High capacity extrachromosomal gene expression vectors.

Journal article

Abstract:: Extrachromosomal gene expression vectors that contain native genomic gene expression elements have numerous advantages over traditional integrating mini-gene vectors. In this protocol chapter we describe our work using episomal vectors where expression of a cDNA is controlled by a 10 kB piece of genomic DNA encompassing the promoter of the low density lipoprotein receptor. We explain methods to sub-clone large genomic inserts into gene expression vectors. We also illustrate various methods employed to ascertain whether expression from these vectors is robust and physiologically relevant by investigating their sensitivity to changes in cellular milieu. Delivery of gene expression vectors in vivo is also described using hydrodynamic tail vein injection, a high pressure, high volume tail vein injection used for liver-directed gene transfer.

Journal:: Methods in molecular biology (Clifton, N.J.) More from this journal
Volume:: 738
Pages:: 19-40
Publication date:: 2011-01-01
DOI:: 10.1007/978-1-61779-099-7_2
EISSN:: 1940-6029
ISSN:: 1064-3745

Language:: English
Keywords:: Genome

Humans

Genetic Vectors

Promoter Regions, Genetic

Genes, Reporter

Organ Specificity

DNA

Cricetinae

Molecular Imaging

Animals

Gene Expression

Protein Transport

Receptors, LDL

Hyperlipoproteinemia Type II

Lipoproteins, LDL

Cricetulus

Plasmids

CHO Cells

Genetic Engineering

Luciferases

Transgenes

Mice

Transfection

Chromosomes, Artificial, Bacterial

Liver

Genetic Therapy
Pubs id:: pubs:127190
UUID:: uuid:1bd994bd-9f45-47e6-b11c-c9142d56a2da
Local pid:: pubs:127190
Source identifiers:: 127190
Deposit date:: 2012-12-19

Licence:: Terms and Conditions of Use for Oxford University Research Archive

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