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Single-molecule localization microscopy and tracking with red-shifted states of conventional BODIPY conjugates in living cells

机译:单分子定位显微镜和活细胞中常规BODIPY偶联物的红移状态跟踪

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摘要

Single-molecule localization microscopy (SMLM) is a rapidly evolving technique to resolve subcellular structures and single-molecule dynamics at the nanoscale. Here, we employ conventional BODIPY conjugates for live-cell SMLM via their previously reported red-shifted ground-state dimers (DII), which transiently form through bi-molecular encounters and emit bright single-molecule fluorescence. We employ the versatility of DII-state SMLM to resolve the nanoscopic spatial regulation and dynamics of single fatty acid analogs (FAas) and lipid droplets (LDs) in living yeast and mammalian cells with two colors. In fed cells, FAas localize to the endoplasmic reticulum and LDs of ~125 nm diameter. Upon fasting, however, FAas form dense, non-LD clusters of ~100 nm diameter at the plasma membrane and transition from free diffusion to confined immobilization. Our reported SMLM capability of conventional BODIPY conjugates is further demonstrated by imaging lysosomes in mammalian cells and enables simple and versatile live-cell imaging of sub-cellular structures at the nanoscale.
机译:单分子定位显微镜(SMLM)是一种快速发展的技术,可以解决亚细胞结构和纳米级的单分子动力学问题。在这里,我们通过其先前报道的红移基态二聚体(DII),将传统的BODIPY缀合物用于活细胞SMLM,其通过双分子相遇而短暂形成并发出明亮的单分子荧光。我们利用DII状态SMLM的多功能性来解决纳米级空间调节和动态酵母和具有两种颜色的哺乳动物细胞中的单个脂肪酸类似物(FAas)和脂质滴(LDs)的动力学。在受精细胞中,FAas定位于内质网和直径约125 nm的LD。然而,禁食时,FAas在质膜上形成直径约100 nm的致密非LD簇,并从自由扩散过渡到有限的固定化。通过对哺乳动物细胞中的溶酶体进行成像,可以进一步证明我们报道的常规BODIPY结合物的SMLM功能,并且可以在纳米级对亚细胞结构进行简单而通用的活细胞成像。

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