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Design of Quantum Dot-Conjugated Lipids for Long-Term High-Speed Tracking Experiments on Cell Surfaces

机译:用于细胞表面长期高速跟踪实验的量子点共轭脂质的设计

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摘要

The current study reports the facile design of quantum dot (QD)-conjugated lipids and their application to high-speed tracking experiments on cell surfaces. CdSe/ZnS core/shell QDs with two types of hydrophilic coatings, 2-(2-aminoethoxy)ethanol (AEE-coating) and a 60:40 molar mixture of 1,2-dipalmitoyl-sn-glycero-3-phosphocholine and 1,2-dipalmitoyl-sn-glycero-3-phosphoethanolamine-N-[methoxy(polyethyleneglycol-2000] (LIPO-coating), are conjugated to sulfhydryl lipids via maleimide reactive groups on the QD surface. Prior to lipid conjugation, the colloidal stability of both types of coated QDs in aqueous solution is confirmed using fluorescence correlation spectroscopy. A sensitive assay based on single lipid tracking experiments on a planar solid-supported phospholipid bilayer is presented that establishes conditions of monovalent conjugation of QDs to lipids. The QD lipids are then employed as single molecule tracking probes in plasma membranes of several cell types. Initial tracking experiments at a frame rate of 30 fps corroborate that QD-lipids diffuse like dye-labeled lipids in the plasma membrane of COS-7, HEK-293, 3T3, and NRK cells, thus confirming monovalent labeling. Finally, QD-lipids are applied for the first time to high-speed single molecule imaging by tracking their lateral mobility in the plasma membrane of NRK fibroblasts with up to 1000 fps. Our high-speed tracking data, which are in excellent agreement to previous tracking experiments with larger 40nm Au labels, not only push the time resolution in long-time, continuous fluorescence-based single molecule tracking, but also show that highly photostable, photoluminescent nanoprobes of 10nm size can be employed (AEE-coated QDs). These probes are also attractive because, unlike Au nanoparticles, they facilitate complex multicolor experiments.
机译:当前的研究报道了量子点(QD)共轭脂质的简便设计及其在细胞表面高速跟踪实验中的应用。具有两种亲水涂层的CdSe / ZnS核/壳QD,2-(2-氨基乙氧基)乙醇(AEE-涂层)和1,2-二棕榈酰基-sn-甘油-3-磷酸胆碱和1的60:40摩尔混合物通过QD表面的马来酰亚胺反应基团将2,2-二棕榈酰基-sn-甘油-3-磷酸乙醇胺-N- [甲氧基(聚乙二醇-2000)(LIPO-涂层)与巯基脂质偶联。在脂质偶联之前,胶体稳定性荧光相关光谱法证实了这两种类型的包被的量子点在液相中固相支持的磷脂双层上基于单脂质跟踪实验的灵敏测定,建立了量子点与脂质单价结合的条件。然后在几种细胞类型的质膜中用作单分子跟踪探针。以30 fps的帧速率进行的初始跟踪实验证实了QD-脂质像染料标记的脂质一样在COS-7,HEK-293、3T3的质膜中扩散和NRK ce lls,从而证实了单价标记。最后,通过以高达1000 fps的速度跟踪NRK成纤维细胞质膜中的横向迁移率,将QD脂质首次应用于高速单分子成像。我们的高速跟踪数据与以前使用较大的40nm Au标签进行的跟踪实验非常吻合,不仅提高了基于连续荧光的长期单分子跟踪的时间分辨率,而且还显示出高度光稳定的光致发光纳米探针可以采用10nm的尺寸(AEE涂层QD)。这些探针也很有吸引力,因为与Au纳米颗粒不同,它们有助于复杂的多色实验。

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