Identification of CHO Endogenous Gene Regulatory Elements

被引:0
|
作者
Jens Pontiller
Andreas Maccani
Martina Baumann
Ingo Klancnik
Wolfgang Ernst
机构
[1] University of Natural Resources and Applied Life Sciences,Department of Biotechnology, Austrian Center of Biopharmaceutical Technology
[2] POLYMUN Scientific Immunbiologische Forschung GmbH,undefined
来源
Molecular Biotechnology | 2010年 / 45卷
关键词
Endogenous promoter; Chinese hamster ovary cells; Recombinant protein expression; Library construction; DNA fragmentation;
D O I
暂无
中图分类号
学科分类号
摘要
The objective of this approach was to identify new CHO endogenous gene regulatory elements that are capable of regulating foreign gene expression in recombinant CHO host cells. The standard technology for the production of many biopharmaceutical products is frequently based on expression vectors that utilize strong mammalian viral promoters like SV40 or CMV which allow for very high expression rates but this may lead to constitutive over-expression resulting in a permanent stress for the cell. In addition, some heterologous promoters are cell-cycle dependent and can be subject to gene silencing generating heterogeneity within the cell population. Here, we describe the construction of a genomic CHO library and the subsequent identification and isolation of selected target sequences that are believed to be responsible for high level expression of the associated genes. The method that was used to isolate these regions of interest relies on gene specific amplification with primer pairs binding on different genes and the vector sequence. Flanking regions of these fragments were identified through Inverse PCR from fragmented and self-ligated genomic DNA. Expression levels of both the initially derived and the mapped fragments were determined through a luciferase reporter assay.
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页码:235 / 240
页数:5
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