以培养的马骨骼肌卫星细胞作为模型系统,评估亮氨酸刺激的蛋白质合成。
Cultured equine satellite cells as a model system to assess leucine stimulated protein synthesis in horse muscle.
机构信息
Department of Animal Science, University of Minnesota, St. Paul, MN.
Department of Veterinary Biomedical Sciences, University of Minnesota, St. Paul, MN.
出版信息
J Anim Sci. 2018 Feb 15;96(1):143-153. doi: 10.1093/jas/skx028.
Leucine has been shown to stimulate the mammalian/mechanistic target of rapamycin (mTOR) signaling pathway which plays numerous key regulatory roles in cell growth, survival, and metabolism including protein synthesis in a number of species. However, previous work with equine satellite cells has suggested distinct species differences in regards to physiological effects and the magnitude of responses to growth factors and regulators. Because there is limited research available regarding the role of leucine in regulating equine skeletal muscle protein synthesis, the objective of this study was to evaluate the effect of leucine on the mTOR signaling pathway in cultured equine satellite. Protein synthesis was evaluated by measuring the incorporation of [3H] Phenylalanine (3HPhe) in equine satellite cell myotube cultures treated with a leucine titration ranging from 0 to 408 µM. Our results show a 1.8-fold increase (P < 0.02) in protein synthesis at levels slightly greater than those found in the general circulation, 204 and 408 µM when compared to a no leucine control (0 µM). Puromycin incorporation, a nonradioactive surface sensing of translation (SUnSET) methodology, was also measured in cells treated with leucine (LEU; 408 µM), a no-leucine control (CON), and a puromycin-negative vehicle (PURO-). These results demonstrated a 180% increase (P = 0.0056) in puromycin incorporation in LEU compared to CON cultures. To evaluate the mTOR signaling pathway, equine satellite cell myotube cultures were treated with leucine (LEU; 408 µM) or a no-leucine control (CON) in the presence or absence of rapamycin (LR and CR, respectively), an inhibitor of mTOR. The mTOR inhibitor, rapamycin, suppressed phosphorylation of mTOR (P < 0.01) and rS6 (P < 0.01) with an increase in phosphorylation of rS6 in leucine-treated cultures observed when compared to control cultures (P < 0.05). Similarly, there was a 27% increase (P < 0.005) in the hyperphosphorylated γ-form of 4E-BP1 compared to total 4E-BP1 in LEU compared to CON cultures with leucine-induced phosphorylation of 4E-BP1 completely blocked by rapamycin with a smaller decrease observed in CR compared to CON cultures. The major finding of this study was that leucine activated the mTOR translation initiation pathway and increased transcription of global proteins in cultured equine satellite cells. Use of the cell culture system with primary equine muscle cell lines provides the opportunity to distinguish the impact of leucine on muscle and protein synthesis, independent of systemic interactions.
亮氨酸已被证明可刺激哺乳动物/雷帕霉素靶蛋白(mTOR)信号通路,该通路在许多物种的细胞生长、存活和代谢中发挥着许多关键的调节作用,包括蛋白质合成。然而,先前对马卫星细胞的研究表明,在生理效应以及对生长因子和调节剂的反应幅度方面,存在明显的物种差异。由于关于亮氨酸在调节马骨骼肌蛋白质合成中的作用的研究有限,因此本研究的目的是评估亮氨酸对培养的马卫星细胞中 mTOR 信号通路的影响。通过测量 [3H]苯丙氨酸(3HPhe)在亮氨酸滴定从 0 到 408 μM 处理的马卫星细胞肌管培养物中的掺入来评估蛋白质合成。与无亮氨酸对照(0 μM)相比,当与无亮氨酸对照(0 μM)相比时,在略高于一般循环水平(204 和 408 μM)时,蛋白质合成增加了 1.8 倍(P <0.02)。还使用亮氨酸(LEU;408 μM)、无亮氨酸对照(CON)和无亮氨酸阴性载体(PURO-)处理的细胞测量了嘌呤霉素掺入,这是一种非放射性表面翻译感应(SUnSET)方法。这些结果表明,与 CON 培养物相比,LEU 中的嘌呤霉素掺入增加了 180%(P = 0.0056)。为了评估 mTOR 信号通路,在存在或不存在雷帕霉素(LR 和 CR,分别)的情况下,用亮氨酸(LEU;408 μM)或无亮氨酸对照(CON)处理马卫星细胞肌管培养物,mTOR 的抑制剂。mTOR 抑制剂雷帕霉素抑制 mTOR(P <0.01)和 rS6(P <0.01)的磷酸化,与对照培养物相比,在亮氨酸处理的培养物中观察到 rS6 的磷酸化增加(P <0.05)。同样,与 CON 培养物相比,LEU 中 4E-BP1 的高磷酸化 γ 形式与总 4E-BP1 相比增加了 27%(P <0.005),并且亮氨酸诱导的 4E-BP1 磷酸化完全被雷帕霉素阻断,与 CON 培养物相比,在 CR 中观察到的减少较小。本研究的主要发现是亮氨酸激活了 mTOR 翻译起始途径,并增加了培养的马卫星细胞中的总蛋白转录。使用具有原发性马肌肉细胞系的细胞培养系统提供了一种机会,可以区分亮氨酸对肌肉和蛋白质合成的影响,而不受全身相互作用的影响。
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