articleScientific ReportsMay 22, 2012GOLD OA

Quantitative assessment on the cloning efficiencies of lentiviral transfer vectors with a unique clone site

GZGang ZhangATAnurag Tandon

University of Toronto

PubMed
Indexed incrossrefdoajpubmed

Abstract

Lentiviral vectors (LVs) are powerful tools for transgene expression in vivo and in vitro. However, the construction of LVs is of low efficiency, due to the large sizes and lack of proper clone sites. Therefore, it is critical to develop efficient strategies for cloning LVs. Here, we reported a combinatorial strategy to efficiently construct LVs using EGFP, hPlk2 wild type (WT) and mutant genes as inserts. Firstly, site-directed mutagenesis (SDM) was performed to create BamH I site for the inserts; secondly, pWPI LV was dephosphorylated after BamH I digestion; finally, the amounts and ratios of the insert and vector DNA were optimized to increase monomeric ligation. Our results showed that the total percentage…

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1,027
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2

Topics & keywords

Topics
Keywords
  • Insert (composites)
  • Cloning (programming)
  • Mutagenesis
  • clone (Java method)
  • Computational biology
  • Biology
  • Transgene
  • Mutant
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