Cells are highly dynamic, squeezing, pulling, and tugging on their surroundings and on each other. Each individualinteractioninvolvesforces.Theseforcesarefeltbyspecificreceptorsandmolecules.Althoughsmall inmagnitude(pN),thesemolecularforcescanhaveprofoundbiologicalimpactsinmanyaspectsofcellularlife includingthefateofdifferentiatingstemcells,celldivision,cancermetastasis,andbloodclotting.Therefore,the ability to characterize the interplay between physical forces and biochemical signals isa critical component of understanding signaling pathways in living systems. There are two main techniques used to study molecular mechanobiology: single molecule force spectroscopy (SMFS) and traction force microscopy (TFM) based methods.Whilepowerful,theseapproachessufferfromseveraldrawbacks.SMFSmeasuresindividualreceptor forces(pN),butitdoessoonlyonemoleculeatatime.ConverselyTFMprovidesspatialmapsofcellularforces, butonthenNscale,ordersofmagnitudelargerthantheforcesappliedbyindividualcellreceptors.Tobridge these approaches, we invented molecular tension fluorescence microscopy (MTFM) which uses conventional fluorescencemicroscopytomapcellularforceswithpNresolutionbyusingacalibratedmolecularforceprobe. ThegoalofthisproposalistotransformthecapabilitiesofMTFMallowingordersofmagnitudeimprovementin spatialandtemporalresolutionaswellasthemappingofforceorientation.Molecularmechanobiologyremains at the fringes of biomedical sciences because of the lack of tools to precisely quantify and link mechanics to cellularbiochemistry.Ourgoalistotransformthefieldofmolecularmechanobiologybydevelopingnewimaging technologies to enable the study cellular forces at unprecedented resolution. These technologies, centered around the DNA-based MTFM probes, will provide a broadly applicable platform of technology to investigate molecularmechanics,andthefunctionaloutcomesofmolecularforces,indiversebiologicalsystems.
In Aim1 wewilladdressthespatialresolutiongap,andleveragetheDNA-basedforceprobestodevelopsuper-resolution force-PAINT with the goal of dynamic force imaging with 20 nm spatial resolution.
In Aim 2 we will probe the dynamicsofforcesandforcefluctuationsbyharnessingthepoweroftwoapproaches,FRAPandFCS,tostudy molecular force dynamics with nsec to msec time resolution. Finally, in Aim 3 we will leverage fluorescence polarization microscopy to measure the 3D orientations of molecular forces. We will use fibroblast focal adhesions, platelet activation and coagulation, and T cell antigen recognition to test and verify our approach. Accomplishmentofthesegoalswillprovideanewtoolkitforunderstandingmolecularforcesandgeneratinga frameworkofhowforceorganizationanddynamicsinfluencecellularfunctioninhealthyanddiseasestates.

Public Health Relevance

The proposal aims to develop new methods to visualize mechanical forces in living cells. If successful, we will be able to reveal the forces that guide cellular processes such as embryonic development, hemostasis, and tumor growth. This will improve our ability to diagnose and treat diseases ranging from cancer metastasis to stroke.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM131099-02
Application #
9843171
Study Section
Cellular and Molecular Technologies Study Section (CMT)
Program Officer
Sammak, Paul J
Project Start
2019-01-01
Project End
2022-12-31
Budget Start
2020-01-01
Budget End
2020-12-31
Support Year
2
Fiscal Year
2020
Total Cost
Indirect Cost
Name
Emory University
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
066469933
City
Atlanta
State
GA
Country
United States
Zip Code
30322