转染至猫角膜内皮细胞的人血小板源性生长因子-B基因的研究

The study of human PDGF-B gene transferred to cat corneal endothelial cells.

作者信息

Luo Wen-Juan, Wang Xiao-Ji, Xing Xiao-Ming, Wang Chuan-Fu

机构信息

Department of Ophthalmology, the Affiliated Hospital of Medical College, Qingdao University, Qingdao 266003, Shandong Province, China.

出版信息

Int J Ophthalmol. 2012;5(1):18-22. doi: 10.3980/j.issn.2222-3959.2012.01.04. Epub 2012 Feb 18.

DOI:10.3980/j.issn.2222-3959.2012.01.04

PMID:22553748

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3340845/

Abstract

AIM

To demonstrate that human platelet-derived growth factor-B (PDGF-B) cDNA could be expressed in primary cultured cat corneal endothelia cells by using gene transfer techniques; to explore a useful tool for the further studies of the molecular mechanisms of corneal endothelium failure and provide a potential effective genetic therapy for the blind patients.

METHODS

Human PDGF-B cDNA was isolated from human placent by RT-PCR and inserted into pcDNA(4) vector to construct recombinant eukaryotic expression plasmid pcDNA(4)-PDGF-B. The full length was confirmed by the DNA sequencing analysis. By tearing endothelium technique we obtained pure single layer of cat corneal endothelial cells. The pcDNA(4)-PDGF-B eukaryotic expression vector was transferred into cat corneal endothelial cells by Effectene™ lipofectine. The transfection efficiency of Effectene™ lipofectine in pcDNA(4)-B was detected with pcDNA(4)-GFP. 5 days later, RT-PCR was used to check the PDGF-B expression. Cell viability was tested by modified tertrozalium salt (MTT) method. Cell morphology was observed under inverted phase contrast microscope.

RESULTS

The human PDGF-B cDNA was isolated successfully from healthy parturien placent tissue and the sequence was confirmed by computer automatic sequence and PCR analysis. Pure single layer cat corneal endothelial cells were successfully cultured by tearing endothelium technique. Effectene™ lipofectine transfection technique could be effectively used to transfer pcDNA(4)-PDGF-B into cat corneal endothelial cells in vitro, the transfection efficiency was 30%. RT-PCR result showed that human PDGF-B gene was highly expressed in transfected cat corneal endothelial cells. The expressed PDGF-BB protein promoted the viability of cat corneal endothelial cells.

CONCLUSION

Human platelet-derived growth factor-B (PDGF-B) cDNA could be highly expressed in cultured cat corneal endothelial cells by gene transfection techniques. Expressed PDGF-BB protein significantly promoted the viability of cat corneal endothelial cells, thus provided a potential effective method for corneal endothelium blindness genetic therapy.

摘要

目的

通过基因转移技术证明人血小板衍生生长因子-B（PDGF-B）cDNA可在原代培养的猫角膜内皮细胞中表达；探索一种用于进一步研究角膜内皮功能衰竭分子机制的有用工具，并为失明患者提供一种潜在有效的基因治疗方法。

方法

通过RT-PCR从人胎盘组织中分离出人PDGF-B cDNA，并将其插入pcDNA(4)载体中构建重组真核表达质粒pcDNA(4)-PDGF-B。通过DNA测序分析确认全长。采用撕除内皮技术获得纯净的单层猫角膜内皮细胞。利用Effectene™脂质体将pcDNA(4)-PDGF-B真核表达载体转染至猫角膜内皮细胞。用pcDNA(4)-GFP检测Effectene™脂质体对pcDNA(4)-B的转染效率。5天后，采用RT-PCR检测PDGF-B的表达。采用改良的噻唑蓝盐（MTT）法检测细胞活力。在倒置相差显微镜下观察细胞形态。

结果

成功从健康产妇胎盘组织中分离出人PDGF-B cDNA，经计算机自动测序和PCR分析确认序列。采用撕除内皮技术成功培养出纯净的单层猫角膜内皮细胞。Effectene™脂质体转染技术可有效将pcDNA(4)-PDGF-B体外转染至猫角膜内皮细胞，转染效率为30%。RT-PCR结果显示人PDGF-B基因在转染的猫角膜内皮细胞中高表达。表达的PDGF-BB蛋白促进了猫角膜内皮细胞的活力。