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首页> 外文期刊>Cell motility and the cytoskeleton >Heterogeneous modes of uptake for latex beads revealed through live cell imaging of phagocytes expressing a probe for phosphatidylinositol-(3,4,5)-trisphosphate and phosphatidylinositol-(3,4)-bisphosphate.
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Heterogeneous modes of uptake for latex beads revealed through live cell imaging of phagocytes expressing a probe for phosphatidylinositol-(3,4,5)-trisphosphate and phosphatidylinositol-(3,4)-bisphosphate.

机译:通过吞噬细胞的活细胞成像揭示了乳胶珠的异质摄取模式,吞噬细胞表达了磷脂酰肌醇-(3,4,5)-三磷酸和磷脂酰肌醇-(3,4)-双磷酸酯的探针。

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摘要

Latex beads are the preferred phagocytic substrate in biochemical studies of phagosome composition and maturation. Using living Dictyostelium cells and fluorescent probes, we compared the properties of phagosomes formed to ingest latex beads or digestible prey. Significant differences were found during the initial steps of phagocytosis. During uptake of bacteria or yeast, PHcrac-GFP, a probe that binds to membranes enriched in PI(3,4,5)P(3) and PI(3,4)P(2), always labeled the nascent phagosome and faded shortly after it sealed. However, labeling of bead-containing phagosomes was highly variable. Beads were engulfed by phagosomes either lacking or displaying the PHcrac-GFP label, and that label, if present, often persisted for many minutes, revealing that early trafficking steps for bead-containing phagosomes are quite heterogeneous. Later stages of the endocytic pathway appeared more similar for phagosomes containing prey and latex beads. Both types of phagosomes fused with acidic endosomes while undergoing transport along microtubules, both acquired the V-ATPase and lost it prior to exocytosis, and both bound the late endosome marker vacuolin B, which was transferred to the plasma membrane upon exocytosis. We conclude that caution is needed in extrapolating results from latex bead phagosomes to phagosomes containing physiological substances, especially in early stages of the endocytic pathway.
机译:在吞噬体组成和成熟的生化研究中,乳胶珠是首选的吞噬底物。我们使用活的Dictyostelium细胞和荧光探针,比较了吞噬乳胶珠或可消化猎物形成的吞噬体的特性。在吞噬作用的初始阶段发现了显着差异。在摄取细菌或酵母的过程中,PHcrac-GFP是一种与富含PI(3,4,5)P(3)和PI(3,4)P(2)的膜结合的探针,始终标记为新生的吞噬体并褪色密封后不久。但是,含珠的吞噬体的标签变化很大。缺少或未显示PHcrac-GFP标签的吞噬体吞没了珠子,并且该标签(如果存在)通常会持续数分钟,这表明含珠子吞噬体的早期运输步骤非常异质。对于包含猎物和乳胶珠的吞噬体,内吞途径的后期显得更为相似。两种类型的吞噬体均与酸性内体融合,同时沿微管运输,都在胞吐之前获得了V-ATPase并丢失了它,并且都与晚期内体标记空泡蛋白B结合,后者在胞吐后转移到质膜上。我们得出结论,在将乳胶珠粒吞噬体的结果推断为含有生理物质的吞噬体的结果时,尤其是在内吞途径的早期阶段,需要谨慎行事。

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