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利用兔成纤维细胞前体和明胶水凝胶进行角膜基质的组织工程研究。

Tissue engineering of corneal stroma with rabbit fibroblast precursors and gelatin hydrogels.

作者信息

Mimura Tatsuya, Amano Shiro, Yokoo Seiichi, Uchida Saiko, Yamagami Satoru, Usui Tomohiko, Kimura Yu, Tabata Yasuhiko

机构信息

Department of Ophthalmology, University of Tokyo Graduate School of Medicine, Tokyo, Japan.

出版信息

Mol Vis. 2008;14:1819-28. Epub 2008 Oct 3.

Abstract

PURPOSE

To isolate fibroblast precursors from rabbit corneal stroma using a sphere-forming assay, to engineer corneal stroma with the precursors and gelatin, and to establish the therapeutic application of precursors in a rabbit corneal stroma.

METHODS

In the in vitro study, a sphere-forming assay was performed to produce precursors from rabbit corneal stroma. Corneal stroma was engineered by cultivating precursors in porous gelatin for one week. In the in vivo study, the engineered corneal stromal sheet with precursors (precursor/gelatin group) or with fibroblasts (fibroblast /gelatin group) or without cells (gelatin group) was transplanted to a pocket of rabbit corneal stroma. Gene expression and extracellular matrix production were examined immunohistochemically in each group one week and four weeks after surgery.

RESULTS

In the in vitro study, cells in the spheres were BrdU-positive, and their progeny were keratocan-positive. The study also showed that the corneas transplanted with a porous gelatin sheet did not show any opacity four weeks after transplantation in any group. In the gelatin sheet of the precursor/gelatin group, a more intense expression of type I collagen was observed relative to the other two groups four weeks after the surgery.

CONCLUSIONS

Our findings demonstrate that the transplantation of fibroblast precursors combined with gelatin hydrogel into the corneal stroma is a possible treatment strategy for corneal stromal regeneration.

摘要

目的

采用成球试验从兔角膜基质中分离成纤维细胞前体细胞,用这些前体细胞和明胶构建角膜基质,并确立前体细胞在兔角膜基质中的治疗应用。

方法

在体外研究中,进行成球试验以从兔角膜基质中产生前体细胞。通过将前体细胞在多孔明胶中培养一周来构建角膜基质。在体内研究中,将带有前体细胞的工程化角膜基质片(前体细胞/明胶组)或带有成纤维细胞的(成纤维细胞/明胶组)或无细胞的(明胶组)移植到兔角膜基质的囊袋中。在术后一周和四周,通过免疫组织化学检查每组中的基因表达和细胞外基质产生情况。

结果

在体外研究中,球体中的细胞BrdU呈阳性,其后代角蛋白聚糖呈阳性。该研究还表明,在任何组中,移植多孔明胶片的角膜在移植后四周均未出现任何混浊。在手术四周后,前体细胞/明胶组的明胶片中观察到I型胶原的表达相对于其他两组更强。

结论

我们的研究结果表明,将成纤维细胞前体细胞与明胶水凝胶联合移植到角膜基质中是角膜基质再生的一种可能治疗策略。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2fce/2566587/2ca6711f1451/mv-v14-1819-f1.jpg

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