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通过细胞内氧感应技术监测细胞氧合和对代谢刺激的反应。

Monitoring of cell oxygenation and responses to metabolic stimulation by intracellular oxygen sensing technique.

机构信息

Biochemistry Department, University College Cork, Cork, Ireland.

出版信息

Integr Biol (Camb). 2010 Sep;2(9):443-51. doi: 10.1039/c0ib00021c. Epub 2010 Jul 26.

Abstract

Quenched-phosphorescence oxygen (O(2)) sensing technique allows non-invasive, real-time monitoring of both intra- and extracellular O(2) concentration in respiring samples. Using this technique we investigated O(2) gradients in populations of neurosecretory PC12 cells cultured in 96-well plates and exposed to graded hypoxia at rest and upon metabolic stimulation. Under high atmospheric O(2) (10-21%) the respiration of resting cells dictated that local O(2) was moderately reduced, and at a certain threshold (6% in galactose medium) cell layer became practically anoxic. Furthermore, cell stimulation triggered a major redistribution of O(2) and a prominent 'hypoxic overshoot' mediated by diffusion. The deep, prolonged cell deoxygenation upon stimulation was matched by an increase in nuclear HIF-1alpha levels. In the presence of nitric oxide the hypoxic overshoot was truncated and HIF-1alpha stabilization inhibited. Thus, the main determinants which impact upon cellular O(2) levels and oxygen-sensitive signaling pathways are the atmospheric O(2), sample geometry, cell density, respiration rate and its dynamics. Changes in any of these parameters can significantly alter the O(2) levels experienced by the cells and the subsequently activated signaling pathways. This technique, which provides simple and reliable monitoring of cell oxygenation, is therefore important for hypoxia research, metabolic studies and experiments with respiring cells.

摘要

猝灭荧光氧(O(2))传感技术允许在呼吸样品中无创、实时监测细胞内和细胞外的 O(2)浓度。使用该技术,我们研究了在休息状态和代谢刺激下暴露于分级缺氧的培养在 96 孔板中的神经分泌 PC12 细胞群体中的 O(2)梯度。在高大气 O(2)(10-21%)下,休息细胞的呼吸导致局部 O(2)适度减少,并且在一定阈值(半乳糖培养基中的 6%)下,细胞层实际上变成乏氧的。此外,细胞刺激引发了 O(2)的主要再分布和由扩散介导的明显“缺氧过冲”。刺激后细胞深度和长时间的去氧与核 HIF-1alpha 水平的增加相匹配。在存在一氧化氮的情况下,缺氧过冲被截断并且 HIF-1alpha 稳定化被抑制。因此,影响细胞 O(2)水平和氧敏感信号通路的主要决定因素是大气 O(2)、样品几何形状、细胞密度、呼吸率及其动力学。这些参数中的任何变化都可能显著改变细胞经历的 O(2)水平和随后激活的信号通路。该技术提供了对细胞氧合作用的简单可靠监测,因此对于缺氧研究、代谢研究和呼吸细胞实验非常重要。

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