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首页> 外文期刊>Molecular & cellular proteomics: MCP >Identification of clinically significant tumor antigens by selecting phage antibody library on tumor cells in situ using laser capture microdissection
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Identification of clinically significant tumor antigens by selecting phage antibody library on tumor cells in situ using laser capture microdissection

机译:通过使用激光捕获显微切割原位选择肿瘤细胞上的噬菌体抗体库来鉴定具有临床意义的肿瘤抗原

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Much work has been done to develop tumor-targeting antibodies by selecting a phage antibody library on cancer cell lines. However, when tumor cells are removed from their natural environment, they may undergo genetic and epigenetic changes yielding different surface antigens than those seen in actual cases of cancer. We developed a strategy that allows selection of phage antibodies against tumor cells in situ on both fresh frozen and paraffin-embedded tissues using laser capture microdissection. By restricting antibody selection to binders of internalizing epitopes, we generated a panel of phage antibodies that target clinically represented prostate cancer antigens. We identified AL-CAM/MEMD/CD166, a newly discovered prostate cancer marker, as the target for one of the selected antibodies, demonstrating the effectiveness of our approach. We further conjugated two single chain Fv fragments to liposomes and demonstrated that these nanotargeting devices were efficiently delivered to the interior of prostate cancer cells. The ability to deliver payload intracellularly and to recognize tumor cells in situ makes these antibodies attractive candidates for the development of targeted cancer therapeutics.
机译:通过选择癌细胞系上的噬菌体抗体库,已经做了很多工作来开发靶向肿瘤的抗体。但是,当肿瘤细胞从自然环境中移出时,它们可能会发生遗传和表观遗传学变化,从而产生与实际癌症病例不同的表面抗原。我们开发了一种策略,允许使用激光捕获显微切割技术在新鲜冷冻和石蜡包埋的组织上原位选择针对肿瘤细胞的噬菌体抗体。通过将抗体选择限制于内在表位的结合物,我们生成了针对临床代表前列腺癌抗原的噬菌体抗体。我们确定AL-CAM / MEMD / CD166(一种新发现的前列腺癌标志物)为所选抗体之一的靶标,证明了我们方法的有效性。我们进一步将两个单链Fv片段缀合到脂质体上,并证明这些纳米靶向装置已有效地传递到前列腺癌细胞的内部。在细胞内递送有效载荷并原位识别肿瘤细胞的能力使这些抗体成为开发靶向癌症治疗剂的有吸引力的候选物。

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