Highlights Catechol-functionalization of a polyamidoamine for tight linkage to SPION surface size 100±28 nm). SPION@ISA23-ND were re-suspended after lyophilization reverting to their pristine dimensions. The SPION@ISA23-ND adsorption of BSA in water, considered as the first stage of phagocytosis, was very low, suggesting that ISA23 could impart stealthiness to SPION@ISA23-ND. 1 H-NMR relaxivity measurements showed an r2 value of 158 s-1 mmol-1 L (vs 100 s-1 mmol-1 L for Endorem) at relevant clinical fields for magnetic resonance imaging (from 0.2 to 1.5 T). SPION@ISA23-ND was tested on HeLa cells and their internalization was visualized by reflectance microscopy. Finally, with the aim of prepare a new dual magneto-optical system, a synthetic procedure to decorate SPION@ISA23-ND with a fluorescent dye was devised, even though the emission intensity of the resultant conjugate was lower than expected, possibly due to luminescence quenching caused by the closeness of emitting moieties to the SPION surface.
Strategies
for endosomal escape and access to the cell nucleus are highly sought
for nanocarriers to deliver their load efficiently following endocytosis.
In this work, we have studied the uptake and intracellular trafficking
of a polycationic polyamidoamine (PAA) endowed with a luminescent
Ru complex, Ru–PhenAN, that shows unique trafficking to the
cell nucleus. Live cell imaging confirmed the capacity of this polymer
to access the nucleus, excluding artifacts due to cell fixation, and
clarified that the mechanism of escape is light-triggered and relies
on the presence of the Ru complexes and their capacity to absorb light
and act as photosensitizers for singlet oxygen production. These results
open up the possibility to use PAA–ruthenium complexes for
targeted light-triggered delivery of genetic material or drugs to
the cytosol and nucleus.
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