用于研究细胞内蛋白质-蛋白质相互作用的生物素化细胞穿透肽
Biotinylated Cell-penetrating Peptides to Study Intracellular Protein-protein Interactions.
作者信息
Jaraíz-Rodríguez Myriam, González-Sánchez Ana, García-Vicente Laura, Medina Jose M, Tabernero Arantxa
机构信息
Instituto de Neurociencias de Castilla y León (INCYL), Departamento de Bioquímica y Biología Molecular, Universidad de Salamanca.
Instituto de Neurociencias de Castilla y León (INCYL), Departamento de Bioquímica y Biología Molecular, Universidad de Salamanca; Centre for Cancer Research & Cell Biology (CCRCB), School of Medicine, Dentistry and Biomedical Sciences, Queen's University Belfast.
出版信息
J Vis Exp. 2017 Dec 20(130):56457. doi: 10.3791/56457.
Here we present a protocol to study intracellular protein-protein interactions that is based on the widely used biotin-avidin pull-down system. The modification presented includes the combination of this technique with cell-penetrating sequences. We propose to design cell-penetrating baits that can be incubated with living cells instead of cell lysates and therefore the interactions found will reflect those that occur within the intracellular context. Connexin43 (Cx43), a protein that forms gap junction channels and hemichannels is down-regulated in high-grade gliomas. The Cx43 region comprising amino acids 266-283 is responsible for the inhibition of the oncogenic activity of c-Src in glioma cells. Here we use TAT as the cell-penetrating sequence, biotin as the pull-down tag and the region of Cx43 comprised between amino acids 266-283 as the target to find intracellular interactions in the hard-to-transfect human glioma stem cells. One of the limitations of the proposed method is that the molecule used as bait could fail to fold properly and, consequently, the interactions found could not be associated with the effect. However, this method can be especially interesting for the interactions involved in signal transduction pathways because they are usually carried out by intrinsically disordered regions and, therefore, they do not require an ordered folding. In addition, one of the advantages of the proposed method is that the relevance of each residue on the interaction can be easily studied. This is a modular system; therefore, other cell-penetrating sequences, other tags, and other intracellular targets can be employed. Finally, the scope of this protocol is far beyond protein-protein interaction because this system can be applied to other bioactive cargoes such as RNA sequences, nanoparticles, viruses or any molecule that can be transduced with cell-penetrating sequences and fused to pull-down tags to study their intracellular mechanism of action.
在此,我们展示了一种基于广泛使用的生物素-抗生物素蛋白下拉系统来研究细胞内蛋白质-蛋白质相互作用的方案。所提出的改进包括将该技术与细胞穿透序列相结合。我们建议设计可与活细胞而非细胞裂解物孵育的细胞穿透诱饵,因此所发现的相互作用将反映细胞内环境中发生的相互作用。连接蛋白43(Cx43)是一种形成间隙连接通道和半通道的蛋白质,在高级别胶质瘤中表达下调。包含氨基酸266 - 283的Cx43区域负责抑制胶质瘤细胞中c-Src的致癌活性。在此,我们使用TAT作为细胞穿透序列,生物素作为下拉标签,并将Cx43氨基酸266 - 283之间的区域作为靶点,以在难以转染的人胶质瘤干细胞中寻找细胞内相互作用。所提出方法的局限性之一是用作诱饵的分子可能无法正确折叠,因此所发现的相互作用可能与该效应无关。然而,该方法对于信号转导途径中涉及的相互作用可能特别有意义,因为它们通常由内在无序区域介导,因此不需要有序折叠。此外,所提出方法的优点之一是可以轻松研究每个残基在相互作用中的相关性。这是一个模块化系统;因此,可以使用其他细胞穿透序列、其他标签和其他细胞内靶点。最后,该方案的范围远远超出蛋白质-蛋白质相互作用,因为该系统可应用于其他生物活性物质,如RNA序列、纳米颗粒、病毒或任何可以通过细胞穿透序列转导并与下拉标签融合以研究其细胞内作用机制的分子。
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