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评估病毒和哺乳动物启动子在小鼠肝脏中驱动转基因表达的能力。

Evaluation of viral and mammalian promoters for driving transgene expression in mouse liver.

作者信息

Al-Dosari Mohammed, Zhang Guisheng, Knapp Joseph E, Liu Dexi

机构信息

Department of Pharmaceutical Sciences, University of Pittsburgh School of Pharmacy, Pittsburgh, PA 15261, USA.

出版信息

Biochem Biophys Res Commun. 2006 Jan 13;339(2):673-8. doi: 10.1016/j.bbrc.2005.11.063. Epub 2005 Nov 21.

DOI:10.1016/j.bbrc.2005.11.063
PMID:16316630
Abstract

Fifteen luciferase plasmid constructs driven by various promoters including cytomegalovirus (CMV), Rous sarcoma virus (RSV), human serum albumin (SA), alpha-1 antitrypsin (AAT), cytochrome P450 CYP1A2, CYP2C9, CYP2C18, CYP2D6, CYP3A4, mouse CYP2b10, human amyloid precursor protein (APP), chicken beta actin (ACT), nuclear factor kappa B (NFkappaB), and heat shock protein 70 (HS) promoters were hydrodynamically introduced into mouse hepatocytes, and the level and persistence of luciferase gene expression were examined. Eight hours post-gene transfer, the CMV and AAT promoters showed the highest activity, followed by the CYP2D6, HS, and RSV promoters which were slightly less active. The human serum albumin promoter exhibited the lowest activity among the promoters examined. The time course of gene expression showed a two-phase decline in luciferase activity with a rapid phase within the first 5-7 days and a slower decline thereafter. Results from Southern and Northern blot analyses revealed a good correlation between the decline of luciferase activity and the decrease in mRNA level, suggesting promoter silencing as the possible mechanism for the observed transient luciferase gene expression. Inclusion of EBN1 and oriP sequences of Epstein-Barr virus into the plasmid extended the period of active transcription for about one week. These results provide important information concerning the role of promoters in regulating transgene expression and for the proper design of plasmids for gene expression and gene therapy.

摘要

将由多种启动子驱动的15种荧光素酶质粒构建体通过流体动力学方法导入小鼠肝细胞,这些启动子包括巨细胞病毒(CMV)、劳氏肉瘤病毒(RSV)、人血清白蛋白(SA)、α-1抗胰蛋白酶(AAT)、细胞色素P450 CYP1A2、CYP2C9、CYP2C18、CYP2D6、CYP3A4、小鼠CYP2b10、人淀粉样前体蛋白(APP)、鸡β-肌动蛋白(ACT)、核因子κB(NFκB)和热休克蛋白70(HS)启动子,然后检测荧光素酶基因表达的水平和持久性。基因转移后8小时,CMV和AAT启动子显示出最高活性,其次是活性稍低的CYP2D6、HS和RSV启动子。在所检测的启动子中,人血清白蛋白启动子活性最低。基因表达的时间进程显示荧光素酶活性呈两阶段下降,第一阶段在前5 - 7天内下降迅速,此后下降较慢。Southern和Northern印迹分析结果显示荧光素酶活性的下降与mRNA水平的降低之间具有良好的相关性,提示启动子沉默可能是观察到的荧光素酶基因瞬时表达的机制。将爱泼斯坦 - 巴尔病毒的EBN1和oriP序列包含在质粒中可使活跃转录期延长约一周。这些结果为启动子在调节转基因表达中的作用以及为基因表达和基因治疗的质粒正确设计提供了重要信息。

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