角质形成细胞无血清培养基条件下构建组织工程皮肤

摘要/Abstract

摘要：

目的探讨在角质形成细胞无血清培养基条件下，用人成纤维细胞、角质形成细胞和黑素细胞接种于人去表皮真皮构建组织工程皮肤。方法胰酶和胶原酶消化处理健康小儿包皮，获得表皮和真皮细胞悬液。分别将角质形成细胞、黑素细胞传至第3代，成纤维细胞传至第5代，调整细胞密度为2.5 × 105/ml。制备人去表皮真皮（含部分基底膜成分），先将成纤维细胞悬液种于6孔板板底， 24 h后将人去表皮真皮放入6孔板，角质形成细胞、黑素细胞悬液接种于人去表皮真皮表面（成纤维细胞、角质形成细胞、黑素细胞比例为1 ∶ 4 ∶ 1。实验组用角质形成细胞无血清培养基培养,对照组用含10% FBS的DMEM、K-SFM、M254，3种培养液比例为1 ∶ 1 ∶ 1的混合培养基培养，人去表皮真皮作为空白对照。液下培养3 d后，空气液面培养相结合的方式进行培养，每3天换液1次，2周后取培养的组织工程皮肤分别行HE染色，Melan-A、S-100、HMB45、CKpan、P63、K5、K6、K14、Ki67、Vimentin、Collagen Ⅳ、Laminin免疫组化染色及PAS染色并取正常皮肤做阳性对照。结果经过14 d的气液培养，实验组出现完整的新生表皮结构, CKpan、P63、K5、K6、K14、Ki67、Melan-A、S-100、HMB45、Collagen Ⅳ、Laminin免疫组化染色阳性；对照组出现完整的新生表皮结构,可见角质层, CKpan、P63、K5/6、K14、Ki67、Laminin免疫组化染色阳性。结论角质形成细胞、黑素细胞及成纤维细胞与人去表皮真皮在角质形成细胞无血清培养基条件下，体外可构建组织工程皮肤。

Abstract:

Lin Jianhong, Wang Yu, Lu Bin, Liu Zhi, Jiang Leiwei, Wang Jinzhao, Zhang Wei, Li Shijun, Lu Hongguang Department of Dermatology, Affiliated Hospital of Guizhou Medical University, Guiyang 550004, China（the current affiliation of the first author was Department of Dermatology, First People′s Hospital of Shaoyang, Shaoyang 422000, Hunan, China） Corresponding author: Lu Hongguang, Email: hongguanglu@hotmail.com 【Abstract】 Objective To reconstruct tissue-engineered skin by co-culture of human fibroblasts, keratinocytes and melanocytes on human de-epidermized dermis with keratinocyte serum-free medium （K-SFM）. Methods Healthy children′s prepuce tissues were treated with pancreatin and collagenase to prepare epidermal and dermal cell suspensions respectively. After keratinocytes and melanocytes were cultured separately up to passage 3 and fibroblasts up to passage 5, the density of these cells was adjusted to 2.5 × 105/ml for the following experiment. Human de-epidermized dermis containing some components of the basement membrane was prepared. Firstly, fibroblast suspensions were seeded at the bottom of 6-well plates followed by 24-hour culture. Subsequently, the prepared de-epidermized dermis was added into the 6-well plates, then, keratinocyte and melanocyte suspensions were seeded on the surface of the de-epidermized dermis with the melanocyte ∶ keratinocyte ∶ fibroblast ratio being 1 ∶ 4 ∶ 1. After 4 hours of culture, the cell mixtures were divided into two groups: an experimental group cultured with K-SFM, a control group cultured with a mixed medium containing DMEM with 10% fetal bovine serum, K-SFM and M254 at a ratio of 1 ∶ 1 ∶ 1. De-epidermized dermis cultured with K-SFM or the mixed medium alone served as blank control groups. After submerged cultivation for 3 days, the tissue cultures were maintained at an air-liquid interface for another 11 days with the culture medium changed every 3 days. Finally, these cultures were subjected to hematoxylin and eosin staining, periodic acid-Schiff （PAS） staining and immunohistochemical staining for Melan-A, S-100, HMB45, cytokeratin-Pan, P63, K5, K6, K14, Ki67, vimentin, collagen Ⅳ and laminin. Results After 14-day submerged and air-liquid interface culture, a well-structured epidermis developed in both the experimental group and control group with the formation of the stratum corneum. The immunohistochemical study showed positive staining for cytokeratin-Pan, P63, K5, K6, K14, Ki67, laminin in both the experimental group and control group, but positive staining for Melan-A, S-100, HMB45 and collagen Ⅳ in only the experimental group. Conclusion Tissue-engineered skin can be constructed using keratinocytes, melanocytes and fibroblasts co-cultured on de-epidermized dermis with K-SFM in vitro.

林建红汪宇卢彬刘志江蕾薇王今朝张伟李世军陆洪光. 角质形成细胞无血清培养基条件下构建组织工程皮肤[J]. 中华皮肤科杂志, 2016, 49(2): 103-107.doi:

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