Engineered FHA domains can bind to a variety of Phosphothreonine-containing peptides

Srinivas S Thota, Grace L Allen, Ashley K Grahn, Brian K Kay
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Abstract

Antibodies play a crucial role in monitoring post-translational modifications, like phosphorylation, which regulates protein activity and location; however, commercial polyclonal and monoclonal antibodies have limitations in renewability and engineering compared to recombinant affinity reagents. A scaffold based on the Forkhead-associated domain (FHA) has potential as a selective affinity reagent for this post-translational modification. Engineered FHA domains, termed phosphothreonine-binding domains (pTBDs), with limited cross-reactivity were isolated from an M13 bacteriophage display library by affinity selection with phosphopeptides corresponding to human mTOR, Chk2, 53BP1, and Akt1 proteins. To determine the specificity of the representative pTBDs, we focused on binders to the pT543 phosphopeptide (536-IDEDGENpTQIEDTEP-551) of the DNA repair protein 53BP1. ELISA and western blot experiments have demonstrated the pTBDs are specific to phosphothreonine, demonstrating the potential utility of pTBDs for monitoring the phosphorylation of specific threonine residues in clinically relevant human proteins.
设计的 FHA 结构域可与多种含磷苏氨酸的肽结合
抗体在监测翻译后修饰(如磷酸化)方面发挥着至关重要的作用,磷酸化可调节蛋白质的活性和位置;然而,与重组亲和试剂相比,商业多克隆和单克隆抗体在可再生性和工程方面存在局限性。基于叉头相关结构域(FHA)的支架有可能成为这种翻译后修饰的选择性亲和试剂。通过与对应于人类 mTOR、Chk2、53BP1 和 Akt1 蛋白的磷酸肽进行亲和选择,从 M13 噬菌体展示文库中分离出了具有有限交叉反应性的工程化 FHA 结构域,称为磷酸苏氨酸结合结构域(phosphothreonine-binding domains,pTBDs)。为了确定代表性 pTBD 的特异性,我们重点研究了与 DNA 修复蛋白 53BP1 的 pT543 磷酸肽(536-IDEDGENpTQIEDTEP-551)的结合者。ELISA 和 Western 印迹实验表明 pTBDs 对磷酸苏氨酸具有特异性,这证明了 pTBDs 在监测临床相关人类蛋白质中特定苏氨酸残基磷酸化方面的潜在用途。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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