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首页> 外文期刊>Hybridoma >Accurate determination of internalization for target binding antibody using papain digestion and flow cytometry.
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Accurate determination of internalization for target binding antibody using papain digestion and flow cytometry.

机译:使用木瓜蛋白酶消化和流式细胞仪准确测定目标结合抗体的内在化。

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Internalization of monoclonal antibodies (MAbs) binding to the targeted cells has drawn great attention to both scientists and anti-cancer drug developmental professionals. Internalization of conjugated MAb is thought to be one of the major mechanisms for tumor cell destruction, and can be studied using several biochemical and microscopic approaches. Here we report a new method based on papain digestion followed by flow cytometry (FCM). This method can identify whether the binding MAb has internalized into the cell, with an additional advantage of accurately quantifying the internalized MAb without altering cell morphology after papain digestion. With this method, we studied the internalization degrees of 3A4 (a mouse anti-human CD45RA MAb) at different time points: 5.3% (15 min), 7.3% (30 min), 36.9% (60 min), 69.2% (120 min), and 72.6% (180 min). This methodology can facilitate our understanding of the efficiency of MAb internalization and allows us to evaluate the targeted killing capacity of the MAb. Our technique can serve as a reference model for future targeted drug development using MAbs. In summary, we established a simple and useful evaluation tool for MAb drug development and research.
机译:与靶细胞结合的单克隆抗体(MAb)的内在化引起了科学家和抗癌药物开发专业人员的极大关注。结合的MAb的内化被认为是破坏肿瘤细胞的主要机制之一,并且可以使用几种生化和显微镜方法进行研究。在这里,我们报告了一种基于木瓜蛋白酶消化然后流式细胞仪(FCM)的新方法。该方法可以识别结合的MAb是否已被内化到细胞中,并具有准确定量内化的MAb而又不改变木瓜蛋白酶消化后细胞形态的额外优势。通过这种方法,我们研究了3A4(小鼠抗人CD45RA MAb)在不同时间点的内在化程度:5.3%(15分钟),7.3%(30分钟),36.9%(60分钟),69.2%(120)分钟)和72.6%(180分钟)。这种方法可以促进我们对单克隆抗体内在化效率的理解,并使我们能够评估靶向单克隆抗体的杀伤能力。我们的技术可以用作将来使用MAb靶向药物开发的参考模型。总之,我们为单克隆抗体药物的开发和研究建立了一个简单而有用的评估工具。

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