by Ruiz-Cabello, Jesus, Walczak, Piotr, Kedziorek, Dorota A, Chacko, Vadappuram P, Schmieder, Anna H, Wickline, Samuel A, Lanza, Gregory M and Bulte, Jeff W M
Abstract:
To optimize (19)F MR tracking of stem cells, we compared cellular internalization of cationic and anionic perfluoro-15-crown-5-ether (PFCE) nanoparticles using cell culture plates with different surface coatings. The viability and proliferation of anionic and cationic PFCE-labeled neural stem cells (NSCs) did not differ from unlabeled cells. Cationic PFCE nanoparticles ((19)F T1/T2 = 580/536 ms at 9.4 Tesla) were superior to anionic particles for intracellular fluorination. Best results were obtained with modified polystyrene culture dishes coated with both carboxylic and amino groups rather than conventional carboxyl-coated dishes. After injecting PFCE-labeled NSCs into the striatum of mouse brain, cells were readily identified in vivo by (19)F MRI without changes in signal or viability over a 2-week period after grafting. These results demonstrate that neural stem cells can be efficiently fluorinated with cationic PFCE nanoparticles without using transfection agents and visualized in vivo over prolonged periods with an MR sensitivity of approximately 140 pmol of PFCE/cell.
Reference:
In vivo “hot spot” MR imaging of neural stem cells using fluorinated nanoparticles. (Ruiz-Cabello, Jesus, Walczak, Piotr, Kedziorek, Dorota A, Chacko, Vadappuram P, Schmieder, Anna H, Wickline, Samuel A, Lanza, Gregory M and Bulte, Jeff W M), In Magn Reson Med, Wiley Subscription Services, Inc., A Wiley Company, volume 60, 2008.
Bibtex Entry:
@article{RuizCabello:2008gvd,
author = {Ruiz-Cabello, Jesus and Walczak, Piotr and Kedziorek, Dorota A and Chacko, Vadappuram P and Schmieder, Anna H and Wickline, Samuel A and Lanza, Gregory M and Bulte, Jeff W M},
title = {{In vivo "hot spot" MR imaging of neural stem cells using fluorinated nanoparticles.}},
journal = {Magn Reson Med},
year = {2008},
volume = {60},
number = {6},
pages = {1506--1511},
month = dec,
publisher = {Wiley Subscription Services, Inc., A Wiley Company},
affiliation = {Russell H. Morgan Department of Radiology and Radiological Science, Division of MR Research, The Johns Hopkins University School of Medicine, Baltimore, Maryland, USA. ruizcabe@farm.ucm.es},
doi = {10.1002/mrm.21783},
pmid = {19025893},
pmcid = {PMC2597664},
language = {English},
rating = {0},
date-added = {2018-03-16T12:58:22GMT},
date-modified = {2020-07-09T13:27:51GMT},
abstract = {To optimize (19)F MR tracking of stem cells, we compared cellular internalization of cationic and anionic perfluoro-15-crown-5-ether (PFCE) nanoparticles using cell culture plates with different surface coatings. The viability and proliferation of anionic and cationic PFCE-labeled neural stem cells (NSCs) did not differ from unlabeled cells. Cationic PFCE nanoparticles ((19)F T1/T2 = 580/536 ms at 9.4 Tesla) were superior to anionic particles for intracellular fluorination. Best results were obtained with modified polystyrene culture dishes coated with both carboxylic and amino groups rather than conventional carboxyl-coated dishes. After injecting PFCE-labeled NSCs into the striatum of mouse brain, cells were readily identified in vivo by (19)F MRI without changes in signal or viability over a 2-week period after grafting. These results demonstrate that neural stem cells can be efficiently fluorinated with cationic PFCE nanoparticles without using transfection agents and visualized in vivo over prolonged periods with an MR sensitivity of approximately 140 pmol of PFCE/cell.},
url = {http://doi.wiley.com/10.1002/mrm.21783},
uri = {url{papers3://publication/doi/10.1002/mrm.21783}}
}