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Time-resolved nanoscale imaging of biomolecules in living cells and tissues: prospects for small animal imaging

机译:活细胞和组织中生物分子的时间分辨纳米级成像:小动物成像的前景

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A major need in non-invasive optical imaging of small animal models is an ability not only to visualize the solid tumors in vivo but to reproducibly quantify the tumor burden and its propensity to metastasize to other organs of the body. It is crucial to non-invasively detect the subtle molecular changes that can make a cell 'abnormal' and cancerous in its very early stage. Currently available methods for non-invasive optical imaging of solid tumors in small animals employ intensity-based detection that are severely affected by spectral artifacts and ubiquitous autofluorescence background. Thus these approaches serve merely as visualization tools and are unable to precisely quantify the size and shape of the tumors in vivo. There is a growing need to establish a reliable, reproducible and non-invasive optical imaging methodology that can provide quantitative information on solid tumors in vivo. This manuscript addresses this vital issue and proposes to employ fluorescence lifetime (rather than intensity) as a contrast parameter to discriminate tumor tissue expressing green fluorescent protein (EGFP) from surrounding autofluorescence background. In this manuscript, we present accurate lifetime measurements in intact living cells and ex vivo tissues and propose that this methodology is a potentially vital approach for whole small animal imaging.
机译:小型动物模型的非侵入性光学成像的主要需求是不仅可以在体内可视化实体肿瘤的能力,而是可重复地量化肿瘤负荷及其转移到身体其他器官的倾向。这对非侵入性地检测到可在其早期阶段进行细胞“异常”和癌症的微妙分子变化至关重要。目前,小动物实体瘤的无侵入光学成像的现有方法采用基于强度的检测,受光谱伪影和普遍存在的自发荧光背景的严重影响。因此,这些方法仅作为可视化工具,并且不能精确地量化体内肿瘤的尺寸和形状。越来越需要建立可靠,可重复的和非侵入性光学成像方法,其可以提供体内实体肿瘤的定量信息。该手稿解决了这个重要问题,并提出了荧光寿命(而不是强度)作为鉴别来自周围的自发荧光背景的肿瘤组织的肿瘤组织(EGFP)。在该稿件中,我们在完整的活细胞和离体组织中呈现精确的寿命测量,并提出这种方法是整个小动物成像的潜在重要方法。

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