Leucine-enriched amino acids maintain peripheral mTOR-Rheb localization independent of myofibrillar protein synthesis and mTORC1 signaling postexercise

被引:19
作者
Hannaian, Sarkis J. [1 ]
Hodson, Nathan [1 ]
Abou Sawan, Sidney [1 ]
Mazzulla, Michael [1 ]
Kato, Hiroyuki [2 ]
Matsunaga, Keiko [2 ]
Waskiw-Ford, Marcus [1 ]
Duncan, Justin [1 ]
Kumbhare, Dinesh A. [3 ]
Moore, Daniel R. [1 ]
机构
[1] Univ Toronto, Fac Kinesiol & Phys Educ, Dept Exercise Sci, Toronto, ON, Canada
[2] Ajinomoto Co Inc, Inst Food Sci & Technol, Technol Dev Ctr, Kawasaki, Kanagawa, Japan
[3] Toronto Rehabil Inst, Toronto, ON, Canada
基金
加拿大自然科学与工程研究理事会;
关键词
signaling; essential amino acids; leucine; mTORC1; muscle protein synthesis; HUMAN SKELETAL-MUSCLE; RESISTANCE EXERCISE; TRANSPORTER EXPRESSION; MECHANISTIC TARGET; WHEY-PROTEIN; INGESTION; ACTIVATION; RAPAMYCIN; RESPONSES; INCREASE;
D O I
10.1152/japplphysiol.00241.2020
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
Postexercise protein ingestion can elevate rates of myofibrillar protein synthesis (MyoPS), mTORC1 activity, and mTOR translocation/proteinprotein interactions. However, it is unclear if leucine-enriched essential amino acids (LEAA) can similarly facilitate intracellular mTOR trafficking in humans after exercise. The purpose of this study was to determine the effect of postexercise LEAA (4 g total EAAs. 1.6 g leucine) on acute MyoPS and mTORC1 translocation and signaling. Recreationally active men performed lower-body resistance exercise (5 x 8-10 leg press and leg extension) to volitional failure. Following exercise participants consumed LEAA (n = 8) or an isocaloric carbohydrate drink (PLA; n = 10). MyoPS was measured over 1.5-4 h of recovery by oral pulse of L-[ring-H-2(5)] -phenylalanine. Phosphorylation of proteins in the mTORC1 pathway were analyzed via immunoblotting and mTORC1-LAMP2/WGA/Rheb colocalization via immunofluorescence microscopy. There was no difference in MyoPS between groups (LEAA = 0.098 +/- 0.01%/h; PL = 0.090 +/- 0.01%/h; P > 0.05). Exercise increased (P < 0.05) rpS6(Ser240/244) (LEAA = 35.3-fold; PLA = 20.6-fold). mTOR(Ser2448 )(LEAA = 1.8-fold; PLA = 1.2-fold) and 4EBP1(T)(hr37/46) (LEAA = 1.5-fold; PLA = 1.4-fold) phosphorylation irrespective of nutrition (P > 0.05). LAT1 and SNAT2 protein expression were not affected by exercise or nutrient ingestion. mTOR-LAMP2 colocalization was greater in LEAA preexercise and decreased following exercise and supplement ingestion (P < 0.05), yet was unchanged in PLA. mTOR-WGA (cell periphery marker) and mTOR-Rheb colocalization was greater in LEAA compared with PLA irrespective of time-point (P < 0.05). In conclusion, the postexercise consumption of 4 g of LEAA maintains mTOR in peripheral regions of muscle fibers, in closer proximity to its direct activator Rheb, during prolonged recovery independent of differences in MyoPS or mTORC1 signaling compared with PLA ingestion. This intracellular localization of mTOR may serve to "prime" the kinase for future anabolic stimuli. NEW & NOTEWORTHY This is the first study to investigate whether postexercise leucine-enriched amino acid (LEAA) ingestion elevates mTORC1 translocation and protein-protein interactions in human skeletal muscle. Here, we observed that although LEAA ingestion did not further elevate postexercise MyoPS or mTORC1 signaling compared with placebo, mTORC1 peripheral location and interaction with Rheb were maintained. This may serve to "prime" mTORC1 for subsequent anabolic stimuli.
引用
收藏
页码:133 / 143
页数:11
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