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Graphene Liquid Enclosure for Single-Molecule Analysis of Membrane Proteins in Whole Cells Using Electron Microscopy

机译:石墨烯液体外壳,用于使用电子显微镜进行全细胞膜蛋白的单分子分子分子

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摘要

Membrane proteins govern many important functions in cells via dynamic oligomerization into active complexes. However, analytical methods to study their distribution and functional state in relation to the cellular structure are currently limited. Here, we introduce a technique for studying single-membrane proteins within their native context of the intact plasma membrane. SKBR3 breast cancer cells were grown on silicon microchips with thin silicon nitride windows. The cells were fixed, and the epidermal growth factor receptor ErbB2 was specifically labeled with quantum dot (QD) nanoparticles. For correlative fluorescence- and liquid-phase electron microscopy, we enclosed the liquid samples by chemical vapor deposited (CVD) graphene films. Depending on the local cell thickness, QD labels were imaged with a spatial resolution of 2 nm at a low electron dose. The distribution and stoichiometric assembly of ErbB2 receptors were determined at several different cellular locations, including tunneling nanotubes, where we found higher levels of homodimerization at the connecting sites. This experimental approach is applicable to a wide range of cell lines and membrane proteins and particularly suitable for studies involving both inter and intracellular heterogeneity in protein distribution and expression.
机译:膜蛋白通过动态低聚将细胞中的许多重要功能控制在活性络合物中。然而,目前有限地研究其与细胞结构有关的分析和功能状态的分析方法。这里,我们介绍一种用于在完整的血浆膜的本地背景下研究单膜蛋白的技术。 Skbr3乳腺癌细胞在具有薄的氮化硅窗口的硅微芯片上生长。固定细胞,并用量子点(QD)纳米颗粒特异性标记表皮生长因子受体ERBB2。对于相关的荧光和液相电子显微镜,我们通过化学气相沉积(CVD)石墨烯薄膜封闭液体样品。取决于局部电池厚度,在低电子剂量下以2nm的空间分辨率对QD标记进行成像。 ErbB2受体的分布和化学计量组装在几个不同的细胞位置测定,包括隧道纳米管,在那里我们在连接位点发现了更高水平的同型二聚体。该实验方法适用于各种细胞系和膜蛋白,特别适用于涉及蛋白质分布和表达中的间型和细胞内异质性的研究。

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