HTRA1 shRNA慢病毒表达载体的构建及感染RPE细胞株的鉴定

眼科 ›› 2013, Vol. 22 ›› Issue (3): 195-200.

HTRA1 shRNA慢病毒表达载体的构建及感染RPE细胞株的鉴定

裴雪婷刘宁朴徐军

100730 首都医科大学附属北京同仁医院北京同仁眼科中心北京市眼科学与视觉科学重点实验室

收稿日期:2013-01-07 出版日期:2013-05-25 发布日期:2013-05-30
通讯作者: 刘宁朴，Email：liuningpu@gmail.com E-mail:liuningpu@gmail.com

Construction of a lentiviral vector of HTRA1 shRNA and identification of its RNA interference effect in a RPE cell line

PEI Xue-ting, LIU Ning-pu, XU Jun

Beijing Ophthalmology and Visual Science Key Laboratory, Beijing Tongren Eye Center, Beijing Tongren Hospital, Capital Medical University, Beijing 100730, China

Received:2013-01-07 Online:2013-05-25 Published:2013-05-30
Contact: LIU Ning-pu, Email: liuningpu@gmail.com E-mail:liuningpu@gmail.com

摘要/Abstract

摘要： 目的构建HTRA1基因的shRNA慢病毒表达载体，并鉴定HTRA1 shRNA慢病毒感染RPE细胞株的效果。设计实验研究。研究对象 HTRA1 shRNA慢病毒载体和RPE细胞。方法设计靶向HTRA1 mRNA的寡核苷酸序列，构建HTRA1 shRNA表达质粒，测序鉴定其序列的正确性。通过载体质粒pGC-LV与辅助质粒pHelper 1.0、pHelper 2.0共转染293T细胞包装慢病毒，收集病毒上清，测定滴度。将包装好的HTRA1 shRNA慢病毒感染RPE细胞，设阴性对照和空白对照，采用实时PCR（RT-PCR）和蛋白印迹法（Western Blot）方法检测HTRA1基因的mRNA水平和蛋白质表达水平的变化。主要指标 HTRA1基因的mRNA和蛋白质表达量。结果 DNA测序证实HTRA1 shRNA表达质粒包装了正确的RNA干扰序列。慢病毒滴度测定为8×108 TU/ml。HTRA1 shRNA慢病毒感染RPE细胞后，HTRA1基因的mRNA水平和蛋白质表达水平较空白对照组和阴性对照组均明显下降，差异均有统计学意义。结论成功构建了HTRA1 shRNA的慢病毒表达载体，该shRNA慢病毒能够有效地抑制RPE细胞株HTRA1基因的表达。

关键词: HTRA1, RPE细胞, 慢病毒, RNA干扰

Abstract: Objective This study was aimed to construct lentivirus-mediated shRNA expression vector targeting HTRA1 and identify the RNA interference effect in a RPE cell line. Design Experimental study. Participants HTRA1 shRNA lentivirus vector and RPE cells. Method One pair of oligonucleotide sequences targeted at human HTRA1 mRNA was designed and synthesized. The annealed oligonucleotide fragments were subcloned into plasmid vector. Virus particles were collected and enveloped into HEK-293T cells．The RPE cells were infected with recombinant lentivirus. Real-time PCR and Western Blot were used respectively to detect the expression of HTRA1 after lentivirus infection. Main Outcome Measures The mRNA and protein expression of HTRA1. Results DNA sequencing demonstrated that the lentivirus shRNA vector of HTRA1 was constructed successfully and the virus was packaged in 293 T cells．The titer of virus was 8×108 TU/ml. The RPE cell line was successfully infected. The mRNA and protein levels of HTRA1 were reduced significantly in RPE cells after lentivirus infection, compared with blank control and negative control． Conclusion It is concluded that the lentiviral shRNA vector of HTRA1 is constructed, and successfully reduced HTRA1 expression in a RPE cell line.

Key words: HTRA1 gene, RPE cell, lentivirus, RNA interference

裴雪婷刘宁朴徐军. HTRA1 shRNA慢病毒表达载体的构建及感染RPE细胞株的鉴定[J]. 眼科, 2013, 22(3): 195-200.

PEI Xue-ting, LIU Ning-pu, XU Jun. Construction of a lentiviral vector of HTRA1 shRNA and identification of its RNA interference effect in a RPE cell line[J]. Ophthalmology in China, 2013, 22(3): 195-200.