大鼠颌下腺离体细胞胰岛素结合位点的鉴定。

G E Scacchi, D Turyn, J M Dellacha
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摘要

从大鼠颌下腺分离的细胞与125i标记的胰岛素结合在一个时间依赖的过程中,在25℃下30-40分钟达到最大值。与细胞结合的放射性可以通过用孵育缓冲液稀释结合位点-激素复合物来解离。在孵育缓冲液中存在未标记的胰岛素,根据添加激素的量抑制125i标记的胰岛素降解。在25℃下孵育10分钟后,与细胞相关的放射性几乎完全被鉴定为完整的125i标记胰岛素。随着时间的增加,与细胞结合的最终降解产物对总放射性的贡献越来越大;然而,在未标记胰岛素存在的情况下,与低分子量产物相关的放射性显著降低。平衡结合数据分析得到一个非线性Scatchard图,其高亲和力组分的解离常数为6.6 +/- 0.4 nM。这些观察结果与大鼠颌下腺细胞中胰岛素结合位点的存在是一致的,这些细胞的特征与其他组织中发现的胰岛素结合位点相似。
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Identification of insulin binding sites in isolated cells from rat submaxillary gland.

Isolated cells from rat submaxillary gland bound 125I-labelled insulin in a time-dependent process that reached a maximum at 30-40 min at 25 degrees C. The radioactivity bound to cells could be dissociated by dilution of the binding site-hormone complex with the incubation buffer. The presence of unlabelled insulin in the incubation buffer inhibited 125I-labelled insulin degradation according to the amount of hormone added. After 10 min of incubation at at 25 degrees C, radioactivity associated to cells was almost exclusively identified as intact 125I-labelled insulin. With increasing times, a greater contribution of final products of degradation in total radioactivity bound to cells was observed; nevertheless, in the presence of unlabelled insulin the radioactivity associated to low molecular weight products markedly decreased. Equilibrium binding data analysis gave rise to a non-linear Scatchard plot, whose high affinity component showed a dissociation constant of 6.6 +/- 0.4 nM. These observations are consistent with the presence of insulin binding sites in rat submaxillary gland cells which are similar in their characteristics to those identified in other tissues.

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