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去唾液酸糖蛋白受体介导的内吞作用:乙醇给药对受体和配体内体分布的影响。

Receptor-mediated endocytosis by the asialoglycoprotein receptor: effect of ethanol administration on endosomal distribution of receptor and ligand.

作者信息

Dalton Shana R, Wiegert Robert L, Casey Carol A

机构信息

Department of Internal Medicine, University of Nebraska Medical Center, Omaha, NE 68198-2000, USA.

出版信息

Liver Int. 2003 Dec;23(6):484-91. doi: 10.1111/j.1478-3231.2003.00874.x.

Abstract

Using the asialoglycoprotein receptor (ASGP-R) and a representative ligand, asialoorosomucoid (ASOR), we have previously shown ethanol-induced impairment of endosomal acidification, receptor recycling and ligand binding, internalization, and degradation. In the current study, we further investigated ethanol-induced alterations in receptor/ligand trafficking by labeling endosomes in vivo with either Texas-Red-ASOR or 125I-ASOR, and then assessing the receptor/ligand content of endosomes. We assessed two fractions after both 5 and 25 min of labeling: 'early endosomes' (EEs; endosomes from the cell periphery) and 'late endosomes' (LEs; endosomes farther into the cell interior). At both time points, significantly more ligand was found in EE fractions isolated from chow- and pair-fed controls (3:1, EE to LE, respectively). However, endosomes isolated from ethanol-fed animals showed a shift over time toward a more equal ligand distribution between endosome fractions (P < or = 0.05). Analysis of the ASGP-R content revealed a distribution pattern between the endosome fractions similar to that observed for ligand distribution. Impairment of receptor-ligand dissociation was assessed in endosome fractions by determining bound/free ligand ratios. Analysis showed that most of the ligand present in both endosome fractions was free (56-99%), although more was bound to receptor in EE vs LE of both control and ethanol animals (P < or = 0.05). At 5 min, more ligand remained bound in endosomes from ethanol-fed animals compared with control endosomes (P < or = 0.05), and the same pattern was observed at the latter time point. These results suggest that delayed dissociation may cause the receptor ligand complexes to travel farther into the cell interior, which may impair proper trafficking of the ligand to lysosomes and alter the receptor recycling.

摘要

利用去唾液酸糖蛋白受体(ASGP-R)和一种代表性配体——去唾液酸血清类黏蛋白(ASOR),我们之前已经证明乙醇会导致内体酸化、受体循环利用以及配体结合、内化和降解受损。在当前研究中,我们通过用Texas-Red-ASOR或¹²⁵I-ASOR在体内标记内体,然后评估内体的受体/配体含量,进一步研究了乙醇诱导的受体/配体运输变化。在标记5分钟和25分钟后,我们评估了两个部分:“早期内体”(EEs;来自细胞周边的内体)和“晚期内体”(LEs;更深入细胞内部的内体)。在这两个时间点,从普通饮食和配对喂养对照组分离的EE部分中发现的配体明显更多(分别为3:1,EE与LE)。然而,从乙醇喂养动物分离的内体显示,随着时间推移,内体部分之间的配体分布变得更加均匀(P≤0.05)。对ASGP-R含量的分析揭示了内体部分之间的分布模式与配体分布相似。通过测定结合/游离配体比率,在内体部分评估了受体-配体解离受损情况。分析表明,两个内体部分中存在的大多数配体是游离的(56-99%),尽管在对照组和乙醇处理动物的EE中与受体结合的配体比LE中更多(P≤0.05)。在5分钟时,与对照内体相比,乙醇喂养动物内体中更多的配体仍与受体结合(P≤0.05),在后期时间点也观察到了相同的模式。这些结果表明,解离延迟可能导致受体配体复合物向细胞内部更深处移动,这可能会损害配体向溶酶体的正常运输,并改变受体的循环利用。

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