1. The transport of ferritin molecules by endothelial cell vesicles has been quantitatively investigated by electron microscopy. Single mesenteric capillaries of pithed frogs were perfused with solutions containing 6.7 g ferritin 100 ml.-1 for known periods before fixation in situ with osmium tetroxide. 2. Two series of experiments were carried out: in the first series the perfusate contained bovine serum albumin (1.0 g 100 ml.-1); in the second series the perfusate contained no protein other than the ferritin. To assess the molecular radius of ferritin in solution, the free diffusion coefficient of ferritin was measured in the presence and absence of albumin. 3. The free diffusion coefficient of ferritin in saline solution (110 m-mole 1.-1) was found to be 0.35 X 10(-6) cm2 sec-1 at 21 degrees C and was not affected by the presence of bovine serum albumin. This indicates that there is no significant binding of albumin to ferritin in solution and yields a value for the Stokes-Einstein radius of ferritin of 6.1 nm. 4. In all perfusion experiments the percentage of luminal vesicles containing ferritin exceeded the percentage of labelled cytoplasmic vesicles, which in turn exceeded the percentage of labelled abluminal vesicles. 5. Labelling of all vesicle populations was seen after perfusions lasting less than 1 sec. At this time luminal vesicles were more heavily labelled in the absence of albumin. 6. The labelling of luminal vesicles increased with lengthening perfusion times up to 30-40 sec, after which steady levels of labelling were achieved. The rate of rise in luminal labelling and the steady-state levels reached were both greater in the absence of albumin. By contrast cytoplasmic labelling increased above its initial value only after perfusions of longer than 10 sec. 7. In the steady state, labelled cytoplasmic vesicles contained, on average, fewer ferritin molecules than labelled luminal vesicles. This finding is inconsistent with translocation of labelled luminal vesicles across the cell. 8. It is suggested that the early constant labelling of cytoplasmic and abluminal vesicles is consistent with the existence of vesicular channels. Later cytoplasmic labelling may result from the transient fusion of cytoplasmic vesicles with labelled luminal vesicles for periods long enough to allow mixing of vesicular contents. Albumin may affect vesicular transport by its interaction with the endothelial glycocalyx.
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机译:1.已经通过电子显微镜定量研究了铁蛋白分子通过内皮细胞囊泡的运输。在原位用四氧化固定之前,先对装有青蛙的单根肠系膜毛细血管灌注含有6.7 g铁蛋白100 ml.-1的溶液。 2.进行了两个系列的实验:在第一个系列中,灌注液中含有牛血清白蛋白(1.0 g 100 ml.-1);在第二系列中,灌注液除铁蛋白外不含任何蛋白质。为了评估溶液中铁蛋白的分子半径,在存在和不存在白蛋白的情况下测量铁蛋白的自由扩散系数。 3.发现铁蛋白在盐水溶液(110 m-mol 1.-1)中的自由扩散系数在21摄氏度下为0.35 X 10(-6)cm2 sec-1,不受牛血清的存在的影响白蛋白。这表明溶液中白蛋白与铁蛋白没有显着结合,铁蛋白的斯托克斯-爱因斯坦半径值为6.1 nm。 4.在所有灌注实验中,含铁蛋白的腔小泡的百分比超过标记的细胞质小泡的百分比,其反过来又超过标记的无囊小泡的百分比。 5.在持续少于1秒的灌注之后,看到所有囊泡种群的标记。此时,在不存在白蛋白的情况下,腔囊囊被更重地标记。 6.腔内囊泡的标记随着灌注时间的延长而增加,最长可达30-40秒,此后达到稳定水平的标记。在没有白蛋白的情况下,管腔标记的增加速率和达到的稳态水平都更大。相比之下,仅在灌注超过10秒后,胞质标记才增加到其初始值以上。 7.在稳态下,标记的细胞质囊泡平均含有的铁蛋白分子少于标记的腔内囊泡。这一发现与标记的腔内小泡跨细胞转运不一致。 8.建议细胞质囊泡和无囊泡的早期恒定标记与囊泡通道的存在是一致的。以后的细胞质标记可能是由于细胞质囊泡与标记的腔内囊泡短暂融合而导致的,其持续时间足以允许囊泡内容物混合。白蛋白可通过其与内皮糖萼的相互作用来影响囊泡运输。
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