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通过扭曲红细胞来加速新陈代谢和跨膜阳离子通量。

Accelerating metabolism and transmembrane cation flux by distorting red blood cells.

机构信息

School of Life and Environmental Sciences, University of Sydney, Sydney, New South Wales, Australia.

出版信息

Sci Adv. 2017 Oct 18;3(10):eaao1016. doi: 10.1126/sciadv.aao1016. eCollection 2017 Oct.

Abstract

Under static conditions, mammalian red blood cells (RBCs) require a continuous supply of energy, typically via glucose, to maintain their biconcave disc shape. Mechanical distortion, in a complementary way, should lead to increased energy demand that is manifest in accelerated glycolysis. The experimental challenge in observing this phenomenon was met by reversibly and reproducibly distorting the cells and noninvasively measuring glycolytic flux. This was done with a gel-distorting device that was coupled with C nuclear magnetic resonance (NMR) spectroscopy. We measured [3-C]l-lactate production from [1,6-C]d-glucose in the RBCs suspended in gelatin gels, and up to 90% rate enhancements were recorded. Thus, for the first time, we present experiments that demonstrate the linkage of mechanical distortion to metabolic changes in whole mammalian cells. In seeking a mechanism for the linkage between shape and energy supply, we measured transmembrane cation flux with Cs (as a K congener) using Cs NMR spectroscopy, and the cation flux was increased up to fivefold. The postulated mechanism for these notable (in terms of whole-body energy consumption) responses is stimulation of Ca-adenosine triphosphatase by increased transmembrane flux of Ca via the channel protein Piezo1 and increased glycolysis because its flux is adenosine triphosphate demand-regulated.

摘要

在静态条件下,哺乳动物的红细胞 (RBC) 需要持续的能量供应,通常通过葡萄糖来维持其双凹盘形。以互补的方式,机械变形会导致能量需求增加,这表现为糖酵解加速。通过可逆和可重复地变形细胞并非侵入性地测量糖酵解通量,解决了观察这一现象的实验挑战。这是通过与 C 核磁共振 (NMR) 光谱学相结合的凝胶变形装置来完成的。我们测量了悬浮在明胶凝胶中的 RBC 中[1,6-C]d-葡萄糖的[3-C]l-乳酸的产生,记录了高达 90%的速率增强。因此,我们首次展示了证明机械变形与整个哺乳动物细胞代谢变化之间联系的实验。在寻找形状和能量供应之间联系的机制时,我们使用 Cs NMR 光谱法测量了跨膜阳离子通量 Cs(作为 K 的同系物),并且阳离子通量增加了五倍。这些显著的(就全身能量消耗而言)反应的假设机制是通过通道蛋白 Piezo1 增加跨膜 Ca 通量刺激 Ca-三磷酸腺苷酶,以及增加糖酵解,因为其通量受三磷酸腺苷需求调节。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7e0a/5647125/7e72a643acb4/aao1016-F1.jpg

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