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[Cloning and functional verification of U6 and 7SK promoter of small RNA from Bama mini-pig in Guangxi].

作者信息

Chen Shi-Jin, Fan Jing, Jiang Qin-Yang, Lan Gan-Qiu, Guo Xiao-Ping, Guo Ya-Fen

机构信息

College of Animal Science and Technology, Guangxi University, Nanning 530005, China.

出版信息

Yi Chuan. 2012 Apr;34(4):445-53. doi: 10.3724/sp.j.1005.2012.00445.

DOI:10.3724/sp.j.1005.2012.00445
PMID:22522162
Abstract

To investigate the functions of U6 and 7SK of Bama mini-pig and produce Bama mini-pig with silenced GGTA1 gene, the siRNA promoters U6 and 7SK were cloned, ligated into pMD18-shEGFP, and co-transfected with PEGFP- N1 into PK-15 kidney cells of pigs to be used in RNAi experiments. The functions of the two promoters in pig cells were verified using pMD18-hU6-shEGFP as the positive control, pMD18-shEGFP vector without promoter as the negative control, PEGFP-N1 as the first blank control, ddH2O in replacement of the plasmid as the second blank control. The results showed that the lengths of U6 and 7SK in Bama mini-pig were 553 bp and 437 bp, respectively. Vectors pMD18-pU6- shEGFP and pMD18-p7SK-shEGFP were constructed and transfected into PK-15 cells from pigs. Promoters pU6 and p7SK proved to express high levels of siRNA activity and can be used in the experiment of silencing α-1,3galactosyltransferase gene.

摘要

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