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Extract2Chip-Bypassing Protein Purification in Drug Discovery Using Surface Plasmon Resonance. | LitMetric

AI Article Synopsis

  • Modern drug discovery involves combinatorial screening to identify drug molecules that target proteins linked to diseases, relying on detailed understanding of these targets through purification.
  • The Extract2Chip method is introduced as an innovative way to study protein interactions directly from cellular extracts without extensive purification, using biotinylated proteins and sensor chips for characterizing molecular interactions via SPR.
  • This method has been validated with specific proteins like Cyclophilin D and has broad applications in drug discovery, helping to investigate challenging targets and potentially reviving unsuccessful campaigns due to protein supply issues.

Article Abstract

Modern drug discovery relies on combinatorial screening campaigns to find drug molecules targeting specific disease-associated proteins. The success of such campaigns often relies on functional and structural information of the selected therapeutic target, only achievable once its purification is mastered. With the aim of bypassing the protein purification process to gain insights on the druggability, ligand binding, and/or characterization of protein-protein interactions, herein, we describe the Extract2Chip method. This approach builds on the immobilization of site-specific biotinylated proteins of interest, directly from cellular extracts, on avidin-coated sensor chips to allow for the characterization of molecular interactions via surface plasmon resonance (SPR). The developed method was initially validated using Cyclophilin D (CypD) and subsequently applied to other drug discovery projects in which the targets of interest were difficult to express, purify, and crystallize. Extract2Chip was successfully applied to the characterization of Yes-associated protein (YAP): Transcriptional enhancer factor TEF (TEAD1) protein-protein interaction inhibitors, in the validation of a ternary complex assembly composed of Dyskerin pseudouridine synthase 1 (DKC1) and RuvBL1/RuvBL2, and in the establishment of a fast-screening platform to select the most suitable NUAK family SNF1-like kinase 2 (NUAK2) surrogate for binding and structural studies. The described method paves the way for a potential revival of the many drug discovery campaigns that have failed to deliver due to the lack of suitable and sufficient protein supply.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10605449PMC
http://dx.doi.org/10.3390/bios13100913DOI Listing

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