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Merck
CN

Tumor cell differentiation by label-free fluorescence microscopy.

Journal of biomedical optics (2012-12-12)
Petra Weber, Michael Wagner, Petra Kioschis, Waltraud Kessler, Herbert Schneckenburger
摘要

Autofluorescence spectra, images, and decay kinetics of U251-MG glioblastoma cells prior and subsequent to activation of tumor suppressor genes are compared. While phase contrast images and fluorescence intensity patterns of tumor (control) cells and less malignant cells are similar, differences can be deduced from autofluorescence spectra and decay kinetics. In particular, upon near UV excitation, the fluorescence ratio of the free and protein-bound coenzyme nicotinamid adenine dinucleotide depends on the state of malignancy and reflects different cytoplasmic (including lysosomal) and mitochondrial contributions. While larger numbers of fluorescence spectra are evaluated by principal component analysis, a multivariate data analysis method, additional information on cell metabolism is obtained from spectral imaging and fluorescence lifetime imaging microscopy.

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产品描述

Sigma-Aldrich
二氯乙酸, ReagentPlus®, ≥99%
Supelco
二氯乙酸, PESTANAL®, analytical standard