Knockdown of fibrillin-1 suppresses retina-blood barrier dysfunction by inhibiting vascular endothelial apoptosis under diabetic conditions.

IF 1.9 4区 医学 Q2 OPHTHALMOLOGY International journal of ophthalmology Pub Date : 2024-08-18 eCollection Date: 2024-01-01 DOI:10.18240/ijo.2024.08.03
Yue Zhang, Xiao-Jing Liu, Xin-Ran Zhai, Yao Yao, Bin Shao, Yu-Han Zhen, Xin Zhang, Zhe Xiao, Li-Fang Wang, Ming-Lian Zhang, Zhi-Min Chen
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Abstract

Aim: To investigate the effects of fibrillin-1 (FBN1) deletion on the integrity of retina-blood barrier function and the apoptosis of vascular endothelial cells under diabetic conditions.

Methods: Streptozotocin (STZ)-induced diabetic mice were used to simulate the diabetic conditions of diabetic retinopathy (DR) patients, and FBN1 expression was detected in retinas from STZ-diabetic mice and controls. In the Gene Expression Omnibus (GEO) database, the GSE60436 dataset was selected to analyze FBN1 expressions in fibrovascular membranes from DR patients. Using lentivirus to knock down FBN1 levels, vascular leakage and endothelial barrier integrity were detected by Evans blue vascular permeability assay, fluorescein fundus angiography (FFA) and immunofluorescence labeled with tight junction marker in vivo. High glucose-induced monkey retinal vascular endothelial cells (RF/6A) were used to investigate effects of FBN1 on the cells in vitro. The vascular endothelial barrier integrity and apoptosis were detected by trans-endothelial electrical resistance (TEER) assay and flow cytometry, respectively.

Results: FBN1 mRNA expression was increased in retinas of STZ-induced diabetic mice and fibrovascular membranes of DR patients (GSE60436 datasets) using RNA-seq approach. Besides, knocking down of FBN1 by lentivirus intravitreal injection significantly inhibited the vascular leakage compared to STZ-DR group by Evans blue vascular permeability assay and FFA detection. Expressions of tight junction markers in STZ-DR mouse retinas were lower than those in the control group, and knocking down of FBN1 increased the tight junction levels. In vitro, 30 mmol/L glucose could significantly inhibit viability of RF/6A cells, and FBN1 mRNA expression was increased under 30 mmol/L glucose stimulation. Down-regulation of FBN1 reduced high glucose (HG)-stimulated retinal microvascular endothelial cell permeability, increased TEER, and inhibited RF/6A cell apoptosis in vitro.

Conclusion: The expression level of FBN1 increases in retinas and vascular endothelial cells under diabetic conditions. Down-regulation of FBN1 protects the retina of early diabetic rats from retina-blood barrier damage, reduce vascular leakage, cell apoptosis, and maintain vascular endothelial cell barrier function.

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在糖尿病条件下,敲除纤维蛋白-1可通过抑制血管内皮细胞凋亡抑制视网膜-血液屏障功能障碍。
目的:研究纤连蛋白-1(FBN1)缺失对糖尿病条件下视网膜-血液屏障功能完整性和血管内皮细胞凋亡的影响:方法:用链脲佐菌素(STZ)诱导的糖尿病小鼠模拟糖尿病视网膜病变(DR)患者的糖尿病状态,检测STZ-糖尿病小鼠和对照组视网膜中FBN1的表达。在基因表达总库(Gene Expression Omnibus,GEO)数据库中,选择了 GSE60436 数据集来分析 FBN1 在 DR 患者纤维血管膜中的表达。利用慢病毒敲除 FBN1 水平,通过埃文斯蓝血管通透性测定、荧光素眼底血管造影(FFA)和体内紧密连接标记免疫荧光检测血管渗漏和内皮屏障完整性。使用高糖诱导的猴视网膜血管内皮细胞(RF/6A)研究 FBN1 在体外对细胞的影响。通过跨内皮电阻(TEER)测定和流式细胞术分别检测了血管内皮屏障的完整性和细胞凋亡:结果:利用RNA-seq方法,STZ诱导的糖尿病小鼠视网膜和DR患者的纤维血管膜(GSE60436数据集)中FBN1 mRNA表达增加。此外,与 STZ-DR 组相比,通过埃文斯蓝血管通透性测定和 FFA 检测,慢病毒玻璃体内注射敲除 FBN1 能显著抑制血管渗漏。STZ-DR 组小鼠视网膜中紧密连接标记物的表达低于对照组,而敲除 FBN1 则提高了紧密连接的水平。在体外,30 mmol/L葡萄糖能显著抑制RF/6A细胞的活力,而FBN1 mRNA的表达在30 mmol/L葡萄糖刺激下有所增加。下调 FBN1 可降低高糖(HG)刺激下视网膜微血管内皮细胞的通透性,增加 TEER,抑制体外 RF/6A 细胞凋亡:结论:在糖尿病条件下,视网膜和血管内皮细胞中 FBN1 的表达水平升高。结论:在糖尿病条件下,FBN1 在视网膜和血管内皮细胞中的表达水平升高,下调 FBN1 可保护早期糖尿病大鼠视网膜免受视网膜-血液屏障损伤,减少血管渗漏和细胞凋亡,维持血管内皮细胞屏障功能。
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CiteScore
2.50
自引率
7.10%
发文量
3141
审稿时长
4-8 weeks
期刊介绍: · International Journal of Ophthalmology-IJO (English edition) is a global ophthalmological scientific publication and a peer-reviewed open access periodical (ISSN 2222-3959 print, ISSN 2227-4898 online). This journal is sponsored by Chinese Medical Association Xi’an Branch and obtains guidance and support from WHO and ICO (International Council of Ophthalmology). It has been indexed in SCIE, PubMed, PubMed-Central, Chemical Abstracts, Scopus, EMBASE , and DOAJ. IJO JCR IF in 2017 is 1.166. IJO was established in 2008, with editorial office in Xi’an, China. It is a monthly publication. General Scientific Advisors include Prof. Hugh Taylor (President of ICO); Prof.Bruce Spivey (Immediate Past President of ICO); Prof.Mark Tso (Ex-Vice President of ICO) and Prof.Daiming Fan (Academician and Vice President, Chinese Academy of Engineering. International Scientific Advisors include Prof. Serge Resnikoff (WHO Senior Speciatist for Prevention of blindness), Prof. Chi-Chao Chan (National Eye Institute, USA) and Prof. Richard L Abbott (Ex-President of AAO/PAAO) et al. Honorary Editors-in-Chief: Prof. Li-Xin Xie(Academician of Chinese Academy of Engineering/Honorary President of Chinese Ophthalmological Society); Prof. Dennis Lam (President of APAO) and Prof. Xiao-Xin Li (Ex-President of Chinese Ophthalmological Society). Chief Editor: Prof. Xiu-Wen Hu (President of IJO Press). Editors-in-Chief: Prof. Yan-Nian Hui (Ex-Director, Eye Institute of Chinese PLA) and Prof. George Chiou (Founding chief editor of Journal of Ocular Pharmacology & Therapeutics). Associate Editors-in-Chief include: Prof. Ning-Li Wang (President Elect of APAO); Prof. Ke Yao (President of Chinese Ophthalmological Society) ; Prof.William Smiddy (Bascom Palmer Eye instituteUSA) ; Prof.Joel Schuman (President of Association of University Professors of Ophthalmology,USA); Prof.Yizhi Liu (Vice President of Chinese Ophtlalmology Society); Prof.Yu-Sheng Wang (Director of Eye Institute of Chinese PLA); Prof.Ling-Yun Cheng (Director of Ocular Pharmacology, Shiley Eye Center, USA). IJO accepts contributions in English from all over the world. It includes mainly original articles and review articles, both basic and clinical papers. Instruction is Welcome Contribution is Welcome Citation is Welcome Cooperation organization International Council of Ophthalmology(ICO), PubMed, PMC, American Academy of Ophthalmology, Asia-Pacific, Thomson Reuters, The Charlesworth Group, Crossref,Scopus,Publons, DOAJ etc.
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