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A Novel Cell-Based Intracellular Protein–Protein Interaction Detection Platform (SOLIS) for Multimodality Screening

细胞内 融合蛋白 生物 蛋白质-蛋白质相互作用 适体 细胞生物学 嵌合体(遗传学) 细胞膜 计算生物学 生物化学 细胞 化学 分子生物学 重组DNA 基因
作者
Daiki Kashima,Miho Kageoka,Yosuke Kimura,Makiko Horikawa,Miwa Miura,Makoto Nakakido,Kouhei Tsumoto,Teruyuki Nagamune,Masahiro Kawahara
出处
期刊:ACS Synthetic Biology [American Chemical Society]
卷期号:10 (5): 990-999 被引量:10
标识
DOI:10.1021/acssynbio.0c00483
摘要

Intervention in protein–protein interactions (PPIs) has tremendous effects in the molecular therapy of many diseases. To fulfill the requirements for targeting intracellular proteins, here we develop SOS-localization-based interaction screening (SOLIS), which elaborately mimics signaling via the Ras-mitogen-activated protein kinase pathway. SOLIS employs two chimeric proteins in which a membrane localization motif (CaaX) is fused at the C-terminus of a protein of interest and the catalytic domain of SOS is fused at the C-terminus of another protein of interest. Interaction between the two proteins of interest induces membrane localization of the SOS chimera and cell proliferation. Thus, the SOLIS system enables enrichment of superior binders based on cell proliferation in an intracellular PPI-dependent manner. This was verified by three major modalities against intracellular PPIs (small molecules, peptide aptamers, and intrabodies). The system worked over a broad range of affinities (KD = 0.32–140 nM). In a screening of a site-directed randomized library, novel intrabody clones were selected on the basis of the potency of cell proliferation. Three other PPI detection methods (NanoBiT, SPR, and pull-down assays) were employed to characterize the SOLIS system, and several intrabody clones were judged as false negatives in these assays. SOLIS signals would be less sensitive to the orientation/conformation of the chimeric proteins, and this feature emerges as the advantage of SOLIS as a mammalian cytosolic PPI detection system with few false negatives.
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