首页
内分泌科 神经内科 心血管内科 消化内科 风湿免疫科 血液科 肾内科 呼吸内科 神经外科 心脏外科 胸部外科 普通外科 肝胆外科 烧伤外科 整形外科 泌尿外科 妇产科 儿科 皮肤性病科 感染科 眼科 急诊科 精神科 口腔科 肿瘤科 骨科 耳鼻咽喉头颈外科
疾病 检查 药品 操作 文献 专题 路径 法规 量表

您的账号已在其他设备登录,您当前账号已强迫下线,
如非您本人操作,建议您在会员中心进行密码修改

确定
首页 > mAbs > Improved decision making for prioritizing tumor targeting antibodies in human xenograf...
Improved decision making for prioritizing tumor targeting antibodies in human xenografts: utility of fluorescence imaging to verify tumor target expression, antibody binding and optimization of dosage and application schedule.
LinkOut
收藏 | 浏览31

Preclinical efficacy studies of antibodies targeting a tumor-associated antigen are only justified when the expression of the relevant antigen has been demonstrated. Conventionally, antigen expression level is examined by immunohistochemistry of formalin-fixed paraffin-embedded tumor tissue section. This method represents the diagnostic "gold standard" for tumor target evaluation, but is affected by a number of factors, such as epitope masking and insufficient antigen retrieval. As a consequence, variances and discrepancies in histological staining results can occur, which may influence decision-making and therapeutic outcome. To overcome these problems, we have used different fluorescence-labeled therapeutic antibodies targeting human epidermal growth factor receptor (HER) family members and insulin-like growth factor-1 receptor (IGF1R) in combination with fluorescence imaging modalities to determine tumor antigen expression, drug-target interaction, and biodistribution and tumor saturation kinetics in non-small cell lung cancer xenografts. For this, whole-body fluorescence intensities of labeled antibodies, applied as a single compound or antibody mixture, were measured in Calu-1 and Calu-3 tumor-bearing mice, then ex vivo multispectral tumor tissue analysis at microscopic resolution was performed. With the aid of this simple and fast imaging method, we were able to analyze the tumor cell receptor status of HER1-3 and IGF1R, monitor the antibody-target interaction and evaluate the receptor binding sites of anti-HER2-targeting antibodies. Based on this, the most suitable tumor model, best therapeutic antibody, and optimal treatment dosage and application schedule was selected. Predictions drawn from obtained imaging data were in excellent concordance with outcome of conducted preclinical efficacy studies. Our results clearly demonstrate the great potential of combined in vivo and ex vivo fluorescence imaging for the preclinical development and characterization of monoclonal antibodies.

作者:Michael, Dobosz;Ute, Haupt;Werner, Scheuer

来源:mAbs 2016 年

循证诊断 循证预后
知识库介绍

临床诊疗知识库该平台旨在解决临床医护人员在学习、工作中对医学信息的需求,方便快速、便捷的获取实用的医学信息,辅助临床决策参考。该库包含疾病、药品、检查、指南规范、病例文献及循证文献等多种丰富权威的临床资源。

详细介绍
热门关注
免责声明:本知识库提供的有关内容等信息仅供学习参考,不代替医生的诊断和医嘱。

Improved decision making for prioritizing tumor targeting antibodies in human xenografts: utility of fluorescence imaging to verify tumor target expression, antibody binding and optimization of dosage and application schedule.
收藏
| 浏览:31
作者:
Michael, Dobosz;Ute, Haupt;Werner, Scheuer
来源:
mAbs 2016 年
标签:
Antibody development Antigen expression Cancer Immunohistochemistry In vivo histology Multispectral fluorescence imaging Optical Imaging Tumor-target evaluation
Preclinical efficacy studies of antibodies targeting a tumor-associated antigen are only justified when the expression of the relevant antigen has been demonstrated. Conventionally, antigen expression level is examined by immunohistochemistry of formalin-fixed paraffin-embedded tumor tissue section. This method represents the diagnostic "gold standard" for tumor target evaluation, but is affected by a number of factors, such as epitope masking and insufficient antigen retrieval. As a consequence, variances and discrepancies in histological staining results can occur, which may influence decision-making and therapeutic outcome. To overcome these problems, we have used different fluorescence-labeled therapeutic antibodies targeting human epidermal growth factor receptor (HER) family members and insulin-like growth factor-1 receptor (IGF1R) in combination with fluorescence imaging modalities to determine tumor antigen expression, drug-target interaction, and biodistribution and tumor saturation kinetics in non-small cell lung cancer xenografts. For this, whole-body fluorescence intensities of labeled antibodies, applied as a single compound or antibody mixture, were measured in Calu-1 and Calu-3 tumor-bearing mice, then ex vivo multispectral tumor tissue analysis at microscopic resolution was performed. With the aid of this simple and fast imaging method, we were able to analyze the tumor cell receptor status of HER1-3 and IGF1R, monitor the antibody-target interaction and evaluate the receptor binding sites of anti-HER2-targeting antibodies. Based on this, the most suitable tumor model, best therapeutic antibody, and optimal treatment dosage and application schedule was selected. Predictions drawn from obtained imaging data were in excellent concordance with outcome of conducted preclinical efficacy studies. Our results clearly demonstrate the great potential of combined in vivo and ex vivo fluorescence imaging for the preclinical development and characterization of monoclonal antibodies.

关于我们 产品特色 专家团队

免责声明:本知识库提供的有关疾病、症状、检查、药品、指南规范、循证文献和病例文献等信息仅供医生学习参考。

2015 北京万方数据股份有限公司 互联网药品信息服务资格证书号:(京)-经营性-2011-0017 京ICP证010071号