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阿片受体介导的125I-β-内啡肽在人多形核白细胞中的内化作用。

Opiate receptor mediated internalization of 125I-beta-endorphin in human polymorphonuclear leucocytes.

作者信息

Falke N E, Fischer E G

出版信息

Cell Biol Int Rep. 1986 Jun;10(6):429-35. doi: 10.1016/0309-1651(86)90038-x.

Abstract

The early events in the interaction of (125I)-Tyr27-beta-endorphin with human polymorphonuclear leucocytes were investigated. Using ultrastructural autoradiography we found that the labeled peptide specifically bound to the plasma membrane and was internalized within two minutes of incubation at 37 degrees C. Both processes could be inhibited by unlabeled beta-endorphin or by the opiate antagonist diprenorphine. This finding was confirmed by radioreceptorassays. With longer incubation times the specific association of the labeled beta-endorphin with the cells decreased. About 10% of the tracer was degraded within 10 min of incubation as shown by gel chromatography. The morphological changes induced by 125I-beta-endorphin in the granulocytes were investigated under the microscope. The labeled peptide had the same biological effect as unlabeled beta-endorphin.

摘要

研究了(125I)-酪氨酰27-β-内啡肽与人多形核白细胞相互作用的早期事件。通过超微结构放射自显影,我们发现标记的肽特异性结合到质膜上,并在37℃孵育两分钟内被内化。这两个过程都可以被未标记的β-内啡肽或阿片拮抗剂二丙诺啡抑制。这一发现通过放射受体分析得到证实。随着孵育时间延长,标记的β-内啡肽与细胞的特异性结合减少。凝胶色谱显示,约10%的示踪剂在孵育10分钟内被降解。在显微镜下研究了125I-β-内啡肽在粒细胞中诱导的形态学变化。标记的肽与未标记的β-内啡肽具有相同的生物学效应。

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