In situ analysis of liposome hard and soft protein corona structure and composition in a single label-free workflow

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Pysyväisosoite

http://hdl.handle.net/10138/311133

Lähdeviite

Kari , O K , Ndika , J , Parkkila , P , Louna , A , Lajunen , T , Puustinen , A , Viitala , T , Alenius , H & Urtti , A 2020 , ' In situ analysis of liposome hard and soft protein corona structure and composition in a single label-free workflow ' , Nanoscale , vol. 12 , no. 3 , pp. 1728-1741 . https://doi.org/10.1039/C9NR08186K

Julkaisun nimi: In situ analysis of liposome hard and soft protein corona structure and composition in a single label-free workflow
Tekijä: Kari, Otto K.; Ndika, Joseph; Parkkila, Petteri; Louna, Antti; Lajunen, Tatu; Puustinen, Anne; Viitala, Tapani; Alenius, Harri; Urtti, Arto
Tekijän organisaatio: Division of Pharmaceutical Biosciences
Drug Delivery Unit
HUMI - Human Microbiome Research
Pharmaceutical biophysics group
Pharmaceutical Nanotechnology
Department of Chemistry
University Management
Division of Pharmaceutical Chemistry and Technology
Drug Research Program
Doctoral Programme in Microbiology and Biotechnology
Drug Delivery
Päiväys: 2020-01-21
Kieli: eng
Sivumäärä: 14
Kuuluu julkaisusarjaan: Nanoscale
ISSN: 2040-3364
DOI-tunniste: https://doi.org/10.1039/C9NR08186K
URI: http://hdl.handle.net/10138/311133
Tiivistelmä: Methodological constraints have limited our ability to study protein corona formation, slowing nanomedicine development and their successful translation into the clinic. We determined hard and soft corona structural properties along with the corresponding proteomic compositions on liposomes in a label-free workflow: surface plasmon resonance and a custom biosensor for in situ structure determination on liposomes and corona separation, and proteomics using sensitive nanoliquid chromatography tandem mass spectrometry with open-source bioinformatics platforms. Undiluted human plasma under dynamic flow conditions was used for in vivo relevance. Proof-of-concept is presented with a regular liposome formulation and two light-triggered indocyanine green (ICG) liposome formulations in preclinical development. We observed formulation-dependent differences in corona structure (thickness, protein-to-lipid ratio, and surface mass density) and protein enrichment. Liposomal lipids induced the enrichment of stealth-mediating apolipoproteins in the hard coronas regardless of pegylation, and their preferential enrichment in the soft corona of the pegylated liposome formulation with ICG was observed. This suggests that the soft corona of loosely interacting proteins contributes to the stealth properties as a component of the biological identity modulated by nanomaterial surface properties. The workflow addresses significant methodological gaps in biocorona research by providing truly complementary hard and soft corona compositions with corresponding in situ structural parameters for the first time. It has been designed into a convenient and easily reproducible single-experiment format suited for preclinical development of lipid nanomedicines.
Avainsanat: 318 Medical biotechnology
PLASMON RESONANCE SENSORS
PEG CHAIN-LENGTH
BIOMOLECULAR CORONA
COMPLEMENT ACTIVATION
BIOLOGICAL IDENTITY
TIME-EVOLUTION
NANOPARTICLES
SURFACE
VIVO
ADSORPTION
PLASMON RESONANCE SENSORS
PEG CHAIN-LENGTH
BIOMOLECULAR CORONA
COMPLEMENT ACTIVATION
BIOLOGICAL IDENTITY
TIME-EVOLUTION
NANOPARTICLES
SURFACE
VIVO
ADSORPTION
Vertaisarvioitu: Kyllä
Tekijänoikeustiedot: cc_by
Pääsyrajoitteet: openAccess
Rinnakkaistallennettu versio: publishedVersion


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