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The generation of olfactory epithelial neurospheres in vitro predicts engraftment capacity following transplantation in vivo.

机译:体外嗅上皮神经球的产生预测了体内移植后的植入能力。

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The stem and progenitor cells of the olfactory epithelium maintain the tissue throughout life and effectuate epithelial reconstitution after injury. We have utilized free-floating olfactory neurosphere cultures to study factors influencing proliferation, differentiation, and transplantation potency of sphere-grown cells as a first step toward using them for therapeutic purposes. Olfactory neurospheres form best and expand most when grown from neonatal epithelium, although methyl bromide-injured or normal adult material is weakly spherogenic. The spheres contain the full range of epithelial cell types as marked by cytokeratins, neuron-specific antigens, E-cadherin, Sox2, and Sox9. Globose basal cells are also prominent constituents. Medium conditioned by growth of phorbol ester-stimulated, immortalized lamina propria-derived cells (LP(Imm)) significantly increases the percentage of Neurog1eGFP(+) progenitors and immature neurons in spheres. Sphere-forming capacity resides within selected populations; FACS-purified, Neurog1eGFP(+) cells were poorly spherogenic, while preparations from DeltaSox2eGFP transgenic mice that are enriched for Sox2(+) basal cells formed spheres very efficiently. Finally, we compared the potency following transplantation of cells grown in spheres vs. cells derived from adherent cultures. The sphere-derived cells engrafted and produced colonies with multiple cell types that incorporated into and resembled host epithelium; cells from adherent cultures did not. Furthermore, cells from spheres grown in conditioned media from the phorbol ester-activated LP(Imm) line gave rise to significantly more neurons after transplantation as compared with control. The current findings demonstrate that sphere formation serves as a biomarker for engraftment capacity and multipotency of olfactory progenitors, which are requirements for their eventual translational use.
机译:嗅上皮的干细胞和祖细胞在整个生命过程中维持组织,并在损伤后实现上皮重建。我们已经利用自由漂浮的嗅觉神经球培养物来研究影响球形生长细胞的增殖,分化和移植潜能的因素,这是将其用于治疗目的的第一步。从新生儿上皮细胞生长时,嗅觉神经球的形成和扩展最多,尽管甲基溴损伤的或正常的成人物质的成球能力较弱。这些球体包含以细胞角蛋白,神经元特异性抗原,E-钙黏着蛋白,Sox2和Sox9标记的上皮细胞类型的全部范围。球状基底细胞也是主要成分。通过佛波酯刺激的,永生化的固有层固有细胞(LP(Imm))生长为条件的培养基显着增加了Neurog1eGFP(+)祖细胞和未成熟神经元在球体中的百分比。形成球的能力驻留在选定的人群中; FACS纯化的Neurog1eGFP(+)细胞的成球性较差,而从DeltaSox2eGFP转基因小鼠制备的富含Sox2(+)基础细胞的制剂非常有效地形成了球体。最后,我们比较了球形细胞与贴壁培养细胞移植后的效力。球形细胞移植并产生具有多种细胞类型的菌落,这些菌落并入宿主上皮并类似于宿主上皮。贴壁培养的细胞没有。此外,与佛波酯激活的LP(Imm)系相比,在佛波酯活化的LP(Imm)系的条件培养基中生长的球形细胞产生的神经元明显多于对照。目前的研究结果表明,球体的形成可以作为嗅觉祖细胞移植能力和多能性的生物标志物,而嗅球祖细胞的最终用途是进行翻译。

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