Improved tumor contrast achieved by single time point dual-reporter fluorescence imaging

Improved tumor contrast achieved by single time point dual-reporter fluorescence imaging

In this study, we demonstrate a method to quantify biomarker expression that uses an exogenous dual-reporter imaging approach to improve tumor signal detection. The uptake of two fluorophores, one nonspecific and one targeted to the epidermal growth factor receptor (EGFR), were imaged at 1 h in thre...

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Veröffentlicht in:Journal of biomedical optics 2012-06, Vol.17 (6), p.066001-066001
Hauptverfasser: Tichauer, Kenneth M, Samkoe, Kimberley S, Sexton, Kristian J, Gunn, Jason R, Hasan, Tayyaba, Pogue, Brian W
Format: Artikel
Sprache:eng
Schlagworte:
Amplification
Animals
Biological
Cell Line, Tumor
Collagen - chemistry
Density
Drug Combinations
ErbB Receptors - metabolism
Fluorescence
Genes, Reporter
Hemodynamics
Humans
Image Processing, Computer-Assisted - methods
Imaging
Laminin - chemistry
Mice
Microscopy, Fluorescence - methods
Models, Chemical
Neoplasm Transplantation
Neoplasms - diagnosis
Neoplasms - pathology
Proteoglycans - chemistry
Rats
Receptors
Research Papers: Imaging
ROC Curve
Therapy
Time Factors
Tumors
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Zusammenfassung:In this study, we demonstrate a method to quantify biomarker expression that uses an exogenous dual-reporter imaging approach to improve tumor signal detection. The uptake of two fluorophores, one nonspecific and one targeted to the epidermal growth factor receptor (EGFR), were imaged at 1 h in three types of xenograft tumors spanning a range of EGFR expression levels (n=6 in each group). Using this dual-reporter imaging methodology, tumor contrast-to-noise ratio was amplified by >6 times at 1 h postinjection and >2 times at 24 h. Furthermore, by as early as 20 min postinjection, the dual-reporter imaging signal in the tumor correlated significantly with a validated marker of receptor density (P
ISSN:1083-3668
1560-2281
DOI:10.1117/1.JBO.17.6.066001