Method Article

A Graphical User Interface for Software-assisted Tracking of Protein Concentration in Dynamic Cellular Protrusions

DOI:

10.3791/55653

July 11th, 2017

In This Article

Summary

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We present a software solution for semi-automated tracking of relative protein concentration along the length of dynamic cellular protrusions.

Abstract

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Filopodia are dynamic, finger-like cellular protrusions associated with migration and cell-cell communication. In order to better understand the complex signaling mechanisms underlying filopodial initiation, elongation and subsequent stabilization or retraction, it is crucial to determine the spatio-temporal protein activity in these dynamic structures. To analyze protein function in filopodia, we recently developed a semi-automated tracking algorithm that adapts to filopodial shape-changes, thus allowing parallel analysis of protrusion dynamics and relative protein concentration along the whole filopodial length. Here, we present a detailed step-by-step protocol for optimized cell handling, image acquisition and software analysis. We further provide instructions for the use of optional features during image analysis and data representation, as well as troubleshooting guidelines for all critical steps along the way. Finally, we also include a comparison of the described image analysis software with other programs available for filopodia quantification. Together, the presented protocol provides a framework for accurate analysis of protein dynamics in filopodial protrusions using image analysis software.

Introduction

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Spatio-temporal control of actin regulatory proteins is associated with filopodium dynamics 1,2. Tracking spatially resolved protein concentration along the whole filopodial length through time is thus crucial to advance our understanding of the mechanisms underlying initiation, elongation, stabilization or collapse of these dynamic structures 3,4. Unlike protein analysis in the cytosol, where many cell shape changes occur at a larger scale, filopodia are dynamic micro structures that constantly buckle 5 and bend, thus precludin....

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Protocol

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1. Cell Culture

  1. Culture HeLa or COS cells in Dulbecco's Modified Eagle Medium (DMEM) containing 4.5 g/L D-glucose, L-alanine-L-glutamine dipeptide, pyruvate, 10% fetal bovine serum, and 10 units/ml of penicillin/streptomycin. Culture neurons in culture-media without L-glutamine, glutamic acid or aspartic acid, supplemented with 0.5 mM L-alanine-L-glutamine dipeptide, serum-free neuronal supplements and 10 units/ml of penicillin/streptomycin.
  2. Once 40% confluency is reached, transfect cells with constructs of choice using a transfection reagent as per manufacturer's instructions. Keep transfected cells in incubator at 37 °C and 5% CO2 fo....

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Results

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Using COS cells transfected with a marker for filamentous actin (f-tractin18, red) and a cytosolic reference (green), we found actin-rich filopodial protrusions (Figure 3A, top panel). Time series showed that filopodia rapidly extend and retract (Figure 3A, middle panel). Using the image analysis software, we then traced individual filopodia. Comparison of filopodial length measured by hand vs. the image a.......

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Discussion

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Here we present a detailed protocol for tracking filopodial growth dynamics and analysis of relative protein concentrations in these dynamic structures via the convex-hull algorithm. Using the software, up to 3 channels can be compared pair-wise in a single run, whereby the relative concentrations of two channels (i.e. proteins) is determined throughout the extension/retraction cycle and stored as image and data files in separate folders. In addition to the routine operations, the software also provides a number.......

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Disclosures

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The authors have nothing to disclose.

Acknowledgements

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The authors acknowledge funding from the DFG (EXC-1003 to MG).

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Materials

List of materials used in this article
NameCompanyCatalog NumberComments
DMEMLife Technologies31966-021
10% Fetal bovine serumBiochrom AGL11-044
Lipofectamine 2000Life Technologies11668-027
1% penicillin/streptomycinBiochrom AG12212
Neurobasal MediumLife Technologies21103-049
B27Life Technologies17504-044
HEPES (1M stock solution)Life Technologies15630
Citrine-N1Addgene54593
LabtechThermo155411
Glutamax-IThermo35050-061
HelaLeibniz Institute DSMZACC-57
COS 7Leibniz Institute DSMZACC-60
3T3 cellsLeibniz Institute DSMZACC-59
MicroscopeNicon Eclipse
CameraAndorDU888 Ultra
Confocal UnitYokagawaCSU-X1
PyruvateGibco31966-021

References

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  1. Dunaevsky, A., Tashiro, A., Majewska, A., Mason, C., Yuste, R. Developmental regulation of spine motility in the mammalian central nervous system. Proc Natl Acad Sci U S A. 96 (23), 13438-13443 (1999).
  2. Matus, A., Brinkhaus, H., Wagner, U.

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Tags

Filopodia TrackingProtein ConcentrationImage Analysis SoftwareProtrusion DynamicsGraphical User InterfaceSpatial Temporal AnalysisProtein LocalizationCell MigrationActin FilamentsRatiometric Protein Analysis

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