Bleed-through correction for rendering and correlation analysis in multi-colour localization microscopy

Kim, Dahan; Curthoys, Nikki M.; Parent, Matthew; Hess, Samuel T.

doi:10.1088/2040-8978/15/9/094011

Cited by 28 publications

(17 citation statements)

References 34 publications

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“…NIH-3T3 (ATCC, Manassas, VA) cells were transfected with Lipofectamine 2000 as per the manufacturer's protocol (Lipofectamine 2000, Invitrogen) with Dendra2-Hemagluttinin (HA)[ 15 ] or Dendra2-actin[ 16 ], PAmCherry-cofilin[ 17 ] or PAmCherry-tropomyosin4[ 16 ], or PAmKate-Transferin Receptor (TfR)[ 8 ]. For antibody labeling, NIH-3T3 cells were first fixed with 4% PFA.…”

Section: Methodsmentioning

confidence: 99%

Super-Resolution Imaging of Molecular Emission Spectra and Single Molecule Spectral Fluctuations

et al. 2016

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Localization microscopy can image nanoscale cellular details. To address biological questions, the ability to distinguish multiple molecular species simultaneously is invaluable. Here, we present a new version of fluorescence photoactivation localization microscopy (FPALM) which detects the emission spectrum of each localized molecule, and can quantify changes in emission spectrum of individual molecules over time. This information can allow for a dramatic increase in the number of different species simultaneously imaged in a sample, and can create super-resolution maps showing how single molecule emission spectra vary with position and time in a sample.

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Section: Methodsmentioning

confidence: 99%

Super-Resolution Imaging of Molecular Emission Spectra and Single Molecule Spectral Fluctuations

et al. 2016

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“…This experimental pitfall can be overcome by imaging two distinguishable sets of molecules to measure their co-distribution 145, 147-149 . This too is not without experimental complexities: fluorescent impurities and spectral overlap can give rise to misidentification and artifactual co-localization 150, 151 . Although the currently available number and types of fluorophores limit these approaches, probe development is an active area of research.…”

Section: Detecting Rafts Using Super-resolution Microscopymentioning

confidence: 99%

The Continuing Mystery of Lipid Rafts

Levental¹,

Veatch

2016

Journal of Molecular Biology

245

251

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Since its initial formalization nearly twenty years ago, the concept of lipid rafts has generated a tremendous amount of attention and interest, and nearly as much controversy. The controversy is perhaps surprising because the notion itself is intuitive: compartmentalization in time and space is a ubiquitous theme at all scales of biology, and therefore the partitioning of cellular membranes into lateral subdivision should be expected. Nevertheless, the physicochemical principles responsible for compartmentalization and the molecular mechanisms by which they are functionalized remain nearly as mysterious today as they were two decades ago. Herein, we review recent literature on this topic with a specific focus on the major open questions in the field, including: (1) what are the best tools to assay raft behavior in living membranes; (2) what is the function of the complex lipidome of mammalian cells with respect to membrane organization; (3) what are the mechanisms that drive raft formation and determine their properties; (4) how can rafts be modulated; (5) how is membrane compartmentalization integrated into cellular signaling. Despite decades of intensive research, this compelling field remains full of fundamental questions.

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“…Nevertheless, successful pairings have been described ( Kozma and Kele, 2019 ), and new FPs have been introduced to facilitate multicolor imaging ( Gunewardene et al., 2011 ). That being said, it is nonetheless important to conduct appropriate controls and correct for bleed-through/cross-talk effects in multicolor experiments ( Bolte and Cordelieres, 2006 ), for which various approaches have been described ( Kim et al., 2013 ; Maddipatla and Tankam, 2020 ). When an adequate combination of fluorophores cannot be found, as is often the case when imaging three or more colors, different techniques can be used to separate the overlapping emissions.…”

Section: Challenges (And Solutions) In Achieving Quantitative Srmmentioning

confidence: 99%

Challenges facing quantitative large-scale optical super-resolution, and some simple solutions

Dankovich

Rizzoli

2021

iScience

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Summary Optical super-resolution microscopy (SRM) has enabled biologists to visualize cellular structures with near-molecular resolution, giving unprecedented access to details about the amounts, sizes, and spatial distributions of macromolecules in the cell. Precisely quantifying these molecular details requires large datasets of high-quality, reproducible SRM images. In this review, we discuss the unique set of challenges facing quantitative SRM, giving particular attention to the shortcomings of conventional specimen preparation techniques and the necessity for optimal labeling of molecular targets. We further discuss the obstacles to scaling SRM methods, such as lengthy image acquisition and complex SRM data analysis. For each of these challenges, we review the recent advances in the field that circumvent these pitfalls and provide practical advice to biologists for optimizing SRM experiments.

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Bleed-through correction for rendering and correlation analysis in multi-colour localization microscopy

Cited by 28 publications

References 34 publications

Super-Resolution Imaging of Molecular Emission Spectra and Single Molecule Spectral Fluctuations

Super-Resolution Imaging of Molecular Emission Spectra and Single Molecule Spectral Fluctuations

The Continuing Mystery of Lipid Rafts

Challenges facing quantitative large-scale optical super-resolution, and some simple solutions

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