Lacrimal gland organoids: A systematic review on development, characterization, molecular profiling and translational potential in dry eye disease

类有机物 肌上皮细胞 生物 诱导多能干细胞 泪腺 干细胞 病理 6号乘客 导管细胞 间充质干细胞 纤毛 细胞分化 细胞生物学 干细胞标记物 电池类型 基因表达谱 上皮 定向微分 细胞培养 体内 眼蛋白 细胞 基因表达 再生(生物学) 羊膜上皮细胞 角膜 蛋白质组学 癌症研究
作者
Mohammad Gufran Siddiqui,Vanessa L.S. LaPointe,Mor M. Dickman,Sayan Basu,Vivek Singh,Swati Singh
出处
期刊:Experimental Eye Research [Elsevier BV]
卷期号:267: 110956-110956
标识
DOI:10.1016/j.exer.2026.110956
摘要

Organoids are mini-organs engineered to mimic the native tissue's organization, cellular structure, and function. Lacrimal gland organoids are considered a potential treatment for patients with dry eye, but the gland's complex heterogeneity has been difficult to replicate. This systematic review summarizes methods for creating lacrimal gland organoids, their characterization, and potential applications. Data collected included organoid source, composition of expansion or differentiation media, biomarkers, gene expression, responses to stimulants, and effects in animal models. The sources of lacrimal gland organoids were human induced pluripotent stem (hiPS) cell lines (n = 2) and tissue biopsies from humans, mice, or pigs (n = 5). Tissue-derived organoids from mice grew for 40 passages, while those from human biopsies lasted up to 20 passages. There is a need to optimize the culture protocol to preserve cell composition and support long-term growth. The organoids expressed epithelial markers (KRT5, KRT13, AQP), mesenchymal markers (Vimentin and α-SMA), and developmental markers (PAX6, TP63, and OCT3/4), though cellular proportions varied between studies. Stimulation studies showed increased calcium influx and β-glucosaminidase activity, indicating secretory capacity. RNA sequencing revealed unique gene expression patterns associated with stemness and functional maturity, including tear proteins and markers of ductal and myoepithelial cells. PAX6 knockout studies confirmed PAX6's essential role in organoid growth. Published studies lack data on epithelial polarity, the coexistence of ductal and acinar cells within organoids, and the in vivo secretory function of organoids. Transplanted organoids into animal models of dry eye disease (two immunosuppressed and two naïve) remained viable for 8 weeks and expressed tear-related markers (AQP5, KRT14, PAX6), although there was no data on tear film or ocular surface changes. Future research could explore the effects of transplantation on the ocular surface and host immune responses.
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