Abstract
Imaging a fluorophore in a living tissue presents several unique problems. The fluorescence from the labeled cell(s) may be weak, the labeled cells may be buried deep within tissue and the presence of a fluorophore may render the cells photo-sensitive. Two-photon laser-scanning microscopy (TPLSM) offers several advantages in meeting these challenges. We show that TPLSM provides greater sensitivity, better resolution and less photo-bleaching, as compared to confocal laser-scanning microscopy. The dramatically reduced photo-bleaching makes it possible to image cells continuously for long periods of time. Therefore, TPLSM allows a safer and higher-resolution means of imaging living cells labeled with a variety of fluorophores, including green fluorescent protein.
Author supplied keywords
Cite
CITATION STYLE
Potter, S. M., Wang, C. M., Garrity, P. A., & Fraser, S. E. (1996). Intravital imaging of green fluorescent protein using two-photon laser-scanning microscopy. In Gene (Vol. 173, pp. 25–31). Elsevier B.V. https://doi.org/10.1016/0378-1119(95)00681-8
Register to see more suggestions
Mendeley helps you to discover research relevant for your work.