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Tracking yeast pheromone receptor Ste2 endocytosis using fluorogen-activating protein tagging

机译:使用荧光激活蛋白标记追踪酵母信息素受体Ste2内吞

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To observe internalization of the yeast pheromone receptor Ste2 by fluorescence microscopy in live cells in real time, we visualized only those molecules present at the cell surface at the time of agonist engagement (rather than the total cellular pool) by tagging this receptor at its N-terminus with an exocellular fluorogen-activating protein (FAP). A FAP is a single-chain antibody engineered to bind tightly a nonfluorescent, cell-impermeable dye (fluorogen), thereby generating a fluorescent complex. The utility of FAP tagging to study trafficking of integral membrane proteins in yeast, which possesses a cell wall, had not been examined previously. A diverse set of signal peptides and propeptide sequences were explored to maximize expression. Maintenance of the optimal FAP-Ste2 chimera intact required deletion of two, paralogous, glycosylphosphatidylinositol (GPI)-anchored extracellular aspartyl proteases (Yps1 and Mkc7). FAP-Ste2 exhibited a much brighter and distinct plasma membrane signal than Ste2-GFP or Ste2-mCherry yet behaved quite similarly. Using FAP-Ste2, new information was obtained about the mechanism of its internalization, including novel insights about the roles of the cargo-selective endocytic adaptors Ldb19/Art1, Rod1/Art4, and Rog3/Art7.
机译:为了通过荧光显微镜实时观察酵母信息素受体Ste2在活细胞中的内在化,我们通过将受体标记在N上来仅观察激动剂参与时细胞表面上存在的那些分子(而不是总细胞池)。 -末端带有胞外氟激活蛋白(FAP)。 FAP是一种单链抗体,经过工程设计可紧密结合非荧光,细胞不可渗透的染料(氟),从而生成荧光复合物。 FAP标记用于研究具有细胞壁的酵母中整合膜蛋白运输的实用性,之前尚未进行过检查。探索了多种信号肽和前肽序列,以最大化表达。要维持最佳的FAP-Ste2嵌合体完整,就需要删除两个旁系的糖基磷脂酰肌醇(GPI)锚定的细胞外天冬氨酰蛋白酶(Yps1和Mkc7)。与Ste2-GFP或Ste2-mCherry相比,FAP-Ste2表现出更明亮和明显的质膜信号,但表现却非常相似。使用FAP-Ste2,可以获得有关其内在化机制的新信息,包括有关货物选择性内吞衔接子Ldb19 / Art1,Rod1 / Art4和Rog3 / Art7的作用的新颖见解。

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