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测量二氯荧光素(DCF)荧光以作为小鼠胰岛中活性氧的一种测量方法。

Measurement of DCF fluorescence as a measure of reactive oxygen species in murine islets of Langerhans.

作者信息

Wang Xue, Roper Michael G

机构信息

Florida State University, Department of Chemistry and Biochemistry, 95 Chieftain Way, Tallahassee, USA.

出版信息

Anal Methods. 2014 May 7;6(9):3019-3024. doi: 10.1039/C4AY00288A.

Abstract

In islets of Langerhans, oxidative stress induced by reactive oxygen species (ROS) is thought to be critically involved in β-cell dysfunction during the development of diabetes. However, ROS have also been hypothesized to play a role in cellular signalling. To aid in delineating the effects of ROS in living islets of Langerhans, the endocrine portion of the pancreas that contain β-cells, we sought to develop a robust and reproducible protocol to measure these species using the fluorescent dye, 2',7'-dichlorodihydrofluorescein diacetate (HDCF-DA). The protocol that was developed minimized photobleaching and leakage of HDCF from murineislets and utilized a normalization procedure to further reduce experimental variability. The method allowed for ~25 min of DCF measurement in living islets. We used the developed protocol to compare DCF fluorescence from batches of islets incubated in varying glucose concentrations and observed ~1.5-fold higher fluorescence signals in 3 vs. 20 mM glucose. The effects of diazoxide, which clamps open K channels reducing intracellular [Ca] ([Ca]) without affecting glucose metabolism, were also investigated. The presence of diazoxide increased DCF fluorescence at all glucose concentrations tested while addition of 30 mM K to increase [Ca] reduced the fluorescence by ~15%. With the developed protocol, all experimental methods tested to increase [Ca] resulted in a decrease in DCF fluorescence, potentially indicating involvement of ROS in intracellular signalling cascades.

摘要

在胰岛中,活性氧(ROS)诱导的氧化应激被认为在糖尿病发生发展过程中β细胞功能障碍中起关键作用。然而,也有假说认为ROS在细胞信号传导中发挥作用。为了有助于阐明ROS在含有β细胞的胰腺内分泌部分——胰岛中的作用,我们试图开发一种可靠且可重复的方案,使用荧光染料2',7'-二氯二氢荧光素二乙酸酯(HDCF-DA)来测量这些物质。所开发的方案将HDCF在小鼠胰岛中的光漂白和泄漏降至最低,并采用归一化程序进一步降低实验变异性。该方法允许在活胰岛中进行约25分钟的DCF测量。我们使用所开发的方案比较了在不同葡萄糖浓度下孵育的多批胰岛的DCF荧光,发现在3 mM葡萄糖与20 mM葡萄糖相比时荧光信号高约1.5倍。还研究了二氮嗪的作用,二氮嗪可使钾通道开放,降低细胞内[Ca]([Ca])而不影响葡萄糖代谢。在所有测试的葡萄糖浓度下,二氮嗪的存在均增加了DCF荧光,而添加30 mM钾以增加[Ca]则使荧光降低了约15%。通过所开发的方案,所有测试的增加[Ca]的实验方法均导致DCF荧光降低,这可能表明ROS参与了细胞内信号级联反应。

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