TY - JOUR
T1 - Tracking of fluorescence nanoparticles with nanometre resolution in a biological system
T2 - Assessing local viscosity and microrheology
AU - Marki, Alex
AU - Ermilov, Eugeny
AU - Zakrzewicz, Andreas
AU - Koller, Akos
AU - Secomb, Timothy W.
AU - Pries, Axel R.
N1 - Funding Information:
Acknowledgments We are grateful to Cathrin Dressler for providing for us the fluorescent nanoparticles, to Thomas Meinel for his help in the data analysis and to Klaus Affeld for his help in capillary viscometer measurements. The work of Alex Marki was supported by the Ernst von Leyden Stipend of the Berlin Cancer Society (Berliner Kreb-sgesellschaft e.V., Berlin, Germany). The project was supported by the Schüchtermann-Foundation (Germany, Dortmund), and the support by H. Warnecke is acknowledged.
PY - 2014/4
Y1 - 2014/4
N2 - The aim of the study was to establish a user-friendly approach for single fluorescence particle 3D localization and tracking with nanometre precision in a standard fluorescence microscope using a point spread function (PSF) approach, and to evaluate validity and precision for different analysis methods and optical conditions with particular application to microcirculatory flow dynamics and cell biology. Images of fluorescent particles were obtained with a standard fluorescence microscope equipped with a piezo positioner for the objective. Whole pattern (WP) comparison with a PSF recorded for the specific set-up and measurement of the outermost ring radius (ORR) were used for analysis. Images of fluorescent particles were recorded over a large range (about 7 μ m) of vertical positions, with and without distortion by overlapping particles as well as in the presence of cultured endothelial cells. For a vertical range of 6.5 μ m, the standard deviation (SD) from the predicted value, indicating validity, was 9.3/8.7 nm (WP/ORR) in the vertical and 8.2/11.7 nm in the horizontal direction. The precision, determined by repeated measurements, was 5.1/3.8 nm in the vertical and 2.9/3.7 nm in the horizontal direction. WP was more robust with respect to underexposure or overlapping images. On the surface of cultured endothelial cells, a layer with 2.5 times increased viscosity and a thickness of about 0.8 μ m was detected. With a validity in the range of 10 nm and a precision down to about 3-5 nm obtained by standard fluorescent microscopy, the PSF approach offers a valuable tool for a variety of experimental investigations of particle localizations, including the assessment of endothelial cell microenvironment.
AB - The aim of the study was to establish a user-friendly approach for single fluorescence particle 3D localization and tracking with nanometre precision in a standard fluorescence microscope using a point spread function (PSF) approach, and to evaluate validity and precision for different analysis methods and optical conditions with particular application to microcirculatory flow dynamics and cell biology. Images of fluorescent particles were obtained with a standard fluorescence microscope equipped with a piezo positioner for the objective. Whole pattern (WP) comparison with a PSF recorded for the specific set-up and measurement of the outermost ring radius (ORR) were used for analysis. Images of fluorescent particles were recorded over a large range (about 7 μ m) of vertical positions, with and without distortion by overlapping particles as well as in the presence of cultured endothelial cells. For a vertical range of 6.5 μ m, the standard deviation (SD) from the predicted value, indicating validity, was 9.3/8.7 nm (WP/ORR) in the vertical and 8.2/11.7 nm in the horizontal direction. The precision, determined by repeated measurements, was 5.1/3.8 nm in the vertical and 2.9/3.7 nm in the horizontal direction. WP was more robust with respect to underexposure or overlapping images. On the surface of cultured endothelial cells, a layer with 2.5 times increased viscosity and a thickness of about 0.8 μ m was detected. With a validity in the range of 10 nm and a precision down to about 3-5 nm obtained by standard fluorescent microscopy, the PSF approach offers a valuable tool for a variety of experimental investigations of particle localizations, including the assessment of endothelial cell microenvironment.
KW - Defocus imaging
KW - Particle tracking
KW - Resolution enhancement
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U2 - 10.1007/s10237-013-0499-7
DO - 10.1007/s10237-013-0499-7
M3 - Article
C2 - 23754460
AN - SCOPUS:84897481756
SN - 1617-7959
VL - 13
SP - 275
EP - 288
JO - Biomechanics and Modeling in Mechanobiology
JF - Biomechanics and Modeling in Mechanobiology
IS - 2
ER -