MODULATION OF MUSCARINIC SIGNALING IN PC12 CELLS OVEREXPRESSING NEURONAL CA2+ SENSOR-1 PROTEIN

被引:3
作者
Guimaraes, M. M. [1 ,2 ]
Reis, H. J. [1 ,3 ]
Guimaraes, L. P. [1 ]
Carneiro, D. S. [1 ,3 ]
Ribeiro, F. M. [4 ]
Gomez, M. V. [1 ]
Jeromin, A. [5 ]
Romano-Silva, M. A. [1 ]
机构
[1] UFMGAv Alfredo Balena, Lab Neurociencia, Dept Saude Mental, INCT Med Mol,Fac Med, BR-30130100 Belo Horizonte, MG, Brazil
[2] Univ Fed Vales Jequitinhonha & Mucuri, Dept Ciencias Basicas, Fac Ciencias Saude, BR-39100000 Diamantina, MG, Brazil
[3] Univ Fed Minas Gerais, Lab Neurofarmacol, Dept Farmacol, Inst Ciencias Biol, BR-31270901 Belo Horizonte, MG, Brazil
[4] Robarts Res Inst, Cell Biol Res Grp, London, ON N6A 5C1, Canada
[5] Univ Texas Austin, Ctr Learning & Memory, Austin, TX 78712 USA
关键词
PC12; cells; NCS-1; Calcium signaling; glutamate release; INOSITOL 1,4,5-TRISPHOSPHATE RECEPTOR; PHOSPHATIDYLINOSITOL 4-OH KINASE; ADRENAL CHROMAFFIN CELLS; CALCIUM-BINDING PROTEIN; CA2+ CHANNELS; GLUTAMATE RELEASE; EXOCYTOSIS; NCS-1; LOCALIZATION; MECHANISM;
D O I
10.1170/130
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
It has been suggested that overexpression of neuronal Ca2+ sensor-1 (NCS-1) protein is implicated in the pathophysiology of neurodisorders such as schizophrenia, bipolar disturbance and X-linked mental retardation. The mechanism by which NCS-1 would be involved in the causes and/or consequences of these neurodisorders is still far from elucidation. Independent evidence has pointed NCS-1 as a key regulator of synaptic efficacy by altering the expression and activity of voltage-gated channels, inhibiting internalization of dopaminergic receptors, and altering phosphoinositide metabolism. In this study, we examined the possible participation of NCS-1 protein in signal transmission dependent on muscarinic receptor activation, using PC12 cells stably expressing NCS-1 (PC12-NCS-1). Carbachol (CCH; 300 mu M) was able to evoke glutamate release more efficiently from PC12-NCS-1 (15.3 +/- 1.0nmol/mg of protein) than wild type cells (PC12-wt; 8.3 +/- 0.9nmol/mg of protein). This increase of glutamate release induced by CCH was independent on extracellular Ca2+ influx. Additionally, a larger increase of cytoplasmic levels of InsP(3) (663.0 +/- 63.0 and 310.0 +/- 39.0% of fluorescence in A.U.) and [Ca2+](i) (766.4 +/- 40.0 and 687.8 +/- 37.1nmol/L) was observed after CCH stimulus of PC12-NCS-1 compared with PC12-wt. Clearly distinction between intracellular Ca2+ dynamics was also observed in PC12-NCS-1 and PC12-wt. A larger increase followed by fast decay of [Ca2+](i) was observed in PC12-NCS-1. A plateau with a delayed decay of [Ca2+](i) was characteristic of PC12-wt [Ca2+](i) response. Both enhancement of InsP3 production and glutamate release observed in PC12-NCS-1 were blocked by atropine (10 mu M). Together, our data show that overexpression of NCS-1 in PC12 cells induces an enhancement of intracellular second messenger and transmitter release dependent on CCH response, suggesting that muscarinic signaling is "up-regulated" in this cell model.
引用
收藏
页码:1138 / 1150
页数:13
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