Noninvasive imaging of the distribution in oxygen in tissue in vivo using near-infrared phosphors.

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Noninvasive imaging of the distribution in oxygen in tissue in vivo using near-infrared phosphors.

S A Vinogradov, L W Lo, W T Jenkins, S M Evans, C Koch and D F Wilson

Department of Biochemistry and Biophysics, Medical School, University of Pennsylvania, Philadelphia 19104, USA. vinograd@mail.med.upenn.edu

ABSTRACT

A newly developed water-soluble phosphor suitable for measuringoxygen pressure in the blood (Green 2W) was used for noninvasive,in vivo imaging of oxygen distribution in the vascular systemsof mice. Oxygen quenches the phosphorescence of Green 2W, measuredin the presence of 2% albumin, according to the Stern-volmerrelationship. This oxygen-dependent quenching of phosphorescencehas been used to obtain digital maps of the oxygen distributionin the tissue vasculature. EMT-6 mammary carcinoma tumors weregrown by injecting 1 x 10(6) cells in 0.1-ml carrier into thesubcutaneous space over the muscle on the hindquarter. Whenthe tumors were approximately 8 mm in diameter, 300 microgramsof phosphorescence probe (Green 2W; absorption maximum 636 nm)was injected into the tail vein. The mice were immobilized withintraperotoneal Ketamine (133 mg/kg) and Xylazine (10 mg/kg)and illuminated with flashes (< 4-microseconds t1/2) of lightof 630 +/- 12 nm. The emitted phosphorescence (790-nm maximum)was imaged an intensified CCD camera. Images were collectedbeginning at 30, 50, 80, 120, 180, 240, 420, and 2500 microsecondsafter the flash and used to calculate digital maps of the phosphorescencelifetimes and oxygen pressure. Both the illumination light andthe phosphorescence were in the near-infrared region of thespectrum, where tissue has greatly decreased absorbance. Thelight therefore readily passed through the skin and centimeterthicknesses of tissue. The oxygen maps could be obtained byilluminating from the side of the mouse opposite the camera(and tumor). The tumors were readily observed as regions withoxygen pressures substantially below those of the surroundingtissue. Thus, phosphorescence measurements can noninvasivelydetect volumes of tissue with below-normal oxygen pressure inthe presence of much larger volumes of tissue with normal oxygenpressures. In addition, tissue oxygen pressures can be monitoredin real time, even through centimeter thicknesses of tissue.

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