A novel chemoproteomic technology to reveal global small molecule-proteome-wide interactions in live cells.

Information

  • Research Project
  • 9669919
  • ApplicationId
    9669919
  • Core Project Number
    R21GM126264
  • Full Project Number
    1R21GM126264-01A1
  • Serial Number
    126264
  • FOA Number
    PAR-17-046
  • Sub Project Id
  • Project Start Date
    2/1/2019 - 5 years ago
  • Project End Date
    1/31/2021 - 3 years ago
  • Program Officer Name
    BACKLUND, PETER S
  • Budget Start Date
    2/1/2019 - 5 years ago
  • Budget End Date
    1/31/2020 - 4 years ago
  • Fiscal Year
    2019
  • Support Year
    01
  • Suffix
    A1
  • Award Notice Date
    1/31/2019 - 5 years ago

A novel chemoproteomic technology to reveal global small molecule-proteome-wide interactions in live cells.

Project Summary/Abstract Small molecules are abundant in nature, where they perform various roles in living cells, as enzyme cofactors, signaling molecules in biological networks or as metabolic components. As a consequence of physical interaction with proteins, they may illicit profound changes in protein function that can have physiological outcomes. Several biophysical and biochemical approaches, including high-throughput screening strategies, have been developed in an effort to globally or individually detect protein-metabolite interactions in vitro, in situ or in vivo. The use of affinity tags and protein overexpression has enabled the detection of metabolome-wide small molecule ligands of each protein target in turn. However, these methods are compounded by a necessity to isolate the protein target of interest from the cell, thus providing lesser physiological relevance and complicating downstream validation and analysis. Excluding the use of protein or small molecule arrays, the remaining in situ or in vivo approaches are limited to permit the identification of proteome-wide targets of each small molecule in turn. These technological restrictions translate to a bottleneck in data acquisition and difficulties in validation when determining important functional roles of small molecules in the context of biological networks. Therefore, currently, there are no technologies to globally identify the proteome-wide targets of all small molecules in live cells without isolation and disturbance of the intact targets within the intracellular milieu. We aim to overcome this limitation by developing a new chemoproteomic technology that will permit direct isolation and characterization by mass spectrometry of metabolome-wide small molecules with their respective proteome-wide targets in situ in a single experiment. This truly global approach will deliver a powerful new tool for the investigator of protein-small molecule interactions by enabling the acquisition of the complete protein-metabolite interactome in live cells. We expect that the information gathered by adopting this technology will yield novel insights in small molecule-protein regulation, providing more comprehensive and larger biological networks for the analysis of signaling pathways of physiological relevance, and facilitating comparisons of entire organism protein-small molecule interactions under different experimental conditions in a similar manner to other current ?omics disciplines.

IC Name
NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES
  • Activity
    R21
  • Administering IC
    GM
  • Application Type
    1
  • Direct Cost Amount
    150000
  • Indirect Cost Amount
    142500
  • Total Cost
    292500
  • Sub Project Total Cost
  • ARRA Funded
    False
  • CFDA Code
    859
  • Ed Inst. Type
  • Funding ICs
    NIGMS:292500\
  • Funding Mechanism
    Non-SBIR/STTR RPGs
  • Study Section
    EBIT
  • Study Section Name
    Enabling Bioanalytical and Imaging Technologies Study Section
  • Organization Name
    MOLECULAR MEDICINE RESEARCH INSTITUTE
  • Organization Department
  • Organization DUNS
    015535594
  • Organization City
    SUNNYVALE
  • Organization State
    CA
  • Organization Country
    UNITED STATES
  • Organization Zip Code
    940854708
  • Organization District
    UNITED STATES