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Nanostructured lipid carriers loaded with resveratrol modulate human dendritic cells

Title
Nanostructured lipid carriers loaded with resveratrol modulate human dendritic cells
Type
Article in International Scientific Journal
Year
2016
Authors
Barbosa, JP
(Author)
Other
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Neves, AR
(Author)
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Silva, AM
(Author)
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Barbosa, MA
(Author)
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Salette Reis
(Author)
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Santos, SG
(Author)
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Journal
Vol. 11
Pages: 3501-3516
ISSN: 1176-9114
Publisher: Dove Medical Press
Other information
Authenticus ID: P-00K-QMR
Abstract (EN): Dendritic cells (DCs) are promising targets for drug delivery, as they can induce immunity or tolerance. The current study aims to examine the potential of using nanostructured lipid carriers (NLC) as delivery systems for human DC by evaluating nanoparticle internalization, cell labeling, and drug activity. NLC were formulated incorporating the fluorochrome fluorescein isothiocyanate (FITC-NLC) or the natural anti-inflammatory molecule resveratrol (rsv-NLC). Primary human DCs were differentiated from peripheral blood monocytes, and the innovative imaging flow cytometry technique was used to examine FITC-NLC internalization. The capacity of rsv-NLC to inhibit DC activation in response to proinflammatory cytokine tumor necrosis factor-alpha (TNF-alpha) was investigated by conventional flow cytometry. A combination of imaging and conventional flow cytometry was used to assess NLC cytotoxicity. The results obtained indicate that both NLC formulations were stable over time, with mean diameter <200 nm and highly negative zeta potential (about-30 mV). When DCs were placed in contact with NLC, imaging flow cytometry clearly showed that DCs efficiently internalized FITC-NLC, with nearly 100% of cells internalizing nanoparticles upon 1 hour of incubation. Both immature and mature DCs internalized NLC to high and comparable levels, and without cytotoxicity. Stimulating DC with TNF-alpha in the presence of rsv-NLC revealed that, using these nanoparticles, very small concentrations of rsv were sufficient to significantly decrease surface expression of activation marker CD83 (5 mu M) and major histocompatibility complex-class II molecule human leukocyte antigen-antigen D related (10 mu M), both upregulated in response to TNF-alpha stimulation. Rsv-NLC were compared with free rsv; at 5 mu M, rsv-NLC were able to inhibit nuclear factor. beta phosphorylation and significantly decrease the level of interleukin-12/23, both upregulated in response to TNF-alpha, while 10 mu M free rsv were needed to promote a similar effect. Taken together, the results presented show that NLC are suitable carriers of fluorescent labels or bioactive molecules for human DCs, leading to inflammation modulation.
Language: English
Type (Professor's evaluation): Scientific
No. of pages: 16
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