Distinctive small molecules blend: Promotes lacrimal gland epithelial cell proliferation in vitro and accelerates lacrimal gland injury repair in vivo

IF 5.9 1区 医学 Q1 OPHTHALMOLOGY
Baihui Zeng , Lina Xu , Guoliang Wang , Ruize Shi , Kerui Wang , Shurong Wang , Cheng Li
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Abstract

Purpose

This study aims to develop a novel serum-free culture strategy containing only two small molecules, Y27632 and SB431542 (2C), for in vitro expansion of mouse lacrimal gland epithelial cells (LGECs) and investigate an innovative therapeutic approach for lacrimal gland (LG) injury.

Methods

LGECs proliferative capacity was assessed by cell counting, crystal violet staining, qRT-PCR and immunofluorescence. Cell differentiation was achieved by manipulating culture conditions and assessed by qRT-PCR and AQP5 immunofluorescence. LGECs were seeded in Matrigel for three-dimensional culture and assessed by qRT-PCR and immunofluorescence. Secretory function of the cultures was assayed by ELISA. In vivo, 2C injection verified its reparative capacity in a mouse LG injury model. Corneal fluorescein staining, phenol red cotton thread, H&E, immunofluorescence and Western blot were used to assess LG injury repair.

Results

LGECs cultured with 2C exhibited high expression of stemness/proliferation markers and maintained morphology and proliferative capacity even after the tenth passage. Removal of 2C was efficacious in achieving LGECs differentiation, characterized by the increased AQP5 expression and LTF secretion. 3D spheroids cultured with 2C demonstrated differentiation potential, forming microglandular structures containing multiple LG cell types with secretory functions after 2C removal. In vivo, 2C improved the structural integrity and function of the injured LG.

Conclusions

We present a small molecule combination, 2C, that promotes LGECs expansion and differentiation in vitro and accelerates LG injury repair in vivo. This approach has potential applications for providing a stable source of seed cells for tissue engineering applications, providing new sights for LG-related diseases treatment.

独特的小分子混合物:体外促进泪腺上皮细胞增殖,体内加速泪腺损伤修复
目的 本研究旨在开发一种新型无血清培养策略,该策略仅含有两种小分子 Y27632 和 SB431542 (2C),用于小鼠泪腺上皮细胞(LGECs)的体外扩增,并研究一种治疗泪腺(LG)损伤的创新方法。方法 通过细胞计数、水晶紫染色、qRT-PCR 和免疫荧光评估 LGECs 的增殖能力。通过调节培养条件实现细胞分化,并通过 qRT-PCR 和 AQP5 免疫荧光进行评估。将 LGECs 接种到 Matrigel 中进行三维培养,并通过 qRT-PCR 和免疫荧光进行评估。培养物的分泌功能通过 ELISA 进行检测。在小鼠 LG 损伤模型中,注射 2C 验证了其体内修复能力。用角膜荧光素染色、酚红棉线、H&E、免疫荧光和 Western blot 评估 LG 损伤修复情况。去除 2C 能有效实现 LGECs 分化,其特征是 AQP5 表达和 LTF 分泌增加。用 2C 培养的三维球体具有分化潜能,去除 2C 后可形成包含多种具有分泌功能的 LG 细胞类型的微腺体结构。结论我们提出了一种小分子组合 2C,它能促进 LGECs 在体外的扩增和分化,并加速 LG 损伤在体内的修复。这种方法有望为组织工程应用提供稳定的种子细胞来源,为 LG 相关疾病的治疗提供新的视角。
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来源期刊
Ocular Surface
Ocular Surface 医学-眼科学
CiteScore
11.60
自引率
14.10%
发文量
97
审稿时长
39 days
期刊介绍: The Ocular Surface, a quarterly, a peer-reviewed journal, is an authoritative resource that integrates and interprets major findings in diverse fields related to the ocular surface, including ophthalmology, optometry, genetics, molecular biology, pharmacology, immunology, infectious disease, and epidemiology. Its critical review articles cover the most current knowledge on medical and surgical management of ocular surface pathology, new understandings of ocular surface physiology, the meaning of recent discoveries on how the ocular surface responds to injury and disease, and updates on drug and device development. The journal also publishes select original research reports and articles describing cutting-edge techniques and technology in the field. Benefits to authors We also provide many author benefits, such as free PDFs, a liberal copyright policy, special discounts on Elsevier publications and much more. Please click here for more information on our author services. Please see our Guide for Authors for information on article submission. If you require any further information or help, please visit our Support Center
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