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Time-domain imaging with quench-based fluorescent contrast agents

机译：基于猝灭的荧光造影剂的时域成像

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Quench-based probes utilize unique characteristics of fluorescence resonance energy transfer (FRET) to enhance contrast upon de-quenching. This mechanism has been used in a variety of molecular probes for imaging of cancer related enzyme activity such as matrix metalloproteinases, cathepsins and caspases. While non-fluorescent upon administration, fluorescence can be restored by separation of donor and acceptor, resulting in higher intensity in the presence of activator. Along with decreased quantum yield, FRET also results in altered fluorescence lifetime. Time-domain imaging can further enhance contrast and information yield from quench-based probes. We present in vivo time-domain imaging for detecting activation of quench-based probes. Quench-based probes utilize unique characteristics of fluorescence resonance energy transfer (FRET) to enhance contrast upon de-quenching. This mechanism has been used in a variety of molecular probes for imaging of cancer related enzyme activity such as matrix metalloproteinases, cathepsins and caspases. While non-fluorescent upon administration, fluorescence can be restored by separation of donor and acceptor, resulting in higher intensity in the presence of activator. Along with decreased quantum yield, FRET also results in altered fluorescence lifetime. Time-domain imaging can further enhance contrast and information yield from quench-based probes. We present in vivo time-domain imaging for detecting activation of quench-based probes. Time-domain diffuse optical imaging was performed to assess the FRET and quenching in living mice with orthotopic breast cancer. Tumor contrast enhancement was accompanied by increased fluorescence lifetime after administration of quenched probes selective for matrix metalloproteinases while no significant change was observed for non-quenched probes for integrin receptors. These results demonstrate the utility of time-domain imaging for detection of cancer-related enzyme activity in vivo.

机译：基于淬灭的探针利用荧光共振能量转移（FRET）的独特特性来增强去淬灭时的对比度。该机制已用于多种分子探针中，用于成像与癌症相关的酶活性，例如基质金属蛋白酶，组织蛋白酶和胱天蛋白酶。虽然在给药时不发荧光，但可以通过分离供体和受体来恢复荧光，从而在活化剂存在下产生更高的强度。随着量子产率的降低，FRET也导致荧光寿命的改变。时域成像可以进一步增强基于淬灭探针的对比度和信息产量。我们目前体内时域成像，用于检测基于淬灭的探针的激活。基于淬灭的探针利用荧光共振能量转移（FRET）的独特特性来增强去淬灭时的对比度。该机制已用于多种分子探针中，用于成像与癌症相关的酶活性，例如基质金属蛋白酶，组织蛋白酶和胱天蛋白酶。虽然在给药时不发荧光，但可以通过分离供体和受体来恢复荧光，从而在活化剂存在下产生更高的强度。随着量子产率的降低，FRET也导致荧光寿命的改变。时域成像可以进一步增强基于淬灭探针的对比度和信息产量。我们目前体内时域成像，用于检测基于淬灭的探针的激活。进行时域漫射光学成像以评估原位乳腺癌活小鼠的FRET和猝灭。施用对基质金属蛋白酶有选择性的淬灭探针后，肿瘤对比增强伴随着荧光寿命的增加，而对于整合素受体的非猝灭探针，未观察到显着变化。这些结果证明了时域成像在体内检测癌症相关酶活性的实用性。

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《Reporters, markers, dyes, nanoparticles, and molecular probes for biomedical applications IV 》|2012年|p.82330G.1-82330G.7|共7页
会议地点 San Francisco CA(US)
作者
Walter J. Akers; Metasebya Solomon; Gail P. Sudlow; Mikhail Berezin; Samuel Achilefu;
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Optical Radiology Laboratory, Departments of Radiology Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110, 4525 Scott Avenue, St. Louis, MO 63108 (USA);

Optical Radiology Laboratory, Departments of Radiology Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110,Biomedical Engineering Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110;

Optical Radiology Laboratory, Departments of Radiology Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110;

Optical Radiology Laboratory, Departments of Radiology Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110;

Optical Radiology Laboratory, Departments of Radiology Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110,Biomedical Engineering Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110,Biochemistry Molecular Biophysics Washington University School of Medicine, 4525 Scott Avenue, St. Louis, MO 63110;

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正文语种 eng
中图分类医用物理学 ;
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Time-domain imaging with quench-based fluorescent contrast agents

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