Literature DB >> 2545834

Fura-2 measurements of cultured rat Purkinje neurons show dendritic localization of Ca2+ influx.

P E Hockberger1, H Y Tseng, J A Connor.   

Abstract

The specific objectives of this study were the following: (1) to characterize the types of calcium currents in cultured PCs using whole-cell voltage-clamp techniques; (2) using fura-2 imaging techniques, to monitor intracellular Ca2+ levels during application of high potassium, glutamate, or glutamate analogs; and (3) to evaluate the types of calcium channels contributing to the calcium fluxes using pharmacological blocking agents. Voltage-clamp analysis of calcium currents proved to be difficult due to space-clamping problems. The latter was presumably due to the unfavorable geometry of cultured PCs. Nevertheless, we found no evidence for inward currents in cells bathed in TTX-TEA-BaCl2 saline. On the other hand, fura-2 measurements demonstrated that free Ca2+ levels were elevated in PCs following local application of either high-potassium saline or glutamate. When individual cells were injected with fura-2 and analyzed in TTX-containing saline, the Ca2+ elevation was usually greater in the dendrites. Since Ca2+ levels were not elevated in all dendrites of the same cell, the smaller responses in the soma wre not simply due to volumetric differences. Together with the voltage-clamp results, the fura-2 data indicate that calcium channels were localized to certain dendrites. Using selective calcium channel blockers, we found evidence for 2 types of calcium conductances in the dendrites of cultured PCs. The Ca conductance induced by high potassium was reduced in a dose-dependent manner by nifedipine (ED50 = 5 X 10(-7) M), indicating that a high-threshold voltage-dependent calcium channel was present. The Ca response to glutamate (or NMDA) was reduced by 2-amino-5-phosphonovaleric acid (ED50 = 10(-4) M), as well as by nifedipine or 10(-4) M LaCl3, indicating that both voltage-dependent and glutamate-coupled channels were opened by glutamate application.

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Year:  1989        PMID: 2545834      PMCID: PMC6569756     

Source DB:  PubMed          Journal:  J Neurosci        ISSN: 0270-6474            Impact factor:   6.167


  13 in total

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Authors:  P Liljelund; J G Netzeband; D L Gruol
Journal:  J Neurosci       Date:  2000-10-01       Impact factor: 6.167

2.  Evaluation of cellular mechanisms for modulation of calcium transients using a mathematical model of fura-2 Ca2+ imaging in Aplysia sensory neurons.

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Authors:  D Hillman; S Chen; T T Aung; B Cherksey; M Sugimori; R R Llinás
Journal:  Proc Natl Acad Sci U S A       Date:  1991-08-15       Impact factor: 11.205

5.  Real-time imaging of calcium influx in mammalian cerebellar Purkinje cells in vitro.

Authors:  M Sugimori; R R Llinás
Journal:  Proc Natl Acad Sci U S A       Date:  1990-07       Impact factor: 11.205

6.  Comparison of quantitative calcium flux through NMDA, ATP, and ACh receptor channels.

Authors:  M Rogers; J A Dani
Journal:  Biophys J       Date:  1995-02       Impact factor: 4.033

7.  Tetrodotoxin induced calcium spikes: in vitro and in vivo studies of normal and deafferented Purkinje cells.

Authors:  A Aubry; C Batini; J M Billard; R T Kado; P Morain
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8.  Dendritic excitability modulates dendritic information processing in a purkinje cell model.

Authors:  Allan D Coop; Hugo Cornelis; Fidel Santamaria
Journal:  Front Comput Neurosci       Date:  2010-03-30       Impact factor: 2.380

9.  A positive feedback signal transduction loop determines timing of cerebellar long-term depression.

Authors:  Keiko Tanaka; George J Augustine
Journal:  Neuron       Date:  2008-08-28       Impact factor: 17.173

10.  Differential Ca2+ binding properties in the human cerebellar cortex: distribution of parvalbumin and calbindin D-28k immunoreactivity.

Authors:  A L Scotti; C Nitsch
Journal:  Anat Embryol (Berl)       Date:  1992
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