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http://dx.doi.org/10.5115/acb.2010.43.3.211

Differential regulation of Purkinje cell dendritic spines in rolling mouse Nagoya ($tg^{rol}/tg^{rol}$), P/Q type calcium channel (${\alpha}1_A/Ca_v2.1$) mutant  

Oda, Sen-Ich (Laboratory of Animal Management, School of Agricultural Science, Nagoya University)
Lee, Kea-Joo (Department of Anatomy, College of Medicine and Human Genetics, Korea University)
Arii, Tatsuo (Section of Brain Structure, Center for Brain Experiment)
Imoto, Keiji (Department of Information Physiology, National Institute for Physiological Sciences)
Hyun, Byung-Hwa (Genetic Resource Center, Korea Research Institute of Bioscience and Biotechnology, KRIBB)
Park, In-Sung (Department of Anatomy, College of Medicine and Human Genetics, Korea University)
Kim, Hyun (Department of Anatomy, College of Medicine and Human Genetics, Korea University)
Rhyu, Im-Joo (Department of Anatomy, College of Medicine and Human Genetics, Korea University)
Publication Information
Anatomy and Cell Biology / v.43, no.3, 2010 , pp. 211-217 More about this Journal
Abstract
Voltage dependent calcium channels (VDCC) participate in regulation of neuronal $Ca^{2+}$. The Rolling mouse Nagoya ($Cacna1a^{tg-rol}$) is a spontaneous P/Q type VDCC mutant, which has been suggested as an animal model for some human neurological diseases such as autosomal dominant cerebellar ataxia (SCA6), familial hemiplegic migraine and episodic ataxia type-2. Morphology of Purkinje cell (PC) dendritic spine is suggested to be regulated by signal molecules such as $Ca^{2+}$ and by interactions with afferent inputs. The amplitude of excitatory postsynaptic current was decreased in parallel fiber (PF) to PC synapses, whereas apparently increased in climbing fiber (CF) to PC synapses in rolling mice Nagoya. We have studied synaptic morphology changes in cerebella of this mutant strain. We previously found altered synapses between PF varicosity and PC dendritic spines. To study dendritic spine plasticity of PC in the condition of insufficient P/Q type VDCC function, we used high voltage electron microscopy (HVEM). We measured the density and length of PC dendritic spines at tertiary braches. We observed statistically a significant decrease in spine density as well as shorter spine length in rolling mice compared to wild type mice at tertiary dendritic braches. In proximal PC dendrites, however, there were more numerous dendritic spines in rolling mice Nagoya. The differential regulation of rolling PC spines at tertiary and proximal dendrites in rolling mice Nagoya suggests that two major excitatory afferent systems may be regulated reciprocally in the cerebellum of rolling mouse Nagoya.
Keywords
Ataxia; Dendritic spine; High voltage electron microscope; Purkinje cell; Voltage dependent calcium channel;
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