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酒精急性拮抗再喂养诱导的骨骼肌 Rag GTPase-Ragulator 复合物的改变。

Alcohol Acutely Antagonizes Refeeding-Induced Alterations in the Rag GTPase-Ragulator Complex in Skeletal Muscle.

机构信息

Department of Surgery, Penn State College of Medicine, Hershey, PA 17033, USA.

Beth Israel Deaconess Medical Center, Department of Surgery, Boston, MA 02215, USA.

出版信息

Nutrients. 2021 Apr 9;13(4):1236. doi: 10.3390/nu13041236.

Abstract

The Ragulator protein complex is critical for directing the Rag GTPase proteins and mTORC1 to the lysosome membrane mediating amino acid-stimulated protein synthesis. As there is a lack of evidence on alcohol's effect on the Rag-Ragulator complex as a possible mechanism for the development of alcoholic skeletal muscle wasting, the aim of our study was to examine alterations in various protein-protein complexes in the Rag-Ragulator pathway produced acutely by feeding and how these are altered by alcohol under in vivo conditions. Mice (C57Bl/6; adult males) were fasted, and then provided rodent chow for 30 min ("refed") or remained food-deprived ("fasted"). Mice subsequently received ethanol (3 g/kg ethanol) or saline intraperitoneally, and hindlimb muscles were collected 1 h thereafter for analysis. Refeeding-induced increases in myofibrillar and sarcoplasmic protein synthesis, and mTOR and S6K1 phosphorylation, were prevented by alcohol. This inhibition was not associated with a differential rise in the intracellular leucine concentration or plasma leucine or insulin levels. Alcohol increased the amount of the Sestrin1•GATOR2 complex in the fasted state and prevented the refeeding-induced decrease in Sestrin1•GATOR2 seen in control mice. Alcohol antagonized the increase in the RagA/C•Raptor complex formation seen in the refed state. Alcohol antagonized the increase in Raptor with immunoprecipitated LAMPTOR1 (part of the Ragulator complex) after refeeding and decreased the association of RagC with LAMPTOR1. Finally, alcohol increased the association of the V domain of v-ATPase with LAMPTOR1 and prevented the refeeding-induced decrease in v-ATPase V1 with LAMPTOR1. Overall, these data demonstrate that acute alcohol intake disrupts multiple protein-protein complexes within the Rag-Ragulator complex, which are associated with and consistent with the concomitant decline in nutrient-stimulated muscle protein synthesis under in vivo conditions.

摘要

Ragulator 蛋白复合物对于指导 Rag GTPase 蛋白和 mTORC1 到溶酶体膜介导氨基酸刺激的蛋白质合成至关重要。由于缺乏关于酒精对 Rag-Ragulator 复合物的影响作为酒精性骨骼肌消耗发展的可能机制的证据,我们的研究旨在检查在体内条件下,急性喂养引起的 Rag-Ragulator 途径中各种蛋白-蛋白复合物的变化,以及酒精如何改变这些复合物。成年雄性 C57Bl/6 小鼠禁食,然后给予 30 分钟的啮齿动物饲料(“再喂养”)或继续禁食。随后,小鼠接受腹腔内注射乙醇(3g/kg 乙醇)或生理盐水,1 小时后收集后肢肌肉进行分析。再喂养诱导的肌原纤维和肌浆蛋白合成增加以及 mTOR 和 S6K1 磷酸化被酒精抑制。这种抑制与细胞内亮氨酸浓度或血浆亮氨酸或胰岛素水平的差异升高无关。酒精增加了禁食状态下 Sestrin1•GATOR2 复合物的数量,并防止了在对照小鼠中观察到的再喂养诱导的 Sestrin1•GATOR2 减少。酒精拮抗了再喂养状态下观察到的 RagA/C•Raptor 复合物形成的增加。酒精拮抗了再喂养后 Raptor 与免疫沉淀的 LAMPTOR1(Ragulator 复合物的一部分)的增加,并减少了 RagC 与 LAMPTOR1 的关联。最后,酒精增加了 v-ATPase V 结构域与 LAMPTOR1 的关联,并防止了再喂养诱导的 v-ATPase V1 与 LAMPTOR1 的减少。总之,这些数据表明,急性酒精摄入破坏了 Rag-Ragulator 复合物内的多个蛋白-蛋白复合物,这些复合物与体内条件下营养刺激的肌肉蛋白质合成的同时下降有关且一致。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4e1b/8070399/802331372ac5/nutrients-13-01236-g001.jpg

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