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首页> 外文期刊>Journal of biomedical optics >Multiphoton fluorescence lifetime contrast in deep tissue imaging: prospects in redox imaging and disease diagnosis
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Multiphoton fluorescence lifetime contrast in deep tissue imaging: prospects in redox imaging and disease diagnosis

机译:深层组织成像中的多光子荧光寿命对比:氧化还原成像和疾病诊断的前景

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Turbid tissues pose serious problems of strong absorption and scattering that make steady state fluorescence imaging methods less successful in imaging tissue layers deeper than a few tens of micrometers. Complications arise as one progresses from imaging cells to tissues to whole animal—which include enormous autofluores-cence background in tissues and poor signal from regions of interest. Since the steady state, intensity-based methods cannot discriminate the photons arising from the fluorophores and the autofluorescence background, it is almost impractical to isolate these two signals. We describe multiphoton fluorescence lifetime imaging methods in the time domain to demonstrate fluorescence lifetime contrast in discriminating autofluorescence background from the fluorescent signals. Since the photophysical schemes of the fluorophore and autofluorescence contributions are distinct, it is feasible to isolate these two contributions in every pixel based only on their decay constants without compromising the SNR. We present preliminary lifetime measurements to characterize autofluorescence in various cell lines and ex vivo tissues obtained from mouse models. Together, these results suggest a novel direction in obtaining quantitative information from endogenous tissue fluorescence without any exogenous staining. The prospects for this approach in metabolic redox imaging and disease diagnosis are discussed.
机译:浑浊的组织构成了严重的强吸收和散射问题,这使得稳态荧光成像方法在对组织层(比几十微米更深)成像时效果不佳。随着人们从成像细胞到组织再到整个动物的发展,出现了并发症,包括组织中巨大的自发荧光背景以及感兴趣区域的不良信号。由于基于强度的稳态方法无法区分由荧光团和自发荧光背景引起的光子,因此隔离这两个信号几乎是不切实际的。我们在时域中描述多光子荧光寿命成像方法,以证明在区分自发荧光背景和荧光信号中的荧光寿命对比。由于荧光团和自发荧光贡献的光物理方案是不同的,因此仅在不损害SNR的情况下,仅基于它们的衰减常数在每个像素中隔离这两个贡献是可行的。我们目前初步的寿命测量,以表征从小鼠模型获得的各种细胞系和离体组织中的自发荧光。在一起,这些结果表明从内源性组织荧光获得定量信息而没有任何外源性染色的新方向。讨论了这种方法在代谢氧化还原成像和疾病诊断中的前景。

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