Brightness experiments

Patrick J. MacDonald; Jolene Johnson; Yan Chen; Joachim D. Mueller

doi:10.1007/978-1-62703-649-8_32

Brightness experiments

Patrick J. MacDonald, Jolene Johnson, Yan Chen, Joachim D. Mueller

Physics and Astronomy (Twin Cities)

Research output: Chapter in Book/Report/Conference proceeding › Chapter

6 Scopus citations

Abstract

This chapter presents an overview of quantitative fluorescence brightness experiments with special emphasis on single-color measurements of protein homo-interactions inside living cells. We discuss practical considerations in the choice of the fluorescent labels and the calibration measurements necessary for quantitative interpretation of brightness experiments. Methods to identify and avoid common pitfalls, such as bleaching and saturation, are addressed. We examine the interpretation of brightness data with moment analysis. In particular, we focus on how to avoid or correct for undersampling, as well as how to characterize and adjust for photon detector effects. We conclude by describing brightness titration experiments which determine the binding curve and stoichiometry of a protein from apparent brightness data.

Original language	English (US)
Title of host publication	Fluorescence Spectroscopy and Microscopy
Subtitle of host publication	Methods and Protocols
Publisher	Humana Press Inc.
Pages	699-718
Number of pages	20
ISBN (Print)	9781627036481
DOIs	https://doi.org/10.1007/978-1-62703-649-8_32
State	Published - 2014

Publication series

Name	Methods in Molecular Biology
Volume	1076
ISSN (Print)	1064-3745

Keywords

Afterpulsing
Autocorrelation
Dead time
Fluctuation
Photobleaching
Photon count moments
Stoichiometry
Titration
Two-photon

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title = "Brightness experiments",

abstract = "This chapter presents an overview of quantitative fluorescence brightness experiments with special emphasis on single-color measurements of protein homo-interactions inside living cells. We discuss practical considerations in the choice of the fluorescent labels and the calibration measurements necessary for quantitative interpretation of brightness experiments. Methods to identify and avoid common pitfalls, such as bleaching and saturation, are addressed. We examine the interpretation of brightness data with moment analysis. In particular, we focus on how to avoid or correct for undersampling, as well as how to characterize and adjust for photon detector effects. We conclude by describing brightness titration experiments which determine the binding curve and stoichiometry of a protein from apparent brightness data.",

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AU - MacDonald, Patrick J.

AU - Johnson, Jolene

AU - Chen, Yan

AU - Mueller, Joachim D.

PY - 2014

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N2 - This chapter presents an overview of quantitative fluorescence brightness experiments with special emphasis on single-color measurements of protein homo-interactions inside living cells. We discuss practical considerations in the choice of the fluorescent labels and the calibration measurements necessary for quantitative interpretation of brightness experiments. Methods to identify and avoid common pitfalls, such as bleaching and saturation, are addressed. We examine the interpretation of brightness data with moment analysis. In particular, we focus on how to avoid or correct for undersampling, as well as how to characterize and adjust for photon detector effects. We conclude by describing brightness titration experiments which determine the binding curve and stoichiometry of a protein from apparent brightness data.

AB - This chapter presents an overview of quantitative fluorescence brightness experiments with special emphasis on single-color measurements of protein homo-interactions inside living cells. We discuss practical considerations in the choice of the fluorescent labels and the calibration measurements necessary for quantitative interpretation of brightness experiments. Methods to identify and avoid common pitfalls, such as bleaching and saturation, are addressed. We examine the interpretation of brightness data with moment analysis. In particular, we focus on how to avoid or correct for undersampling, as well as how to characterize and adjust for photon detector effects. We conclude by describing brightness titration experiments which determine the binding curve and stoichiometry of a protein from apparent brightness data.

KW - Afterpulsing

KW - Autocorrelation

KW - Dead time

KW - Fluctuation

KW - Photobleaching

KW - Photon count moments

KW - Stoichiometry

KW - Titration

KW - Two-photon

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EP - 718

BT - Fluorescence Spectroscopy and Microscopy

PB - Humana Press Inc.

ER -

Brightness experiments

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