Release, transfer and partition of fluorescent dyes from polymeric nanocarriers to serum proteins monitored by asymmetric flow field-flow fractionation.

Oliveira, Maria Alice de; Lana, Gwenaelle Elza Nathalie Pound; Oliveira, Patricia Capelari de; Pontífice, Thaís Godinho; Silva, Sabrina Emanuelle Dias; Machado, Marina Guimarães Carvalho; Postacchini, Bruna Bueno; Mosqueira, Vanessa Carla Furtado

Use este identificador para citar ou linkar para este item: http://www.repositorio.ufop.br/jspui/handle/123456789/14122

Título:	Release, transfer and partition of fluorescent dyes from polymeric nanocarriers to serum proteins monitored by asymmetric flow field-flow fractionation.
Autor(es):	Oliveira, Maria Alice de Lana, Gwenaelle Elza Nathalie Pound Oliveira, Patricia Capelari de Pontífice, Thaís Godinho Silva, Sabrina Emanuelle Dias Machado, Marina Guimarães Carvalho Postacchini, Bruna Bueno Mosqueira, Vanessa Carla Furtado
Palavras-chave:	Lipophilicity Dye-protein binding
Data do documento:	2021
Referência:	OLIVEIRA, M. A. de et al. Release, transfer and partition of fluorescent dyes from polymeric nanocarriers to serum proteins monitored by asymmetric flow field-flow fractionation. Journal of Chromatography A, v. 1641, p. 461959, 2021. Disponível em: <https://www.sciencedirect.com/science/article/abs/pii/S0021967321000832>. Acesso em: 10 jun. 2021.
Resumo:	Fluorescent probes are used in drug nanocarrier pre-clinical studies or as active compounds in theranostics and photodynamic therapy. In the biological medium, nanoparticles interact with proteins, which can result in the off-target release of their cargo. The present study used asymmetric flow field-flow fractionation with online multi-angle laser light scattering and fluorescence detection (AF4-MALLS-FLD) to study the release, transfer, and partition of fluorescent dyes from polymeric nanoparticles (NP). NP formulations containing the dyes Rose Bengal, Rhodamine B, DiI, 3-(α-azidoacetyl)coumarin and its polymer conjugate, Nile Red, and IR780 and its polymer conjugate were prepared. NP suspensions were incubated in a medium with serum proteins and then analyzed by AF4. AF4 allowed efficient separation of proteins (< 10 nm) from fluorescently labeled NP (range of 54 – 180 nm in diameters). The AF4 analyses showed that some dyes, such as Rose Bengal, IR780, and Coumarin were transferred to a high extent (68-77%) from NP to proteins. By contrast, for DiI and dye-polymer conjugates, transfer occured to a lower extent. The studies of dye release kinetics showed that the transfer of IR780 from NP to proteins occurs at a high extent (~50%) and rate, while Nile Red was slowly released from the NP over time with reduced association with proteins (~20%). This experiment assesses the stability of fluorescence labeling of nanocarriers and probes the transfer of fluorescent dyes from NP to proteins, which is otherwise not accessible with commonly used techniques of separation, such as dialysis and ultrafiltration/centrifugation employed in drug encapsulation and release studies of nanocarriers. Determining the interaction and transfer of dyes to proteins is of utmost importance in the pre-clinical evaluation of drug nanocarriers for improved correlation between in vitro and in vivo studies.
URI:	http://www.repositorio.ufop.br/jspui/handle/123456789/14122
Link para o artigo:	https://www.sciencedirect.com/science/article/abs/pii/S0021967321000832
DOI:	https://doi.org/10.1016/j.chroma.2021.461959
ISSN:	0021-9673
Aparece nas coleções:	DEFAR - Artigos publicados em periódicos

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