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Directed immobilization of peptide ligands to accessible pore sites by conjugation with a placeholder molecule

机译:通过与占位符分子缀合将肽配体定向固定到可到达的孔位

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When small ligands are immobilized onto a porous chromatography medium, only a limited number of binding sites contributes to the interaction with the target molecule. The main part of the ligand molecules is distributed on sites that are not accessible for the target protein due to steric hindrance. To direct the ligand into a well-accessible position, the ligand was conjugated to a large molecule that acted as a placeholder during the immobilization step. Then the placeholder molecule was cleaved off and washed out. Two linear peptides with affinity for lysozyme and human blood coagulation factor VIII, respectively, were studied as model systems. The protected peptide ligand was covalently linked to a 20-kDa poly(ethylene glycol) molecule containing an acid-labile linker. After selective deprotection of the peptide and purification, immobilization of this conjugate on a preactivated chromatography matrix was performed alternatively through the free N-terminus, the epsilon-amino group of lysine, or the sulfohydryl group of cysteine. After the immobilization reaction, the spacer molecule and remaining protecting groups were cleaved off and the gels were tested by affinity chromatography. This novel immobilization technique substantially increased the binding capacity and the ligand utilization for the target protein, and site-specific immobilization could be demonstrated. [References: 18]
机译:当小的配体固定在多孔色谱介质上时,只有有限数量的结合位点有助于与靶分子的相互作用。由于空间位阻,配体分子的主要部分分布在靶蛋白无法接近的位点上。为了将配体引导到易于接近的位置,将配体与固定步骤中充当占位符的大分子缀合。然后将占位符分子裂解并洗掉。研究了分别对溶菌酶和人凝血因子VIII有亲和力的两种线性肽作为模型系统。将受保护的肽配体共价连接至包含酸不稳定接头的20 kDa聚乙二醇分子。在对肽进行选择性脱保护并纯化后,可通过游离的N端,赖氨酸的ε-氨基或半胱氨酸的巯基将该缀合物固定在预活化的色谱基质上。固定化反应后,将间隔物分子和剩余的保护基团切除,并通过亲和色谱法测试凝胶。这种新颖的固定技术大大提高了对目标蛋白的结合能力和配体利用率,并且可以证明位点特异性固定。 [参考:18]

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