AI Article Synopsis

  • The first-generation vector pCMViR-TSC shows significantly higher gene expression (10- to 100-fold) compared to standard plasmids but is limited to transient gene expression in mammalian cells.
  • To address this limitation, a new second-generation vector, pSAKA-4B, is introduced, enabling stable integration of genes into mammalian DNA with high efficiency.
  • This improved vector system allows for indefinite gene expression, making it valuable for basic research and potential clinical applications like gene therapy.

Article Abstract

The first-generation pCMViR-TSC, implemented through the promoter sandwich rule, yields 10- to 100-fold higher gene expression than the standard plasmid used with the CMV (cytomegalovirus) or CAG promoter. However, the vector's shortcomings limit its utility to transient expression only, as it is not suitable for establishing stable transformants in mammalian cells. To overcome this weakness, we here introduce the improved plasmid vector pSAKA-4B, derived from pCMViR-TSC as a second-generation chromosome-insertable vector. This vector facilitates the linear entry of the expression unit into the TTAA site of DNA universally with transposase assistance. The vector is helpful for the indefinite expression of our target gene. The new vector system is proven here to be efficient in establishing stable transformants with a high likelihood of positive clones that exhibit significantly elevated expression levels of the delivered foreign gene. This system, alongside the first-generation vector, is therefore instrumental for diverse basic research endeavors concerning genes, proteins, cells, and animals, and potentially for clinical applications such as gene therapy.

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Source
http://dx.doi.org/10.1007/s11626-024-00992-2DOI Listing
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11655592PMC

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