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Real-time analysis of the binding of fluorescent VEGF₁₆₅a to VEGFR2 in living cells: Effect of receptor tyrosine kinase inhibitors and fate of internalized agonist-receptor complexes

机译:实时分析活细胞中荧光VEGF₁₆₅a与VEGFR2的结合:受体酪氨酸激酶抑制剂的作用和内在激动剂-受体复合物的命运

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摘要

Vascular endothelial growth factor (VEGF) is an important mediator of angiogenesis. Here we have used a novel stoichiometric protein-labeling method to generate a fluorescent variant of VEGF (VEGF₁₆₅a-TMR) labeled on a single cysteine within each protomer of the antiparallel VEGF homodimer. VEGF₁₆₅a-TMR has then been used in conjunction with full length VEGFR2, tagged with the bioluminescent protein NanoLuc, to undertake a real time quantitative evaluation of VEGFR2 binding characteristics in living cells using bioluminescence resonance energy transfer (BRET). This provided quantitative information on VEGF-VEGFR2 interactions. At longer incubation times, VEGFR2 is internalized by VEGF₁₆₅a-TMR into intracellular endosomes. This internalization can be prevented by the receptor tyrosine kinase inhibitors (RTKIs) cediranib, sorafenib, pazopanib or vandetanib. In the absence of RTKIs, the BRET signal is decreased over time as a consequence of the dissociation of agonist from the receptor in intracellular endosomes and recycling of VEGFR2 back to the plasma membrane.
机译:血管内皮生长因子(VEGF)是血管生成的重要介质。在这里,我们使用了一种新型的化学计量蛋白质标记方法来生成在反平行VEGF同型二聚体的每个前体内单个半胱氨酸上标记的VEGF荧光变体(VEGF₁₆₅a-TMR)。然后,VEGF₁₆₅a-TMR已与标记有生物发光蛋白NanoLuc的全长VEGFR2结合使用,利用生物发光共振能量转移(BRET)进行了活细胞中VEGFR2结合特性的实时定量评估。这提供了关于VEGF-VEGFR2相互作用的定量信息。在更长的孵育时间中,VEGFRa-TMR将VEGFR2内化为细胞内内体。受体酪氨酸激酶抑制剂(RTKIs)西地尼布,索拉非尼,帕唑帕尼或vandetanib可防止这种内在化。在不存在RTKI的情况下,由于激动剂从胞内内体中的受体解离并且VEGFR2循环回到质膜,BRET信号随时间降低。

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