том 13 издание 10 страницы 2200-2216

Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy

Тип публикацииJournal Article
Дата публикации2018-09-14
scimago Q1
wos Q1
БС1
SJR5.854
CiteScore27.6
Impact factor16.0
ISSN17542189, 17502799
General Biochemistry, Genetics and Molecular Biology
Краткое описание
The goal of mechanobiology is to understand the links between changes in the physical properties of living cells and normal physiology and disease. This requires mechanical measurements that have appropriate spatial and temporal resolution within a single cell. Conventional atomic force microscopy (AFM) methods that acquire force curves pointwise are used to map the heterogeneous mechanical properties of cells. However, the resulting map acquisition time is much longer than that required to study many dynamic cellular processes. Dynamic AFM (dAFM) methods using resonant microcantilevers are compatible with higher-speed, high-resolution scanning; however, they do not directly acquire force curves and they require the conversion of a limited number of instrument observables to local mechanical property maps. We have recently developed a technique that allows commercial AFM systems equipped with direct cantilever excitation to quantitatively map the viscoelastic properties of live cells. The properties can be obtained at several widely spaced frequencies with nanometer–range spatial resolution and with fast image acquisition times (tens of seconds). Here, we describe detailed procedures for quantitative mapping, including sample preparation, AFM calibration, and data analysis. The protocol can be applied to different biological samples, including cells and viruses. The transition from dAFM imaging to quantitative mapping should be easily achievable for experienced AFM users, who will be able to set up the protocol in <30 min.This protocol describes a dynamic atomic force microscopy (dAFM) approach for high-speed and high-resolution mapping of the viscoelastic properties of live cells. The procedure describes sample preparation, AFM calibration, and data analysis.
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ГОСТ |
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Efremov Y. M. et al. Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy // Nature Protocols. 2018. Vol. 13. No. 10. pp. 2200-2216.
ГОСТ со всеми авторами (до 50) Скопировать
Efremov Y. M., Cartagena-Rivera A. X., Athamneh A. I. M., Suter D. M., Raman A. Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy // Nature Protocols. 2018. Vol. 13. No. 10. pp. 2200-2216.
RIS |
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TY - JOUR
DO - 10.1038/s41596-018-0031-8
UR - https://doi.org/10.1038/s41596-018-0031-8
TI - Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy
T2 - Nature Protocols
AU - Efremov, Yuri M
AU - Cartagena-Rivera, Alexander X
AU - Athamneh, Ahmad I M
AU - Suter, Daniel M
AU - Raman, Arvind
PY - 2018
DA - 2018/09/14
PB - Springer Nature
SP - 2200-2216
IS - 10
VL - 13
PMID - 30218102
SN - 1754-2189
SN - 1750-2799
ER -
BibTex |
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BibTex (до 50 авторов) Скопировать
@article{2018_Efremov,
author = {Yuri M Efremov and Alexander X Cartagena-Rivera and Ahmad I M Athamneh and Daniel M Suter and Arvind Raman},
title = {Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy},
journal = {Nature Protocols},
year = {2018},
volume = {13},
publisher = {Springer Nature},
month = {sep},
url = {https://doi.org/10.1038/s41596-018-0031-8},
number = {10},
pages = {2200--2216},
doi = {10.1038/s41596-018-0031-8}
}
MLA
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Efremov, Yuri M., et al. “Mapping heterogeneity of cellular mechanics by multi-harmonic atomic force microscopy.” Nature Protocols, vol. 13, no. 10, Sep. 2018, pp. 2200-2216. https://doi.org/10.1038/s41596-018-0031-8.