Establishment of a three-dimensional corneal stroma extracellular matrix fibrosis model induced by transforming growth factor-β1 in vitro
10.3760/cma.j.issn.2095-0160.2015.05.005
- VernacularTitle:转化生长因子-β1介导的角膜基质细胞外基质纤维化体外三维培养模型的构建
- Author:
He, JIN
;
Shinan, LUO
;
Zixi, FAN
;
Jie, LI
;
Weiwei, ZHOU
;
Xia, LI
- Publication Type:Journal Article
- Keywords:
Corneal keratocyte;
Wound healing;
Cell culture techniques/methods;
Transforming growth factor-β1;
Extracellular matrix;
Fibrosis;
Collagen type Ⅰ;
Collagen type Ⅲ
- From:
Chinese Journal of Experimental Ophthalmology
2015;33(5):406-411
- CountryChina
- Language:Chinese
-
Abstract:
Background Extracellular matrix (ECM) fibrosis leads to corneal scaring during the process of cornea wound healing.Transforming growth factor-β1 (TGF-β1) is known to mediate overproduce of ECM components.Our previous study developed a three-dimensional model for corneal stromal cells culture in vitro.Objective The hypothesis of this study was to apply TGF-β1 in the three-dimensional culture system to establish a corneal stroma ECM fibrosis model.Methods Fresh bovine corneas were extracted for the culture of bovine keratocytes in constructed three-dimension culture system.The Pellets were cultured in the DMEM/F12+ 10% fetal bovine serum (FBS) medium with 0.5 ng/ml or 1.0 ng/ml TGF-β1 or without TGF-β1,respectively.Calcein AM/(propidium iodide) PI staining was employed to assay the cell viability 2 weeks after culture.The expressions of α-smooth muscle actin (α-SMA),type Ⅰ collagen (Col Ⅰ) and Col Ⅲ mRNA and protein in the cells were detected by real-time PCR and Western blot respectively 48 hours,1 week and 2 weeks after cultured.The results were statistically analyzed.Results Cultured for 48 hours in the Pellet system,corneal stromal cells clustered and was identified alive by Calcein-AM/PI staining in 2 weeks.The relative expression levels of α-SMA,Col Ⅰ and Col m mRNA were elevated in both the 0.5 ng/ml and 1.0 ng/ml TGF-β1 supplement groups in comparison with the only DMEM/F12+10% FBS group,with marked difference among the three groups (Fgroup =696.745,P<0.001;Fgroup =35.166,P<0.001;Fgroup =33.677,P<0.001),and the expression levels increased with the lapse of culture time (Ftime =5.863,P<0.05;Ftime =298.614,P<0.001;Ftime =607.472,P<0.001).The synthetic rate of Col Ⅲ mRNA was obviously faster than that of Col Ⅰ mRNA.Western blot showed that only a trace of α-SMA,Col Ⅰ and Col Ⅲ were detected 48 hours and 1 week after culture.The expression levels of α-SMA,Col Ⅰ and Col Ⅲ in Pellet system in 0.5 ng/ml TGF-β1 medium were 0.395±0.208,1.060±0.175 and 0.629±0.382,and in 1.0 ng/ml TGF-β1 medium were 0.758±0.228,1.201 ±0.187 and 0.753±0.468,respectively 2 weeks after culture,significant differences were shown among the three groups (α-SMA:F=10.691,P<0.05;Col Ⅰ:F=14.094,P<0.05;Col Ⅲ:F=10.995,P<0.05).Conclusions Addition of TGF-β1 and serum enhance the assembly and fibrosis of ECM,showing the higher expressions of specific fibrotic markers in bovine keratocytes Pellet.This culture systerm can be used as a candidate three-dimensional model for corneal stroma ECM fibrosis.
