Mechanical fluidity of fully suspended biological cells

John M. Maloney; Eric Lehnhardt; Alexandra F. Long; Krystyn J. Van Vliet

doi:10.1016/j.bpj.2013.08.040

Mechanical fluidity of fully suspended biological cells

John M. Maloney, Eric Lehnhardt, Alexandra F. Long, Krystyn J. Van Vliet

Biology

Research output: Contribution to journal › Article › peer-review

21 Scopus citations

Abstract

Mechanical characteristics of single biological cells are used to identify and possibly leverage interesting differences among cells or cell populations. Fluidity - hysteresivity normalized to the extremes of an elastic solid or a viscous liquid - can be extracted from, and compared among, multiple rheological measurements of cells: creep compliance versus time, complex modulus versus frequency, and phase lag versus frequency. With multiple strategies available for acquisition of this nondimensional property, fluidity may serve as a useful and robust parameter for distinguishing cell populations, and for understanding the physical origins of deformability in soft matter. Here, for three disparate eukaryotic cell types deformed in the suspended state via optical stretching, we examine the dependence of fluidity on chemical and environmental influences at a timescale of ∼1 s. We find that fluidity estimates are consistent in the time and frequency domains under a structural damping (power-law or fractional-derivative) model, but not under an equivalent-complexity, lumped-component (spring-dashpot) model; the latter predicts spurious time constants. Although fluidity is suppressed by chemical cross-linking, we find that ATP depletion in the cell does not measurably alter the parameter, and we thus conclude that active ATP-driven events are not a crucial enabler of fluidity during linear viscoelastic deformation of a suspended cell. Finally, by using the capacity of optical stretching to produce near-instantaneous increases in cell temperature, we establish that fluidity increases with temperature - now measured in a fully suspended, sortable cell without the complicating factor of cell-substratum adhesion.

Original language	English
Pages (from-to)	1767-1777
Number of pages	11
Journal	Biophysical Journal
Volume	105
Issue number	8
DOIs	https://doi.org/10.1016/j.bpj.2013.08.040
State	Published - Oct 15 2013

Funding

This work was supported by the Singapore-MIT Alliance for Research and Technology (SMART) Centre (BioSyM IRG), National Science Foundation CAREER CBET-0644846 (K.J.V.V.), National Science Foundation REU DBI-1005055 (E.L. and A.F.L.), and the National Institutes of Health/National Institute of Biomedical Engineering and Bioengineering Molecular, Cellular, Tissue and Biomechanics Training Grant EB006348 (J.M.M.).

Funders	Funder number
National Institute of Biomedical Engineering and Bioengineering Molecular, Cellular, Tissue and Biomechanics Training	EB006348
U.S. Department of Energy Chinese Academy of Sciences Guangzhou Municipal Science and Technology Project Oak Ridge National Laboratory Extreme Science and Engineering Discovery Environment National Science Foundation National Energy Research Scientific Computing Center National Natural Science Foundation of China	CBET-0644846, REU DBI-1005055
U.S. Department of Energy Chinese Academy of Sciences Guangzhou Municipal Science and Technology Project Oak Ridge National Laboratory Extreme Science and Engineering Discovery Environment National Science Foundation National Energy Research Scientific Computing Center National Natural Science Foundation of China
National Institutes of Health (NIH)
National Institute of Biomedical Imaging and Bioengineering	T32EB006348
National Institute of Biomedical Imaging and Bioengineering
Singapore-MIT Alliance for Research and Technology Centre

ASJC Scopus subject areas

Biophysics

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10.1016/j.bpj.2013.08.040

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title = "Mechanical fluidity of fully suspended biological cells",

abstract = "Mechanical characteristics of single biological cells are used to identify and possibly leverage interesting differences among cells or cell populations. Fluidity - hysteresivity normalized to the extremes of an elastic solid or a viscous liquid - can be extracted from, and compared among, multiple rheological measurements of cells: creep compliance versus time, complex modulus versus frequency, and phase lag versus frequency. With multiple strategies available for acquisition of this nondimensional property, fluidity may serve as a useful and robust parameter for distinguishing cell populations, and for understanding the physical origins of deformability in soft matter. Here, for three disparate eukaryotic cell types deformed in the suspended state via optical stretching, we examine the dependence of fluidity on chemical and environmental influences at a timescale of ∼1 s. We find that fluidity estimates are consistent in the time and frequency domains under a structural damping (power-law or fractional-derivative) model, but not under an equivalent-complexity, lumped-component (spring-dashpot) model; the latter predicts spurious time constants. Although fluidity is suppressed by chemical cross-linking, we find that ATP depletion in the cell does not measurably alter the parameter, and we thus conclude that active ATP-driven events are not a crucial enabler of fluidity during linear viscoelastic deformation of a suspended cell. Finally, by using the capacity of optical stretching to produce near-instantaneous increases in cell temperature, we establish that fluidity increases with temperature - now measured in a fully suspended, sortable cell without the complicating factor of cell-substratum adhesion.",

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AU - Lehnhardt, Eric

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N2 - Mechanical characteristics of single biological cells are used to identify and possibly leverage interesting differences among cells or cell populations. Fluidity - hysteresivity normalized to the extremes of an elastic solid or a viscous liquid - can be extracted from, and compared among, multiple rheological measurements of cells: creep compliance versus time, complex modulus versus frequency, and phase lag versus frequency. With multiple strategies available for acquisition of this nondimensional property, fluidity may serve as a useful and robust parameter for distinguishing cell populations, and for understanding the physical origins of deformability in soft matter. Here, for three disparate eukaryotic cell types deformed in the suspended state via optical stretching, we examine the dependence of fluidity on chemical and environmental influences at a timescale of ∼1 s. We find that fluidity estimates are consistent in the time and frequency domains under a structural damping (power-law or fractional-derivative) model, but not under an equivalent-complexity, lumped-component (spring-dashpot) model; the latter predicts spurious time constants. Although fluidity is suppressed by chemical cross-linking, we find that ATP depletion in the cell does not measurably alter the parameter, and we thus conclude that active ATP-driven events are not a crucial enabler of fluidity during linear viscoelastic deformation of a suspended cell. Finally, by using the capacity of optical stretching to produce near-instantaneous increases in cell temperature, we establish that fluidity increases with temperature - now measured in a fully suspended, sortable cell without the complicating factor of cell-substratum adhesion.

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Mechanical fluidity of fully suspended biological cells

Abstract

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