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Improved Lentiviral Gene Delivery to Mouse Liver by Hydrodynamic Vector Injection through Tail Vein.

Mol Ther Nucleic Acids. 2018-09; 
DalsgaardTrine,CecchiClaudia R,AskouAnne Louise,BakRasmus O,AndersenPernille O,HougaardDavid,JensenThomas G,Dagnæs-HansenFrederik,MikkelsenJacob Giehm,CorydonThomas J,Aagaard
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Gene Synthesis … The human elongation factor-1α (EF1α) promoter was PCR-amplified with ClaI- and BamHI-tagged primers from a custom-made vector harboring a shortened version of the EF1α promoter (pUC57-mirvector, Genscript, Piscataway, USA) … Get A Quote

摘要

Delivery of genes to mouse liver is routinely accomplished by tail-vein injections of viral vectors or naked plasmid DNA. While viral vectors are typically injected in a low-pressure and -volume fashion, uptake of naked plasmid DNA to hepatocytes is facilitated by high pressure and volumes, also known as hydrodynamic delivery. In this study, we compare the efficacy and specificity of delivery of vesicular stomatitis virus G glycoprotein (VSV-G) pseudotyped lentiviral vectors to mouse liver by a number of injection schemes. Exploiting in vivo bioluminescence imaging as a readout after lentiviral gene transfer, we compare delivery by (1) "conventional" tail-vein injections, (2) "primed" injections, (... More

关键词

gene transfer,hepatocytes,high-pressure tail-vein injection,hydrodynamic delivery,in vivo,lentivirus,liver gene the