研究目的
To engineer biosensors that can detect and measure the metastatic "potential" of single living cancer cells by identifying and targeting a metastasis-related phosphoprotein.
研究成果
The IMP biosensors can measure the diversity and plasticity of metastatic potential of tumor cells in a sensitive and unbiased way, providing a novel tool for detecting metastasis-initiating cells (MICs) and potentially guiding personalized cancer therapy.
研究不足
Further evolution of the probes is needed before they can be used for in vivo imaging studies. The signaling event localizes to focal adhesions, which may complicate sorting-related applications. Increased ROS production in tumor cells may affect the signaling pathways monitored with IMPs or the IMP probes themselves.
1:Experimental Design and Method Selection:
Comprehensive analysis of the pan-cancer phosphoproteome to identify actin remodelers required for cell migration. Design of FRET-based biosensors targeting the identified phosphoprotein.
2:Sample Selection and Data Sources:
Use of various cancer cell lines with known metastatic potential, including MDA-MB-231, PC-9, and H2030, and their metastatic subclones.
3:List of Experimental Equipment and Materials:
Confocal microscopy for FRET imaging, immunoblotting for protein analysis, and various growth factors and inhibitors for cell stimulation.
4:Experimental Procedures and Operational Workflow:
Transfection of cells with IMP probes, stimulation with ligands, and FRET imaging to measure metastatic potential.
5:Data Analysis Methods:
Quantitative analysis of FRET efficiency to assess the metastatic potential of single cells.
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