Technetium-99m-Labeled Fibroblast Activation Protein-Targeted Nanobody Radiotracer: from Preclinical Development to Clinical Translation in Cancer Imaging

IF 3.7 Q1 CHEMISTRY, MEDICINAL

ACS Pharmacology and Translational Science Pub Date : 2025-07-16 DOI:10.1021/acsptsci.5c00256

Chenzhen Li, Xinru Li, Yuchen Wang, Zhidong Bai, Yuanbo Wang, Rui Gao and Bing Jia*,

{"title":"Technetium-99m-Labeled Fibroblast Activation Protein-Targeted Nanobody Radiotracer: from Preclinical Development to Clinical Translation in Cancer Imaging","authors":"Chenzhen Li, Xinru Li, Yuchen Wang, Zhidong Bai, Yuanbo Wang, Rui Gao and Bing Jia*, ","doi":"10.1021/acsptsci.5c00256","DOIUrl":null,"url":null,"abstract":"Fibroblast activation protein (FAP) is a highly expressed marker in cancer-associated fibroblasts (CAFs) across various epithelial cancers, making it an attractive target for diagnostic imaging. To address the limitations of existing FAP-targeted radiopharmaceuticals, such as poor tumor retention and off-target uptake, this study aimed to establish a comprehensive FAP nanobody library. Through systematic screening, we sought to identify a nanobody with cross-reactivity to both human and murine FAP, optimized for technetium-99m (99mTc) labeling, and suitable for single-photon emission computed tomography (SPECT) imaging. A library of anti-FAP nanobodies (AFNs) was constructed and screened for binding affinity and specificity to human and murine FAP. Selected nanobodies were labeled with 99mTc using a site-specific radiolabeling process. In vitro assays were conducted to evaluate binding kinetics and cross-reactivity, while in vivo studies assessed pharmacokinetics, biodistribution, and imaging performance in murine tumor models. Finally, a first-in-human clinical study was performed to validate the safety and diagnostic efficacy of the lead nanobody-based radiotracer. From the nanobody library, three candidates were identified with high specificity for FAP: AFN01 (murine-specific), AFN05 (human-specific), and AFN13 (cross-reactive to both human and murine FAP). Among them, [99mTc]Tc-AFN13 demonstrated excellent binding affinity (dissociation constants: 2.16 ± 0.16 nM for murine FAP and 6.82 ± 0.54 nM for human FAP) and favorable pharmacokinetics. In vivo SPECT imaging revealed rapid tumor accumulation, prolonged retention, and minimal off-target uptake (e.g., tumor uptake of 4.41 ± 0.13% ID/cc at 30 min postinjection, declining to 2.35 ± 0.17% ID/cc at 12 h). Preliminary clinical imaging in patients confirmed the safety and specificity of [99mTc]Tc-AFN13 for FAP-expressing lesions, with no adverse events observed. In conclusion, this study successfully established a FAP nanobody library and identified [99mTc]Tc-AFN13 as a novel radiotracer with cross-reactivity to human and murine FAP. Its robust preclinical performance and promising clinical results highlight its potential for SPECT imaging in FAP-expressing cancers, paving the way for further clinical translation and theranostic applications.","PeriodicalId":36426,"journal":{"name":"ACS Pharmacology and Translational Science","volume":"8 8","pages":"2673–2682"},"PeriodicalIF":3.7000,"publicationDate":"2025-07-16","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"ACS Pharmacology and Translational Science","FirstCategoryId":"1085","ListUrlMain":"https://pubs.acs.org/doi/10.1021/acsptsci.5c00256","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"CHEMISTRY, MEDICINAL","Score":null,"Total":0}

引用次数: 0

Abstract

Fibroblast activation protein (FAP) is a highly expressed marker in cancer-associated fibroblasts (CAFs) across various epithelial cancers, making it an attractive target for diagnostic imaging. To address the limitations of existing FAP-targeted radiopharmaceuticals, such as poor tumor retention and off-target uptake, this study aimed to establish a comprehensive FAP nanobody library. Through systematic screening, we sought to identify a nanobody with cross-reactivity to both human and murine FAP, optimized for technetium-99m (^99mTc) labeling, and suitable for single-photon emission computed tomography (SPECT) imaging. A library of anti-FAP nanobodies (AFNs) was constructed and screened for binding affinity and specificity to human and murine FAP. Selected nanobodies were labeled with ^99mTc using a site-specific radiolabeling process. In vitro assays were conducted to evaluate binding kinetics and cross-reactivity, while in vivo studies assessed pharmacokinetics, biodistribution, and imaging performance in murine tumor models. Finally, a first-in-human clinical study was performed to validate the safety and diagnostic efficacy of the lead nanobody-based radiotracer. From the nanobody library, three candidates were identified with high specificity for FAP: AFN01 (murine-specific), AFN05 (human-specific), and AFN13 (cross-reactive to both human and murine FAP). Among them, [^99mTc]Tc-AFN13 demonstrated excellent binding affinity (dissociation constants: 2.16 ± 0.16 nM for murine FAP and 6.82 ± 0.54 nM for human FAP) and favorable pharmacokinetics. In vivo SPECT imaging revealed rapid tumor accumulation, prolonged retention, and minimal off-target uptake (e.g., tumor uptake of 4.41 ± 0.13% ID/cc at 30 min postinjection, declining to 2.35 ± 0.17% ID/cc at 12 h). Preliminary clinical imaging in patients confirmed the safety and specificity of [^99mTc]Tc-AFN13 for FAP-expressing lesions, with no adverse events observed. In conclusion, this study successfully established a FAP nanobody library and identified [^99mTc]Tc-AFN13 as a novel radiotracer with cross-reactivity to human and murine FAP. Its robust preclinical performance and promising clinical results highlight its potential for SPECT imaging in FAP-expressing cancers, paving the way for further clinical translation and theranostic applications.

Abstract Image

查看原文本刊更多论文

锝-99m标记的成纤维细胞活化蛋白靶向纳米体放射性示踪剂：从临床前开发到癌症成像的临床转化

成纤维细胞激活蛋白（FAP）是各种上皮癌中癌症相关成纤维细胞（CAFs）中高度表达的标志物，使其成为诊断成像的一个有吸引力的靶标。为了解决现有靶向FAP的放射性药物的局限性，如肿瘤保留率差和脱靶摄取，本研究旨在建立一个全面的FAP纳米体文库。通过系统筛选，我们试图鉴定出一种对人类和小鼠FAP具有交叉反应性的纳米体，该纳米体对锝-99m （99mTc）标记进行了优化，并适用于单光子发射计算机断层扫描（SPECT）成像。构建抗FAP纳米体（afn）文库，并对其与人和鼠FAP的结合亲和力和特异性进行筛选。选定的纳米体使用特定位点的放射性标记过程用99mTc标记。体外实验评估了结合动力学和交叉反应性，而体内研究评估了小鼠肿瘤模型的药代动力学、生物分布和成像性能。最后，进行了首次人体临床研究，以验证基于铅纳米体的放射性示踪剂的安全性和诊断有效性。从纳米体文库中，鉴定出三种候选FAP具有高特异性：AFN01（小鼠特异性），AFN05（人类特异性）和AFN13（对人和小鼠FAP均有交叉反应）。其中，[99mTc]Tc-AFN13具有良好的结合亲和力（解离常数：小鼠FAP为2.16±0.16 nM，人FAP为6.82±0.54 nM）和良好的药代动力学。体内SPECT成像显示肿瘤积聚迅速，滞留时间长，脱靶摄取最小（例如，注射后30分钟肿瘤摄取为4.41±0.13% ID/cc， 12小时降至2.35±0.17% ID/cc）。患者的初步临床影像学证实了[99mTc]Tc-AFN13对表达fap的病变的安全性和特异性，未观察到不良事件。综上所述，本研究成功建立了FAP纳米体文库，并鉴定出[99mTc]Tc-AFN13是一种新型的对人和鼠FAP具有交叉反应性的放射性示踪剂。其强大的临床前表现和有希望的临床结果突出了其在表达fap的癌症中SPECT成像的潜力，为进一步的临床转化和治疗应用铺平了道路。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

ACS Pharmacology and Translational Science Medicine-Pharmacology (medical)

CiteScore

10.00

自引率

3.30%

发文量

133

期刊介绍： ACS Pharmacology & Translational Science publishes high quality, innovative, and impactful research across the broad spectrum of biological sciences, covering basic and molecular sciences through to translational preclinical studies. Clinical studies that address novel mechanisms of action, and methodological papers that provide innovation, and advance translation, will also be considered. We give priority to studies that fully integrate basic pharmacological and/or biochemical findings into physiological processes that have translational potential in a broad range of biomedical disciplines. Therefore, studies that employ a complementary blend of in vitro and in vivo systems are of particular interest to the journal. Nonetheless, all innovative and impactful research that has an articulated translational relevance will be considered. ACS Pharmacology & Translational Science does not publish research on biological extracts that have unknown concentration or unknown chemical composition. Authors are encouraged to use the pre-submission inquiry mechanism to ensure relevance and appropriateness of research.