人GJB6基因Tet-on HaCaT细胞稳定株的构建与鉴定

摘要/Abstract

摘要：

目的以Tet-on慢病毒为载体建立稳定表达GJB6基因及其突变体的HaCaT细胞株，为后续研究有汗性外胚层发育不良的发病机制奠定实验基础。方法利用PCR技术扩增人GJB6基因野生型与突变型（A88V）基因，重组Tet-on慢病毒质粒，经基因测序及酶切技术对其鉴定，再将重组慢病毒转染入HaCaT细胞，经嘌呤霉素筛选出稳定表达编码缝隙连接蛋白Cx30的GJB6基因的细胞株。细胞株加四环素诱导后，通过RT-PCR检测GJB6基因的mRNA表达量，同时通过Western印迹检测Cx30与FLAG标签肽的表达，从而对稳定表达GJB6基因的HaCaT细胞株进行鉴定。用CCK8法检测GJB6基因野生型与突变型经四环素诱导表达后对细胞增殖的影响。结果经酶切、测序鉴定，重组慢病毒质粒构建成功。RT-PCR检测到稳定转染的HaCaT细胞中GJB6基因mRNA表达量明显增加，感染野生型Tet-on慢病毒的HaCaT细胞组（WT组）加四环素GJB6基因表达丰度是WT组不加四环素的113.369倍（P < 0.05），感染突变型（A88V）Tet-on慢病毒的HaCaT细胞组（MU组）加四环素GJB6基因表达丰度是MU组不加四环素的3.249倍（P < 0.05）；Western印迹可检测到经四环素处理的WT组和MU组稳定表达Cx30与FLAG，而未经四环素处理的细胞和感染阴性对照病毒的HaCaT细胞组（NC组）未检测到Cx30与FLAG目的条带。NC组加与不加入四环素在4、8、12、24、36、48 h时的A值差异均无统计学意义（P ＞ 0.05）；WT组加与不加入四环素在4、8、12、24、36 h时的A值差异均有统计学意义（P < 0.05）；MU组加与不加入四环素在4、8、12、24、36、48 h时的A值差异均有统计学意义（P < 0.05）。结论成功构建出稳定表达GJB6基因野生型及其突变体A88V的HaCaT细胞株。

Abstract:

Lu Yuting, Wang Zhenying, Song Yali, Ji Cancan, Zhang Li Department of Dermatology, Shandong Provincial Hospital Affiliated to Shandong University, Jinan 250021, China Corresponding author: Zhang Li, Email: zhangliwenzhe@medmail.com.cn 【Abstract】 Objective To construct HaCaT cell lines stably expressing the wild type human GJB6 gene or its mutant by using a Tet-On lentiviral vector, and to lay an experimental foundation for studies on pathogenesis of hidrotic ectodermal dysplasia. Methods The wild-type human GJB6 gene and its mutant （A88V） were amplified by PCR, and then inserted into the Tet-on lentivirus plasmid to construct recombinant lentivirus vectors. The recombinants were identified by gene sequencing and enzymatic digestion. Cultured HaCaT cells were classified into three groups to be transfected with a negative control lentiviral vector （NC group）, the lentivirus vector expressing the wild-type human GJB6 gene （WT group）, or the lentivirus vector expressing the mutant human GJB6 gene （MU group）. Puromycin was used to select HaCaT cell clones stably expressing the GJB6 gene which encodes the connexin 30 （Cx30） protein. The selected HaCaT cell clones were cultured with or without tetracycline for 48 hours, thereafter, real-time PCR （RT-PCR） was performed to detect GJB6 gene mRNA , Western-blot analysis to measure s of Cx30 and FLAG-tag proteins, and cell counting kit 8 （CCK8） assay to evaluate cellular proliferative activity. Results Enzymatic digestion and gene sequencing showed that recombinant lentivirus plasmids were successfully constructed. RT-PCR showed evidently increased mRNA of the GJB6 gene in stably transfected HaCaT cells. Moreover, the abundance of the GJB6 gene was 112.369 times higher in the WT group induced by tetracycline than in that without tetracycline treatment （P < 0.05）, and 2.249 times higher in the MU group induced by tetracycline than in that without tetracycline treatment （P < 0.05）. Western-blot analysis showed that Cx30 and FLAG-tag proteins were stably expressed in the WT group and MU group after induction with tetracycline, while neither of them was observed in the WT group or MU group without tetracycline treatment, or in the NC group. Significant differences were noted in cellular proliferative activity （expressed as the absorbance value at 450 nm） between the MU group with and without tetracycline treatment and between the WT group with and without tetracycline treatment at 4, 8, 12, 24, 36 and 48 hours（all P < 0.05）, but not between the NC group with and without tetracycline treatment at any of the above time points （all P > 0.05）. Conclusion HaCaT cell lines which stably express the wild-type GJB6 gene or its mutant （A88V） are successfully constructed.

中图分类号:

R246.7

路雨婷王震英宋亚丽姬灿灿张莉. 人GJB6基因Tet-on HaCaT细胞稳定株的构建与鉴定[J]. 中华皮肤科杂志, 2016, 49(4): 265-270.

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