TY - JOUR
T1 - Internalization and Cellular Fate of Protein Corona-Coated Nanoparticles by Multimodal Multi-Scale Microscopy
AU - Galdino, Flávia E.
AU - Rabelo, Renata S.
AU - Scarpa, Isabella
AU - Yoneda, Juliana S.
AU - Consonni, Sílvio R.
AU - Paes Leme, Adriana F.
AU - Smith, Andrew M.
AU - Harkiolaki, Maria
AU - Cardoso, Mateus B.
N1 - The authors gratefully acknowledge the financial support provided by the Funda\u00E7\u00E3o de Amparo \u00E0 Pesquisa do Estado de S\u00E3o Paulo (FAPESP \u2013 Process: 2018/09555\u20109, 2019/00720\u20100, and 2021/12071\u20106). M.B.C. acknowledges the Conselho Nacional de Desenvolvimento Cient\u00EDfico e Tecnol\u00F3gico (CNPq) for a productivity fellowship. The authors also extend their appreciation to the ME laboratory of LNNano for granting access to the electron microscopy facility (Proposal TEM\u201020210286), LNBio for providing access to the NMR spectrometer (Proposal RMN\u201020220629), and LC\u2010MS spectrometer (MAS\u201020220870), LNLS for granting access to the CD at the Cedro beamline (CEDRO\u201020241155), and the Diamond Light Source for the use of cryo\u2010SIM and cryo\u2010SXT at the B24 beamline (BI32901 and BI33390). The authors also express their gratitude to iNext (PID 26134 VID 44140) for their financial support during the analysis conducted at Diamond Light Source. Special thanks are due to Silvana A. Rocco for her assistance with NMR, and to Bianca A. Pauletti, Romenia R. Domingues, Lindomar Albuquerque, and Iris R. S. Ribeiro for their assistance with LC\u2010MS. Additionally, the authors appreciate the contributions of Opeyemi H. Arogundade in TIRF, and Talitha F. Stefanello and Maiara F. Terra in the apoptosis experiments. The authors are also grateful to Juliana T. T. Carvalho for her assistance with CD experiments.
PY - 2024/12/8
Y1 - 2024/12/8
N2 - Upon exposure to biological environments, nanoparticles are rapidly coated with biomolecules, predominantly proteins, which alter their colloidal stability, biodistribution, and cell interactions. Despite extensive efforts to investigate the nanoparticles' fate, only a few studies use high-resolution characterization methods that allow in-depth characterization, and the existing methodologies are unable to differentiate particles internalized at the onset of incubation from those taken up toward the end of an incubation period. In this study, these limitations related to incubation disparities are overcame and precisely monitored the spatiotemporal displacement of colloidally stable protein corona-coated nanoparticles within cells. An unprecedented application of cryogenic X-ray nanotomography, combined with high-resolution, super-resolution, and correlative microscopy techniques, revealed the migration of nanoparticles to the perinuclear region while monitoring the evolution of cellular organelles in fully hydrated cells under near-native conditions, without the need for contrasting agents. Notably, this tracking indicates the progressive fusion of vesicles carrying the nanoparticles intracellularly. This strategy demonstrates the potential for uncovering the temporal aspects of nanoparticle behavior within cells and can be adaptable to a wide range of nanoparticles and cell types, offering a versatile and powerful tool to follow nanoparticles in cellular environments.
AB - Upon exposure to biological environments, nanoparticles are rapidly coated with biomolecules, predominantly proteins, which alter their colloidal stability, biodistribution, and cell interactions. Despite extensive efforts to investigate the nanoparticles' fate, only a few studies use high-resolution characterization methods that allow in-depth characterization, and the existing methodologies are unable to differentiate particles internalized at the onset of incubation from those taken up toward the end of an incubation period. In this study, these limitations related to incubation disparities are overcame and precisely monitored the spatiotemporal displacement of colloidally stable protein corona-coated nanoparticles within cells. An unprecedented application of cryogenic X-ray nanotomography, combined with high-resolution, super-resolution, and correlative microscopy techniques, revealed the migration of nanoparticles to the perinuclear region while monitoring the evolution of cellular organelles in fully hydrated cells under near-native conditions, without the need for contrasting agents. Notably, this tracking indicates the progressive fusion of vesicles carrying the nanoparticles intracellularly. This strategy demonstrates the potential for uncovering the temporal aspects of nanoparticle behavior within cells and can be adaptable to a wide range of nanoparticles and cell types, offering a versatile and powerful tool to follow nanoparticles in cellular environments.
KW - correlative microscopy
KW - cryogenic X-ray nanotomography
KW - electron microscopy
KW - intracellular fate
KW - nanoparticles
KW - protein corona
KW - super-resolution fluorescence microscopy
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U2 - 10.1002/smll.202409065
DO - 10.1002/smll.202409065
M3 - Article
C2 - 39648571
AN - SCOPUS:85211319459
SN - 1613-6810
VL - 21
JO - Small
JF - Small
IS - 22
M1 - 2409065
ER -