Stem Cells. 2008 Sep;26(9):2349-60. Epub 2008 Jun 12.

Fate mapping and lineage analyses demonstrate the production of a large number of striatal neuroblasts after transforming growth factor alpha and noggin striatal infusions into the dopamine-depleted striatum.

de Chevigny A, Cooper O, Vinuela A, Reske-Nielsen C, Lagace DC, Eisch AJ, Isacson O.

Source

Udall Parkinson Disease Research Center of Excellence, Center for Neuroregeneration Research, McLean Hospital/Harvard Medical School, Belmont, Massachusetts, USA.

Abstract

Infusion of transforming growth factor alpha (TGFalpha) into the adult dopamine (DA)-depleted striatum generates a local population of nestin(+)/proliferating cell nuclear antigen (PCNA)(+) newborn cells. The precise origin and fate of these new striatal cells are unknown, making it difficult to direct them for neural repair in Parkinson's disease. Experiments in rats using 5-bromo-2'-deoxyuridine (BrdU) to label neural progenitor cells showed that during TGFalpha infusion in the DA-depleted striatum, newborn striatal cells formed a homogeneous population of precursors, with the majority coexpressing nestin, Mash1, Olig2, and epidermal growth factor receptor, consistent with the phenotype of multipotent C cells. Upon TGFalpha pump withdrawal, the subventricular zone (SVZ) was repopulated by neuroblasts. Strikingly, during this period, numerous clusters of doublecortin(+)/polysialylated neuronal cell adhesion molecule(+) neuroblasts were also produced in the ipsilateral medial striatum. In parallel, striatal BrdU(+)/glial fibrillary acidic protein(+) astrocytes were generated, but no BrdU(+)/O4(+)/CNPase(+) oligodendrocytes were generated. Infusion of the neuralizing bone morphogenetic protein antagonist noggin after TGFalpha pump withdrawal increased the neuroblast-to-astrocyte ratio among new striatal cells by blocking glial differentiation but did not alter striatal neurogenesis. At no time or treatment condition were differentiated neurons generated, including DA neurons. Using 6-hydroxydopamine-lesioned nestin-CreER(T2)/R26R-YFP mice that allow genetic fate-mapping of SVZ nestin(+) cells, we show that TGFalpha-generated striatal cells originate from SVZ nestin(+) precursors that confirmed data from the rats on the phenotype and fate of striatal nestin(+)/PCNA(+) cells upon TGFalpha withdrawal. This work demonstrates that a large population of multipotent striatal C-like cells can be generated in the DA-depleted striatum that do not spontaneously differentiate into DA neurons.

PMID:: 18556510; [PubMed - indexed for MEDLINE]
PMCID:: PMC2649803

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Figure 6

6-OHDA lesioned nestin-CreER^T2/R26R-YFP mice show that TGFα-induced C-like cells and their progeny arise from SVZ nestin⁺ cells

(A) Mice that received an intrastriatal infusion of PBS for 2 weeks showed YFP⁺ cells (green) that were restricted to SVZs (left panel), RMS (middle panel) and olfactory bulbs (right panel). (B) Strikingly, mice that received an intrastriatal infusion of TGFα for 14 days exhibited an increased number of YFP⁺ cells (green) in SVZs (left), RMS (middle) and olfactory bulbs (right). Such cells contributed to YFP⁺ cellular waves in the ipsilateral striatum, septum as well as corpus callosum and deep cortical layers (see left and middle panels). (C) YFP⁺ cells (green) in the ipsilateral striatum coexpressed PCNA (red) and nestin (blue). (D) Most ipsilateral striatal YFP⁺ cells (green) expressed BrdU (red), thus confirming a proliferative state. (E) Single plan confocal scan showing that no YFP⁺ cells (green) were GFAP⁺ astrocytes (red) in mice sacrificed during TGFα infusion. (F) YFP⁺ cells (green) coexpressing EGFR (red) and Olig2 (blue) in the DA-depleted striatum. (G) At a lower magnification, most ipsilateral striatal YFP⁺ cells (green) coexpressed Olig2 (red). (G–I) Distribution and phenotypes of SVZ-derived NPCs 2 weeks after TGFα withdrawal. (G) Numerous YFP⁺ cells (green) were observed in the SVZs, ipsilateral striatum, septum (left), RMS (middle) and olfactory bulbs (right). (H) Numerous ipsilateral striatal YFP⁺ cells (green, left) coexpressed GFAP (red, middle). Right panel depicts a merged image. (I) Other striatal YFP⁺ cells (green, left) coexpressed PSANCAM (red, middle), indicating a neuroblast phenotype (see right panel for a merged image). Scale bars: A, B, H, 500 µm; C, D, 10 µm, E, 400 µm; F, 5 µm; G, 50 µm, I, J, 20 µm.

Fate Mapping and Lineage Analyses Demonstrate the Production of a Large Number of Striatal Neuroblasts after TGFα and Noggin Striatal Infusions into the Dopamine-depleted Striatum

Stem Cells. Stem Cells;26(9):2349-2360.

Figure 3

Distribution of immature dividing cells during PBS or during and after TGF-alpha withdrawal

(A, C) Distribution of immature dividing cells in the ipsilateral striatum. (A) During PBS infusion in the DA-depleted striatum, PCNA⁺ (green) dividing cells were present in the ipsilateral SVZ, but rarely detected in the adjacent striatum. (B) TGFα striatal infusion for 2 weeks induced a large population of PCNA⁺ cells in the ipsilateral DA-depleted striatum. (C) Two weeks after withdrawal of the TGFα infusing pump, the distribution of PCNA⁺ cells resembled that of PBS infused rats. (D–F) Distribution of BrdU⁺ cells. (D) During PBS infusion, BrdU⁺ cells (red) were confined to the ipsilateral and contralateral SVZs. (E) During TGFα infusion, BrdU⁺ cells formed a striatal wave in the ipsilateral striatum (right panel), while in the contralateral hemisphere they formed hyper-proliferative nodules protruding from the SVZ towards the source of TGFα (left panel). (F) Two weeks after TGFα withdrawal, contralateral ventricular BrdU⁺ hyper-proliferative nodules were not found (left panel). BrdU⁺ cells were observed in the ipsilateral striatum (right), although their distribution pattern (C, right) and number had changed. Note the ~ 35% reduction in total BrdU⁺ cell number after TGFα withdrawal (G). (H–K) Programmed cell death is induced by TGFα treatment. (H, I) TUNEL⁺ cells in ipsilateral SVZ and striatum of rats infused with PBS (H) or TGFα (I), 2 weeks after its withdrawal. Arrowheads show TUNEL⁺ cells. The number of TUNEL⁺ cells was significantly higher in rats sacrificed after TGFα infusion than in their control counterparts (K). (J) In one rat that died 5 days after TGFα withdrawal, ventricular nodules were found and contained a high proportion of TUNEL⁺ cells. Scale bars: A–B, 50 µm; D–F, 100 µm; H, I, 200 µm; J, 50 µm.

Fate Mapping and Lineage Analyses Demonstrate the Production of a Large Number of Striatal Neuroblasts after TGFα and Noggin Striatal Infusions into the Dopamine-depleted Striatum

Stem Cells. Stem Cells;26(9):2349-2360.

PubMed

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Fate mapping and lineage analyses demonstrate the production of a large number of striatal neuroblasts after transforming growth factor alpha and noggin striatal infusions into the dopamine-depleted striatum.

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