fluorescence lifetime imaging of polyq protein aggregation in caenorhabditis elegans neurons

Fluorescence Lifetime Imaging of PolyQ Protein Aggregation in Caenorhabditis elegans Neurons

Make sure the nematodes are completely immobile. Open the FLIM acquisition software. Locate the Tab button and press Enable Outputs. Place the slide with the mounted&#160;C. elegans on the stage and, using a 10 times magnification lens in transmission mode, localize the position of the nematodes on the slide. Remove the slide, switch the objective to a 63 times magnification lens, and apply the required immersion medium.Place the slide on the stage and localize the nematodes. Start scanning the sample. Select a region of interest and focus on its maximum projection plane. On the interface of the FLIM software, preview the number of photons detected. The ADC value should be between 1 times 10 to the fourth and 1 times 10 to the fifth. If necessary, shift the focus on a different plane or increase the laser power to collect more photons.- Ensure that you avoid photon pileup, but collect a sufficient amount of photons to create a good lifetime fit and measurement.- In the menu bar, select the tab to set the acquisition parameters. Select Scan Sync In to allow for single photon detection. Set the acquisition to a fixed amount of time or a fixed number of photons. Press Start to begin acquisition. Open the software and import FLIM data files via File, Load FLIM Data. Load all the samples from one condition, even if obtained in different sessions and from different biological repeats.If necessary, segment a single nematode for many FLIM picture via Segmentation, Segmentation Manager. Drag the cropping tool around the area of interest until it is highlighted. Once completed, press OK. Select a small region where the intensity-based image of a&#160;C. elegans appears. The decay curve of that region appears in the large decay window on the right side of the interface.To extrapolate the lifetime on the Data tab, set an arbitrary integrated minimum value between 40 to 300 to exclude any pixels that are too dim to produce a good fit. Select a time minimum and a time maximum number to limit the FLIM signal to these values. Do not change the preset counts photon of one. Input the repetition rate in megahertz of the laser utilized during acquisition.Input a gate max value to exclude all saturated pixels. On the Lifetime tab, select a global fitting to be used. Do not change any other parameter except the number of exponential selection if it is known that the chosen fluorescence decay is multiexponential and exhibits more than a single lifetime.Upload the IRF via the IRF menu. To estimate the IRF shift, select IRF, Estimate, IRF Shift. A set of values automatically appears on the IRF tab. Once this is established, do not change any other parameters of this tab. Once all parameters are set, press Fit Data Set. The resulting fit highlighted in a blue line should overlap with all the events. A good fit is obtained when all events are aligned along the fit.Click the Parameters tab located within the top right menus of the software's interface, and select statistic, weighted mean, and check that the chi-square value is as close as possible to one. The lifetime value of the selected image is thus revealed as tau 1. Export any information of interest through File, Export Intensity Images, Fit Result Table, Images, Histograms.

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Source:&#160;Pigazzini, M. L.,&#160;et. al. Characterization of Amyloid Structures in Aging&#160;C. Elegans Using Fluorescence Lifetime Imaging.&#160;J. ...

Begin with anesthetized, age-matched control and chaperone-deficient&#160;Caenorhabditis elegans worms.&#160;Both groups express fluorophore-tagged polyQ proteins in their neurons that are prone to misfolding.&#160;In control worms, chaperone proteins limit misfolded polyQ aggregation, whereas, in chaperone-deficient worms, misfolded polyQ readily forms aggregates.&#160;Place the control slide on a confocal microscope stage for Fluorescence Lifetime Imaging Microscopy (FLIM).&#160;Illuminate the worms using a pulsed laser.&#160;The laser excites the fluorophore, which emits a photon as it returns to the ground state.&#160;FLIM measures fluorescence lifetime&#8212;the duration the fluorophore remains in its excited state.In chaperone-deficient worms, polyQ aggregation clusters fluorophores, promoting energy transfer between adjacent fluorophores instead of photon emission, thereby reducing fluorescence lifetime. &#160;&#160;The FLIM software processes these lifetimes to generate color-coded maps, enabling aggregation visualization.A reduced fluorescence lifetime in chaperone-deficient worms, compared to controls, indicates increased polyQ aggregation.

33 Views. Fluorescence Lifetime Imaging of PolyQ Protein Aggregation in Caenorhabditis elegans Neurons

Video: Fluorescence Lifetime Imaging of PolyQ Protein Aggregation in Caenorhabditis elegans Neurons - Experiment

Imaging Amyloid Tissues Stained with Luminescent Conjugated Oligothiophenes by Hyperspectral Confocal Microscopy and Fluorescence Lifetime Imaging

Proteins that deposit as amyloid in tissues throughout the body can be the cause or consequence of a large number of diseases. Among these we find neurodegenerative diseases such as Alzheimer&#39;s and Parkinson&#39;s disease afflicting primarily the central nervous system, and systemic amyloidosis where serum amyloid A, transthyretin and IgG light chains deposit as amyloid in liver, carpal tunnel, spleen, kidney, heart, and other peripheral tissues. Amyloid has been known and studied for more than a century, often using amyloid specific dyes such as Congo red and Thioflavin T (ThT) or Thioflavin (ThS). In this paper, we present heptamer-formyl thiophene acetic acid (hFTAA) as an example of recently developed complements to these dyes called luminescent conjugated oligothiophenes (LCOs). hFTAA is easy to use and is compatible with co-staining in immunofluorescence or with other cellular markers. Extensive research has proven that hFTAA detects a wider range of disease associated protein aggregates than conventional amyloid dyes. In addition, hFTAA can also be applied for optical assignment of distinct aggregated morphotypes to allow studies of amyloid fibril polymorphism. While the imaging methodology applied is optional, we here demonstrate hyperspectral imaging (HIS), laser scanning confocal microscopy and fluorescence lifetime imaging (FLIM). These examples show some of the imaging techniques where LCOs can be used as tools to gain more detailed knowledge of the formation and structural properties of amyloids. An important limitation to the technique is, as for all conventional optical microscopy techniques, the requirement for microscopic size of aggregates to allow detection. Furthermore, the aggregate should comprise a repetitive &#946;-sheet structure to allow for hFTAA binding. Excessive fixation and/or epitope exposure that modify the aggregate structure or conformation can render poor hFTAA binding and hence pose limitations to accurate imaging.

Amyloid deposition is a hallmark of different diseases and afflicts many different organs. This paper describes the application of luminescent conjugated oligothiophene fluorescence staining in combination with fluorescence microscopy techniques. This staining method represents a powerful tool for detection and exploration of protein aggregates in both clinical and scientific setups.

Proteins that deposit as amyloid in tissues throughout the body can be the cause or consequence of a large number of diseases. Among these we find ...

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Biochemistry

Visualizing Intracellular SNARE Trafficking by Fluorescence Lifetime Imaging Microscopy

Soluble N-ethylmaleimide sensitive fusion protein (NSF) attachment protein receptor (SNARE) proteins are key for membrane trafficking, as they catalyze membrane fusion within eukaryotic cells. The SNARE protein family consists of about 36 different members. Specific intracellular transport routes are catalyzed by specific sets of 3 or 4 SNARE proteins that thereby contribute to the specificity and fidelity of membrane trafficking. However, studying the precise function of SNARE proteins is technically challenging, because SNAREs are highly abundant and functionally redundant, with most SNAREs having multiple and overlapping functions. In this protocol, a new method for the visualization of SNARE complex formation in live cells is described. This method is based on expressing SNARE proteins C-terminally fused to fluorescent proteins and measuring their interaction by F&#246;rster resonance energy transfer (FRET) employing fluorescence lifetime imaging microscopy (FLIM). By fitting the fluorescence lifetime histograms with a multicomponent decay model, FRET-FLIM allows (semi-)quantitative estimation of the fraction of the SNARE complex formation at different vesicles. This protocol has been successfully applied to visualize SNARE complex formation at the plasma membrane and at endosomal compartments in mammalian cell lines and primary immune cells, and can be readily extended to study SNARE functions at other organelles in animal, plant, and fungal cells.

This protocol describes a new method allowing for the quantitative visualization of complex formation of SNARE proteins, based on F&#246;rster resonance energy transfer, and fluorescence lifetime imaging microscopy.

Soluble N-ethylmaleimide sensitive fusion protein (NSF) attachment protein receptor (SNARE) proteins are key for membrane trafficking, as they catalyze ...

Immunology and Infection

Effect of Fluorescent Proteins on Fusion Partners Using Polyglutamine Toxicity Assays in Yeast

For the investigation of protein localization and trafficking using live cell imaging, researchers often rely on fusing their protein of interest to a fluorescent reporter. The constantly evolving list of genetically encoded fluorescent proteins (FPs) presents users with several alternatives when it comes to fluorescent fusion design. Each FP has specific optical and biophysical properties that can affect the biochemical, cellular, and functional properties of the resulting fluorescent fusions. For instance, several FPs tend to form nonspecific oligomers that are susceptible to impede on the function of the fusion partner. Unfortunately, only a few methods exist to test the impact of FPs on the behavior of the fluorescent reporter. Here, we describe a simple method that enables the rapid assessment of the impact of FPs using polyglutamine (polyQ) toxicity assays in the budding yeast Saccharomyces cerevisiae. PolyQ-expanded huntingtin proteins are associated with the onset of Huntington&#39;s disease (HD), where the expanded huntingtin aggregates into toxic oligomers and inclusion bodies. The aggregation and toxicity of polyQ expansions in yeast are highly dependent on the sequences flanking the polyQ region, including the presence of fluorescent tags, thus providing an ideal experimental platform to study the impact of FPs on the behavior of their fusion partner.

This article describes protocols to assess the effect of fluorescent proteins on the aggregation and toxicity of misfolded polyglutamine expansion for the rapid evaluation of a newly uncharacterized fluorescent protein in the context of fluorescent reporters.

For the investigation of protein localization and trafficking using live cell imaging, researchers often rely on fusing their protein of interest to a ...

Fluorescence Lifetime Imaging of PolyQ Protein Aggregation in Caenorhabditis elegans Neurons

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Fluorescence Lifetime Imaging of PolyQ Protein Aggregation in Caenorhabditis elegans Neurons