解构自身荧光:细胞和组织中生物化学的无创检测和监测(会议报告)

SPIE BiOS Pub Date : 2016-05-17 DOI:10.1117/12.2212443
E. Goldys, M. Gosnell, A. Anwer, J. C. Cassano, C. Sue, S. Mahbub, S. M. Pernichery, D. Inglis, Partho P. Adhikary, J. Jazayeri, M. Cahill, S. Saad, C. Pollock, M. Sutton-Mcdowall, Jeremy G. Thompson
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引用次数: 1

摘要

能够处理复杂生物异质性的非侵入性细胞监测的自动化和公正方法对生物学和医学至关重要。无标记细胞成像提供了内源性荧光代谢物、酶和辅助因子在细胞中的信息。然而,迄今为止,从天然荧光成像中提取高含量信息是不可能的。在这里,我们定量表征细胞群在不同的组织类型,活的或固定的,通过使用新的图像处理和一个简单的多光谱升级的宽视场荧光显微镜。多光谱本征荧光成像应用于患者嗅神经球源性细胞,人类代谢性疾病MELAS(线粒体肌病、脑肌病、乳酸酸中毒、卒中样综合征)的细胞模型。通过使用内源性对比源,在其完整的形态学背景下,在活细胞之间检测到细微的代谢变化,这使得在治疗前后区分健康细胞和病变细胞成为可能。天然荧光团、黄素、结合和游离NADH和类维生素a的细胞图谱揭示了微妙的代谢特征,并帮助揭示了重要的细胞亚群,特别是线粒体功能受损的亚群。通过检测癌症基因突变、无创监测CD90表达、无标记跟踪干细胞分化、识别具有不同功能特征的干细胞亚群、糖尿病组织诊断和评估植入前胚胎状况,进一步说明了我们方法的多功能性。我们的最佳判别方法使统计假设检验和直观的可视化,以前无法察觉的差异变得清晰明显。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Deconstructing autofluorescence: non-invasive detection and monitoring of biochemistry in cells and tissues (Conference Presentation)
Automated and unbiased methods of non-invasive cell monitoring able to deal with complex biological heterogeneity are fundamentally important for biology and medicine. Label-free cell imaging provides information about endogenous fluorescent metabolites, enzymes and cofactors in cells. However extracting high content information from imaging of native fluorescence has been hitherto impossible. Here, we quantitatively characterise cell populations in different tissue types, live or fixed, by using novel image processing and a simple multispectral upgrade of a wide-field fluorescence microscope. Multispectral intrinsic fluorescence imaging was applied to patient olfactory neurosphere-derived cells, cell model of a human metabolic disease MELAS (mitochondrial myopathy, encephalomyopathy, lactic acidosis, stroke-like syndrome). By using an endogenous source of contrast, subtle metabolic variations have been detected between living cells in their full morphological context which made it possible to distinguish healthy from diseased cells before and after therapy. Cellular maps of native fluorophores, flavins, bound and free NADH and retinoids unveiled subtle metabolic signatures and helped uncover significant cell subpopulations, in particular a subpopulation with compromised mitochondrial function. The versatility of our method is further illustrated by detecting genetic mutations in cancer, non-invasive monitoring of CD90 expression, label-free tracking of stem cell differentiation, identifying stem cell subpopulations with varying functional characteristics, tissue diagnostics in diabetes, and assessing the condition of preimplantation embryos. Our optimal discrimination approach enables statistical hypothesis testing and intuitive visualisations where previously undetectable differences become clearly apparent.
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