JoVE Journal

Biochemistry

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Simultaneous Interference Reflection and Total Internal Reflection Fluorescence Microscopy for Imaging Dynamic Microtubules and Associated Proteins

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3.4K Views

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06:43 min

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May 3rd, 2022

DOI :

10.3791/63730-v

May 3rd, 2022

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Yazgan Tuna¹, Amer Al-Hiyasat¹, Jonathon Howard¹^,²

¹Department of Molecular Biophysics & Biochemistry, Yale University, ²Department of Physics, Yale University

Podsumowanie

We present a protocol for implementing interference-reflection microscopy and total-internal-reflection-fluorescence microscopy for the simultaneous imaging of dynamic microtubules and fluorescently labeled microtubule-associated proteins.

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Simultaneous Interference Reflection

Total Internal Reflection Fluorescence Microscopy

Dynamic Microtubules

Label free Imaging

PDMS Polymer Preparation

Plasma Cleaning

Fluorescent Microbeads

Tubulin Extension Mixture

Rozdziały w tym wideo

0:05

Introduction

0:29

Preparation of PDMS Channels

2:15

Preparation for Imaging

3:02

Growing Dynamic Guanosine Diphosphate “Extensions”

3:46

Kinesin Motility Assay

4:23

Image Processing and Analysis

5:22

Results: Imaging of Dynamic Microtubules and Fluorescently Labeled Microtubule-Associated Proteins

5:57

Conclusion

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