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Co-localization of fluorescent labeled lipid nanoparticles with specifically tagged subcellular compartments by single particle tracking at low nanoparticle to cell ratios

机译:通过在低纳米颗粒下以低纳米颗粒进行单颗粒跟踪,用特异标记的亚细胞隔室具有特异性标记的亚细胞间隔的荧光标记脂质纳米颗粒的共定位

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We utilized quantitative high-resolution single particle tracking to study the internalization and endosomal sorting of lipid nanoparticles (LNPs) by HeLa cells in vitro to gain a better understanding of how cells process LNPs that are used for siRNA delivery. We compared the trafficking of three formulations that have been demonstrated to deliver siRNA into cells. They were composed of either a tritratable anionic lipid, formulation of cholesterol hemisuccinate (CHEMS), or a titratatable cationic lipid formulation of 1,2-dilinoleyloxy-3-dimethylaminopropane (DLinDMA) or a non-titratable cationic formulation lipid formulation of 1,2-dioleoyl-3-trimethylammonium-propane (DOTAP). They also contained either a substantial percentage of 1,2-dioleoyl-sn-glycero-3-phosphoethanolamine (DOPE) or cholesterol and 5mole percent 1,2-dimyristoyl-sn-glycerol-[methoxy(polyethylene glycol)-2000 (PEG-DMG). We optically measured the endosomal pH experienced by individual LNPs, observed the internalization pathways used and tracked the particles as they co-localized with fluorescent protein tags on compartment-specific proteins, during endosomal sorting to the lysosome. The data revealed significant differences in the accumulation in subcellular compartments among the three formulations, which help to explain the observed effects LNP composition exerts on in vitro delivery efficiency.
机译:我们利用定量高分辨率单粒子跟踪来研究脂质纳米颗粒(LNP)的内化和内体分选,在体外,更好地理解用于SiRNA递送的细胞过程LNP。我们比较了已经证明将siRNA送入细胞的三种配方的贩运。它们由涂料的阴离子脂质,制剂的胆固醇半眼(Chems),或1,2-稀释氧基-3-二甲基氨基丙烷(Dlindma)的滴定阳离子脂质制剂或1,2的不可滴定阳离子制剂脂质制剂组成-dioleyl-3-三甲基铵 - 丙烷(dotap)。它们还含有大量的1,2-Dioleyl-sn-甘油-3-磷乙醇胺(掺杂)或胆固醇,5摩尔百分比1,2-二维酰基-N-甘油 - [甲氧基(聚乙二醇)-2000(PEG- dmg)。我们光学测量单个LNP所经历的内体pH值,观察到使用的内化途径,并在孤房分类期间将荧光蛋白标签与杂物组上的荧光蛋白标签共定位。该数据揭示了三种制剂中亚细胞隔室积累的显着差异,这有助于解释观察到的LNP组合物对体外递送效率施加。

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