4.6 Article

Discovery of functional interactions among actin regulators by analysis of image fluctuations in an unperturbed motile cell system

Publisher

ROYAL SOC
DOI: 10.1098/rstb.2017.0110

Keywords

actin; system redundancy; real-time; imaging; signalling; fluctuations

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Funding

  1. NIH [R01 GM071868]
  2. NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES [R01GM071868] Funding Source: NIH RePORTER

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Cell migration is driven by propulsive forces derived from polymerizing actin that pushes and extends the plasma membrane. The underlying actin network is constantly undergoing adaptation to new mechano-chemical environments and intracellular conditions. As such, mechanisms that regulate actin dynamics inherently contain multiple feedback loops and redundant pathways. Given the highly adaptable nature of such a system, studies that use only perturbation experiments (e.g. knockdowns, overexpression, pharmacological activation/inhibition, etc.) are challenged by the nonlinearity and redundancy of the pathway. In these pathway configurations, perturbation experiments at best describe the function(s) of a molecular component in an adapting (e.g. acutely drug-treated) or fully adapted (e.g. permanent gene silenced) cell system, where the targeted component now resides in a non-native equilibrium. Here, we propose how quantitative live-cell imaging and analysis of constitutive fluctuations of molecular activities can overcome these limitations. We highlight emerging actin filament barbed-end biology as a prime example of a complex, nonlinear molecular process that requires a fluctuation analytic approach, especially in an unperturbed cellular system, to decipher functional interactions of barbed-end regulators, actin polymerization and membrane protrusion.

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