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树状聚合物-肽-核酸缀合物的制备及体外扩增前靶向评价的研究。

Research on preparation and in vitro evaluation of the dendrimer-peptide nuclear acid conjugate for amplification pretargeting.

机构信息

Radiopharmaceuticals Center, Shanghai Institute of Applied Physics, Chinese Academy of Sciences, Shanghai, China.

Shanghai Institute of Applied Physics, University of Chinese Academy of Sciences, Beijing, China.

出版信息

J Labelled Comp Radiopharm. 2021 Sep;64(11):428-439. doi: 10.1002/jlcr.3937. Epub 2021 Aug 10.

DOI:10.1002/jlcr.3937
PMID:34330148
Abstract

Amplification pretargeting has the potential to increase the tracer's accumulation in the tumor. This study aimed to develop a three-step amplification pretargeting strategy in nuclear medicine with a polymer conjugated with multiple copies of peptide nuclear acid (PNA). In this study, the tracer F-labeled complementary PNA ( F-cPNA) was prepared by click-chemistry with high radiochemical purity (>99%) and great stability in vitro. The PAMMA dendrimer generation 4 (G4) was conjugated with multiple copies of PNAs. The average number of PNA groups in the G4-PNA conjugate was determined by matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) and the accessibility to the F-cPNA was identified by size-exclusion high-performance liquid chromatography (SE-HPLC). There were approximately 11.7 of 64 carboxyl groups modified with PNAs, of which more than 99% were accessible to F-cPNA. F-cPNA was added to a mixture of CC49-cPNA and G4-PNA, and the complex exhibited a single peak on high-performance liquid chromatography (HPLC) as evidence of complete hybridization between F-cPNA and CC49-cPNA/G4-PNA. The LS174T tumor cells were incubated with CC49-cPNA followed by G4-PNA as an amplification platform before F-cPNA was added to hybridize with CC49-cPNA/G4-PNA. Compared with conventional pretargeting without G4-PNA, the radioactivity signal was amplified about four times, which demonstrated that the dendrimer-PNA conjugate plays a crucial role in signal amplification.

摘要

扩增前靶向具有增加示踪剂在肿瘤中积累的潜力。本研究旨在开发一种三步扩增前靶向策略,在核医学中使用与多个肽核酸(PNA)拷贝结合的聚合物。在这项研究中,通过点击化学制备了放射性核素 F 标记的互补 PNA( F-cPNA),具有>99%的高放射化学纯度和体外稳定性。将多拷贝 PNA 与 PAMMA 树状聚合物第 4 代(G4)连接。通过基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)确定 G4-PNA 缀合物中的 PNA 基团的平均数量,通过尺寸排阻高效液相色谱(SE-HPLC)鉴定 F-cPNA 的可及性。大约有 11.7 个 64 个羧基被 PNA 修饰,其中超过 99%的 PNA 是可及的 F-cPNA。将 F-cPNA 加入 CC49-cPNA 和 G4-PNA 的混合物中,高效液相色谱(HPLC)显示复合物呈现单个峰,证明 F-cPNA 与 CC49-cPNA/G4-PNA 完全杂交。LS174T 肿瘤细胞先用 CC49-cPNA 孵育,然后用 G4-PNA 作为扩增平台,然后加入 F-cPNA 与 CC49-cPNA/G4-PNA 杂交。与没有 G4-PNA 的常规前靶向相比,放射性信号放大了约四倍,这表明树枝状聚合物-PNA 缀合物在信号放大中起着关键作用。

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