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Daniel Axelrod

Researcher at University of Michigan

Publications -  124
Citations -  13841

Daniel Axelrod is an academic researcher from University of Michigan. The author has contributed to research in topics: Total internal reflection fluorescence microscope & Microscopy. The author has an hindex of 48, co-authored 121 publications receiving 13264 citations. Previous affiliations of Daniel Axelrod include University of California, Berkeley & Cornell University.

Papers
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Journal ArticleDOI

Mobility measurement by analysis of fluorescence photobleaching recovery kinetics.

TL;DR: The theoretical basis and some practical guidelines for simple, rigorous analysis of FPR experiments are presented and some model experiments on aqueous solutions of rhodamine 6G are described.
Journal ArticleDOI

Total internal reflection fluorescence microscopy in cell biology.

TL;DR: This review describes a microscopy technique based on total internal reflection fluorescence which is well suited for optical sectioning at cell‐substrate regions with an unusually thin region of fluorescence excitation.
Journal ArticleDOI

Cell-substrate contacts illuminated by total internal reflection fluorescence.

TL;DR: Total internal reflection fluorescence examination of cells appears to have promising applications, including visualization of the membrane and underlying cytoplasmic structures at cell-substrate contacts, dramatic reduction of autofluorescence from debris and thick cells, mapping of membranes topography, and visualization of reversible bound fluorescent ligands at membrane receptors.
Journal ArticleDOI

Total internal reflection fluorescence

TL;DR: TIRF is an optical effect particularly well-suited to the study of molecular and cellular phenomena at liquid/solid interfaces that is central to a wide range of biochemical and biophysical processes.
Journal ArticleDOI

Carbocyanine dye orientation in red cell membrane studied by microscopic fluorescence polarization

Daniel Axelrod
- 01 Jun 1979 - 
TL;DR: To interpret the experimental data, formulae are derived to account for the effect of high aperture observation on fluorescence polarization ratios, and are generally applicable to any high aperture polarization studied on microscopic samples, such as portions of single cells.