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一种用于检测细胞裂解物中蛋白激酶活性的肽微阵列。

A peptide microarray for detecting protein kinase activity in cell lysates.

作者信息

Han Xiaoming, Katayama Yoshiki

机构信息

Graduate School of System Life Sciences, Kyushu University, Fukuoka, Japan.

出版信息

Methods Mol Biol. 2010;669:183-94. doi: 10.1007/978-1-60761-845-4_15.

Abstract

Protein kinases (PKs) are widely recognized as valuable targets for disease diagnosis and drug discovery. For this reason, we have developed a sensitive peptide microarray for detecting intracellular PK activity. Peptides are immobilized on a glutaraldehyde-premodified high-amino terminal glass slide, by spotting 2 nL volumes of substrate peptide solutions with an automated microarray spotter. After the peptides are phosphorylated by cell lysates, phosphorylation is specifically recognized by a fluorescence-labeled antiphosphotyrosine antibody for tyrosine kinases, or Phos-tag biotin (a biotinylated phosphate-specific ligand based on Zn(2+) complex), which is subsequently bound with fluorescence-labeled streptavidin, for serine/threonine kinases. The fluorescence signal is then detected by an automatic microarray scanner. The peptide microarray system involves simple peptide immobilization, requires low sample volumes and provides a high density array. Importantly, it provides high sensitivity for detecting PK activities in cell lysates. Thus, the peptide microarray system is expected to be useful for a high-throughput kinase assay to investigate intracellular kinase activity and has potential applications in disease diagnosis and drug discovery.

摘要

蛋白激酶(PKs)被广泛认为是疾病诊断和药物研发的重要靶点。基于此,我们开发了一种用于检测细胞内PK活性的灵敏肽微阵列。通过使用自动微阵列点样仪点样2 nL体积的底物肽溶液,将肽固定在戊二醛预修饰的高氨基末端载玻片上。肽被细胞裂解物磷酸化后,酪氨酸激酶的磷酸化可被荧光标记的抗磷酸酪氨酸抗体特异性识别,而丝氨酸/苏氨酸激酶的磷酸化则可被Phos-tag生物素(一种基于Zn(2+)络合物的生物素化磷酸特异性配体)特异性识别,随后Phos-tag生物素与荧光标记的链霉亲和素结合。然后通过自动微阵列扫描仪检测荧光信号。该肽微阵列系统涉及简单的肽固定,所需样品体积小,并提供高密度阵列。重要的是,它对检测细胞裂解物中的PK活性具有高灵敏度。因此,该肽微阵列系统有望用于高通量激酶测定以研究细胞内激酶活性,并在疾病诊断和药物研发中具有潜在应用。

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