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多光子显微镜检查过程中大鼠嗜碱性白血病细胞中还原型烟酰胺腺嘌呤二核苷酸的光漂白及高荧光损伤的形成

Photobleaching of reduced nicotinamide adenine dinucleotide and the development of highly fluorescent lesions in rat basophilic leukemia cells during multiphoton microscopy.

作者信息

Tiede LeAnn M, Nichols Michael G

机构信息

Department of Biomedical Sciences, Creighton University, Omaha, NE, USA.

出版信息

Photochem Photobiol. 2006 May-Jun;82(3):656-64. doi: 10.1562/2005-09-19-RA-689.

Abstract

Endogenous reduced nicotinamide adenine dinucleotide (NADH) fluorescence provides an intrinsic indicator of the cellular metabolic state, but prolonged monitoring is limited by photobleaching and/or phototoxicity. Multiphoton excitation of NADH by ultrashort, 740-nm laser pulses provides a significant improvement over UV excitation by eliminating peripheral photobleaching; however, molecules within the subfemtoliter excitation volume remain susceptible. We have investigated the photophysical mechanisms responsible for multiphoton photobleaching of NADH in living cells to permit the imaging technique to be optimized. The loss of fluorescence because of multiphoton photobleaching was measured by repetitively imaging individual planes within rat basophilic leukemia cells. The photobleaching rate was proportional to the fourth power of the laser intensity. Based on these measurements, we propose a double-biphotonic, four-photon photobleaching mechanism and estimate the quantum yield of photobleaching of intracellular NADH to be 0.0073 +/- 0.0002 by this mechanism. In addition to photobleaching, the development of bright, punctate fluorescent lesions can also be observed. The frequency of lesion formation also increased approximately as the fourth power of the laser intensity after an intensity-dependent threshold number of images had been exceeded. The consequences for two-photon metabolic imaging are discussed.

摘要

内源性还原型烟酰胺腺嘌呤二核苷酸(NADH)荧光可提供细胞代谢状态的内在指标,但长时间监测受光漂白和/或光毒性限制。用740纳米超短激光脉冲对NADH进行多光子激发,通过消除周边光漂白,相较于紫外线激发有显著改进;然而,亚飞升激发体积内的分子仍易受影响。我们研究了活细胞中NADH多光子光漂白的光物理机制,以便优化成像技术。通过对大鼠嗜碱性白血病细胞内单个平面进行重复成像,测量了多光子光漂白导致的荧光损失。光漂白速率与激光强度的四次方成正比。基于这些测量结果,我们提出了一种双双光子、四光子光漂白机制,并估计通过该机制细胞内NADH的光漂白量子产率为0.0073±0.0002。除了光漂白,还能观察到明亮的点状荧光损伤的形成。在超过强度依赖性阈值图像数量后,损伤形成频率也大约随激光强度的四次方增加。讨论了对双光子代谢成像的影响。

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