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使用新型酶传感可激活大分子光学探针进行淋巴结的近红外荧光成像。

Near-infrared fluorescence imaging of lymph nodes using a new enzyme sensing activatable macromolecular optical probe.

作者信息

Wunderbaldinger Patrick, Turetschek Karl, Bremer Christoph

机构信息

Department of Radiology, University of Vienna, Waehringer Guertel 18-20, 1090 Vienna, Austria.

出版信息

Eur Radiol. 2003 Sep;13(9):2206-11. doi: 10.1007/s00330-003-1932-6. Epub 2003 Jun 12.

Abstract

The aim of this study was to validate the use of near infrared fluorescence imaging (NIRF) using enzyme-sensitive optical probes for lymph node detection. An optical contrast probe that is activated by cystein proteases, such as cathepsin B, was used to visualize lymph nodes by NIRF reflectance imaging. In order to quantitate the uptake of the optical probe in lymphatic tissue, the biodistribution was assessed using the Indium-111 labeled optical probe. Sixteen Balb-c mice were injected either intravenously (i.v.) or subcutaneously (s.c.) with the NIRF-probe (2 micromol cyanine (Cy)/animal; i.v., n=10; s.c., n=6) and imaged 24 h after injection. Signal intensities and target-to-background ratios of various lymph nodes were measured by manual regions of interest (ROIs). Additional signal intensity measurements were performed of excised lymph nodes (n=21) from i.v. injected mice (24 h after injection) and compared with excised lymph nodes (n=8) of non-injected mice. The probe employed in this study was lymphotropic with approximately 3-4% accumulation in lymph nodes (3.4+/-0.8% ID/g). Measurements of the excised lymph nodes (after i.v. injection) confirmed a significant increase in lymph node fluorescence signal from baseline 26+/-7.6 arbitary units (AU) to 146+/-10.9 AU (p<0.0001). A significant increase in lymph node fluorescence signal was also seen in vivo throughout the body after i.v. injection (96+/-7.8 AU) and/or regionally after s.c. injection (141+/-11.5 AU) in comparison with baseline autofluorescence (26+/-7.6 AU). Target-to-background ratio was significantly higher after s.c. injection (6.6%+/-0.81) compared with i.v. injection (4.8+/-0.67%). Detection and visualization of lymph nodes is feasible by NIRF imaging using a cystein-protease sensitive optical probe.

摘要

本研究的目的是验证使用对酶敏感的光学探针的近红外荧光成像(NIRF)用于淋巴结检测的效果。一种由半胱氨酸蛋白酶(如组织蛋白酶B)激活的光学造影探针,被用于通过NIRF反射成像来可视化淋巴结。为了定量光学探针在淋巴组织中的摄取,使用铟-111标记的光学探针评估生物分布。16只Balb-c小鼠通过静脉内(i.v.)或皮下(s.c.)注射NIRF探针(2微摩尔花菁(Cy)/动物;静脉注射,n = 10;皮下注射,n = 6),并在注射后24小时进行成像。通过手动感兴趣区域(ROIs)测量各种淋巴结的信号强度和靶本比。对静脉注射小鼠(注射后24小时)切除的淋巴结(n = 21)进行了额外的信号强度测量,并与未注射小鼠切除的淋巴结(n = 8)进行比较。本研究中使用的探针具有亲淋巴性,在淋巴结中的蓄积率约为3 - 4%(3.4±0.8% ID/g)。对切除的淋巴结(静脉注射后)的测量证实,淋巴结荧光信号从基线的26±7.6任意单位(AU)显著增加到146±10.9 AU(p < 0.0001)。与基线自发荧光(26±7.6 AU)相比,静脉注射后全身(96±7.8 AU)和/或皮下注射后局部(141±11.5 AU)的淋巴结荧光信号也有显著增加。皮下注射后的靶本比(6.6%±0.81)显著高于静脉注射(4.8±0.67%)。使用对半胱氨酸蛋白酶敏感的光学探针通过NIRF成像检测和可视化淋巴结是可行的。

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