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 | This article was the subject of an educational assignment in 2013 Q3. Further details were available on the "Education Program:Georgia Institute of Technology/Introduction to Neuroscience (Fall 2013)" page, which is now unavailable on the wiki. |
Background[edit]
Neurogenesis is the mechanism for neuron proliferation and differentiation. It entails many different complex processes which are all time and ordered depenedent.[1] Processes such as neuron proliferation, fate specification, differentiation, maturation, and functional integration of newborn cells into existing neuronal networks are all interconnected.[2] In the past decade many epigenetic regulatory mechanisms have been shown to play a large role in the timing and determination of neural stem cell lineage. [1]
Relevant Mechanisms & Definitions[edit]
Three important methods of epigenetic regulation include Histone modification, DNA methylation and demethylation, and MicroRNA (miRNA) expression. While there are many different types of Histone modifications, in neural epigenetics there are two primary mechanisms which have been explored: histone methylation and histone acetylation. [1][3] In the former, methyl groups are either added or removed to the histone altering it's structure and exposing chromatin and leading to gene activation or deactivation. In the latter, histone acetylation causes the histone to hold the DNA more loosely, allowing for more gene activation. DNA Methylation, in which methyl groups are added to cytosine or adenosine redisdues on the DNA, is a more lasting method of gene inactivation than histone modification, though is still reversible in some cases. [1][3] MicroRNAs are a small form of non-coding RNA (ncRNA) which often act as "fine-tuning" mechanisms for gene expression by repressing or inducing messenger RNA (mRNA) in neural cells but can also act directly with transcription factors to guide neurogenesis.[1][3][4] [5]
Epigenetic Regulation in the Brain[edit]
Embryonic Neurogenesis[edit]
Histone Modifications:[edit]
Neural Stem Cells generate the cortex in a precise "inside out" manner with carefully controlled timing mechanisms. Early born neurons form deep layers in the cortex while newer born form the upper layers. This timing program is seen in vitro as well as in vivo. [1][3] Histone methylation has been shown to be one of the epigenetic regulatory mechanisms which alters the proportionate production of deep layer and upper layer neurons. Specifically, deletion of Ezh2 encoding histone methyltransferase led to a two fold reduction of BRN2-expressing and SATB2 expressing upper layer neurons without affecting the number of neurons in layer V and VI. Similiarly, histone acetylation through histone deacetylase (HDAC) inhibitor Valproic Acid, an epilepsy therapeutic, in mouse embryonic stem cell (ESC) derived neural proginetors not only induces neuronal differentiation, but also selectively enriched the upper layer neuronal population. As such, it has been proposed that HDAC inhibition promotes the progression of neuronal differentiation, leading to a fate-switch from deep-layer producing progenitors into upper-layer progenitors. However, the reasons behind this selective differentiation and timing control as a result of HDAC inhibition are not yet fully understood. [3]
DNA Methylation:[edit]
DNA methylation's critical nature to corticogenesis has been shown through knockout experiments in mice. When DNMT3b and DNMT1 were ablated in mouse embryos, each separately, embryonic lethality followed due to impairment of neural tube development. DNMT3a ablation did not cause embryonic lethality, but did result in a severe detriment in postnatal neurogenesis.[1][3] This is largely due to the timing in which these epigenetic mechanisms are active. DNMT3b is expressed in early neural progenitor cells and decrease as neural development proceeds and DNMT3a is barely detectable up until embryonic day 10 (E.10). However, at E.10, DNMT3a expression increases significantly from E13.5 and well into adulthood. In the postnatal forebrain, DNMT3a is expressed in the subventricular zone (SVZ) and the hippocampal dentate gyrus, the primary locations for adult neurogenesis.[1][2] The loss of DNMT3a in post natal neural progenitor cells leads to the down-regulation of neuronic genes such as Dlx2, Neurog2, and Sp8; but upregulation of genes involved in astroglial and oligodendroglial differentiation, indicating a role in the cell-fate switch from neurogenesis to gliogenesis. DNA demethylation, as well as methylation, of certain genes allows for neurogenesis to proceed in a time dependent manner. One such gene is Hes5, hypermethylated in E7.5 Embryos but completely demethylated by E9.5, which is one of the target genes in the Notch Signaling pathway. GCM1 and GCM2 demethylate the Hes5 promoter, allowing it to respond to NOTCH signaling and initiating the generation of neural stem cells.[1] Another example is the Gfap gene which is required for astrocyte differentiation. The ability to differentiate into glial cells is repressed in neural stem cells with a neuronal cell fate. This repression is due largely to an irresponsiveness of neural stem cells towards astrocyte-inducing stimulations. The neural stem cells are non-responsive due to hypermethylated DNA in the promoter regions of astrocyte genes such as Gfap. The STAT3 binding site in the promoter region of Gfap is hypermethylated at E11.5 and barely so at E14.5, at which point it is able to recieve astrocyte inducing stimulations and begin cytokine-inducible astrocyte differentiation. [3]
miRNAs:[edit]
Studies done by De Pietri Tonelli and Kawase-Koga have shown conditional knockout of Dicer, an enzyme largely used for miRNA synthesis, in mouse neocortex resulted in reduced cortical size, increased neuronal apoptosis, and deficient corticol layering. Neuroepithelial cells and neuroprogenitor cells were not affected until E.14, at which point they also underwent apoptosis. This doesn't show which miRNAs were responsible for the varying factors affected, but it does show that there is a stage-specific requirement for miRNA expression in cortical development.[1][5][6][7] miR-124, the most abundant microRNA in the central nervous system, controls the lineage progression of subventricular zone neural progenitor cells into neuroblasts by suppressing protein production by targeting Sox9. Another major microRNA player is miR-9/9*. In embryonic neurogenesis miR-9 has been shown to regulate neuronal differentiation and self-renewal.[1][5][4] Ectopic expression of miR-9 in the developing mouse cortex led to premature neuronal differentiation and disrupted the migration of new neurons throough targeting Foxg1.[1]
Contrary to the idea that microRNAs are only fine-tuning mechanisms, recent studies have shown that miR-9 and miR-124 can act together to guide fibroblasts into neural cells. Transcription factors and regulatory genes, such as Neurod1, Ascr1, and Myt1l, which were previously thought to be responsible for this phenomena did not transform human fibroblasts in the abscence of miR-9 and miR-124, but in the prescence of the microRNAs and the abscence of the transcription factors human fibroblast transformation proceeded, albeit in a less efficient manner. [1][4][5]
Adult Neurogenesis[edit]
DNA Methylation[edit]
Neurogenesis continues after development well through adulthood. [2]Growth arrest and DNA-damage-inducible, beta (GADD45b) is required for the demethylation of promoters of critical genes responsible for new-born neuron development such as brain-derived neurotrophic factor (BDNF) and Basic fibroblast growth factor (FGF2).[8] As such, upregulation of GADD45b leads to increased demethylation, increased BDNF and FGF2, and ultimately more neural progenitor cells. [1][8]
Histone Modification[edit]
Histone deacetylation also plays a large role in the proliferation and self renewal of post-natal neural stem cells. Neural-expressed HDACs interact with Tlx, an essential neural stem cell regulator, to suppress TLX target genes. This includes the cyclin-dependent kinase inhibitor P21 and the tumor supressor gene Pten to promote neural stem cell proliferation. Inhibition of HDACS by the antiepileptic drug valproic acid induces neuronal differentiation as in embryonic neurogenesis, but also inhibits glial cell differentiation of adult neural stem cells. This is likely mediated through upregulation of neuronal specific genes such as the neurogeneic basic helix-loop-helix transcription factors NEUROD, NEUROGENENIN1, and Math1. Conditional loss of HDAC1 and HDAC2 in neural progenitor cells prevented them from differentiating into neurons and their loss in oligodendrytic progenitor cells disrupted oligodendrocyte formations, suggesting that histone deacetlyation plays important but varying roles in different stages of neuronal development. [1]
miRNAs[edit]
miR-9 targets the nuclear receptor TLX in adult neurogenesis to promote neural differentiation and inhibit neural stem cell proliferation. It also influences neuronal subtype specification and regulates axonal growth, branching, and targeting in the central nervous system through interactions with HES1, a neural stem cell homeostasis molecule.[1][5] miR-124 promotes cell cycle exit and neuronal differentiation in adult neurogensis. Mouse studies have shown that ectopic expression of miR-124 showed premature neural progenitor cell differentiation and exhaustion is the subventricular zone.[5]
In Memory[edit]
Histone acetylation has a dynamic role in controlling memory formation and synaptic plasticity. HDAC inhibitors exhibited positive effects on mice with cognitive defects such as Alzheimers disease and improved the cognition of wild type mice. HDAC2 has been shown to play a negative role in memory and learning. Sirt1, a histone acetylase, reduces memory formation ability by promoting the expression of miR-134, which targets the critical activity-dependent transcription factor (CREB) essential for learning and memory.[8]
The Growth Arrest and DNA Damage inducible 45 (Gadd45) gene family plays a large role in the hippocampus. Gadd45 facilitates hippocampal long-term potentiation and enhances persisting memory for motor performance, aversive conditioning, and spatial navigation.[9] Additionally, DNA methylation has been shown to be important for activity-dependent modulation of adult neurogenesis in the hippocampus, which is mediated by GADD45b. GADD45b seems to act as a sensor in mature neurons for environmental changes which it expresses through these methylation changes. [1] This was determined by examining the effects of applying an electric stimulus to the hippocampal dentate gyrus (DG) in normal and GADD45b knockout mice. In normal mice application of electrical stimulation to the DG increased neurogenesis by increasing BDNF. However, in GADD45b defficient mice the electrical stimulus had less of an effect. Further examination revealed that around 1.4% of CpG islands in DG neurons are actively methylated and demthylated upon electric shock. This shows that the post-mitotic methylation states of neurons are not static and given that electric shock equipment such as that used in the study has been shown to have therapeutic effects to human patients with depression and other psychiatric disorders, the possibility remains that epigenetic mechanisms may play an important role in the pathophysiology of neuropsychiatric disorders.[2][8] DNMT1 and DNMT3a are both required in conjunction for learning, memory, and synaptic plasticity.[8]
Epigenetic Misregulation & Neurological Disorders[edit]
Alterations on epigenomic machinery cause DNA methylation and Histone acetylation processes to go rogue, leading to alterations on the transcriptional level of genes involved in the pathogenesis of neural degenerative diseases such as Parkinsons Disease, Alzheimer's Disease, Schizophrenia, and Bipolar Disease.[1] [10]
Parkinson's Disease:[edit]
Common epigenetic regulatory mechanisms which cover neuronal death can lead to neurodegenerative disorders such as Parkinson's disease when they cease functioning properly. [8]
Alzheimer's Disease:[edit]
MicroRNA expression is critical for neurogenesis. In patients with Alzheimer's disease miR-9 and miR-128 is upregulated, while miR-15a is downregulated.[4] AD patients also show decreases in brain-derived neurotrophic factor, which has been shown to be repressed through DNA methylation. [8]
References[edit]
- ^ a b c d e f g h i j k l m n o p q r Hu, X.L. (2012). "Epigenetic control on cell fate choice in neural stem cells". Protein & Cell. 3 (4): 278–290. doi:10.1007/s13238-012-2916-6.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ a b c d Faigle, Roland (2013). "Signaling mechanisms regulating adult neural stem cells and neurogenesis". Biochimica et Biophysica Acta. 1830 (2): 2435–2448.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ a b c d e f g MuhChyi, Chai (2013). "Epigenetic regulation of neural stem cell fate during corticogenesis". International Journal of Developmental Neuroscience. 31 (6): 424–433. doi:10.1016/j.ijdevneu.2013.02.006.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help); Unknown parameter|month=ignored (help) - ^ a b c d Ji, Fen (2013). "The Role of MicroRNAs in Neural Stem Cells and Neurogenesis". Journal of Genetics and Genomics. 40 (2): 61–66. doi:10.1016/j.jgg.2012.12.008.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help); Unknown parameter|month=ignored (help) - ^ a b c d e f Sun, Alfred X (2013). "MicroRNAs: regulators of neuronal fate". Current Opinion in Cell Biology. 25 (2): 215–221. doi:10.1016/j.ceb.2012.12.007.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help); Unknown parameter|month=ignored (help) - ^ De Pietri Tonelli, D. (23 October 2008). "miRNAs are essential for survival and differentiation of newborn neurons but not for expansion of neural progenitors during early neurogenesis in the mouse embryonic neocortex". Development. 135 (23): 3911–3921. doi:10.1242/dev.025080.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ Kawase-Koga, Y. (26 January 2010). "RNAase-III enzyme Dicer maintains signaling pathways for differentiation and survival in mouse cortical neural stem cells". Journal of Cell Science. 123 (4): 586–594. doi:10.1242/jcs.059659.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ a b c d e f g Lv, Jingwen (2013). "The Epigenetic Switches for Neural Development and Psychiatric Disorders". Journal of Genetics and Genomics. 40: 339–346.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ Sultan, Faraz (2012). "Genetic Deletion of gadd45b, a Regulator of Active DNA Demethylation, Enhances Long-Term Memory and Synaptic Plasticity". The Journal of Neuroscience. 32 (48): 17059–17066.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help) - ^ Dempster, E. L. (9 September 2011). "Disease-associated epigenetic changes in monozygotic twins discordant for schizophrenia and bipolar disorder". Human Molecular Genetics. 20 (24): 4786–4796. doi:10.1093/hmg/ddr416.
{{cite journal}}: Unknown parameter|coauthors=ignored (|author=suggested) (help)CS1 maint: date and year (link)