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通过 MRI 采用亲和素/生物素放大途径进行靶标可视化:生物素-Gd-DOTA 单酰胺三聚体的合成与测试。

Target visualization by MRI using the avidin/biotin amplification route: synthesis and testing of a biotin-Gd-DOTA monoamide trimer.

机构信息

Dipartimento di Scienze dell'Ambiente e della Vita, Università del Piemonte Orientale Amedeo Avogadro, Viale T. Michel 11, 15121 Alessandria, Italy.

出版信息

Chemistry. 2010 Jul 19;16(27):8080-7. doi: 10.1002/chem.201000508.

DOI:10.1002/chem.201000508
PMID:20533461
Abstract

To design efficient targeting strategies in magnetic resonance (MR) molecular imaging applications, the formation of supramolecular adducts between (strept)avidin ((S)Av) and tribiotinylated Gd-DOTA-monoamide complexes (DOTA=1,4,7,10-tetraazacyclododecane-N,N',N'',N'''-tetraacetic acid) was explored. Two compounds based on the trivalent core of tris(2-aminoethyl)amine each containing three biotin molecules and one (L1) or three (L2) DOTA-monoamide (DOTAMA) ligands were synthesized. In these tribiotinylated derivatives the biotins are spaced far enough apart to allow the formation of the supramolecular adduct with the protein and to host the chelating units in between the (S)Av layers. Size exclusion HPLC analyses indicated complete formation of very high molecular weight polymers (>2 MDa) with (S)Av in solution. A (1)H NMR spectroscopy relaxometric study on the obtained polymeric adducts showed a marked increase of the relaxivity at 35-40 MHz as a consequence of the lengthening of the tumbling time due to the formation of Gd-chelates/(S)Av polymers. The most efficient Gd(3)L2/(S)Av polymeric system was used for a test in cell cultures. The target is represented by a neural cell adhesion molecule (NCAM), which is overexpressed in Kaposi's sarcoma cells and tumor endothelial cells (TEC) and that is efficiently recognized by a biotinylated tetrameric peptide (C3d-Bio). In vitro experiments showed that only cells incubated with both C3d-Bio and Gd(3)L2/SAv polymer were hyperintense with respect to the control. Relaxation rates of cell pellets incubated with Gd(3)L2/SAv alone were not significantly different from the untreated cells demonstrating the absence of a specific binding.

摘要

为了在磁共振(MR)分子成像应用中设计高效的靶向策略,探索了(链)亲和素((S)Av)和三生物素化 Gd-DOTA-单酰胺配合物(DOTA=1,4,7,10-四氮杂环十二烷-N,N',N'',N'''-四乙酸)之间形成超分子加合物的情况。合成了两种基于三(2-氨基乙基)胺三价核的化合物,每个化合物都含有三个生物素分子和一个(L1)或三个(L2)DOTA-单酰胺(DOTAMA)配体。在这些三生物素化衍生物中,生物素之间的间隔足够远,允许与蛋白质形成超分子加合物,并在(S)Av 层之间容纳螯合单元。尺寸排阻 HPLC 分析表明,在溶液中与(S)Av 完全形成非常高分子量聚合物(>2 MDa)。对获得的聚合物加合物进行(1)H NMR 光谱弛豫研究表明,由于形成 Gd-配合物/(S)Av 聚合物导致旋转时间延长,弛豫率在 35-40 MHz 处显著增加。Gd(3)L2/(S)Av 聚合物体系最有效,用于细胞培养中的测试。靶标是神经细胞粘附分子(NCAM),其在卡波西肉瘤细胞和肿瘤内皮细胞(TEC)中过度表达,并且被生物素化四聚肽(C3d-Bio)有效地识别。体外实验表明,只有与 C3d-Bio 和 Gd(3)L2/SAv 聚合物孵育的细胞相对于对照显示出超强度。单独用 Gd(3)L2/SAv 孵育的细胞沉淀的弛豫率与未处理的细胞没有显著差异,证明不存在特异性结合。

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