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Functional expression of distinct NMDA channel subunits tagged with green fluorescent protein in hippocampal neurons in culture
被引:84
作者:
Luo, JH
Fu, ZY
Losi, G
Kim, BG
Prybylowski, K
Vissel, B
Vicini, S
机构:
[1] Georgetown Univ, Sch Med, Dept Physiol & Biophys, Washington, DC 20007 USA
[2] Salk Inst Biol Studies, Mol & Neurobiol Lab, La Jolla, CA USA
关键词:
NMDA receptors;
green fluorescent protein;
excitatory postsynaptic current;
development;
D O I:
10.1016/S0028-3908(01)00188-5
中图分类号:
Q189 [神经科学];
学科分类号:
071006 ;
摘要:
We generated expression vectors for N-terminally green fluorescent protein-tagged NR2A and NR2B subunits (GFP-NR2A and GFP-NR2B). Both constructs expressed GFP and formed functional NMDA channels with similar properties to untagged controls when co-transfected with NR1 subunit partner in HEK293 cells. Primary cultured hippocampal neurons were transfected at five days in vitro with these vectors. Fifteen days after transfection, well-defined GFP clusters were observed for both GFP-NR2A and GFP-NR2B subunits being co-localized with endogenous NR1 subunit. Whole-cell recordings showed that the GFP-NR2A subunit determined the decay of NMDA-mediated miniature spontaneous excitatory postsynaptic currents (NMDA-mEPSCs) in transfected neurons. Live staining with anti-GFP antibody demonstrated the surface expression of GFP-NR2A and GFP-NR2B subunits that was partly co-localized a presynaptic marker. Localization of NMDA receptor clusters in dendrites was studied by co-transfection of CFP-actin and GFP-NR2 subunits followed by anti-GFP surface staining. Within one week after plating most surface NMDAR clusters were distributed on dendritic shafts. Later in development, a large portion of surface clusters for both GFP-NR2A and GFP-NR2B subunits were clearly localized at dendritic spines. Our report provides the basis for studies of NMDA receptor location together with dendritic dynamics in living neurons during synaptogenesis in vitro. (C) 2002 Published by Elsevier Science Ltd.
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页码:306 / 318
页数:13
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