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[羊膜提取对兔角膜准分子激光角膜切削术后上皮伤口愈合和基质重塑的影响]

[Effects of amniotic extraction on epithelial wound healing and stromal remodelling after excimer laser keratectomy in rabbit cornea].

作者信息

Xiao Qiguo, Chen Yuan, Du Juan, Wang Hua, Li Wei, Liu Zuguo

机构信息

Department of Ophthalmology, the Second Affiliated Hospital of South China University, Hengyang 421001, China.

Email:

出版信息

Zhonghua Yan Ke Za Zhi. 2014 Jan;50(1):42-50.

Abstract

OBJECTIVE

To investigate the effects and mechanism of amniotic extraction on corneal healing after photorefractive keratectomy (PRK).

METHODS

Experimental Study. Thirty-six New Zealand rabbit corneas were performed with PRK models (-10 diopters, 6.5 mm diameter). According to random number table, all eyes were divided into three groups, including treated with amniotic extraction, 0.1% dexamethasone and excipient respectively after operation. Clinical and histopathologic examinations were taken by slit-lamp microscope and light microscope. Corneal epithelium reparation was observed by fluorescent staining. Corneal stroma cell apoptosis was evaluated by terminal deoxyribonucleotidyl transferase-mediated deoxyuridine triphosphate nick end labeling (TUNEL) assay. Myofibroblast generation was evaluated by immunofluorescence checking the expression of alpha-smooth muscle actin (α-SMA). The number of TUNEL and α-SMA positive cells was analyzed to explore the effects on corneal haze. The haze grading was compared between groups using Kruskal-Wallis H test. Mean values for each experiment were compared between groups using a one-way analysis of variance and LSD-t test.Spearman rank analysis was used to evaluate the correlation between the haze grading and the expression of TUNEL positive cells and α-SMA.

RESULTS

The corneas of seventy-two eyes reepithelialized in 6 days after operation. The average epithelium repair time of the AE group was (4.12 ± 0.62) d, the dexamethasone group was (5.25 ± 0.78) d, and the excipient group was (4.96 ± 0.73) d. The progression of reepithelialization was significantly faster in the AE group than the other two groups (F = 14.144, P < 0.01). The haze appeared in the first week after the PRK in all three groups, increased after 3-4 weeks, and relieved after 8 weeks. The degree of haze was significantly lower in the AE group than the other two groups in the first week (Vs. dexamethasone group, H = 3.995, P < 0.05; vs. excipient group, H = 12.77, P < 0.01), in the 4th week (Vs. dexamethasone group, H = 4.468, P < 0.05;vs. excipient group, H = 9.003, P < 0.01), and 8th week (Vs dexamethasone group, H = 4.397, P < 0.05;vs. excipient group, H = 5.744, P < 0.05) after PRK. The TUNEL-positive cells appeared in the central anterior stroma at the first week after surgery. And the number of TUNEL-positive cells in the AE group was (2.2500 ± 0.3750) cells/HP, the dexamethasone group was (4.5000 ± 0.7500) cells/HP, and the excipient group was (7.1250 ± 0.9063) cells/HP. The number of TUNEL-positive cells in AE group was less than those in the other two groups (Vs. dexamethasone group, t = 4.26, P < 0.01; vs. excipient group, t = 8.13, P < 0.01). The TUNEL-positive cells were only found in the excipient group (2.8750 ± 0.6563)/HP in 4th week after operation.It was significantly different between the dexamethasone group and the excipient group (t = 9.01, P < 0.01). There were no significant TUNEL-positive cells in 8th weeks in all three groups.α-SMA-positive cells started to appear apparently at the first week after surgery in the dexamethasone and excipient groups, and the peaks appeared at the 4th week after treatments, and there were still a lot of α-SMA-positive cells in corneal stroma at the 8th week after operation in both groups.On the contrary, there were no significant α-SMA-positive cells in the AE group all the time after surgery. The statistical significant difference can be found between the AE group vs. the dexamethasone and excipient groups in the first week (t = 28.62, 36.55;P < 0.01), in the 4th week (t = 30.40, 35.96; P < 0.01), and in the 8th week (t = 34.02, 38.32; P < 0.01).Spearman rank analysis demonstrated that the formation of haze was proportional to the expression of TUNEL positive cells (r = 0.881, P < 0.01) and α-SMA (r = 0.710, P < 0.01).

CONCLUSION

Amniotic extraction can reduce the formation of haze, which was more effective than 0.1% dexamethasone.It might release certain factors which were transported into corneal matrix, then affected the healing of epithelial cell by interacting with the corneal cell factors, reducing the cell apoptosis, corneal wound healing response and rebuilding the corneal matrix with less myofibroblast, collagen and scar and finally reduce the formation of haze.

摘要

目的

探讨羊膜提取对准分子激光角膜切削术(PRK)后角膜愈合的影响及机制。

方法

实验研究。对36只新西兰兔角膜制作PRK模型(-10屈光度,直径6.5mm)。根据随机数字表,将所有眼分为三组,分别于术后给予羊膜提取、0.1%地塞米松和赋形剂处理。采用裂隙灯显微镜和光学显微镜进行临床和组织病理学检查。通过荧光染色观察角膜上皮修复情况。采用末端脱氧核苷酸转移酶介导的脱氧尿苷三磷酸缺口末端标记法(TUNEL)检测角膜基质细胞凋亡。通过免疫荧光检测α平滑肌肌动蛋白(α-SMA)的表达评估成肌纤维细胞的生成。分析TUNEL和α-SMA阳性细胞数量以探讨对角膜混浊的影响。采用Kruskal-Wallis H检验比较各组间的混浊分级。采用单因素方差分析和LSD-t检验比较各组间各实验的平均值。采用Spearman秩相关分析评估混浊分级与TUNEL阳性细胞和α-SMA表达之间的相关性。

结果

72只眼的角膜术后6天重新上皮化。羊膜提取组的平均上皮修复时间为(4.12±0.62)天,地塞米松组为(5.25±0.78)天,赋形剂组为(4.96±0.73)天。羊膜提取组的上皮化进程明显快于其他两组(F=14.144,P<0.01)。所有三组在PRK术后第一周均出现混浊,3-4周后加重,8周后减轻。在术后第一周(与地塞米松组相比,H=3.995,P<0.05;与赋形剂组相比,H=12.77,P<0.01)、第4周(与地塞米松组相比,H=4.468,P<0.05;与赋形剂组相比,H=9.003,P<0.01)和第8周(与地塞米松组相比,H=4.397,P<0.05;与赋形剂组相比,H=5.744,P<0.05),羊膜提取组的混浊程度明显低于其他两组。术后第一周,TUNEL阳性细胞出现在中央前基质中。羊膜提取组的TUNEL阳性细胞数量为(2.2500±0.3750)个/HP,地塞米松组为(4.5000±0.7500)个/HP,赋形剂组为(7.1250±0.9063)个/HP。羊膜提取组的TUNEL阳性细胞数量少于其他两组(与地塞米松组相比,t=4.26,P<0.01;与赋形剂组相比,t=8.13,P<0.01)。术后第4周,仅在赋形剂组发现TUNEL阳性细胞(2.8750±0.6563)/HP。地塞米松组和赋形剂组之间差异有统计学意义(t=9.01,P<0.01)。所有三组在第8周均未发现明显的TUNEL阳性细胞。地塞米松组和赋形剂组在术后第一周α-SMA阳性细胞开始明显出现,在治疗后第4周达到峰值,两组在术后第8周角膜基质中仍有大量α-SMA阳性细胞。相反,羊膜提取组在术后一直未发现明显的α-SMA阳性细胞。在术后第一周(t=28.62,36.55;P<0.01)、第4周(t=30.40,35.96;P<0.01)和第8周(t=34.02,38.32;P<0.01),羊膜提取组与地塞米松组和赋形剂组之间存在统计学显著差异。Spearman秩相关分析表明,混浊的形成与TUNEL阳性细胞(r=0.881,P<0.01)和α-SMA(r=0.710,P<0.01)的表达成正比。

结论

羊膜提取可减少混浊的形成,比0.1%地塞米松更有效。它可能释放某些因子,这些因子进入角膜基质,然后通过与角膜细胞因子相互作用影响上皮细胞的愈合,减少细胞凋亡、角膜伤口愈合反应,并以较少的成肌纤维细胞、胶原蛋白和瘢痕重建角膜基质,最终减少混浊的形成。

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