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ASCL1的动态表达驱动幼年和成年猕猴穆勒胶质细胞向未成熟视网膜神经节细胞的神经发生。

Dynamic expression of ASCL1 drives neurogenesis from infant and adult macaque Müller glia into immature retinal ganglion cells.

作者信息

Pavlou Marina, Wohlschlegel Juliette, Hahn Josh, Kaplan Lew, Rieke Fred, Manookin Michael B, Ortuño-Lizarán Isabel, Probst Marlene, Prieve Aric R, Reh Thomas A

出版信息

bioRxiv. 2025 Aug 25:2025.08.21.671552. doi: 10.1101/2025.08.21.671552.

DOI:10.1101/2025.08.21.671552
PMID:40909711
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12407719/
Abstract

Strategies to stimulate the regeneration of neurons in the adult central nervous system can offer universal solutions for neurodegenerative diseases. Taking lessons from naturally regenerating species, such as the zebrafish, we have previously shown that vector-mediated expression of proneural transcription factors can stimulate neurogenesis from the resident Müller glia (MG) population in the adult mouse retina, both and . To bring this closer to translation, we now show that vector-mediated expression of the proneural transcription factor ASCL1 can reprogram adult macaque MG into functional neurons. To this end, we established purified MG cultures and show they retain a mature transcriptomic profile that correlates with foveal and peripheral MG. Importantly, MG-derived neurons express retinal ganglion cell markers, can fire action potentials and have a transcriptome that overlaps with developing human and adult macaque retinal ganglion cells. To refine this approach for clinical application, we incorporated microRNA-124 target sites in the reprogramming cassette and show that this restricts expression to MG in mixed primary cultures and intact explant cultures of adult macaque retina. Regulating ASCL1 expression with microRNA-124 target sites maintained the reprogramming efficiency from adult MG cultures and improved the yield of RGC-like neurons from infant MG cultures. Most importantly, with this vector cassette we successfully reprogrammed macaque MG from both adult and infant retina into HuC/D+ neurons. Our findings demonstrate that ASCL1 can induce neurogenesis from macaque MG across ages and provide a targeted, effective strategy for potential clinical translation in retinal repair.

摘要

刺激成体中枢神经系统中神经元再生的策略可为神经退行性疾病提供通用解决方案。从斑马鱼等自然再生物种中汲取经验,我们之前已经表明,前神经转录因子的载体介导表达可刺激成年小鼠视网膜中常驻的米勒胶质细胞(MG)群体产生神经发生。为了使其更接近临床应用,我们现在表明,前神经转录因子ASCL1的载体介导表达可将成年猕猴的MG重编程为功能性神经元。为此,我们建立了纯化的MG培养物,并表明它们保留了与中央凹和周边MG相关的成熟转录组图谱。重要的是,MG衍生的神经元表达视网膜神经节细胞标志物,能够产生动作电位,并且具有与发育中的人类和成年猕猴视网膜神经节细胞重叠的转录组。为了优化这种方法以用于临床应用,我们在重编程盒中纳入了微小RNA-124靶位点,并表明这将表达限制在成年猕猴视网膜的混合原代培养物和完整外植体培养物中的MG。用微小RNA-124靶位点调节ASCL1表达可维持成年MG培养物的重编程效率,并提高幼年MG培养物中RGC样神经元的产量。最重要的是,使用这种载体盒,我们成功地将成年和幼年视网膜的猕猴MG重编程为HuC/D+神经元。我们的研究结果表明,ASCL1可诱导不同年龄猕猴MG的神经发生,并为视网膜修复的潜在临床应用提供了一种有针对性的有效策略。

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