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Biology
Imaging locale Ca 2+ Segnali in cellule di mammifero coltivate
Imaging locale Ca 2+ Segnali in cellule di mammifero coltivate
JoVE Journal
Biology
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JoVE Journal Biology
Imaging Local Ca2+ Signals in Cultured Mammalian Cells

Imaging locale Ca 2+ Segnali in cellule di mammifero coltivate

Full Text
11,508 Views
09:30 min
March 3, 2015

DOI: 10.3791/52516-v

Jeffrey T. Lock1, Kyle L. Ellefsen1, Bret Settle1, Ian Parker1,2, Ian F. Smith1

1Neurobiology and Behavior,University of California, Irvine, 2Physiology and Biophysics,University of California, Irvine

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Please note that some of the translations on this page are AI generated. Click here for the English version.

Overview

This article presents techniques for imaging local IP3-mediated Ca2+ events in intact mammalian cells using fluorescence microscopy. The method involves loading cells with calcium indicators and employing an algorithm for automated event identification and analysis.

Key Study Components

Area of Science

  • Neuroscience
  • Cell Biology
  • Fluorescence Microscopy

Background

  • Understanding calcium signaling is crucial for cellular processes.
  • IP3 plays a significant role in mediating calcium release from the endoplasmic reticulum.
  • Fluorescence microscopy allows for real-time imaging of calcium dynamics.
  • Automated analysis enhances the efficiency of data interpretation.

Purpose of Study

  • To demonstrate the acquisition of local IP3-mediated calcium signals.
  • To illustrate the detection and analysis of these signals in live cells.
  • To provide a protocol for researchers to replicate the imaging technique.

Methods Used

  • Culturing mammalian cells on glass bottom cover dishes.
  • Loading cells with cell membrane permeable fluorescent calcium indicators.
  • Using an inverted microscope with 488 nm light for excitation.
  • Inducing local calcium signals with a brief pulse of UV light.

Main Results

  • Successful imaging of local calcium signals in intact cells.
  • Demonstrated automation in the identification of calcium events.
  • Provided a clear protocol for future studies in calcium signaling.
  • Highlighted the role of IP3 in mediating calcium release.

Conclusions

  • The technique effectively captures local calcium signaling dynamics.
  • Automation improves the analysis of complex calcium events.
  • This method can be applied to various studies involving calcium signaling.

Frequently Asked Questions

What is the significance of IP3 in calcium signaling?
IP3 is crucial for mediating calcium release from the endoplasmic reticulum, impacting various cellular functions.
How does fluorescence microscopy aid in studying calcium events?
Fluorescence microscopy allows for real-time visualization of calcium dynamics within live cells.
What are the advantages of using automated analysis?
Automated analysis enhances efficiency and accuracy in identifying and quantifying calcium signaling events.
Can this method be applied to other types of cells?
Yes, the technique can be adapted for various cell types to study calcium signaling.
What are the key steps in the imaging protocol?
Key steps include culturing cells, loading indicators, and using specific light wavelengths for excitation.
What role does UV light play in this study?
UV light is used to photo-liberate IP3 from a caged precursor, initiating calcium release.

Qui presentiamo tecniche per l'imaging di eventi locali di Ca2+ mediati da IP3 utilizzando la microscopia a fluorescenza in cellule di mammifero intatte caricate con indicatori di Ca2+ insieme a un algoritmo che automatizza l'identificazione e l'analisi di questi eventi.

L'obiettivo generale di questa procedura è dimostrare l'acquisizione, il rilevamento e l'analisi dei segnali di calcio mediati da IP 3 locali in cellule di mammifero intatte utilizzando l'imaging basato su telecamera. Ciò si ottiene coltivando prima le cellule sui piatti di copertura del fondo di vetro e caricandole con le forme permeabili alla membrana cellulare dell'indicatore di calcio fluorescente. CAL cinque 20 e IP in gabbia tre.

Il secondo passo consiste nel posizionare il vetro di copertura sul tavolino di un microscopio invertito e illuminare il campione con luce a 488 nanometri per eccitare il colorante fluorescente sensibile al calcio Cal five 20. Successivamente, i segnali locali di calcio vengono indotti esponendo le cellule a un breve impulso di luce UV. Questa foto libera l'IP 3 da un precursore in gabbia in modo tale che ora possa legarsi al recettore dell'acetolo trisfosfato e mediare il rilascio di calcio dal reticolo endoplasmatico.

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