111In-BnDTPA-F3:一种靶向核仁素的发射俄歇电子的放射性治疗药物。
111In-BnDTPA-F3: an Auger electron-emitting radiotherapeutic agent that targets nucleolin.
机构信息
Department of Oncology, Cancer Research UK/Medical Research Council Gray Institute for Radiation Oncology and Biology, University of Oxford, Old Road Campus Research Building, Off Roosevelt Drive, Oxford, OX3 7DQ, UK.
出版信息
EJNMMI Res. 2012 Feb 20;2:9. doi: 10.1186/2191-219X-2-9.
INTRODUCTION
The F3 peptide (KDEPQRRSARLSAKPAPPKPEPKPKKAPAKK), a fragment of the human high mobility group protein 2, binds nucleolin. Nucleolin is expressed in the nuclei of normal cells but is also expressed on the membrane of some cancer cells. The goal was to investigate the use of 111In-labeled F3 peptide for Auger electron-targeted radiotherapy.
METHODS
F3 was labeled with fluorescein isothiocyanate (FITC) for confocal microscopy and conjugated to p-SCN-benzyl-diethylenetriaminepentaacetic acid (BnDTPA) for labeling with 111In to form 111In-BnDTPA-F3. MDA-MB-231-H2N (231-H2N) human breast cancer cells were exposed to 111In-BnDTPA-F3 and used in cell fractionation, γH2AX immunostaining (a marker of DNA double-strand breaks), and clonogenic assays. In vivo, biodistribution studies of 111In-BnDTPA-F3 were performed in 231-H2N xenograft-bearing mice. In tumor growth delay studies, 111In-BnDTPA-F3 (3 μg, 6 MBq/μg) was administered intravenously to 231-H2N xenograft-bearing mice once weekly for 3 weeks.
RESULTS
Membrane-binding of FITC-F3 was observed in 231-H2N cells, and there was co-localization of FITC-F3 with nucleolin in the nuclei. After exposure of 231-H2N cells to 111In-BnDTPA-F3 for 2 h, 1.7% of 111In added to the medium was membrane-bound. Of the bound 111In, 15% was internalized, and of this, 37% was localized in the nucleus. Exposure of 231-H2N cells to 111In-BnDTPA-F3 (1 μM, 6 MBq/μg) resulted in a dose-dependent increase in γH2AX foci and in a significant reduction of clonogenic survival compared to untreated cells or cells exposed to unlabeled BnDTPA-F3 (46 ± 4.1%, 100 ± 1.8%, and 132 ± 7.7%, respectively). In vivo, tumor uptake of 111In-BnDTPA-F3 (3 μg, 6 MBq/μg) at 3-h post-injection was 1% of the injected dose per gram (%ID/g), and muscle uptake was 0.5%ID/g. In tumor growth delay studies, tumor growth rate was reduced 19-fold compared to untreated or unlabeled BnDTPA-F3-treated mice (p = 0.023).
CONCLUSION
111In-BnDTPA-F3 is internalized into 231-H2N cells and translocates to the nucleus. 111In-BnDTPA-F3 has a potent cytotoxic effect in vitro and an anti-tumor effect in mice bearing 231-H2N xenografts despite modest total tumor accumulation.
简介
F3 肽(KDEPQRRSARLSAKPAPPKPEPKPKKAPAKK)是人类高迁移率族蛋白 2 的一个片段,与核仁蛋白结合。核仁蛋白在正常细胞的核内表达,但也在一些癌细胞的膜上表达。目的是研究 111In 标记的 F3 肽用于 Auger 电子靶向放射治疗。
方法
F3 用异硫氰酸荧光素(FITC)标记用于共聚焦显微镜,与 p-SCN-苄基-二乙三胺五乙酸(BnDTPA)缀合用于用 111In 标记形成 111In-BnDTPA-F3。MDA-MB-231-H2N(231-H2N)人乳腺癌细胞暴露于 111In-BnDTPA-F3 中,并用于细胞分馏、γH2AX 免疫染色(DNA 双链断裂的标志物)和集落形成测定。在体内,231-H2N 荷瘤小鼠进行了 111In-BnDTPA-F3 的生物分布研究。在肿瘤生长延迟研究中,231-H2N 荷瘤小鼠每周静脉注射 111In-BnDTPA-F3(3μg,6MBq/μg)一次,共 3 周。
结果
在 231-H2N 细胞中观察到 FITC-F3 的膜结合,并且在核内 FITC-F3 与核仁蛋白存在共定位。231-H2N 细胞暴露于 111In-BnDTPA-F3 2 小时后,加入培养基的 111In 的 1.7%与膜结合。结合的 111In 中有 15%被内化,其中 37%定位于核内。与未经处理的细胞或暴露于未标记的 BnDTPA-F3(分别为 46±4.1%、100±1.8%和 132±7.7%)相比,231-H2N 细胞暴露于 111In-BnDTPA-F3(1μM,6MBq/μg)导致 γH2AX 焦点的剂量依赖性增加,并导致集落形成存活显著降低。在体内,3 小时后注射 111In-BnDTPA-F3(3μg,6MBq/μg)的肿瘤摄取为每克注入剂量的 1%(%ID/g),肌肉摄取为 0.5%ID/g。在肿瘤生长延迟研究中,与未经处理或未标记的 BnDTPA-F3 治疗的小鼠相比,肿瘤生长速度降低了 19 倍(p=0.023)。
结论
111In-BnDTPA-F3 被内化到 231-H2N 细胞中并转移到细胞核中。111In-BnDTPA-F3 在体外具有很强的细胞毒性作用,在 231-H2N 异种移植小鼠中具有抗肿瘤作用,尽管总肿瘤积累适中。
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