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A role of microRNA-29b-mediated β-catenin signaling in the mouse brain development : 뇌 발생과정중 microRNA-29b에 의한 베타-카테닌 신호전달의 기능 연구
| DC Field | Value | Language |
|---|---|---|
| dc.contributor.advisor | 서유헌-김혜선 | - |
| dc.contributor.author | 신재경 | - |
| dc.date.accessioned | 2017-07-14T06:03:21Z | - |
| dc.date.available | 2018-07-04T02:22:53Z | - |
| dc.date.issued | 2014-08 | - |
| dc.identifier.other | 000000020897 | - |
| dc.identifier.uri | https://hdl.handle.net/10371/125399 | - |
| dc.description | 학위논문 (박사)-- 서울대학교 대학원 : 협동과정뇌과학전공, 2014. 8. 서유헌-김혜선. | - |
| dc.description.abstract | INTRODUCTION: β-catenin has been widely implicated in the regulation of mammalian development and homeostasis. However, in vivo mechanisms by which Wnt/β-catenin signaling components regulate physiological events during brain development remain undetermined. Inhibitor of β-catenin and T cell factor (ICAT) interferes the association of β-catenin with T cell factor. Deficiency of ICAT in mice results in severe malformation of the forebrain and craniofacial bones, suggesting its critical role in regulation of the Wnt signaling in the CNS. The microRNA-29 family is abundantly expressed in the adult cortex, but not in the embryonic brain. However, its physiological role in neuronal development has not been well-studied. The purpose of this study is to determine if deregulated ICAT by miR-29 results in a defective neurogenesis toward neuronal cell lineages and whether these pathologies are due to impaired β-catenin-mediated signaling events.
METHODS: To mimic in vivo micro-environment, neural stem cells (NSCs) were cultured in 3D microfluidics device. Then qRT-PCR, BrdU-pulse and immunofluorescence were performed to characterize NSCs stemness in the niche, such as proliferation and self-renewal properties. In addition, luciferase activity was examined whether miR-29b directly targets the 3-untranslated region (3-UTR) of ICAT. Furthermore, in utero electroporation method was applied to investigate the roles of miR-29b in vivo during fetal corticogenesis under technical cooperation with a research lab at Hallym University. RESULTS: miR-29b, but not miR-29a or c, is increased in differentiated NSCs which is reverse-correlated with the decreased levels of ICAT. I also found that miR 29b diminished NSCs proliferation and self-renewal capabilities, and controlled their fate, directing their differentiation along certain cell lineages. A luciferase reporter assay revealed that the 3-UTR of the ICAT mRNA (also known as CTNNBIP 1 gene) is the direct target of miR-29b. In vivo results show that applied anti-sense miR-29b by in utero electroporation in corticogenesis led to the proliferative defect and premature outward migration. CONCLUSIONS: I showed that miR-29b regulates neurogenesis by controlling Wnt/β-catenin signaling during brain development via inhibition of ICAT expression. Furthermore, these research findings may identify novel therapeutic approaches to modulate ICAT-mediated Wnt/β-catenin signaling to treat or prevent neurological disorders in humans. | - |
| dc.description.tableofcontents | Abstract in English i
Contents iv List of tables and figures viii List of Abbreviations x Introduction 1 1. Cerebral cortical development 1 1.1 Corticogenesis in mammals 1 1.2 Characterization of the neurogenic niche 2 1.3 Development of stem cells in the neurogenic niche 4 2. Signal transduction in the stem cell niche 6 2.1 Influence of growth factors and other extrinsic signals 6 2.2 An integrated shift: from FGF-receptor to GSK-3β 10 2.3 Wnt/β-catenin signaling related to intracellular mechanisms 11 3. Stem cells, Wnt/β-catenin and ICAT 12 3.1 β-catenin and associated mediators in the brain 12 3.2 Structural properties of β-catenin and its functions 13 3.3 The negative regulatory effect of ICAT 15 4. Overview of microRNAs 16 4.1 microRNAs as an intrinsic regulator 16 4.2 miRNA biogenesis and its mechanism 17 4.3 Identification of miRNAs in the developing mouse brain 20 4.4 Classification of miRNA-29a, b, and c families and their targets 22 Material and Methods 23 1. Establishment of primary mouse embryonic neurosphere cultures 23 2. cDNA synthesis and qRT-PCR analysis 24 3. Micro-device array fabrication and preparation 25 4. 3D NSC culture in the micro-device 28 5. Western blot analysis 29 6. Immunofluorescence 30 7. Luciferase reporter assay 31 8. BrdU incorporation assay 34 9. Expansion and proliferation assays 34 10. In utero electroporation 35 11. Histological approaches 36 12. Statistical analysis 36 Results 38 1. Wnt signaling components are expressed in 3D cultured NSCs 38 2. miR-29b reduces NSC proliferation and self-renewal 38 3. Nuclear β-catenin is necessary for NSC differentiation 40 4. miR-29 directly targets the 3-UTR of ICAT 41 5. miR-29b antisense induces a profound proliferative defect during brain development 43 Discussion 56 References 62 Abstract in Korean 80 | - |
| dc.format | application/pdf | - |
| dc.format.extent | 15988424 bytes | - |
| dc.format.medium | application/pdf | - |
| dc.language.iso | en | - |
| dc.publisher | 서울대학교 대학원 | - |
| dc.subject | neurogenesis | - |
| dc.subject | β-catenin | - |
| dc.subject | ICAT | - |
| dc.subject | microRNA-29b | - |
| dc.subject.ddc | 611 | - |
| dc.title | A role of microRNA-29b-mediated β-catenin signaling in the mouse brain development | - |
| dc.title.alternative | 뇌 발생과정중 microRNA-29b에 의한 베타-카테닌 신호전달의 기능 연구 | - |
| dc.type | Thesis | - |
| dc.contributor.AlternativeAuthor | JAEKYUNG SHIN | - |
| dc.description.degree | Doctor | - |
| dc.citation.pages | xi, 82 | - |
| dc.contributor.affiliation | 자연과학대학 협동과정뇌과학전공 | - |
| dc.date.awarded | 2014-08 | - |
| dc.embargo.terms | 2017-07-26 | - |
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