McNeil P L, Tanasugarn L, Meigs J B, Taylor D L
J Cell Biol. 1983 Sep;97(3):692-702. doi: 10.1083/jcb.97.3.692.
We have measured changes of pH in a protein's microenvironment consequent on its binding to the cell surface and incorporation into pinosomes. Changes of pH were measured from single, living cells and selected regions of cells by the fluorescence ratio technique using a photon-counting microspectrofluorimeter. The chemotactic agent and pinocytosis inducer, ribonuclease, labeled with fluorescein (FTC-RNase), adsorbed to the surface of Amoeba proteus, and was pinocytosed by cells in culture media at pH 7.0. The FTC-RNase entered an apparently acidic microenvironment, pH approximately 6.1, upon binding to the surface of amoebae. Once enclosed within pinosomes, this protein's microenvironment became steadily more acidic, reaching a minimum of pH approximately 5.6 in less than 10 min. FTC-RNase pinocytosed by the giant amoeba, Chaos carolinensis, entered pinosomes whose pH was correlated with their cytoplasmic location during the initial 30-40 min after pinocytosis. The majority of pinosomes containing FTC-RNase clustered in the tail ectoplasm of C. carolinensis during this interval and had a pH of approximately 6.5; those released into endoplasm and carried into the tip of cells had a pH below 5.0. As pinosomes became distributed at random in C. carolinensis (1-2 h after initial pinocytosis), differences in pH between tip and tail pinosomes vanished. We have also measured the pH within single phagosomes of A. proteus. Phagosomal pH dropped steadily to approximately 5.4 within 5 min after particle ingestion in 70% of the cells measured, and reached this level of acidity within 10 min in 90% of the cells measured. By contrast, stain for the lysosomal enzyme, acid phosphatase, was evident within only 20% of 5-min-old phagosomes visualized by light microscopy, and within only 40% of 10-min-old phagosomes. A microfluorimetric assay was used to simultaneously record changes in pH, and the initial deposition of lysosomal esterases, within phagosomes of single, living Amoeba proteus. Near complete acidification of the phagosome was recorded from some cells before phagosomal fusion was evident by this microfluorimetric assay. From other cells, however, continued acidification of phagosomes was recorded after lysosomal fusion was initiated. We conclude that acidification of phagosomes by A. proteus is initiated but not necessarily completed prior to phagosome-lysosome formation, and that the two events are closely linked in time. Initial acidification of endosomes is a property intrinsic to the plasma membrane which envelops particles at the cell surface, rather than the result of lysosomal fusion with phagosomes.
我们已经测量了蛋白质与细胞表面结合并被纳入吞噬体后其微环境中的pH变化。使用光子计数显微分光荧光计,通过荧光比率技术从单个活细胞和细胞的选定区域测量pH变化。趋化剂和胞饮作用诱导剂——用荧光素标记的核糖核酸酶(FTC-RNase)吸附在变形虫表面,并在pH 7.0的培养基中被培养细胞胞饮。FTC-RNase与变形虫表面结合后进入一个明显呈酸性的微环境,pH约为6.1。一旦被包裹在吞噬体内,这种蛋白质的微环境会逐渐变得更酸,在不到10分钟内达到最低pH约5.6。由巨型变形虫卡罗琳混沌菌胞饮的FTC-RNase进入吞噬体,其pH与胞饮后最初30 - 40分钟内它们在细胞质中的位置相关。在此期间,大多数含有FTC-RNase的吞噬体聚集在卡罗琳混沌菌的尾部外质中,pH约为6.5;那些释放到内质中并被带到细胞顶端的吞噬体pH低于5.0。随着吞噬体在卡罗琳混沌菌中随机分布(初始胞饮后1 - 2小时),顶端和尾部吞噬体之间的pH差异消失。我们还测量了变形虫单个吞噬体内的pH。在70%被测量的细胞中,吞噬颗粒后5分钟内吞噬体pH稳步下降至约5.4,在90%被测量的细胞中10分钟内达到这种酸度水平。相比之下,通过光学显微镜观察,仅20%的5分钟龄吞噬体中溶酶体酶酸性磷酸酶的染色明显,10分钟龄吞噬体中仅40%有明显染色。使用微荧光测定法同时记录单个活变形虫吞噬体内pH的变化以及溶酶体酯酶的初始沉积。在通过这种微荧光测定法明显观察到吞噬体融合之前,从一些细胞中记录到吞噬体几乎完全酸化。然而,从其他细胞中,在溶酶体融合开始后记录到吞噬体持续酸化。我们得出结论,变形虫对吞噬体的酸化在吞噬体 - 溶酶体形成之前就已开始,但不一定完成,并且这两个事件在时间上紧密相连。内体的初始酸化是细胞膜的固有特性,细胞膜在细胞表面包裹颗粒,而不是溶酶体与吞噬体融合的结果。
