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Castration alters protein balance after high-frequency muscle contraction

机译:去势改变高频肌肉收缩后的蛋白质平衡

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摘要

Resistance exercise increases muscle mass by shifting protein balance in favor of protein accretion. Androgens independently alter protein balance, but it is unknown whether androgens alter this measure after resistance exercise. To answer this, male mice were subjected to sham or castration surgery 7–8 wk before undergoing a bout of unilateral, high-frequency, electrically induced muscle contractions in the fasted or refed state. Puromycin was injected 30 min before euthanasia to measure protein synthesis. The tibialis anterior was analyzed 4 h postcontraction. In fasted mice, neither basal nor stimulated rates of protein synthesis were affected by castration despite lower phosphorylation of mechanistic target of rapamycin in complex 1 (mTORC1) substrates [p70S6K1 (Thr389) and 4E-BP1 (Ser65)]. Markers of autophagy (LC3 II/I ratio and p62 protein content) were elevated by castration, and these measures remained elevated above sham values after contractions. Furthermore, in fasted mice, the protein content of Regulated in Development and DNA Damage 1 (REDD1) was correlated with LC3 II/I in noncontracted muscle, whereas phosphorylation of uncoordinated like kinase 1 (ULK1) (Ser757) was correlated with LC3 II/I in the contracted muscle. When mice were refed before contractions, protein synthesis and mTORC1 signaling were not affected by castration in either the noncontracted or contracted muscle. Conversely, markers of autophagy remained elevated in the muscles of refed, castrated mice even after contractions. These data suggest the castration-mediated elevation in baseline autophagy reduces the absolute positive shift in protein balance after muscle contractions in the refed or fasted states.>NEW & NOTEWORTHY In the absence of androgens, markers of autophagy were elevated, and these could not be normalized by muscle contractions. In the fasted state, REDD1 was identified as a potential contributor to autophagy in noncontracted muscle, whereas phosphorylation of ULK1 may contribute to this process in the contracted muscle. In the refed state, markers of autophagy remain elevated in both noncontracted and contracted muscles, but the relationship with REDD1 and ULK1 (Ser757) no longer existed.
机译:抵抗运动通过改变蛋白质平衡而有利于蛋白质积聚来增加肌肉质量。雄激素独立地改变蛋白质平衡,但是尚不清楚雄激素是否在抵抗运动后改变该措施。为了回答这个问题,雄性小鼠在禁食或反射状态下进行了单侧,高频,电诱导的肌肉收缩,然后进行了7-8周的假手术或去势手术。安乐死前30分钟注射嘌呤霉素以测量蛋白质合成。收缩后4小时分析胫骨前。在禁食的小鼠中,尽管复合物1(mTORC1)底物[p70S6K1(Thr389)和4E-BP1(Ser65)]中雷帕霉素的机械靶标磷酸化程度较低,但去势既不影响蛋白质的基础合成速率,也不刺激蛋白质的刺激速率受去势影响。自噬的标志物(LC3 II / I比值和p62蛋白含量)通过去势而升高,并且这些措施在收缩后仍高于假值。此外,在禁食的小鼠中,未收缩肌肉中调节发育和DNA损伤1(REDD1)的蛋白质含量与LC3 II / I相关,而未配位的激酶1(ULK1)(Ser757)的磷酸化与LC3 II / I相关。我在收缩的肌肉中。当小鼠在收缩前被拒食时,未收缩或收缩的肌肉中的去势均不会影响蛋白质合成和mTORC1信号传导。相反,自噬标志物即使在收缩后,在去势,去势小鼠的肌肉中仍保持升高。这些数据表明,去势或空腹状态下肌肉收缩后,去势介导的基线自噬水平升高降低了蛋白质平衡的绝对正向移位。>新与重要在没有雄激素的情况下,自噬标记物升高了,而肌肉收缩无法将其归一化。在禁食状态下,REDD1被认为是非收缩肌肉自噬的潜在贡献者,而ULK1的磷酸化可能有助于收缩肌肉的这一过程。在反射状态下,自噬标志物在未收缩和收缩的肌肉中均保持升高,但与REDD1和ULK1(Ser757)的关系不再存在。

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