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含有α2-巨球蛋白的内吞小泡的快速酸化。

Rapid acidification of endocytic vesicles containing alpha 2-macroglobulin.

作者信息

Tycko B, Maxfield F R

出版信息

Cell. 1982 Mar;28(3):643-51. doi: 10.1016/0092-8674(82)90219-7.

Abstract

We have used fluorescein-labeled alpha 2-macroglobulin (F-alpha 2M) to measure pH changes in the microenvironment of internalized ligands following receptor-mediated endocytosis. Fluorescence intensities of single BALB/c 3T3 mouse fibroblasts were measured by using a microscope spectrofluorometer with narrow bandpass excitation filters. The pH was determined from the ratio of fluorescein fluorescence intensities with 450 nm and 490 nm excitation. A standard pH curve was obtained by incubating cells with F-alpha 2M for 30 min at 37 degrees C followed by fixation and incubation in buffers of varying pH. To measure the pH of endocytic vesicles, cells were incubated with F-alpha 2M for 15 min at 37 degrees C. Fluorescence intensities were measured on living cells within 5 min of rinsing. Under these conditions, the pH of the F-alpha 2M microenvironment was 5.0 +/- 0.2. Using colloidal gold-alpha 2M for electron microscopic localizations we have verified that, under these conditions, alpha 2M is predominantly in uncoated vesicles that are negative for acid phosphatase activity. With further incubation for 1/2 hr, we obtained a pH of 5.0 +/- 0.2 for the F-alpha 2M. Using fluorescein dextran, we obtained a lysosomal pH of 4.6 +/- 0.2. These results indicate that endocytic vesicles become acidic prior to fusion with lysosomes.

摘要

我们使用荧光素标记的α2-巨球蛋白(F-α2M)来测量受体介导的内吞作用后内化配体微环境中的pH变化。通过使用带有窄带通激发滤光片的显微镜分光荧光计测量单个BALB/c 3T3小鼠成纤维细胞的荧光强度。根据450nm和490nm激发下荧光素荧光强度的比值确定pH值。通过在37℃下将细胞与F-α2M孵育30分钟,然后固定并在不同pH的缓冲液中孵育来获得标准pH曲线。为了测量内吞小泡的pH值,将细胞在37℃下与F-α2M孵育15分钟。在漂洗后5分钟内对活细胞测量荧光强度。在这些条件下,F-α2M微环境的pH值为5.0±0.2。使用胶体金-α2M进行电子显微镜定位,我们已经证实,在这些条件下,α2M主要存在于对酸性磷酸酶活性呈阴性的无被小泡中。进一步孵育半小时后,我们测得F-α2M的pH值为5.0±0.2。使用荧光素葡聚糖,我们测得溶酶体的pH值为4.6±0.2。这些结果表明,内吞小泡在与溶酶体融合之前就会变成酸性。

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