Abstract

A fundamental problem in developmental neurobiology is how the relationship between cell proliferation and pattern formation is coordinated. Studies during the previous funding period have identified a message form of the D2 cyclin gene, MN20, in selected neural precursors making their final divisions and in recently post-mitotic neurons. In cerebellum, MN20/D2 cyclin is expressed in the ventricular zone and is up-regulated in post mitotic cells, such as those contributing to the deep cerebellar nuclei. While absent in the granule cell precursors as they originate and migrate from the embryonic rhombic lip, MN20/D2 cyclin is heavily expressed in these cells only after they reach the external germinal layer in the early postnatal period. Therefore, D2 cyclin expression in granule cell precursors coincides with the time and location in which these cells become competent to differentiate. Its developmental expression pattern suggest that D2 cyclin plays a role in the final rounds of division and differentiation of selected neurons. Preliminary investigation using antisense oligonucleotides indicate that down-regulation of D2 cyclin in granule cell precursors reduces BrdU incorporation and prevents neurite extension. This project will test the hypothesis that the expression of cell cycle regulatory genes is important for primary neurogenesis and regional neuronal differentiation. Specifically, our goal is to examine how cell division is regulated during cerebellar histogenesis and to establish whether cell cycle components, like D2 cyclin, can interact with developmentally important gene products to influence cellular differentiation and organization.
Aim 1 a will test the role of cell cycle progression and cytokinesis in neuronal differentiation by disrupting the cycle at various points using antisense oligonucleotides to reduced expression of other regulatory proteins active in G1 or G2 phase.
Aim 1 b will test the hypothesis that the influence of the cycle on cerebellar neural differentiation may be mediated through G1 active proteins via their control of the E2F transcription factor family.
Aim 2 will use yeast two hybrid selection to test the hypothesis that D2 cyclin may interact directly with developmentally important gene products to influence cerebellar pattern formation.
Aim 2 will use mice that lack D2 cyclin, D2 cyclin or both to examine their role in cerebellar development, taking advantage of in vivo and in vitro experimental systems. Together, the proposed experiments will provide insights into mechanisms that integrate the control of proliferation and differentiation in cerebellar neural lineages.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Program Projects (P01)
Project #
5P01NS031318-09
Application #
6579424
Study Section
Project Start
2002-04-01
Project End
2003-03-31
Budget Start
1997-10-01
Budget End
1998-09-30
Support Year
9
Fiscal Year
2002
Total Cost
$293,069
Indirect Cost

  Institution

Name
University of Minnesota Twin Cities
Department
Type
DUNS #
168559177
City
Minneapolis
State
MN
Country
United States
Zip Code
55455

  Publications

Kuceyeski, Amy; Navi, Babak B; Kamel, Hooman et al. (2016) Structural connectome disruption at baseline predicts 6-months post-stroke outcome. Hum Brain Mapp 37:2587-601
Chen, Gang; Gao, Wangcai; Reinert, Kenneth C et al. (2005) Involvement of kv1 potassium channels in spreading acidification and depression in the cerebellar cortex. J Neurophysiol 94:1287-98
Goswami, Jaideep; Martin, Loren A; Goldowitz, Daniel et al. (2005) Enhanced Purkinje cell survival but compromised cerebellar function in targeted anti-apoptotic protein transgenic mice. Mol Cell Neurosci 29:202-21
Brodie, Christopher R; Khaliq, Mahmooda; Yin, Jerry C P et al. (2004) Overexpression of CREB reduces CRE-mediated transcription: behavioral and cellular analyses in transgenic mice. Mol Cell Neurosci 25:602-11
Reinert, Kenneth C; Dunbar, Robert L; Gao, Wangcai et al. (2004) Flavoprotein autofluorescence imaging of neuronal activation in the cerebellar cortex in vivo. J Neurophysiol 92:199-211
Dunbar, R L; Chen, G; Gao, W et al. (2004) Imaging parallel fiber and climbing fiber responses and their short-term interactions in the mouse cerebellar cortex in vivo. Neuroscience 126:213-27
Beitz, Alvin J; Saxon, Dale (2004) Harmaline-induced climbing fiber activation causes amino acid and peptide release in the rodent cerebellar cortex and a unique temporal pattern of Fos expression in the olivo-cerebellar pathway. J Neurocytol 33:49-74
Zhang, Yi; Forster, Colleen; Milner, Teresa A et al. (2003) Attenuation of activity-induced increases in cerebellar blood flow by lesion of the inferior olive. Am J Physiol Heart Circ Physiol 285:H1177-82
Yang, Guang; Zhang, Yi; Ross, M Elizabeth et al. (2003) Attenuation of activity-induced increases in cerebellar blood flow in mice lacking neuronal nitric oxide synthase. Am J Physiol Heart Circ Physiol 285:H298-304
Gao, Wangcai; Dunbar, Robert L; Chen, Gang et al. (2003) Optical imaging of long-term depression in the mouse cerebellar cortex in vivo. J Neurosci 23:1859-66

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