Literature DB >> 20059251

Wavelength-dependent backscattering measurements for quantitative real-time monitoring of apoptosis in living cells.

Christine S Mulvey1, Carly A Sherwood, Irving J Bigio.   

Abstract

Apoptosis--programmed cell death--is a cellular process exhibiting distinct biochemical and morphological changes. An understanding of the early morphological changes that a cell undergoes during apoptosis can provide the opportunity to monitor apoptosis in tissue, yielding diagnostic and prognostic information. There is avid interest regarding the involvement of apoptosis in cancer. The initial response of a tumor to successful cancer treatment is often massive apoptosis. Current apoptosis detection methods require cell culture disruption. Our aim is to develop a nondisruptive optical method to monitor apoptosis in living cells and tissues. This would allow for real-time evaluation of apoptotic progression of the same cell culture over time without alteration. Elastic scattering spectroscopy (ESS) is used to monitor changes in light-scattering properties of cells in vitro due to apoptotic morphology changes. We develop a simple instrument capable of wavelength-resolved ESS measurements from cell cultures in the backward direction. Using Mie theory, we also develop an algorithm that extracts the size distribution of scatterers in the sample. The instrument and algorithm are validated with microsphere suspensions. For cell studies, Chinese hamster ovary (CHO) cells are cultured to confluence on plates and are rendered apoptotic with staurosporine. Backscattering measurements are performed on pairs of treated and control samples at a sequence of times up to 6-h post-treatment. Initial results indicate that ESS is capable of discriminating between treated and control samples as early as 10- to 15-min post-treatment, much earlier than is sensed by standard assays for apoptosis. Extracted size distributions from treated and control samples show a decrease in Rayleigh and 150-nm scatterers, relative to control samples, with a corresponding increase in 200-nm particles. Work continues to correlate these size distributions with underlying morphology. To our knowledge, this is the first report of the use of backscattering spectral measurements to quantitatively monitor apoptosis in viable cell cultures in vitro.

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Year:  2009        PMID: 20059251      PMCID: PMC2794414          DOI: 10.1117/1.3259363

Source DB:  PubMed          Journal:  J Biomed Opt        ISSN: 1083-3668            Impact factor:   3.170


  39 in total

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4.  Index-of-refraction-dependent subcellular light scattering observed with organelle-specific dyes.

Authors:  Jeremy D Wilson; William J Cottrell; Thomas H Foster
Journal:  J Biomed Opt       Date:  2007 Jan-Feb       Impact factor: 3.170

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Review 6.  Apoptosis detection: an overview.

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Journal:  Exp Gerontol       Date:  1998-09       Impact factor: 4.032

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Review 9.  Apoptosis. Basic concepts and implications in coronary artery disease.

Authors:  P J Best; D Hasdai; G Sangiorgi; R S Schwartz; D R Holmes; R D Simari; A Lerman
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Review 10.  Apoptosis. Its significance in cancer and cancer therapy.

Authors:  J F Kerr; C M Winterford; B V Harmon
Journal:  Cancer       Date:  1994-04-15       Impact factor: 6.860

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  17 in total

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Journal:  J Biomed Opt       Date:  2011-11       Impact factor: 3.170

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8.  Wide-field quantitative imaging of tissue microstructure using sub-diffuse spatial frequency domain imaging.

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9.  Detection of doxorubicin-induced apoptosis of leukemic T-lymphocytes by laser tweezers Raman spectroscopy.

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