Transplantation of tissue-engineered human corneal epithelium in limbal stem cell deficiency rabbit models

AIM: To evaluate the biological functions of tissue-engineered human corneal epithelium (TE-HCEP) by corneal transplantation in limbal stem cell deficiency (LSCD) rabbit models. METHODS: TE-HCEPs were reconstructed with DiI-labeled untransfected HCEP cells and denuded amniotic membrane (dAM) in air-liquid interface culture, and their morphology and structure were characterized by hematoxylin-eosin (HE) staining of paraffin-sections, immunohistochemistry and electron microscopy. LSCD models were established by mechanical and alcohol treatment of the left eyes of New Zealand white rabbits, and their eyes were transplanted with TE-HCEPs with dAM surface outside by lamellar keratoplasty (LKP). Corneal transparency, neovascularization, thickness, and epithelial integrality of both traumatic and post transplantation eyes were checked once a week by slit-lamp corneal microscopy, a corneal pachymeter, and periodic acid-Schiff (PAS) staining. At day 120 post surgery, the rabbits in each group were sacrificed and their corneas were examined by DiI label observation, HE staining, immunohistochemistry and electron microscopy. RESULTS: After cultured for 5 days on dAM, HCEP cells, maintaining keratin 3 expression, reconstructed a 6-7 layer TE-HCEP with normal morphology and structure. The traumatic rabbit corneas, entirely opaque, conjunctivalized and with invaded blood vessels, were used as LSCD models for TE-HCEP transplantation. After transplantation, obvious edema was not found in TE-HCEP-transplanted corneas which became more and more transparent, the invaded blood vessels reduced gradually throughout the monitoring period. The corneas decreased to normal thickness on day 25, while those of dAM eyes were over 575 mu m in thickness during the monitoring period. A 45 layer of epithelium consisting of TE-HCEP originated cells attached tightly to the anterior surface of stroma was reconstructed 120 days after TE-HCEP transplantation, which was similar to the normal control eye in morphology and structure. In contrast, intense corneal edema, turbid, invaded blood vessels were found in dAM eyes, and no multilayer epithelium was found but only a few scattered conjunctiva-like cells appeared. CONCLUSION: The TE-HCEP, with similar morphology and structure to those of innate HCEP, could reconstruct a multilayer corneal epithelium with normal functions in restoring corneal transparency and thickness of LSCD rabbits after transplantation. It may be a promising HCEP equivalent for clinical therapy of corneal epithelial disorders.

兔角膜缘干细胞的研究进展

目前,角膜移植是临床上治疗角膜疾患的最有效途径,但供体角膜非常有限。新近兴起的干细胞技术,为组织工程角膜的研制和应用提供了契机。对于以角膜缘干细胞缺乏或功能障碍为特征的疾病也有治疗效果。采取角膜缘干细胞移植应是一种合理有效的治疗手段。本文主要介绍了兔角膜缘干细胞的体外分离、培养、鉴定及一些生长因子对其增殖的影响。

自体角膜缘移植术治疗角膜缘缺陷症的实验与临床研究

目的探讨自体角膜缘移植术在局限性或全角膜缘缺陷症治疗中的作用。方法动物实验以兔眼前节碱烧伤制作全角膜缘缺陷症模型，烧伤后实施自体角膜缘移植术治疗。结果动物手术组角膜上皮愈合快，角膜新生血管及炎细胞浸润均轻于对照组。临床研究中所有翼状胬肉均未见复发。结论自体角膜缘移植术治疗角膜缘缺陷症效果显著，是一种符合生理机制的、安全的手术方式。

兔自体骨髓间充质干细胞移植对角膜缘干细胞损伤的初步疗效研究

目的探讨兔自体骨髓间充质干细胞(BMSCs)移植对角膜缘干细胞(LSCs)损伤的初步疗效。方法 36只大白兔分为三组:BMSCs组、LSCs组与羊膜对照组,每组12只。BMSCs组采用附着有BMSCs的羊膜治疗角膜缘干细胞损伤,LSCs组将附着有角膜内皮细胞的羊膜治疗角膜缘干细胞损伤,羊膜对照组则仅将羊膜用缝合线固定于浅层巩膜上治疗角膜缘干细胞损伤。于术前、术后1周、术后2周、3周和4周对眼表的形态进行评分;并于术前、术后1周、4周、8周利用聚焦显微镜观察细胞密度和表面积。结果在移植手术实施之前三组兔的眼表形态综合评分之间的差异无统计学意义(P>0.05);手术之后4周BMSCs组和LSCs组兔的眼表形态评分得以显著改善,差异有统计学意义(P<0.05);手术之后4周羊膜对照组兔的眼表形态评分与手术前相比,差异无统计学意义(P>0.05);手术之后4周BMSCs组和LSCs组之间的眼表形态评分之间差异无统计学意义(P>0.05)。与羊膜对照组相比,其它两组手术4周之后的眼表形态评分改善更显著,差异有统计学意义(P<0.05)。经过共焦显微镜观察,BMSCs组兔移植1周之后的细胞形态为圆形,而非初始的梭边形,细胞较小,密度较高,而随着时间推移,个数逐渐减少,体积变大。随着时间的推移BMSCs组与LSCs组兔移植后的平均细胞密度出现下降。手术前BMSCs组与LSCs组细胞表面积差异无统计学意义(P>0.05);手术后1周、4周BMSCs组的细胞表面积显著低于LSCs组,差异有统计学意义(P<0.05),手术之后8周和12周时BMSCs组与LSCs组细胞表面积差异无统计学意义(P>0.05)。结论与角膜缘干细胞相似,兔自体骨髓间充质干细胞移植治疗角膜缘干细胞可以重建受损的眼表,减轻水肿,抑制血管生成。

神经生长因子(NGF)对兔角膜缘干细胞增殖的影响

目的：探讨神经生长因子（NGF）对兔角膜缘干细胞增殖作用的影响及最佳有效浓度。方法：取成年大耳白兔角膜缘组织，应用组织块消化培养法进行原代培养，取第2代生长状态良好的干细胞，以5×10^3个／ml细胞浓度接种于96孔细胞培养板中，依次加入不同浓度的NGF．培养48h后，采用MTT法测定细胞增殖情况。结果：10ng／ml、50ng／ml、100ng／ml、200ng／ml不同浓度组的NGF均有促进角膜缘干细胞的增殖作用，与对照组比较差异均有显著性（P〈0．01）。1ng／ml组与对照组、50ng／ml组与200ng／ml组比较差异均无显著性（P〉0．05）。结论：NGF可有效促进培养角膜缘干细胞的生长，培养的适宜浓度为10～100ng／ml，为角膜缘干细胞移植患者术后及角膜外伤或溃疡时局部应用NGF提供了理论依据。

家兔角膜缘干细胞缺失病理模型的制作

根据角膜缘干细胞定位于角膜缘上皮基底层,为角膜上皮增殖分化的源泉并保持角膜上皮完整性的理论。将20只家兔随机分为4组,每组5只,分别将角膜缘上皮全周或半周板层手术切除,或用1mol/LNaOH直接擦除等方法破坏角膜缘干细胞,探索制作角膜缘干细胞完全缺失病理模型的有效途径。结果表明,处理后4周,全周角膜缘上皮板层手术切除,中央角膜上皮层用1mol/LNaOH擦除的5只试验家兔角膜表面全部血管化、结膜化,未发生睑球粘连,角膜基质胶原纤维完整未见溃疡、穿孔等病变,细胞印迹学检查为结膜表型,可作为实验性角膜缘干细胞移植的病理模型;全周角膜缘上皮板层手术切除,中央角膜上皮用生理盐水擦除的5只试验家兔,有2只为结膜表型,另3只为角膜表型,观察期内结果不稳定;半周角膜缘上皮板层手术切除,中央角膜上皮层用生理盐水擦除的5只试验家兔,角膜表面透明,全部为角膜表型;直接用1mol/LNaOH擦除角膜缘和中央角膜上皮的试验家兔,有4只角膜基质胶原纤维断裂、溶解,并伴有严重的溃疡、穿孔、睑球粘连等病变,不能用于移植试验,另1只角膜表面透明,未见结膜和新生血管长入,细胞印迹学检查为角膜表型。

兔角膜缘干细胞体外培养方法的研究

目的探讨兔角膜缘干细胞培养方法,并获得兔角膜缘干细胞。方法采用组织块培养法,对兔角膜缘干细胞行体外培养;对原代培养第7 d的细胞进行p63、AE5免疫组织化学鉴定。结果原代培养的细胞通常在7 d左右即可达到80%～90%的融合,细胞呈椭圆形或多边形,核质比例大,表现出较强的增生能力。结论采用组织块培养法对兔角膜缘组织进行体外培养,可获得较纯、未分化、有增生能力的角膜缘干细胞。

以干燥脱水法保存的异种角膜基质为载体构建人工生物角膜上皮组织

目的:观察以干燥脱水法保存的鸵鸟角膜基质为载体构建人工生物角膜上皮组织的生物学特性。方法:采用组织块培养法获得新西兰大白兔角膜缘干细胞,经胰蛋白酶消化法获得细胞,种植于干燥脱水法保存的鸵鸟角膜板层基质上,采用气液界面培养法进行培养,通过倒置显微镜、透射电子显微镜、荧光显微镜观察其形态学、生长特点,超微结构及免疫学特征。结果:在干燥脱水法保存的鸵鸟角膜基质上种植兔角膜缘干细胞,接种72h后,细胞形成单层,移置气液交界面后继续培养7～10d,逐渐形成复层。经光镜、透射电镜、及免疫学检测显示其具有角膜上皮组织的生物学特性。结论:兔角膜缘干细胞能够在干燥脱水法保存的鸵鸟角膜基质载体上生长,并可形成复层,基本具有正常角膜上皮细胞的形态、超微结构和生物学特性。

以脱细胞角膜基质为载体的组织工程化兔角膜的构建及移植

目的进行体外分离和培养兔角膜缘干细胞,使之成为一种上皮组织,以便进行角膜移植。方法组织块法体外培养兔角膜缘干细胞:角膜缘组织块作为外植体,在脱细胞猪角膜基质上培养;获得的复合角膜上皮组织移植于兔眼,观察并记录兔角膜组织生长情况,待角膜组织生长良好后做免疫组织化学鉴定。结果兔角膜缘组织应用组织块法在脱细胞角膜基质上生长9~10 d后达到80%汇合状态,显微镜下动态观察细胞生长良好,增殖能力较高,将组织工程化角膜上皮作异体板层角膜移植于兔眼后,4~5 d角膜上皮光滑,20~21 d角膜变为透明,荧光素染色只见缝线处少许着色,期间未见角膜移植排斥反应。术后30 dHE染色显示角膜组织与宿主角膜组织结合良好,上皮细胞可见4~5层结构,可见角膜缘干细胞多呈卵圆形;免疫荧光染色可见培养的细胞P63,CK3单克隆抗体呈阳性表达。结论以组织块法生长的以脱细胞角膜基质为载体的组织工程化兔角膜可在角膜缘干细胞缺乏的兔眼上生长良好。