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小鼠胚胎中靶向VEGFR2的分子成像:肿瘤模型的替代方法。

VEGFR2-targeted molecular imaging in the mouse embryo: an alternative to the tumor model.

作者信息

Denbeigh Janet M, Nixon Brian A, Hudson John M, Puri Mira C, Foster F Stuart

机构信息

Sunnybrook Research Institute, Department of Medical Biophysics, University of Toronto, Toronto, Ontario, Canada.

Sunnybrook Research Institute, Department of Medical Biophysics, University of Toronto, Toronto, Ontario, Canada.

出版信息

Ultrasound Med Biol. 2014 Feb;40(2):389-99. doi: 10.1016/j.ultrasmedbio.2013.09.022. Epub 2013 Dec 15.

DOI:10.1016/j.ultrasmedbio.2013.09.022
PMID:24342913
Abstract

As a tumor surrogate, the mouse embryo presents as an excellent alternative for examining the binding of angiogenesis-targeting microbubbles and assessing the quantitative nature of molecular ultrasound. We establish the validity of this model by developing a robust method to study microbubble kinetic behavior and investigate the reproducibility of targeted binding in the murine embryo. Vascular endothelial growth factor receptor 2 (VEGFR2)-targeted (MBV), rat immunoglobulin G2 (IgG2) control antibody-targeted (MBC) and untargeted (MBU) microbubbles were introduced into vasculature of living mouse embryos. Non-linear contrast-specific and B-mode ultrasound imaging, performed at 21 MHz with a Vevo-2100 scanner, was used to collect basic perfusion parameters and contrast mean power ratios for all bubble types. We observed a twofold increase (p < 0.001) in contrast mean power ratios for MBV (4.14 ± 1.78) compared with those for MBC (1.95 ± 0.78) and MBU (1.79 ± 0.45). Targeted imaging of endogenous endothelial cell surface markers in mouse embryos is possible with labeled microbubbles. The mouse embryo thus presents as a versatile model for testing the performance of ultrasound molecular targeting, where further development of quantitative imaging techniques may enable rapid evaluations of biomarker expression in studies of vascular development, disease and angiogenesis.

摘要

作为肿瘤替代物,小鼠胚胎是检测血管生成靶向微泡结合以及评估分子超声定量特性的绝佳选择。我们通过开发一种强大的方法来研究微泡动力学行为,并研究小鼠胚胎中靶向结合的可重复性,从而确立了该模型的有效性。将血管内皮生长因子受体2(VEGFR2)靶向微泡(MBV)、大鼠免疫球蛋白G2(IgG2)对照抗体靶向微泡(MBC)和非靶向微泡(MBU)引入活小鼠胚胎的脉管系统。使用Vevo - 2100扫描仪在21 MHz频率下进行非线性对比特异性和B模式超声成像,以收集所有气泡类型的基本灌注参数和对比平均功率比。我们观察到,与MBC(1.95±0.78)和MBU(1.79±0.45)相比,MBV的对比平均功率比增加了两倍(p < 0.001)(4.14±1.78)。使用标记的微泡可以对小鼠胚胎中的内源性内皮细胞表面标志物进行靶向成像。因此,小鼠胚胎是测试超声分子靶向性能的通用模型,在血管发育、疾病和血管生成研究中,定量成像技术的进一步发展可能有助于快速评估生物标志物的表达。

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