Literature DB >> 29755164

Mass Measurements of Focal Adhesions in Single Cells Using High Resolution Surface Plasmon Resonance Microscopy.

Alexander W Peterson1, Michael Halter1, Alessandro Tona1, Anne L Plant1, John T Elliott1.   

Abstract

Surface plasmon resonance microscopy (SPRM) is a powerful label-free imaging technique with spatial resolution approaching the optical diffraction limit. The high sensitivity of SPRM to small changes in index of refraction at an interface allows imaging of dynamic protein structures within a cell. Visualization of subcellular features, such as focal adhesions (FAs), can be performed on live cells using a high numerical aperture objective lens with a digital light projector to precisely position the incident angle of the excitation light. Within the cell-substrate region of the SPRM image, punctate regions of high contrast are putatively identified as the cellular FAs. Optical parameter analysis is achieved by application of the Fresnel model to the SPRM data and resulting refractive index measurements are used to calculate protein density and mass. FAs are known to be regions of high protein density that reside at the cell-substratum interface. Comparing SPRM with fluorescence images of antibody stained for vinculin, a component in FAs, reveals similar measurements of FA size. In addition, a positive correlation between FA size and protein density is revealed by SPRM. Comparing SPRM images for two cell types reveals a distinct difference in the protein density and mass of their respective FAs. Application of SPRM to quantify mass can greatly aid monitoring basic processes that control FA mass and growth and contribute to accurate models that describe cell-extracellular interactions.

Entities:  

Keywords:  SPRM; Surface plasmon; cells; density; focal adhesions; mass; proteins

Year:  2018        PMID: 29755164      PMCID: PMC5947864          DOI: 10.1117/12.2290776

Source DB:  PubMed          Journal:  Proc SPIE Int Soc Opt Eng        ISSN: 0277-786X


  15 in total

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Authors:  S K Sastry; K Burridge
Journal:  Exp Cell Res       Date:  2000-11-25       Impact factor: 3.905

2.  Quantitative angle-resolved SPR imaging of DNA-DNA and DNA-drug kinetics.

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Authors:  Anne L Plant; Kiran Bhadriraju; Tighe A Spurlin; John T Elliott
Journal:  Biochim Biophys Acta       Date:  2008-11-05

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Authors:  Benjamin Geiger; Joachim P Spatz; Alexander D Bershadsky
Journal:  Nat Rev Mol Cell Biol       Date:  2009-01       Impact factor: 94.444

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Journal:  Annu Rev Cell Dev Biol       Date:  1995       Impact factor: 13.827

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Authors:  K Burridge; M Chrzanowska-Wodnicka
Journal:  Annu Rev Cell Dev Biol       Date:  1996       Impact factor: 13.827

7.  Live-cell mass profiling: an emerging approach in quantitative biophysics.

Authors:  Thomas A Zangle; Michael A Teitell
Journal:  Nat Methods       Date:  2014-12       Impact factor: 28.547

8.  Nanoscale architecture of integrin-based cell adhesions.

Authors:  Pakorn Kanchanawong; Gleb Shtengel; Ana M Pasapera; Ericka B Ramko; Michael W Davidson; Harald F Hess; Clare M Waterman
Journal:  Nature       Date:  2010-11-25       Impact factor: 49.962

9.  Step-by-step quantitative analysis of focal adhesions.

Authors:  Utku Horzum; Berrin Ozdil; Devrim Pesen-Okvur
Journal:  MethodsX       Date:  2014-07-07

10.  High resolution surface plasmon resonance imaging for single cells.

Authors:  Alexander W Peterson; Michael Halter; Alessandro Tona; Anne L Plant
Journal:  BMC Cell Biol       Date:  2014-12-01       Impact factor: 4.241

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  1 in total

1.  In Situ Analysis of Membrane-Protein Binding Kinetics and Cell-Surface Adhesion Using Plasmonic Scattering Microscopy.

Authors:  Pengfei Zhang; Xinyu Zhou; Jiapei Jiang; Jayeeta Kolay; Rui Wang; Guangzhong Ma; Zijian Wan; Shaopeng Wang
Journal:  Angew Chem Int Ed Engl       Date:  2022-08-23       Impact factor: 16.823

  1 in total

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