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JoVE Journal
Biology
Misurazioni FLIM-FRET delle interazioni proteina-proteina nei batteri vivi.
Misurazioni FLIM-FRET delle interazioni proteina-proteina nei batteri vivi.
JoVE Journal
Biology
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JoVE Journal Biology
FLIM-FRET Measurements of Protein-Protein Interactions in Live Bacteria.

Misurazioni FLIM-FRET delle interazioni proteina-proteina nei batteri vivi.

Full Text
10,038 Views
09:26 min
August 25, 2020

DOI: 10.3791/61602-v

Hanna Manko1, Vincent Normant2,3, Quentin Perraud2,3, Tania Steffan1, Véronique Gasser2,3, Emmanuel Boutant1, Éléonore Réal1, Isabelle J. Schalk2,3, Yves Mély1, Julien Godet1,4

1Université de Strasbourg,Laboratoire de Bioimagerie et Pathologies, UMR CNRS 7021, 2Université de Strasbourg, UMR 7242, ESBS, 3CNRS, UMR 7242, ESBS, 4Groupe Méthode Recherche Clinique,Hôpitaux Universitaires de Strasbourg

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Overview

This study presents a protocol for characterizing protein-protein interactions in live Pseudomonas aeruginosa through FLIM-FRET measurements. The approach focuses on analyzing interactions between two proteins expressed at significantly different levels within the native cellular environment.

Key Study Components

Research Area

  • Protein-protein interactions
  • Live cell imaging
  • Molecular biology techniques

Background

  • The necessity of studying protein interactions in native cellular contexts.
  • FLIM-FRET as an advanced method for investigating these interactions.
  • Challenges in analyzing unbalanced donor and acceptor protein ratios.

Methods Used

  • FLIM-FRET measurements
  • Pseudomonas aeruginosa as the biological model organism
  • Data acquisition and analysis using microscopy and RStudio

Main Results

  • Demonstrated successful identification of protein interactions in live cells.
  • Established that differences in protein expression levels can affect FRET efficiency.
  • Provided insights into the stoichiometry of proteins and their interactions.

Conclusions

  • The study validates the use of FLIM-FRET for probing protein interactions in living systems.
  • Findings contribute to the understanding of molecular interactions crucial for cellular processes.

Frequently Asked Questions

What is FLIM-FRET?
FLIM-FRET is a technique used to measure protein-protein interactions in live cells by analyzing fluorescence lifetime changes.
Why is studying protein-protein interactions important?
Protein-protein interactions are vital for understanding cellular processes and signaling pathways, affecting function and regulation.
What organisms were used in this study?
Pseudomonas aeruginosa was the primary organism used for the experiments.
How can unbalanced donor and acceptor ratios affect results?
Unbalanced ratios can lead to inaccurate interpretations of FRET data, impacting the understanding of molecular interactions.
What software was utilized for data analysis?
RStudio was used to perform statistical analysis on the collected FLIM-FRET data.
Can FLIM-FRET be used for other biological systems?
Yes, FLIM-FRET can potentially be applied to various systems beyond Pseudomonas aeruginosa to study protein interactions.
What is the significance of the findings?
The findings enhance the understanding of protein interactions in living cells, which are essential for cellular function and signaling.

Descriviamo qui un protocollo per caratterizzare le interazioni proteina-proteina tra due proteine espresse in modo molto diverso nelle Pseudomonas aeruginosa vive usando misurazioni FLIM-FRET. Il protocollo include costruzioni di ceppo batterico, immobilizzazione dei batteri, routine di analisi dei dati di imaging e post-imaging.

FILM-FRET è una tecnica potente che consente di confermare le interazioni proteina-proteina sospette o previste. In questo protocollo, presentiamo un modo per analizzare i dati in particolari casi di quantità di donatori e accettori squilibrati. FILM-FRET è in grado di fornire informazioni sulle interazioni proteina-proteina direttamente nelle cellule vive.

È importante indagare le interazioni personali-proteiche nell'ambiente cellulare nativo, in particolare quando le proteine fluorescenti sono espresse nel livello endogeno. Inizia coltivando batteri aiutanti P.aeruginosa, E.coli TOP10 ed E.coli ciascuno in cinque millilitri di LB senza antibiotico a 30 gradi Celsius mentre tremano durante la notte. Il giorno successivo, misurare la densità ottica delle colture e mescolare una quantità uguale di P.aeruginosa, E.coli TOP10 ed E.coli aiutante in un microtubo da 1,5 millilitri.

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Biologia Numero 162 FRET-FLIM interazioni proteina-proteina Pseudomonas aeruginosa batteri imaging fluorescenza

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