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The use of phage display to generate conformation-sensor recombinant antibodies

机译:使用噬菌体展示产生构象传感器重组抗体

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摘要

We describe a phage display approach that we have previously used to generate conformation-sensor antibodies that specifically recognize and stabilize the oxidized, inactive conformation of protein tyrosine phosphatase 1B (PTP1B). We use a solution-based panning and screening strategy conducted in the presence of reduced active PTP1B, which enriches antibodies to epitopes unique to the oxidized form while excluding antibodies that recognize epitopes common to oxidized and reduced forms of PTP1B. This strategy avoids conventional solid-phase immobilization owing to its inherent potential for denaturation of the antigen. In addition, a functional screening strategy selects single-chain variable fragments (scFvs) directly for their capacity for both specific binding and stabilization of the target enzyme in its inactive conformation. These conformation-specific scFvs illustrate that stabilization of oxidized PTP1B is an effective strategy to inhibit PTP1B function; it is possible that this approach may be applicable to the protein tyrosine phosphatase (PTP) family as a whole. With this protocol, isolation and characterization of specific scFvs from immune responsive animals should take ~6 weeks.
机译:我们描述了一种噬菌体展示方法,我们以前用来生成构象传感器抗体,可以特异性识别并稳定蛋白质酪氨酸磷酸酶1B(PTP1B)的氧化,无活性构象。我们使用在减少的活性PTP1B存在下进行的基于溶液的淘选和筛选策略,该方法可丰富针对氧化形式独特的表位的抗体,而排除识别PTP1B氧化和还原形式共有的表位的抗体。由于其固有的抗原变性潜力,该策略避免了常规的固相固定。另外,功能性筛选策略直接选择单链可变片段(scFv),因为它们具有特异性结合和稳定靶酶非活性构象的能力。这些构象特异性的scFvs表明,氧化的PTP1B的稳定化是抑制PTP1B功能的有效策略。整个方法可能适用于蛋白质酪氨酸磷酸酶(PTP)家族。通过此协议,从免疫反应动物中分离和鉴定特定scFv的过程大约需要6周。

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