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Binding internalization and lysosomal association of 125I-human growth hormone in cultured human lymphocytes: a quantitative morphological and biochemical study

机译:培养的人淋巴细胞中125 I-人生长激素的结合内在化和溶酶体缔合:定量形态学和生化研究

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摘要

125I-human growth hormone (125I-hGH) binds specifically to receptors on cultures human lymphocytes (IM-9). When this process is studied by use of quantitative EM radioautography, under conditions of incubation at 15 degrees C for 5 min, the ligand is localized to the plasma membrane of the cell. At 30 degrees and 37 degrees C, however, 125I-hGH is progressively internalized by the cell as a function of time. The internalized ligand is found predominantly in the Golgi region of the cells, with a five-fold preferential localization to membrane-bounded structures with the morphological and cytochemical characteristics of lysosomes. Up to 59% of these lysosome-like structures are positive for the acid phosphatase reaction under the conditions of incubation at 37 degrees C for 120 min. When the cell associated radioactivity after 15- 120 min of incubation at 37 degrees C is extracted in 1 M acetic acid and filtered on a Sephadex G-100 column, 58-73% of the material elutes as intact hGH. When cells are incubated with 125I-hGH at 37 degrees C for 15-120 min, separated from the incubation medium, and washed and diluted 100-fold, the percent 125I-hGH dissociable decreases as a function of increasing time of incubation. When cells are incubated with 125I-hGH for 15 min at 37 degrees C and the radioactivity that dissociates from the cells during 15-90 min is studied, the labeled material appearing in the incubation medium is progressively degraded as a function of time of incubation. When the dissociation process is studied radioautographically, grains are found both in plasma membrane and intracelluar compartments after 30 min of association, but after 30 and 120 min of dissociation a higher proportion of grains are in the intracellular compartment. After 120 min of association, there is less dissociation from either compartment and a preferential increase of grains in the intracellular compartment. These data suggest that receptor-linked internalization of a polypeptide hormone provides a mechanism that couples degradation of the ligand with loss of the cell surface receptor.
机译:125I-人类生长激素(125I-hGH)与人类淋巴细胞(IM-9)培养物上的受体特异性结合。当使用定量EM放射自显影技术研究此过程时,在15摄氏度下孵育5分钟的条件下,配体位于细胞的质膜上。然而,在30度和37摄氏度下,125I-hGH作为时间的函数被细胞逐渐内在化。内化的配体主要存在于细胞的高尔基体区域,具有溶酶体的形态学和细胞化学特征的五倍优先定位于膜结合结构。这些溶酶体样结构中有多达59%在37°C孵育120分钟的条件下对酸性磷酸酶反应呈阳性。当在1M乙酸中提取37°C孵育15-120分钟后与细胞相关的放射性并在Sephadex G-100柱上过滤时,58-73%的物质以完整的hGH洗脱。当将细胞与125I-hGH在37摄氏度下孵育15-120分钟,与孵育介质分离,洗涤并稀释100倍时,可分解的125I-hGH百分比随孵育时间的增加而降低。当将细胞与125I-hGH在37°C下孵育15分钟并研究在15-90分钟内从细胞中解离的放射性时,在孵育培养基中出现的标记物质会随着孵育时间的增长而逐渐降解。通过放射自显影研究解离过程时,缔合30分钟后在质膜和细胞内隔室中均发现了颗粒,但解离30和120分钟后,细胞内室中有更高比例的颗粒。缔合120分钟后,从任一隔室解离的次数减少,并且细胞内隔室中的颗粒优先增加。这些数据表明多肽激素的受体连接的内在化提供了一种机制,该机制将配体的降解与细胞表面受体的损失耦合在一起。

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