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禁食对人和小鼠体内血液的代谢影响。

Metabolic effects of fasting on human and mouse blood in vivo.

作者信息

Pietrocola Federico, Demont Yohann, Castoldi Francesca, Enot David, Durand Sylvère, Semeraro Michaela, Baracco Elisa Elena, Pol Jonathan, Bravo-San Pedro Jose Manuel, Bordenave Chloé, Levesque Sarah, Humeau Juliette, Chery Alexis, Métivier Didier, Madeo Frank, Maiuri M Chiara, Kroemer Guido

机构信息

a Equipe 11 labellisée Ligue contre le Cancer, Centre de Recherche des Cordeliers, INSERM U 1138 , Paris , France.

b Université Paris Descartes, Sorbonne Paris Cité , Paris , France.

出版信息

Autophagy. 2017 Mar 4;13(3):567-578. doi: 10.1080/15548627.2016.1271513. Epub 2017 Jan 6.

Abstract

Starvation is a strong physiological stimulus of macroautophagy/autophagy. In this study, we addressed the question as to whether it would be possible to measure autophagy in blood cells after nutrient deprivation. Fasting of mice for 48 h (which causes ∼20% weight loss) or starvation of human volunteers for up to 4 d (which causes <2% weight loss) provokes major changes in the plasma metabolome, yet induces only relatively minor alterations in the intracellular metabolome of circulating leukocytes. White blood cells from mice and human volunteers responded to fasting with a marked reduction in protein lysine acetylation, affecting both nuclear and cytoplasmic compartments. In circulating leukocytes from mice that underwent 48-h fasting, an increase in LC3B lipidation (as assessed by immunoblotting and immunofluorescence) only became detectable if the protease inhibitor leupeptin was injected 2 h before drawing blood. Consistently, measurement of an enhanced autophagic flux was only possible if white blood cells from starved human volunteers were cultured in the presence or absence of leupeptin. Whereas all murine leukocyte subpopulations significantly increased the number of LC3B puncta per cell in response to nutrient deprivation, only neutrophils from starved volunteers showed signs of activated autophagy (as determined by a combination of multi-color immunofluorescence, cytofluorometry and image analysis). Altogether, these results suggest that white blood cells are suitable for monitoring autophagic flux. In addition, we propose that the evaluation of protein acetylation in circulating leukocytes can be adopted as a biochemical marker of organismal energetic status.

摘要

饥饿是巨自噬/自噬的一种强烈生理刺激因素。在本研究中,我们探讨了在营养剥夺后是否能够检测血细胞中的自噬。小鼠禁食48小时(导致体重减轻约20%)或人类志愿者饥饿长达4天(导致体重减轻<2%)会引起血浆代谢组的重大变化,但仅诱导循环白细胞细胞内代谢组相对较小的改变。来自小鼠和人类志愿者的白细胞对禁食的反应是蛋白质赖氨酸乙酰化显著降低,影响细胞核和细胞质部分。在禁食48小时的小鼠的循环白细胞中,只有在采血前2小时注射蛋白酶抑制剂亮抑酶肽,才能检测到LC3B脂化增加(通过免疫印迹和免疫荧光评估)。同样,只有在饥饿的人类志愿者的白细胞在有或没有亮抑酶肽的情况下培养时,才能测量到增强的自噬通量。虽然所有小鼠白细胞亚群在营养剥夺后每个细胞的LC3B斑点数量都显著增加,但只有饥饿志愿者的中性粒细胞显示出自噬激活的迹象(通过多色免疫荧光、细胞荧光测定和图像分析相结合确定)。总之,这些结果表明白细胞适合用于监测自噬通量。此外,我们建议将循环白细胞中蛋白质乙酰化的评估作为机体能量状态的生化标志物。

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