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内化过程中表皮生长因子受体的配体介导自磷酸化活性。

Ligand-mediated autophosphorylation activity of the epidermal growth factor receptor during internalization.

作者信息

Lai W H, Cameron P H, Doherty J J, Posner B I, Bergeron J J

机构信息

Department of Anatomy, McGill University, Montreal, Quebec, Canada.

出版信息

J Cell Biol. 1989 Dec;109(6 Pt 1):2751-60. doi: 10.1083/jcb.109.6.2751.

Abstract

The association of EGF with its receptor in endosomes isolated from rat liver homogenates was assessed biochemically by polyethylene glycol precipitation and morphologically by electron microscope radioautography. The proportion of receptor-bound ligand in endosomes at 15 min after the injection of doses of 0.1 and 1 microgram EGF/100 g body weight was 57%. This value increased to 77% for the dose of 10 micrograms EGF injected. Quantitative electron microscope radioautography carried out on endosomes isolated at 15 min after the injection of 10 micrograms 125I-EGF demonstrated that most radiolabel was over the endosomal periphery thereby indicating that ligand-receptor complexes were in the bounding membrane but not in intraluminal vesicles of the content. EGF receptor autophosphorylation activity during internalization was evaluated in plasmalemma and endosome fractions. This activity was markedly but transiently reduced on the cell surface shortly after the administration of saturating doses of EGF. The same activity, however, was augmented and prolonged in endosomes for up to 30 min after EGF injection. The transient desensitization of cell surface activity was not due to prior in vivo phosphorylation since receptor dephosphorylation in vitro failed to restore autophosphorylation activity. Transient desensitization of cell surface autophosphorylation activity coincided with a diminished capacity for endocytosis of 125I-EGF with endocytosis returning to normal after the restoration of cell surface autophosphorylation activity. The inhibition of cell surface autophosphorylation activity and the activation of endosomal autophosphorylation activity coincident with downregulation suggest that EGF receptor traffic is governed by ligand-regulated phosphorylation activity.

摘要

通过聚乙二醇沉淀法进行生物化学评估,并通过电子显微镜放射自显影法进行形态学评估,来检测从大鼠肝脏匀浆中分离出的内体中表皮生长因子(EGF)与其受体的结合情况。注射剂量为0.1和1微克EGF/100克体重后15分钟,内体中与受体结合的配体比例为57%。注射10微克EGF时,该值升至77%。对注射10微克125I-EGF后15分钟分离出的内体进行定量电子显微镜放射自显影显示,大多数放射性标记位于内体周边,从而表明配体-受体复合物存在于边界膜而非内容物的腔内小泡中。在质膜和内体组分中评估内化过程中EGF受体的自身磷酸化活性。给予饱和剂量的EGF后不久,细胞表面的这种活性显著但短暂降低。然而,在EGF注射后长达30分钟内,内体中的相同活性增强且持续时间延长。细胞表面活性的短暂脱敏并非由于体内预先磷酸化,因为体外受体去磷酸化未能恢复自身磷酸化活性。细胞表面自身磷酸化活性的短暂脱敏与125I-EGF内吞能力的降低同时发生,细胞表面自身磷酸化活性恢复后,内吞作用恢复正常。与下调同时发生的细胞表面自身磷酸化活性的抑制和内体自身磷酸化活性的激活表明,EGF受体的转运受配体调节的磷酸化活性控制。

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