| Literature DB >> 26185052 |
Kangqiang Qiu1, Bole Yu1, Huaiyi Huang1, Pingyu Zhang1, Juanjuan Huang1, Shanshan Zou1, Yu Chen1, Liangnian Ji1, Hui Chao1.
Abstract
Fluorescent tracking gene delivery could provide us with a better understanding of the critical steps in the transfection process. However, for in vivo tracking applications, a small diameter (<10 nm) is one of the rigorous requirements for tracking vectors. Herein, we have demonstrated a new paradigm for two-photon tracking gene delivery based on a dendritic nano-sized hexanuclear ruthenium(II) polypyridyl complex. Because thisEntities:
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Year: 2015 PMID: 26185052 PMCID: PMC4505312 DOI: 10.1038/srep10707
Source DB: PubMed Journal: Sci Rep ISSN: 2045-2322 Impact factor: 4.379
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Figure 3(a) Agarose gel electrophoresis of pBR 322 DNA (45 μM) after incubation with Ru6L at various +/− ratios in aqueous solution; (b) Hydrodynamic diameter and (c) zeta potential of the pBR 322 DNA (1.5 μM) incubation with Ru6L at various +/− ratios in an aqueous solution,as determined by DLS.
Figure 4(a) AFM images of the condensation process, starting with2 kb DNA (1.5 μM), induced by incubation with Ru6L at +/− ratios of 1 (a1), 2 (a2), 4 (a3), and 20 (a4), respectively. (b) Schematic representation of the stepwise DNA compaction by RuL.
Figure 5Cellular uptake and intracellular localization of Ru6L-pEGFP DNA particles at the +/− ratio of 20 monitored, as by TEM. The DNA concentration was 1.5 μM, N: nucleus, C: cytoplasm.
Figure 6Time-dependent confocal microscopy images of entry and transportation of Ru6L-pEGFP DNA particles at the +/− ratio of 20 in HeLa cells. The DNA concentration was 1.5 μM. The red luminescence is RuL, the blue florescence is Hoechst 33258 and the green florescence is GFP.
Figure 7Transfection efficiencies of Ru6L-pGL3 DNA particles in HeLa cells, as determined by luciferase assays; the DNA concentration was 1.5 μM. As a control, DNAand lipofectamine 2000 were also investigated.
Figure 8The cell viability of Ru6L and Ru6L-pEGFP DNA particles in HeLa cells, as determined by MTT assays; the DNA concentration was 1.5 μM.