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单链抗体的细胞表面表达及其在体内基因表达成像中的应用。

Cell surface expression of single chain antibodies with applications to imaging of gene expression in vivo.

作者信息

Northrop Jeffrey P, Bednarski Mark, Barbieri Susan O, Lu Amy T, Nguyen Dee, Varadarajan John, Osen Maureen, Li King C, Star-Lack Josh

机构信息

Affymax Research Institute, Palo Alto, CA, USA.

出版信息

Eur J Nucl Med Mol Imaging. 2003 Sep;30(9):1292-8. doi: 10.1007/s00259-003-1237-7. Epub 2003 Jun 25.

DOI:10.1007/s00259-003-1237-7
PMID:12827313
Abstract

Imaging of gene expression in vivo has many potential uses for biomedical research and drug discovery, ranging from the study of gene regulation and cancer to the non-invasive assessment of gene therapies. To streamline the development of imaging marker gene technologies for nuclear medicine, we propose a new approach to the design of reporter/probe pairs wherein the reporter is a cell surface-expressed single chain antibody variable fragment that has been raised against a low molecular weight imaging probe with optimized pharmacokinetic properties. Proof of concept of the approach was achieved using a single chain antibody variable fragment that binds with high affinity to fluorescein and an imaging probe consisting of fluorescein isothiocyanate coupled to the chelator diethylene triamine penta-acetic acid labeled with the gamma-emitter (111)In. We demonstrate specific high-affinity binding of this probe to the cell surface-expressed reporter in vitro and assess the in vivo biodistribution of the probe both in wild-type mice and in mice harboring tumor xenografts expressing the reporter. Specific uptake of the probe by, and in vivo imaging of, tumors expressing the reporter are shown. Since ScFvs with high affinities can be raised to almost any protein or small molecule, the proposed methodology may offer a new flexibility in the design of imaging tracer/reporter pairs wherein both probe pharmacokinetics and binding affinities can be readily optimized.

摘要

体内基因表达成像在生物医学研究和药物发现方面有许多潜在用途,范围从基因调控和癌症研究到基因治疗的非侵入性评估。为了简化用于核医学的成像标记基因技术的开发,我们提出了一种设计报告基因/探针组对的新方法,其中报告基因是一种细胞表面表达的单链抗体可变片段,它是针对具有优化药代动力学特性的低分子量成像探针产生的。使用与荧光素具有高亲和力结合的单链抗体可变片段和由异硫氰酸荧光素与用γ发射体(111)铟标记的螯合剂二乙烯三胺五乙酸偶联而成的成像探针,实现了该方法的概念验证。我们在体外证明了该探针与细胞表面表达的报告基因的特异性高亲和力结合,并评估了该探针在野生型小鼠和携带表达报告基因的肿瘤异种移植物的小鼠体内的生物分布。展示了表达报告基因的肿瘤对探针的特异性摄取以及体内成像。由于可以针对几乎任何蛋白质或小分子产生具有高亲和力的单链抗体可变片段,因此所提出的方法可能在成像示踪剂/报告基因对的设计中提供新的灵活性,其中探针的药代动力学和结合亲和力都可以很容易地优化。

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