Abstract

The adult hippocampus continuously generates new dentate granule neurons from neural stem cells. A number of factors that preferentially activate hippocampal circuits, such as exercise, enriched environment, and many pathological conditions, regulate new neuron development. Neurons transmit activity from cell to cell mainly through synapses. However, synapses of new neurons do not form until at least two weeks after birth. This suggests the presence of diffusible factors from active circuits to regulate new neuron development. This speculation has motivated us to examine signaling pathways reacting to circuit activity to regulate new neuron development. Sphingolipid signaling recently caught massive attention because of its role in mediating activity across cells in the immune system. In a pilot study, we tested the existence of this pathway in the dentate gyrus and found that sphingosine 1-phosphate receptor 1 (S1PR1) is enriched in new neurons. Moreover, both sphingosine kinase 1 and SPNS2 are enriched in existing but not new dentate granule cells. We therefore speculate that the SPNS2-S1PR1 pathway transmits the existing circuit activity to regulate the integration of newborn neurons. To test this hypothesis, we propose the following experiments: First, we will genetically perturb theSPNS2-S1PR1 pathway and test optogenetic activation of dentate granule cells-induced development of new dentate granule cells. Second, in the S1PR1 over-expressing new dentate granule cells, we will use a retroviral method to manipulate the Cdc42 and Akt pathways to examine their roles in mediating the S1PR1 regulation to new neuron development. We will perform the same genetic manipulation of the Cdc42 and Akt pathways in optogenetic-induced development of new dentate granule cells. Third, we will use pilocarpine-induced seizures as a model system to test the development of new neurons after genetically manipulating the SPNS2-S1PR1 pathway. Moreover, we will monitor epileptic activity after disrupting the SPNS2-S1PR1 pathway of new neurons. Our proposal aims to reveal the role of the SPNS2-S1PR1 pathway in propagating neural circuit activity to regulate new neuron development. This study will provide insights towards understanding how existing neural circuits dictate the development of new neurons. Our results may introduce a novel therapeutic target for the treatment of epilepsy.

Public Health Relevance

Disease, degeneration or traumatic injury of the nervous system are among the greatest public health concerns in the United States and are generally considered irreparable, often causing catastrophic damage to the functional capacity of the individual. Now, however, characterization of neural stem cells residing within specific germinal centers of the brain and in cell culture raises hope that functional regeneration of nervous tissue may be feasible, if we learn to exploit adult neurogenesis for clinical benefit. The research proposal here aims to study how existing brain cells control the integration of new members derived from endogenous neural stem cells. If successful, this proposal will lead to improved understanding of neural stem cell biology, possibly leading to the development of new drugs for repair and regeneration of the nervous system.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
1R01NS089770-01A1
Application #
8987244
Study Section
Special Emphasis Panel (ZRG1-MDCN-P (02))
Program Officer
Fureman, Brandy E
Project Start
2015-09-30
Project End
2020-06-30
Budget Start
2015-09-30
Budget End
2016-06-30
Support Year
1
Fiscal Year
2015
Total Cost
$362,674
Indirect Cost
$99,125

  Institution

Name
State University New York Stony Brook
Department
Neurosciences
Type
Schools of Medicine
DUNS #
804878247
City
Stony Brook
State
NY
Country
United States
Zip Code
11794

  Publications

Kirschen, Gregory W; Ge, Shaoyu; Park, Il Memming (2018) Probability of viral labeling of neural stem cells in vivo. Neurosci Lett 681:17-18
Kirschen, Gregory W; Kéry, Rachel; Ge, Shaoyu (2018) The Hippocampal Neuro-Glio-Vascular Network: Metabolic Vulnerability and Potential Neurogenic Regeneration in Disease. Brain Plast 3:129-144
Mukherjee, Shradha; Hsieh, Jenny (2018) Genome-Wide Identification of Transcription Factor-Binding Sites in Quiescent Adult Neural Stem Cells. Methods Mol Biol 1686:265-286
Thodeson, Drew M; Brulet, Rebecca; Hsieh, Jenny (2018) Neural stem cells and epilepsy: functional roles and disease-in-a-dish models. Cell Tissue Res 371:47-54
Rao, Sneha; Kirschen, Gregory W; Szczurkowska, Joanna et al. (2018) Repositioning of Somatic Golgi Apparatus Is Essential for the Dendritic Establishment of Adult-Born Hippocampal Neurons. J Neurosci 38:631-647
Kirschen, Gregory W; Kéry, Rachel; Liu, Hanxiao et al. (2018) Genetic dissection of the neuro-glio-vascular machinery in the adult brain. Mol Brain 11:2
Brulet, Rebecca; Matsuda, Taito; Zhang, Ling et al. (2017) NEUROD1 Instructs Neuronal Conversion in Non-Reactive Astrocytes. Stem Cell Reports 8:1506-1515
Kirschen, Gregory W; Shen, Jia; Tian, Mu et al. (2017) Active Dentate Granule Cells Encode Experience to Promote the Addition of Adult-Born Hippocampal Neurons. J Neurosci 37:4661-4678
Brulet, Rebecca; Zhu, Jingfei; Aktar, Mahafuza et al. (2017) Mice with conditional NeuroD1 knockout display reduced aberrant hippocampal neurogenesis but no change in epileptic seizures. Exp Neurol 293:190-198
Matsui, Takeshi; Nieto-Estévez, Vanesa; Kyrychenko, Sergii et al. (2017) Retinoblastoma protein controls growth, survival and neuronal migration in human cerebral organoids. Development 144:1025-1034

Showing the most recent 10 out of 15 publications