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首页> 外文期刊>Bioconjugate Chemistry >Development of an Indole-Based Chemically Cleavable Linker Concept for Immobilizing Bait Compounds for Protein Pull-Down Experiments
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Development of an Indole-Based Chemically Cleavable Linker Concept for Immobilizing Bait Compounds for Protein Pull-Down Experiments

机译:基于吲哚的化学可切割连接子概念的开发,用于固定诱饵化合物用于蛋白质下拉实验

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摘要

A novel linker chemistry based on a malondialdehyde—indole condensation reaction has been developed for the affinity-independent elution of targeted protein pull-downs. Previously developed in our lab for the tagging of tryptophan residues on proteins or peptides, the concept was extended for the design of a chemically cleavable linker system. Target molecules for interaction studies are immobilized on a solid support including the linker scaffold, and a typical pull-down experiment is carried out. After purification, the linker is cleaved by incubation with SO mM pyrrolidine. A specific tyrosine kinase inhibitor, bosutinib, was coupled to agarose and acrylamide beads, respectively, via the new linker system, and a protein pull-down experiment of putative interaction partners from a K562 whole cell lysate was performed. The system was found to be compatible with targeted protein pull-downs; during the cleavage step, no protein hydrolysis or any degradation of amino acid side-chains was apparent. From the pull-down experiment, key targets of bosutinib such as the tyrosine kinase, Btk, were identified by liquid chromatography—tandem mass spectrometry.
机译:已经开发出一种基于丙二醛-吲哚缩合反应的新型接头化学,用于不依赖亲和力的靶向蛋白下拉反应的洗脱。该概念先前在我们的实验室中开发,用于标记蛋白质或肽上的色氨酸残基,后来扩展到了可化学裂解的接头系统的设计。用于相互作用研究的目标分子被固定在包括连接支架的固体支持物上,并进行了典型的下拉实验。纯化后,通过与SO mM吡咯烷一起温育来切割接头。通过新的接头系统,将特定的酪氨酸激酶抑制剂bosutinib分别与琼脂糖和丙烯酰胺珠偶联,并进行了从K562全细胞裂解物中推定的相互作用伴侣的蛋白质下拉实验。发现该系统与目标蛋白下拉序列兼容;在切割步骤中,没有蛋白质水解或氨基酸侧链的任何降解是明显的。通过下拉实验,通过液相色谱-串联质谱法鉴定了波舒替尼的关键靶标,例如酪氨酸激酶Btk。

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