| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 1425020 | Journal of Controlled Release | 2011 | 8 Pages |
Cellular uptake and nuclear localization are two barriers to gene delivery. Here, we designed new gene delivery carriers with an N-terminal stearylated (STR) nuclear localization signal (NLS), PKKKRKV, present in the Simian Virus 40 large T antigen with the aim to overcome limitations, such as cell membrane and nuclear pores, offering attractive possibilities to enhance gene delivery. Four vectors with different structures of N-stearylated nuclear localization signal-octaarginine peptide (STR-PKKKRKV-R8 or STR-NLS-R8, STR-VKRKKKP-R8 or STR-reverse NLS-R8, PKKKRKV-R8 or NLS-R8, and VKRKKKP-R8 or reverse NLS-R8) were compared. The gene expression mediated by these vectors in dividing and non-dividing cells (both in 293T and HeLa cell lines) was investigated. The most efficient N/P ratio was 4 for STR-PKKKRKV-R8, STR-VKRKKKP-R8, and 0.25 for PKKKRKV-R8, VKRKKKP-R8. The maximum transfection activity of these vehicles (VKRKKKP-R8) was up to 80% as effective as jetPEI™ and the vehicles did not exhibit cytotoxicity. Interestingly, N-stearylated peptides presented lower transfection activity compared to peptides without N-stearylation at lower N/P ratios (0.25 to 1). Confocal study showed that the vectors could effectively promote the nuclear translocation.
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