 subunits and other NR1 domains, we chose to isolate the contribution of NR1 C-terminal domains using Tac-NR1 chimeras.…”
Section: Discussionmentioning
confidence: 99%
“…1 A). When expressed alone in heterologous cells, these subtypes exhibit differential subcellular localization (Ehlers et al, 1995) and are differentially expressed at the cell surface (Okabe et al, 1999;Standley et al, 2000) (data not shown). To determine which domains of NR1 are responsible for regulating NR1 surface expression, we constructed chimeric receptor molecules consisting of the human interleukin-2 receptor ␣ subunit (Tac) tagged with portions of the intracellular C terminal domain of the NR1 subunit (Leonard et al, 1983;Tan et al, 1998;Craven and Bredt, 2000).…”
Section: Identification Of Trafficking Signals In the C Terminal Domamentioning
Formation of mature excitatory synapses requires the assembly and delivery of NMDA receptors to the neuronal plasma membrane. A key step in the trafficking of NMDA receptors to synapses is the exit of newly assembled receptors from the endoplasmic reticulum (ER). Here we report the identification of an RXR-type ER retention/retrieval motif in the C-terminal tail of the NMDA receptor subunit NR1 that regulates receptor surface expression in heterologous cells and in neurons. In addition, we show that PKC phosphorylation and an alternatively spliced consensus type I PDZ-binding domain suppress ER retention. These results demonstrate a novel quality control function for alternatively spliced C-terminal domains of NR1 and implicate both phosphorylation and potential PDZ-mediated interactions in the trafficking of NMDA receptors through early stages of the secretory pathway.
“…3 Alternative splicing of the C2 cassette regulates cellular trafficking and cell surface expression of the NMDA receptor. [14][15][16] NMDA receptors are predominantly expressed in the postsynaptic membrane where they interact with an intracellularly organized multiprotein complex termed the postsynaptic density (PSD). 17,18 Proteins of the membrane-associated guanylate-kinase family (MAGUKs), a group of PSD-associated proteins characterized by the presence of guanylate kinase, PDZ and Src homology 3 (SH3) protein-interacting domains, function as scaffolding and organizer proteins of the PSD.…”
Abnormal expression of the N-Methyl-D-Aspartate (NMDA) receptor and its interacting molecules of the postsynaptic density (PSD) are thought to be involved in the pathophysiology of schizophrenia. Frontal regions of neocortex including dorsolateral prefrontal (DLPFC) and anterior cingulate cortex (ACC) are essential for cognitive and behavioral functions that are affected in schizophrenia. In this study, we have measured protein expression of two alternatively spliced isoforms of the NR1 subunit (NR1 C2 and NR1 C2 0 ) as well as expression of the NR2A-D subunits of the NMDA receptor in DLPFC and ACC in post-mortem samples from elderly schizophrenic patients and a comparison group. We found significantly increased expression of NR1 C2 0 but not of NR1 C2 in ACC, suggesting altered NMDA receptor cell membrane expression in this cortical area. We did not find significant changes in the expression of either of the NR1 isoforms in DLPFC. We did not detect changes of any of the NR2 subunits studied in either cortical area. In addition, we studied expression of the NMDAinteracting PSD molecules NF-L, SAP102, PSD-95 and PSD-93 in ACC and DLPFC at both transcriptional and translational levels. We found significant changes in the expression of NF-L in DLPFC, and PSD-95 and PSD-93 in ACC; increased transcript expression was associated with decreased protein expression, suggesting abnormal translation and/or accelerated protein degradation of these molecules in schizophrenia. Our findings suggest abnormal regional processing of the NMDA receptor and its associated PSD molecules, possibly involving transcription, translation, trafficking and protein stability in cortical areas in schizophrenia.
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