人全长PLCγ1基因真核表达载体的构建及鉴定

南方医科大学学报 ›› 2004, Vol. 24 ›› Issue (08): 849-853.

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人全长PLCγ1基因真核表达载体的构建及鉴定

李秀梅, 邓凡, 曾位森, 华亮, 陆地, 李明, 王宏, 刘忠英, 罗深秋

第一军医大学细胞生物学教研室, 广东, 广州, 510515

出版日期:2004-08-20 发布日期:2004-08-20
基金资助:
作者简介:LI Xiu-mei (1972-),PhD,Tel: 86-20-61648207,E-mail: hlxm1234@hotmail.com
通讯作者:LUO Shen-qiu,Professor,specialized in the research of cellular signal transduction,Te1:86-20- 61648208,E-mail:luoshq888@163.com

Construction and identification of eukaryotic expression vector of human full-length PLCγ1 gene

LI Xiu-mei, DENG Fan, ZENG Wei-sen, HUA Liang, LU Di, LI Ming, WANG Hong, LIU Zhong-ying, LUO Shen-qiu

第一军医大学细胞生物学教研室, 广东, 广州, 510515

Online:2004-08-20 Published:2004-08-20

摘要/Abstract

摘要： 目的构建人全长PLCγ1基因真核表达载体,以便进一步研究PLCγ1的作用及其机制。方法自行设计一对带有HindⅢ和NotⅠ酶切位点的引物,采用RT-PCR技术从MG63细胞中扩增人全长PLCγ1cDNA(3878bp),纯化后,经HindⅢ-NotⅠ酶切,插入真核表达载体pLNCX2中,构建重组质粒pLNCX2/PLCγ1。通过PCR,限制性酶切分析及DNA直接测序对所构建的重组质粒进行鉴定。同时经瞬时转染后,利用RT-PCR及Westernblotting转染后LoVo细胞中PLCγ1的表达。结果 RT-PCR产物经琼脂糖电泳分析所得片段大小与预期相符(3878bp)。重组质粒经HindⅢ-NotⅠ酶切后,得到3878bp(PLCγ1基因)及6100bp(载体pLNCX2)两个片段,同时重组质粒经HindⅢ-BglⅡ酶切后,得到约1300bp及约8500bp两个片段,与预期一致。DNA测序也证实了重组质粒的正确。经RT-PCR和Westernblot分析证实转染pLNCX2/PLCγ1的LoVo细胞中PLCγ1的表达均高于转染空质粒pLNCX2的LoVo细胞及未转染的LoVo细胞。结论成功构建了人全长PLCγ1基因真核表达载体pLNCX2/PLCγ1,为进一步研究PLCγ1的作用奠定了基础。

Abstract: Objective To construct the eukaryotic expression vector of human full-length PLCγ1 gene for further study of the role of PLCγ1 in cancer invasion. Methods Reverse transcription-polymerase chain reaction (RT-PCR) technique was used to amplify human full-length PLCγ1 gene from MG63 cells with a pair of specific primers containing the restriction sites for Hindb Ⅲ and Not Ⅰ. After purification, the product of RT-PCR was digested with Hindb Ⅲ and Not Ⅰ before insertion into the corresponding sites of eukaryotic expression vector pLNCX2, yielding the recombinant plasmid pLNCX2/PLCγ1. PCR, restriction endonuclease analysis and DNA sequencing were performed to identify the recombinant eukaryotic expression vector pLNCX2/PLCγ1. RT-PCR and Western blotting were used to detect the expression of the PLCγ1 gene in LoVo cells after transient transfection via Lipofectamine TM 2000. Results A 3 878-bp full-length PLCγ1 gene fragment was successfully amplified by RT-PCR and inserted into eukaryotic expression vector pLNCX2. After digestion by Hindb Ⅲ and Not Ⅰ, the recombinant eukaryotic expression vector pLNCX2/PLCγ1 yielded a 3 878-bp fragment (PLCγ1 gene) and a 6 100 bp fragment (vector). Hindb Ⅲ-Bgla! digestion was also done to verify the correctness of the recombinant plasmid, resulting in the identification of the fragments as expected. Sequencing analysis further confirmed the results. In addition, RT-PCR and Western blotting verified that the PLCγ1 could overexpress in LoVo cells after transfection with recombinant eukaryotic expression vector pLNCX2/PLCγ1. Conclusion The recombinant eukaryotic expression vector pLNCX2/PLCγ1 has been constructed successfully.

中图分类号:

Q785

李秀梅, 邓凡, 曾位森, 华亮, 陆地, 李明, 王宏, 刘忠英, 罗深秋. 人全长PLCγ1基因真核表达载体的构建及鉴定[J]. 南方医科大学学报, 2004, 24(08): 849-853.

LI Xiu-mei, DENG Fan, ZENG Wei-sen, HUA Liang, LU Di, LI Ming, WANG Hong, LIU Zhong-ying, LUO Shen-qiu. Construction and identification of eukaryotic expression vector of human full-length PLCγ1 gene[J]. Journal of Southern Medical University, 2004, 24(08): 849-853.

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人全长PLCγ1基因真核表达载体的构建及鉴定

Construction and identification of eukaryotic expression vector of human full-length PLCγ1 gene

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