Regulation of Postnatal Forebrain Amoeboid Microglial Cell Proliferation and Development by the Transcription Factor Runx1

Zusso, Morena; Methot, Laurent; Lo, Rita; Greenhalgh, Andrew D.; David, Samuel; Stifani, Stefano

doi:10.1523/jneurosci.6182-11.2012

Cited by 140 publications

(102 citation statements)

References 43 publications

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“…Common opinion holds that yolk sac-derived myeloid precursors colonize the developing murine CNS between embryonic days 7 and 7.5 [36], where they proliferate extensively during embryonic and early postnatal development, eventually giving rise to mature ramified microglia [29,37]. Proliferation is rapidly restricted in the first 2 postnatal weeks [29], with adult microglia displaying low turnover [38] and highly limited replacement by peripheral monocytes under non-pathological conditions [39].…”

Section: Discussionmentioning

confidence: 99%

“…These observations of similar microglial densities in LPS-administered P7, P21 and P74 animals could speculatively suggest that there may be a target or maximum density in the brain and that control of microglial proliferation may be juxtacrine in nature. Indeed microglia express both Notch-1 receptor and its ligands Jagged-1 and Delta-1 [41], and Notch activation induces expression of the Runx1 (Runt-related) transcription factor [42], which in turn inhibits amoeboid microglial progenitor proliferation and facilitates progression from amoeboid precursor to ramified microglia [37]. Having observed an LPS-mediated acute increase in microglial cell density at P7, we asked whether these additional microglia were derived from endogenous microglia/myeloid precursor cell proliferation or peripheral monocyte recruitment.…”

Section: Discussionmentioning

confidence: 99%

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Neonatal Peripheral Immune Challenge Activates Microglia and Inhibits Neurogenesis in the Developing Murine Hippocampus

Smith¹,

Hagberg²,

Naylor³

et al. 2014

Dev Neurosci

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The early postnatal period represents an important window in rodent hippocampal development with peak hilar neurogenesis and widespread microgliogenesis occurring in the first week of life. Inflammation occurring during this period may negatively influence development, potentially facilitating or increasing susceptibility to later-life pathology. We administered the Gram-negative bacterial coat protein lipopolysaccharide (LPS) systemically at postnatal day 5 (1 mg/kg i.p.) and assessed potential effects on microgliogenesis, inflammation and neurogenesis in the developing hippocampus. LPS administration led to an acute but transient increase in absolute number and density of ionized calcium-binding adaptor molecule 1-immunoreactive microglia, a change attributable to increased proliferation of central nervous system-resident microglia/microglial precursor cells but not infiltration of peripheral monocyte-derived macrophages. qRT-PCR analysis of hippocampal gene expression showed these LPS-mediated changes to be associated with persistent dysregulation of genes associated with both M1 and M2 microglial phenotypes, indicating prolonged alteration in hippocampal inflammatory status. Further, analysis of progenitor cell regulation in the hippocampal subgranular zone revealed a transient inhibition of the neuronal differentiation pathway up to 2 weeks after LPS administration, a change occurring specifically through effects on type 3 neural progenitor cells and independently of altered cell proliferation or survival of newly born cells. Together, our results show that systemic inflammation occurring during the early neonatal period is sufficient to alter inflammatory status and dysregulate the ongoing process of neurogenesis in the developing hippocampal germinal niche.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Neonatal Peripheral Immune Challenge Activates Microglia and Inhibits Neurogenesis in the Developing Murine Hippocampus

Smith¹,

Hagberg²,

Naylor³

et al. 2014

Dev Neurosci

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“…Primary neural progenitor cells from E13.5 mouse neocortices were obtained and cultured as described. 11,12,37 Double-label immunofluorescence analysis of endogenous proteins was performed as described 11,41 using the following primary antibodies: rat anti-Gro/TLE (1 : 10), rabbit anti-Pin1 (1 : 500), mouse anti-Pin1 (1 : 200; R&D Systems) or rabbit anti-HIPK2 42 (1 : 300). For differentiation assays, cells were transfected as described 11,12,37 after 48 h in vitro using the following plasmids in the combinations indicated in the appropriate figure legend: pEGFP (0.1 mg/well) alone or in combination with pCMV2-FLAG-Gro/TLE1 (0.4 mg/well), pCMV2-FLAGHes1 (0.4 mg/well), pFLAG-HIPK2 or pFLAG-HIPK2(K221R) (0.4 mg/well) and pcDNA3-Pin1-HA (0.4 mg/well).…”

Section: Discussionmentioning

confidence: 99%

“…11,12,15,37 Three days following transfection, cells were analyzed by immunofluorescence using antibodies against Ki67 (1 : 500; BD Pharmingen), nestin (1 : 100; Millipore), Sox2 (1 : 250; R&D Systems), type III b-tubulin (1 : 1000; Promega, Madison, WI, USA), MAP2 (1 : 1000; Sigma-Aldrich) and NeuN (1 : 250; Millipore), as described. 41,43 Cells were counterstained with Hoechst 33258 (Sigma-Aldrich) before examination by fluorescence microscopy. Grayscale images were digitally assigned to the appropriate red or green channel using Northern Eclipse software (Empix Imaging, Inc., Mississauga, ON, Canada).…”

Section: Discussionmentioning

confidence: 99%

Prolyl isomerase Pin1 and protein kinase HIPK2 cooperate to promote cortical neurogenesis by suppressing Groucho/TLE:Hes1-mediated inhibition of neuronal differentiation

et al. 2013

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The Groucho/transducin-like Enhancer of split 1 (Gro/TLE1):Hes1 transcriptional repression complex acts in cerebral cortical neural progenitor cells to inhibit neuronal differentiation. The molecular mechanisms that regulate the anti-neurogenic function of the Gro/TLE1:Hes1 complex during cortical neurogenesis remain to be defined. Here we show that prolyl isomerase Pin1 (peptidyl-prolyl cis-trans isomerase NIMA-interacting 1) and homeodomain-interacting protein kinase 2 (HIPK2) are expressed in cortical neural progenitor cells and form a complex that interacts with the Gro/TLE1:Hes1 complex. This association depends on the enzymatic activities of both HIPK2 and Pin1, as well as on the association of Gro/TLE1 with Hes1, but is independent of the previously described Hes1-activated phosphorylation of Gro/TLE1. Interaction with the Pin1:HIPK2 complex results in Gro/TLE1 hyperphosphorylation and weakens both the transcriptional repression activity and the anti-neurogenic function of the Gro/ TLE1:Hes1 complex. These results provide evidence that HIPK2 and Pin1 work together to promote cortical neurogenesis, at least in part, by suppressing Gro/TLE1:Hes1-mediated inhibition of neuronal differentiation. Cell Death and Differentiation (2014) 21, 321-332; doi:10.1038/cdd.2013.160; published online 22 November 2013During mammalian brain development, the ventricular zone of the dorsolateral region of the alar telencephalon (neocortex) contains undifferentiated neural progenitor cells that initially undergo symmetric (proliferative) divisions to generate two new progenitor cells and later undergo asymmetric (differentiative) divisions to give rise to a new mitotic progenitor and a post-mitotic neuron.

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“…Finally, it is important to mention that Runx1 can contribute to nervous system development and repair in an additional manner, namely by modulating the activity of microglia, the resident immune cells of the nervous system (Zusso et al 2012). Microglia survey the nervous system for signs of infection, injury or disease and mediate immune responses during many neuropathological conditions (Ransohoff and El Khoury 2015;Shemer et al 2015).…”

Section: Discussionmentioning

confidence: 99%

Roles of Runx Genes in Nervous System Development

Wang

Stifani

2017

Advances in Experimental Medicine and Biology

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Runt-related (Runx) transcription factors play essential roles during development and adult tissue homeostasis and are responsible for several human diseases. They regulate a variety of biological mechanisms in numerous cell lineages. Recent years have seen significant progress in our understanding of the functions performed by Runx proteins in the developing and postnatal mammalian nervous system. In both central and peripheral nervous systems, Runx1 and Runx3 display remarkably specific expression in mostly non-overlapping groups of postmitotic neurons. In the central nervous system, Runx1 is involved in the development of selected motor neurons controlling neural circuits mediating vital functions such as chewing, swallowing, breathing, and locomotion. In the peripheral nervous system, Runx1 and Runx3 play essential roles during the development of sensory neurons involved in circuits mediating pain, itch, thermal sensation and sense of relative position. Runx1 and Runx3 orchestrate complex gene expression programs controlling neuronal subtype specification and axonal connectivity. Runx1 is also important in the olfactory system, where it regulates the progenitor-to-neuron transition in undifferentiated neural progenitor cells in the olfactory epithelium as well as the proliferation and developmental maturation of specific glial cells termed olfactory ensheathing cells. Moreover, upregulated Runx expression is associated with brain injury and disease. Increasing knowledge of the functions of Runx proteins in the developing and postnatal nervous system is therefore expected to improve our understanding of nervous system development, homeostasis and disease.

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Regulation of Postnatal Forebrain Amoeboid Microglial Cell Proliferation and Development by the Transcription Factor Runx1

Cited by 140 publications

References 43 publications

Neonatal Peripheral Immune Challenge Activates Microglia and Inhibits Neurogenesis in the Developing Murine Hippocampus

Neonatal Peripheral Immune Challenge Activates Microglia and Inhibits Neurogenesis in the Developing Murine Hippocampus

Prolyl isomerase Pin1 and protein kinase HIPK2 cooperate to promote cortical neurogenesis by suppressing Groucho/TLE:Hes1-mediated inhibition of neuronal differentiation

Roles of Runx Genes in Nervous System Development

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