Your search keyword '"Fluorescent Dyes analysis"' showing total 143 results

1. DIGE Analysis of Fish Tissues.

Author

Nynca J, Dietrich MA, and Ciereszko A

Subjects

Animals, Staining and Labeling, Two-Dimensional Difference Gel Electrophoresis methods, Isoelectric Focusing, Proteins, Fishes, Electrophoresis, Gel, Two-Dimensional methods, Proteomics methods, Fluorescent Dyes analysis

Abstract

Two-dimensional difference gel electrophoresis (2D-DIGE) appears to be especially useful in quantitative approaches, allowing the co-separation of proteins of control samples and proteins of treated/disease samples on the same gel, eliminating gel-to-gel variability. The principle of 2D-DIGE is to label proteins prior to isoelectric focusing and use three spectrally resolvable fluorescent dyes, allowing the independent labeling of control and experimental samples. This procedure makes it possible to reduce the number of gels in an experiment, allowing the accurate and reproducible quantification of multiple samples. 2D-DIGE has been found to be an excellent methodical tool in several areas of fish research, including environmental pollution and toxicology, the mechanisms of development and disorders, reproduction, nutrition, evolution, and ecology., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

2. Comparative Two-Dimensional Fluorescence Gel Electrophoresis.

Author

Ackermann D and König S

Subjects

Reproducibility of Results, Electrophoresis, Gel, Two-Dimensional methods, Fluorescent Dyes analysis, Two-Dimensional Difference Gel Electrophoresis methods, Electrophoresis, Polyacrylamide Gel, Proteomics methods, Proteome

Abstract

Two-dimensional comparative fluorescence gel electrophoresis (CoFGE) uses an internal standard to increase the reproducibility of coordinate assignment for protein spots visualized on 2D polyacrylamide gels. This is particularly important for samples that need to be compared without the availability of replicates and thus cannot be studied using differential gel electrophoresis (DIGE). CoFGE corrects for gel-to-gel variability by co-running with the sample proteome a standardized marker grid of 80-100 nodes, which is formed by a set of purified proteins. Differentiating of reference and analyte is possible by the use of two fluorescent dyes. Variations in the y-dimension (molecular weight) are corrected by the marker grid. For the optional control of the x-dimension (pI), azo-dyes can be used. Experiments are possible in both vertical and horizontal (h) electrophoresis devices, but hCoFGE is much easier to perform. The CoFGE experimental principle can additionally be used for protein quantification. For data analysis, commercial software has been adapted., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

3. Choosing Fluorescent Probes and Labeling Systems.

Author

Jacoby-Morris K and Patterson GH

Subjects

Animals, COS Cells, Chlorocebus aethiops, Fluorescent Dyes chemistry, Humans, Molecular Structure, Nanoparticles, Single Molecule Imaging, Fluorescent Dyes analysis, Microscopy, Fluorescence methods, Staining and Labeling methods

Abstract

Fluorescence microscopy is advantageous for investigating biological processes and mechanisms in living cells. One of the most important considerations when designing an experiment is the selection of an appropriate fluorescent probe. Equally important is deciding how the probe will be attached to the protein of interest. The advantages and disadvantages of different fluorescent probe types and their respective labeling methods are discussed to provide an overview on selecting appropriate fluorophores and labeling systems for fluorescence-based assays. Protocols are outlined when appropriate.

Published

2021

4. FRET Analysis of RNA -Protein Interactions Using Spinach Aptamers.

Author

Gerhard L and Hennig S

Subjects

Amino Acid Sequence, Bacteriophages chemistry, Base Sequence, Capsid Proteins genetics, Capsid Proteins metabolism, Chromatography, Gel methods, Cloning, Molecular methods, Dimerization, Luminescent Proteins genetics, Nucleic Acid Conformation, Protein Binding, RNA isolation & purification, RNA metabolism, Red Fluorescent Protein, Aptamers, Nucleotide metabolism, Fluorescence Resonance Energy Transfer methods, Fluorescent Dyes analysis, Luminescent Proteins analysis, RNA-Binding Proteins metabolism

Abstract

The method development to analyze direct RNA-protein interaction is of high importance as not many homogeneous assay formats are available.The discovery of fluorescent light-up aptamers (FLAPs), short RNA aptamers that switch the fluorescence of small, cell-permeable, and nontoxic organic chromophores on, paved the road for their utilization in direct RNA -protein interactions. The combination with fluorescent proteins as biological fluorophores enabled the development of homogeneous assays that are in principle even encodable on genomic level.Here the rules and methods to design a homogeneous in vitro assay for the detection and quantification of a direct RNA -protein interaction will be described. The design and application of a homogeneous assay to observe and quantify the interaction of the Pseudomonas aeruginosa bacteriophage coat protein 7 (PP7) with its binding RNA sequence (pp7-RNA) will be shown. For this, the Spinach-DFHBI aptamer as RNA fusion and the red fluorescent mCherry as protein fusion was used.The methods presented here do not require any chemical modification of proteins or RNAs which make them relatively easy to use and to adopt on other systems. As all fluorophores are fusion tags to the according biomolecules, standard cloning strategies and molecular biology technologies are sufficient and make this method available for a broad community of researchers.

Published

2021

5. Live-Cell Imaging of Sirtuin Activity Using a One-Step Fluorescence Probe.

Author

Kawaguchi M and Nakagawa H

Subjects

Enzyme Inhibitors pharmacology, Fluorescent Dyes chemistry, HEK293 Cells, Humans, Sirtuin 1 antagonists & inhibitors, Diagnostic Imaging methods, Fluorescent Dyes analysis, Microscopy, Fluorescence methods, Sirtuin 1 metabolism

Abstract

Sirtuins (SIRTs) are a family of NAD + -dependent histone deacetylases (HDACs). In mammals, dysfunction of SIRTs is associated with age-related metabolic diseases, cancers, and even aging. Therefore, the detection of SIRT activity in living cells or tissues would be helpful for diagnosis of a wide range of SIRT-associated diseases. Here, we present methodology to measure SIRT activity in living cells by using our newly developed SIRT fluorescence probe, KST-F-DA.

Published

2021

6. Live Cell Imaging Using Riboswitch-Spinach tRNA Fusions as Metabolite-Sensing Fluorescent Biosensors.

Author

Manna S, Kellenberger CA, Hallberg ZF, and Hammond MC

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Benzyl Compounds, Cloning, Molecular methods, Cyclic GMP analogs & derivatives, Cyclic GMP metabolism, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Imidazolines, Isopropyl Thiogalactoside pharmacology, Nucleic Acid Conformation, Phosphorus-Oxygen Lyases genetics, Phosphorus-Oxygen Lyases metabolism, Plasmids, Aptamers, Nucleotide genetics, Biosensing Techniques methods, Flow Cytometry methods, Fluorescent Dyes analysis, Intravital Microscopy methods, Microscopy, Fluorescence methods, RNA genetics, RNA, Transfer genetics, Riboswitch genetics

Abstract

The development of fluorescent biosensors is motivated by the desire to monitor cellular metabolite levels in real time. Most genetically encodable fluorescent biosensors are based on receptor proteins fused to fluorescent protein domains. More recently, small molecule-binding riboswitches have been adapted for use as fluorescent biosensors through fusion to the in vitro selected Spinach aptamer, which binds a profluorescent, cell-permeable small molecule mimic of the GFP chromophore, DFHBI. Here we describe methods to prepare and analyze riboswitch-Spinach tRNA fusions for ligand-dependent activation of fluorescence in vivo. Example procedures describe the use of the Vc2-Spinach tRNA biosensor to monitor perturbations in cellular levels of cyclic di-GMP using either fluorescence microscopy or flow cytometry. In this updated chapter, we have added procedures on using biosensors in flow cytometry to detect exogenously added compounds. The relative ease of cloning and imaging of these biosensors, as well as their modular nature, should make this method appealing to other researchers interested in utilizing riboswitch-based biosensors for metabolite sensing.

Published

2021

7. Detection of Neutrophils in the Sciatic Nerve Following Peripheral Nerve Injury.

Author

Niemi JP, Lindborg JA, and Zigmond RE

Subjects

Animals, Antigens, Ly analysis, Axotomy, Biomarkers, CD11b Antigen analysis, Cell Separation, Fluorescent Dyes analysis, Frozen Sections, Indoles analysis, Mice, Peripheral Nerve Injuries immunology, Peroxidase analysis, Phagocytosis, Sciatic Nerve injuries, Sciatic Nerve pathology, Staining and Labeling methods, Wallerian Degeneration immunology, von Willebrand Factor analysis, Flow Cytometry methods, Immunohistochemistry methods, Neutrophils enzymology, Neutrophils pathology, Peripheral Nerve Injuries pathology, Wallerian Degeneration pathology

Abstract

Injury to the sciatic nerve leads to degeneration and debris clearance in the area distal to the injury site, a process known as Wallerian degeneration. Immune cell infiltration into the distal sciatic nerve plays a major role in the degenerative process and subsequent regeneration of the injured motor and sensory axons. While macrophages have been implicated as the major phagocytic immune cell participating in Wallerian degeneration, recent work has found that neutrophils, a class of short-lived, fast responding white blood cells, also significantly contribute to the clearance of axonal and myelin debris. Detection of specific myeloid subtypes can be difficult as many cell-surface markers are often expressed on both neutrophils and monocytes/macrophages. Here we describe two methods for detecting neutrophils in the axotomized sciatic nerve of mice using immunohistochemistry and flow cytometry. For immunohistochemistry on fixed frozen tissue sections, myeloperoxidase and DAPI are used to specifically label neutrophils while a combination of Ly6G and CD11b are used to assess the neutrophil population of unfixed sciatic nerves using flow cytometry.

Published

2020

8. In Vivo Visualization of Moving Synaptic Cargo Complexes within Drosophila Larval Segmental Axons.

Author

Banerjee R, White JA 2nd, and Gunawardena S

Subjects

Amyloid beta-Protein Precursor analysis, Amyloid beta-Protein Precursor genetics, Animals, Axons metabolism, Computer Systems, Drosophila Proteins analysis, Drosophila Proteins genetics, Drosophila melanogaster growth & development, Fluorescent Dyes analysis, GTP Phosphohydrolases analysis, GTP Phosphohydrolases genetics, Kymography, Larva, Luminescent Proteins analysis, Luminescent Proteins genetics, R-SNARE Proteins analysis, R-SNARE Proteins genetics, Software, Synaptic Vesicles physiology, Axonal Transport, Drosophila melanogaster metabolism, Intravital Microscopy methods, Microscopy, Fluorescence methods, Synaptic Vesicles ultrastructure

Abstract

Identifying moving synaptic vesicle complexes and isolating specific proteins present within such complexes in vivo is challenging. Here we detail a protocol that we have developed that is designed to simultaneously visualize the axonal transport of two fluorescently tagged synaptic vesicle proteins in living Drosophila larval segmental nerves in real time. Using a beam-splitter and split view software, larvae expressing GFP-tagged Synaptobrevin (Syb) and mRFP-tagged Rab4-GTPase or YFP-tagged Amyloid Precursor protein (APP) and mRFP-tagged Rab4-GTPase are imaged simultaneously using separate wavelengths. Merged kymographs from the two wavelengths are evaluated for colocalization analysis. Vesicle velocity analysis can also be done. Such analysis enables us to visualize the motility behaviors of two synaptic proteins present on a single vesicle complex and identify candidate proteins moving on synaptic vesicles in vivo, under physiological conditions.

Published

2020

9. In Vivo Imaging of Anterograde and Retrograde Axonal Transport in Rodent Peripheral Nerves.

Author

Sleigh JN, Tosolini AP, and Schiavo G

Subjects

Animals, Endosomes ultrastructure, Fluorescent Dyes administration & dosage, Fluorescent Dyes analysis, Fluorescent Dyes pharmacokinetics, Genes, Reporter, Injections, Intramuscular, Intravital Microscopy instrumentation, Kinesins physiology, Muscle, Skeletal, Organelles ultrastructure, Peripheral Nerves ultrastructure, Rodentia, Sciatic Nerve physiology, Sciatic Nerve ultrastructure, Axonal Transport physiology, Intravital Microscopy methods, Nerve Degeneration pathology, Peripheral Nerves physiology

Abstract

Axonal transport, which is the process mediating the active shuttling of a variety cargoes from one end of an axon to the other, is essential for the development, function, and survival of neurons. Impairments in this dynamic process are linked to diverse nervous system diseases and advanced ageing. It is thus essential that we quantitatively study the kinetics of axonal transport to gain an improved understanding of neuropathology as well as the molecular and cellular mechanisms regulating cargo trafficking. One of the best ways to achieve this goal is by imaging individual, fluorescent cargoes in live systems and analyzing the kinetic properties of their progression along the axon. We have therefore developed an intravital technique to visualize different organelles, such as signaling endosomes and mitochondria, being actively transported in the axons of both motor and sensory neurons in live, anesthetized rodents. In this chapter, we provide step-by-step instructions on how to deliver specific organelle-targeting, fluorescent probes using several routes of administration to image individual cargoes being bidirectionally transported along axons within the exposed sciatic nerve. This method can provide detailed, physiologically relevant information on axonal transport, and is thus poised to elucidate mechanisms regulating this process in both health and disease.

Published

2020

10. Transcutaneous Measurement of Glomerular Filtration Rate in Rodents.

Author

Daniele C, Nardozi D, Torelli A, Khan AUM, and Gretz N

Subjects

Animals, Fluorescent Dyes administration & dosage, Fluorescent Dyes pharmacokinetics, Glomerular Filtration Rate physiology, Injections, Intravenous, Kidney Function Tests instrumentation, Mice, Rats, Renal Elimination physiology, Software, Spectroscopy, Near-Infrared instrumentation, Spectroscopy, Near-Infrared methods, Fluorescent Dyes analysis, Kidney metabolism, Kidney Function Tests methods

Abstract

Glomerular filtration rate (GFR) is considered the gold standard to test kidney function. However, the serial blood and/or urine sample collection required for the calculation of the GFR is stressful for the animal and time consuming for the experimenter. Here, we describe a transcutaneous assessment of renal function in conscious animals that does not require plasma or urine sampling and/or deep anesthesia. For the measurement, we use a near-infrared (NIR) device that records the excretion kinetic of the renal marker ABZWCY-HPβCD. ABZWCY-HPβCD is a new hydrophilic, stable, and nontoxic NIR fluorescent agent that can be used as a renal marker as it is filtrated and completely excreted through the kidneys into the urine without reabsorption or secretion and without accumulation in the skin. The data recorded in the device are then analyzed with "GFRmeasure," an open-source, freely downloadable, and user-friendly software.

Published

2020

11. Analyzing Subcellular Reorganization During Early Arabidopsis Embryogenesis Using Fluorescent Markers.

Author

Liao CY and Weijers D

Subjects

Arabidopsis cytology, Arabidopsis ultrastructure, Microscopy, Confocal instrumentation, Seeds cytology, Seeds ultrastructure, Arabidopsis embryology, Fluorescent Dyes analysis, Microscopy, Confocal methods, Seeds embryology

Abstract

Virtually all growth, developmental, physiological, and defense responses in plants are accompanied by reorganization of subcellular structures to enable altered cellular growth, differentiation or function. Visualizing cellular reorganization is therefore critical to understand plant biology at the cellular scale. Fluorescently labeled markers for organelles, or for cellular components are widely used in combination with confocal microscopy to visualize cellular reorganization. Early during plant embryogenesis, the precursors for all major tissues of the seedling are established, and in Arabidopsis, this entails a set of nearly invariant switches in cell division orientation and directional cell expansion. Given that these cellular reorganization events are genetically regulated and coupled to formative events in plant development, they offer a good model to understand the genetic control of cellular reorganization in plant development. Until recently, it has been challenging to visualize subcellular structures in the early Arabidopsis embryo for two reasons: embryos are deeply embedded in seed coat and fruit, and in addition, no dedicated fluorescent markers, expressed in the embryo, were available. We recently established both an imaging approach and a set of markers for the early Arabidopsis embryo. Here, we describe a detailed protocol to use these new tools in imaging cellular reorganization.

Published

2020

12. Single-Cell Live Imaging.

Author

Hiratsuka T and Komatsu N

Subjects

Animals, Cell Culture Techniques methods, Cell Survival, Cells, Cultured, Equipment Design, Fluorescence Resonance Energy Transfer instrumentation, Fluorescence Resonance Energy Transfer methods, Fluorescent Dyes analysis, Imaging, Three-Dimensional instrumentation, Imaging, Three-Dimensional methods, Mice, Microscopy, Fluorescence instrumentation, Optical Imaging instrumentation, Single-Cell Analysis instrumentation, Whole Body Imaging instrumentation, Whole Body Imaging methods, Microscopy, Fluorescence methods, Optical Imaging methods, Single-Cell Analysis methods

Abstract

Recent fluorescence microscopy allows for high-throughput acquisition of 5D (X, Y, Z, T, and Color) images in various targets such as cultured cells, 3D spheroid/organoid, and even living tissue with single-cell resolution. The technology is considered promising to augment insights on heterogeneous features of both physiological and pathological cell phenotypes, for instance, distinct responses of cancer cells to anticancer drug treatment. Here we overview microscopic applications to capture live cell events for different types of targets, together with a couple of proof of concepts. The 2D live imaging will be exemplified by a FRET-based time-lapse cultured cell imaging, and 3D tissue imaging protocol will be complemented with a method for mouse skin live imaging.

Published

2019

13. Correlative Live-Cell Imaging and Super-Resolution Microscopy of Autophagy.

Author

Karanasios E

Subjects

Adaptor Proteins, Signal Transducing analysis, Adaptor Proteins, Signal Transducing metabolism, Autophagosomes metabolism, Autophagosomes ultrastructure, Autophagy-Related Proteins analysis, Autophagy-Related Proteins metabolism, Cell Culture Techniques methods, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, HEK293 Cells, Humans, Image Processing, Computer-Assisted methods, Recombinant Proteins analysis, Recombinant Proteins metabolism, Transfection methods, Autophagy, Microscopy, Fluorescence methods, Optical Imaging methods

Abstract

Correlative live-cell imaging and super-resolution microscopy of autophagy was developed to combine the temporal resolution of time-lapse fluorescence microscopy with the spatial resolution of super-resolution microscopy. HEK293 cells that express recombinant proteins of interest fused to fluorescent tags are imaged live to capture the formation of autophagosomes, fixed on stage to "snap-freeze" these structures, stained with appropriate antibodies, relocated, and imaged at super resolution by direct stochastic optical reconstruction microscopy. This chapter provides an easy-to-follow protocol along with practical tips and background information to help set up and perform an experiment.

Published

2019

14. In Vitro Characterization of a Multidomain Glycosyltransferase Using Fluorescently Tagged Synthetic Acceptors.

Author

Williams DM, Ovchinnikova OG, and Whitfield C

Subjects

Bacterial Proteins chemistry, Chromatography, Thin Layer methods, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Glycosyltransferases chemistry, Humans, Klebsiella Infections microbiology, Klebsiella pneumoniae chemistry, Klebsiella pneumoniae metabolism, Mass Spectrometry methods, Nuclear Magnetic Resonance, Biomolecular methods, O Antigens metabolism, Protein Domains, Bacterial Proteins metabolism, Glycosyltransferases metabolism, Klebsiella pneumoniae enzymology

Abstract

In vitro assays using fluorescently tagged sugar residues can facilitate the characterization of glycosyltransferase function. Here we describe the use of in vitro assays to characterize the three glycosyltransferase modules of the protein designated WbbB from Klebsiella pneumoniae O12. This protein combines key activities necessary to synthesize the O antigenic polysaccharide portion of lipopolysaccharide. The specificities of the three glycosyltransferases were investigated in vitro, using purified proteins, the activated donor sugars (dTDP-Rha, UDP-GlcNAc and CMP-β-Kdo) and synthetic acceptors terminating in either α1,3-linked Rha or β1,4-linked GlcNAc. The reaction products were verified by mass spectrometry and nuclear magnetic resonance methods.

Published

2019

15. Laboratory Screening Protocol to Identify Novel Oleaginous Yeasts.

Author

Sitepu IR, Garay AL, Cajka T, Fiehn O, and Boundy-Mills KL

Subjects

Chromatography, Liquid methods, Fluorescent Dyes analysis, Lipidomics methods, Mass Spectrometry methods, Microscopy, Fluorescence methods, Oxazines analysis, Staining and Labeling methods, Triglycerides analysis, Lipids analysis, Yeasts chemistry

Abstract

Oleaginous microbes, which contain over 20% intracellular lipid, predominantly triacylglycerols (TG), by dry weight, have been discovered to have high oil content by many different protocols, ranging from simple staining to more complex chromatographic methods. In our laboratory, a methodical process was implemented to identify high oil yeasts, designed to minimize labor while optimizing success in identifying high oil strains among thousands of candidates. First, criteria were developed to select candidate yeast strains for analysis. These included observation of buoyancy of the yeast cell mass in 20% glycerol, and phylogenetic placement near known oleaginous species. A low-labor, semiquantitative Nile red staining protocol was implemented to screen numerous yeast cultures for high oil content in 96-well plates. Then, promising candidates were selected for more quantitative analysis. A more labor-intensive and quantitative gravimetric assay was implemented that gave consistent values for intracellular oil content for a broad range of yeast species. Finally, an LC-MS protocol was utilized to quantify and identify yeast triacylglycerols. This progressive approach was successful in identifying 30 new oleaginous yeast species, out of over 1000 species represented in the Phaff Yeast Culture Collection.

Published

2019

16. Isolation and Propagation of Single Inclusion-Derived Chlamydia Using Laser Microdissection.

Author

Podgorny OV, Polina NF, and Lazarev VN

Subjects

Boron Compounds analysis, Chlamydia Infections microbiology, Fluorescent Dyes analysis, HeLa Cells, Humans, Microscopy, Fluorescence methods, Staining and Labeling methods, Chlamydia Infections pathology, Chlamydia trachomatis isolation & purification, Laser Capture Microdissection methods

Abstract

Other than its routine application for capturing pure cell populations from fixed tissue sections for diverse downstream molecular assays, laser microdissection enables isolation of single live cells. Here we describe a method for the isolation of single Chlamydia trachomatis-infected cells using a laser microdissection system, in which the dissected samples are captured via gravity. Cells infected by C. trachomatis at low multiplicity of infection are marked with the fluorescent Golgi-specific probe BODIPY ® FL C5-ceramide, to facilitate identification of the cells with chlamydial inclusions under the microscope. Individual C. trachomatis-infected cells are harvested into separate wells with a pregrown host cell monolayer. Inclusions in harvested cells maturate, and the released elementary bodies infect the host cell monolayer, thus initiating propagation of single inclusion-derived Chlamydia. The method can be used for generation of microbiological clones of C. trachomatis and recovery of transformants and mutants. Isolated single Chlamydia-infected cells can also be examined by diverse downstream molecular assays to reveal unknown features of the Chlamydia replication at a single inclusion level.

Published

2019

17. Utilization of Fluorescently Tagged Synthetic Acceptor Molecules for In Vitro Characterization of a Dual-Domain Glycosyltransferase Enzyme, KpsC, from Escherichia coli.

Author

Doyle L, Ovchinnikova OG, and Whitfield C

Subjects

Chromatography, Thin Layer methods, Escherichia coli metabolism, Fluorescent Dyes analysis, Glycosyltransferases analysis, Mass Spectrometry methods, Nuclear Magnetic Resonance, Biomolecular methods, Substrate Specificity, Enzyme Assays methods, Escherichia coli enzymology, Fluorescent Dyes metabolism, Glycosyltransferases metabolism

Abstract

The incorporation of fluorescent tags into synthetic acceptor molecules for in vitro biochemical assays allows quick and easy detection of enzyme activity. Reaction products can be separated via thin-layer chromatography and visualized under UV light for rapid detection of reaction progress. Subsequent structural analysis of these reaction products through the use of NMR spectroscopy and mass spectrometry allows for complete functional characterization of enzyme activity. Here we describe an application of this technique which was previously used to functionally characterize a dual-domain glycosyltransferase enzyme, KpsC, involved in capsular polysaccharide biosynthesis in Escherichia coli.

Published

2019

18. Assay Methods for the Glycosyltransferases Involved in Synthesis of Bacterial Polysaccharides.

Author

Abukar T, Buenbrazo N, Janesch B, Kell L, and Wakarchuk W

Subjects

Bacteria chemistry, Bacteria metabolism, Biosynthetic Pathways, Boron Compounds analysis, Chromatography, High Pressure Liquid methods, Chromatography, Thin Layer methods, Fluorescent Dyes analysis, Oxidation-Reduction, Polysaccharides, Bacterial analysis, Recombinant Proteins metabolism, Bacteria enzymology, Boron Compounds metabolism, Enzyme Assays methods, Fluorescent Dyes metabolism, Glycosyltransferases metabolism, Polysaccharides, Bacterial metabolism

Abstract

Glycans play many important roles in bacterial biology and the complexity of the glycan structures requires biochemical assays in place to help characterize the biosynthetic pathways. Our focus has been on the use of enzymes from pathogens which make molecular mimics of host glycans. We have been examining glycosyltransferases that make strategic linkages in biologically active glycans which can be also exploited for potential therapeutic glycoconjugate synthesis. This chapter will provide details on assays for a variety of bacterial glycosyltransferases that we and others have used for the characterization of pathogen glycoconjugate biosynthetic pathways, and for the in vitro synthesis of human-like glycans produced by bacterial pathogens. The methods presented here should enable other assays to be developed for new pathway characterization.

Published

2019

19. Determination of Cell-Surface Hyaluronan Through Flow Cytometry.

Author

Vitale DL, Spinelli FM, and Alaniz L

Subjects

Animals, Cell Line, Fluorescent Dyes analysis, Humans, Staining and Labeling methods, Cell Membrane chemistry, Flow Cytometry methods, Hyaluronic Acid analysis

Abstract

Hyaluronan is the major glycosaminoglycan present in the extracellular matrix of several cell types; its synthesis occurs on the cellular plasma membrane. Variations in its expression are related to alterations in cell proliferation, adhesion, and migration. It is able to interact with different binding proteins called hyaladherins, which can be conjugated to different fluorochromes and analyzed by flow cytometry.

Published

2019

20. Measuring Calcium and ROS by Genetically Encoded Protein Sensors and Fluorescent Dyes.

Author

Gibhardt CS, Vultur A, and Bogeski I

Subjects

Cell Culture Techniques methods, HEK293 Cells, Humans, Luminescent Proteins genetics, Reactive Oxygen Species analysis, Biosensing Techniques methods, Calcium analysis, Fluorescent Dyes analysis, Hydrogen Peroxide analysis, Luminescent Proteins analysis, Microscopy, Fluorescence methods

Abstract

Oxidative modifications of cellular building blocks such as proteins, lipids, and DNA have a major impact on cell behavior, fate, and clinical outcome. Reactive oxygen species (ROS) are important factors that influence these redox processes. Calcium ion (Ca 2+ ) dynamics and signals are also essential regulators of key cellular processes. Therefore, the combined and precise monitoring of ROS and Ca 2+ in single cells, with a high spatial and temporal resolution and in physiological environments, is essential to better understand their functional impact. Here, we describe protocols to detect one of the most prominent ROS (hydrogen peroxide, H 2 O 2 ) using genetically encoded protein sensors and fluorescent dyes. We also provide guidelines on how to simultaneously detect Ca 2+ and H 2 O 2 and how to examine the influence of Ca 2+ signals on cellular ROS production and vice versa.

Published

2019

21. Using FM Dyes to Study Endomembranes and Their Dynamics in Plants and Cell Suspensions.

Author

Jelínková A, Malínská K, and Petrášek J

Subjects

Arabidopsis ultrastructure, Cell Membrane ultrastructure, Fluorescent Dyes analysis, Optical Imaging methods, Plant Roots ultrastructure, Nicotiana ultrastructure, Arabidopsis cytology, Endocytosis, Microscopy, Fluorescence methods, Plant Roots cytology, Nicotiana cytology

Abstract

FM (Fei-Mao) styryl dyes are commonly used for the fluorescence imaging of plasma membrane (PM) and endocytosis in vivo. Thanks to their amphiphilic character, these dyes are incorporated in the outer leaflet of the PM lipid bilayer and emit fluorescence in its hydrophobic environment. The endocytic pathway of FM dye uptake starts with rapid PM staining and continues in PM invaginations and membrane vesicles during endocytosis, followed by staining of trans-Golgi network (TGN) and ending in tonoplast (vacuolar membrane). FM dyes do not stain endoplasmic reticulum and nuclear membrane. The time-lapse fluorescence microscopy could track endocytic vesicles and characterize the rate of endocytosis in vivo. On the other hand, fixable FM dyes (FX) can be used for the visualization of particular steps in the FM dye uptake in situ. Staining with FM dyes and subsequent microscopic observations could be performed on both tissue and cellular level. Here, we describe simple procedures for the effective FM dye staining and destaining in root tip of Arabidopsis thaliana seedlings and suspension-cultured tobacco cells.

Published

2019

22. Evaluation of Bacterial Lipid Production: Quantitative and Qualitative Measurements: Tips and Guidelines.

Author

Modiri S, Zahiri HS, and Noghabi KA

Subjects

Cyanobacteria chemistry, Fluorescent Dyes analysis, Lipids isolation & purification, Oxazines analysis, Spectrometry, Fluorescence methods, Staining and Labeling methods, Cyanobacteria metabolism, Lipid Metabolism, Lipids analysis

Abstract

Over the last decade, finding bacterial strains with ability to accumulate high concentrations of lipids has gained increasing interest, since these lipids may be used in different industries. Here we describe two methods for evaluation of lipid accumulation in cyanobacteria, following by our personal reflection on issues surrounding the use of these methods. First, we present the Bligh and Dyer protocol as a traditional extraction method using organic solvents for quantitative determination of lipids and next Nile red, a selective fluorescent stain, that has been used as a rapid approach for both qualitative and quantitative measurement of lipids.

Published

2019

23. Method for Determining Gelatinolytic Activity in Tissue Extracts: Real-Time Gelatin Zymography.

Author

Hadler-Olsen E and Winberg JO

Subjects

Animals, Cell Line, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Furans analysis, Furans metabolism, Gelatin analysis, Gelatin metabolism, Gelatinases analysis, Humans, Kidney chemistry, Kidney enzymology, Liver chemistry, Liver enzymology, Mice, Mice, Inbred BALB C, Skin chemistry, Skin enzymology, Electrophoresis, Polyacrylamide Gel methods, Enzyme Assays methods, Gelatinases metabolism

Abstract

To explore the physiological or pathological roles of proteases, it is important to be able to detect and precisely localize them in a tissue, to differentiate between inactive and active forms, as well as to quantify and determine the nature of the enzyme that degrades a given substrate. Here we present a protocol for real-time gelatin zymography that is very useful for the detection of gelatin-degrading proteases in tissue extracts. This method uses fluorescence-labeled gelatin and therefore we also present an easy, fast, and cheap method for labeling gelatin with 2-methoxy-2,4-diphenyl-3(2H)-furanone (MDPF).

Published

2019

24. Method for Determining Gelatinolytic Activity in Tissue: In Situ Gelatin Zymography.

Author

Hadler-Olsen E and Winberg JO

Subjects

Animals, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Gelatin analysis, Gelatin metabolism, Gelatinases analysis, Humans, Mammary Glands, Human chemistry, Mammary Glands, Human enzymology, Mammary Glands, Human ultrastructure, Mice, Substrate Specificity, Tissue Embedding methods, Tissue Fixation methods, Enzyme Assays methods, Gelatinases metabolism, Microscopy, Fluorescence methods, Microtomy methods

Abstract

To explore the physiological or pathological roles of proteases, it is important to be able to detect and precisely localize them in a tissue, to differentiate between inactive and active forms, as well as to quantify and determine the nature of the enzyme that degrades a given substrate. Here we present an in situ gelatin zymography method that allows for a precise localization of active gelatin-degrading enzymes in a tissue section. In this method, dye-quenched gelatin is put on top of a tissue section. During an incubation period, active gelatinolytic enzymes will degrade the substrate and fluorescent signals are emitted from the locations of these enzymes.

Published

2019

25. Transient Gene Expression as a Tool to Monitor and Manipulate the Levels of Acidic Phospholipids in Plant Cells.

Author

Noack LC, Pejchar P, Sekereš J, Jaillais Y, and Potocký M

Subjects

Fluorescent Dyes metabolism, Gene Expression, Luminescent Proteins analysis, Luminescent Proteins genetics, Microscopy, Confocal methods, Phosphatidylinositols analysis, Phosphatidylinositols metabolism, Phospholipids metabolism, Plant Cells metabolism, Pollen chemistry, Pollen genetics, Nicotiana chemistry, Nicotiana genetics, Transformation, Genetic, Fluorescent Dyes analysis, Microscopy, Fluorescence methods, Phospholipids analysis, Plant Cells chemistry, Nicotiana cytology

Abstract

Anionic phospholipids represent only minor fraction of cell membranes lipids but they are critically important for many membrane-related processes, including membrane identity, charge, shape, the generation of second messengers, and the recruitment of peripheral proteins. The main anionic phospholipids of the plasma membrane are phosphoinositides phosphatidylinositol 4-phosphate (PI4P), phosphatidylinositol 4,5-bisphosphate (PI4,5P 2 ), phosphatidylserine (PS), and phosphatidic acid (PA). Recent insights in the understanding of the nature of protein-phospholipid interactions enabled the design of genetically encoded fluorescent molecular probes that can interact with various phospholipids in a specific manner allowing their imaging in live cells. Here, we describe the use of transiently transformed plant cells to study phospholipid-dependent membrane recruitment.

Published

2019

26. The Photoconvertible Fluorescent Protein Dendra2 Tag as a Tool to Investigate Intracellular Protein Dynamics.

Author

Lešková A, Kusá Z, Labajová M, Krausko M, and Jásik J

Subjects

Arabidopsis chemistry, Arabidopsis ultrastructure, Intracellular Membranes chemistry, Light, Luminescent Proteins analysis, Plant Roots chemistry, Plant Roots ultrastructure, Arabidopsis cytology, Arabidopsis Proteins analysis, Fluorescent Dyes analysis, Intracellular Membranes ultrastructure, Microscopy, Confocal methods, Synaptotagmin I analysis

Abstract

Fluorescence proteins changing spectral properties after exposure to light with a specific wavelength have recently become outstanding aids in the study of intracellular protein dynamics. Herein we show using Arabidopsis SYNAPTOTAGMIN 1 as a model protein that the Dendra2 green to red photoconvertible protein tag in combination with confocal scanning laser microscopy is a useful tool to study membrane protein intracellular dynamics.

Published

2019

27. Vacuole Dynamics in Rice Cells Invaded by the Blast Fungus Magnaporthe oryzae.

Author

Jones K and Khang CH

Subjects

Fluoresceins analysis, Fluorescent Dyes analysis, Host-Pathogen Interactions, Magnaporthe physiology, Oryza ultrastructure, Magnaporthe isolation & purification, Microscopy, Confocal methods, Oryza microbiology, Plant Diseases microbiology, Vacuoles microbiology, Vacuoles ultrastructure

Abstract

We describe a fluorescence imaging method to visualize the dynamics of the central vacuole in rice cells during invasion by the blast fungus Magnaporthe oryzae. This method utilizes the combination of confocal microscopy, rice sheath cells (optically transparent), fluorescently tagged M. oryzae (red fluorescence), and fluorescein diacetate staining (green fluorescence; visualizing vacuole dynamics). Using this method, we demonstrate that the vacuole undergoes progressive shrinkage and collapse during M. oryzae infection.

Published

2018

28. MethyLight and Digital MethyLight.

Author

Campan M, Weisenberger DJ, Trinh B, and Laird PW

Subjects

CpG Islands, Epigenesis, Genetic, Humans, Sulfites, DNA Methylation, Fluorescent Dyes analysis, Real-Time Polymerase Chain Reaction methods

Abstract

MethyLight is a quantitative, fluorescence-based, real-time PCR method to sensitively detect and quantify DNA methylation of candidate regions of the genome. MethyLight is uniquely suited for detecting low-frequency methylated DNA regions against a high background of unmethylated DNA, as it combines methylation-specific priming with methylation-specific fluorescent probing. The quantitative accuracy of real-time PCR and the ability to design bisulfite-dependent, DNA methylation-independent control reactions together allow for a quantitative assessment of these low frequency methylation events. Here we describe the experimental steps of MethyLight analysis in detail. Furthermore, we present principles and design examples for three types of quality control reactions. QC-1 reactions are methylation-independent reactions to monitor sample quantity and integrity. QC-2 reactions are bisulfite-independent reactions to monitor recovery efficiencies of the bisulfite conversion methodology used. QC-3 reactions are bisulfite-independently primed reactions with variable bisulfite-dependent probing to monitor completeness of the sodium bisulfite treatment. We show that these control reactions perform as expected in a time course experiment interrupting sodium bisulfite conversion at various timepoints. Finally, we describe Digital MethyLight, in which MethyLight is combined with Digital PCR, for the highly sensitive detection of individual methylated molecules, with use in disease detection and screening.

Published

2018

29. Isolation of Vacuoles from the Leaves of the Medicinal Plant Catharanthus roseus.

Author

Carqueijeiro I, Noronha H, Bettencourt S, Guedes JG, Duarte P, Gerós H, and Sottomayor M

Subjects

Benzenesulfonates analysis, Blotting, Western methods, Catharanthus metabolism, Enzyme Assays methods, Fluoresceins analysis, Fluorescent Dyes analysis, Hydrolysis, Microscopy, Fluorescence methods, Neutral Red analysis, Optical Imaging methods, Osmotic Pressure, Plant Leaves metabolism, Plant Proteins analysis, Plant Proteins metabolism, Plants, Medicinal cytology, Plants, Medicinal metabolism, Protoplasts cytology, Protoplasts metabolism, Protoplasts ultrastructure, Pyridinium Compounds analysis, Quaternary Ammonium Compounds analysis, Staining and Labeling methods, Vacuolar Proton-Translocating ATPases analysis, Vacuolar Proton-Translocating ATPases metabolism, Catharanthus cytology, Cell Fractionation methods, Plant Leaves cytology, Vacuoles metabolism, Vacuoles ultrastructure

Abstract

The isolation of vacuoles is an essential step to unravel the important and complex functions of this organelle in plant physiology. Here, we describe a method for the isolation of vacuoles from Catharanthus roseus leaves involving a simple procedure for the isolation of protoplasts, and the application of a controlled osmotic/thermal shock to the naked cells, leading to the release of intact vacuoles, which are subsequently purified by density gradient centrifugation. The purity of the isolated intact vacuoles is assayed by microscopy, western blotting, and measurement of vacuolar (V)-H + -ATPase hydrolytic activity. Finally, membrane functionality and integrity is evaluated by measuring the generation of a transtonoplast pH gradient by the V-H + -ATPase and the V-H + -pyrophosphatase, also producing further information on vacuole purity.

Published

2018

30. Plant Cell Vacuoles: Staining and Fluorescent Probes.

Author

Stefano G, Renna L, and Brandizzi F

Subjects

Arabidopsis chemistry, Arabidopsis ultrastructure, Luminescent Proteins analysis, Neutral Red analysis, Pyridinium Compounds analysis, Quaternary Ammonium Compounds analysis, Vacuoles chemistry, Arabidopsis cytology, Arabidopsis Proteins analysis, Fluorescent Dyes analysis, Microscopy, Confocal methods, Staining and Labeling methods, Vacuoles ultrastructure

Abstract

In plant cells, vacuoles are extremely important for growth and development, and influence important cellular functions as photosynthesis, respiration, and transpiration. Plant cells contain lytic and storage vacuoles, whose size can be different depending on cell type and tissue developmental stage. One of the main roles of vacuoles is to regulate the cell turgor in response to different stimuli. Thus, studying the morphology, dynamics, and physiology of vacuole is fundamentally important to advance knowledge in plant cell biology at large. The availability of fluorescent probes allows marking vacuoles in multiple ways. These may be fast, when using commercially available chemical dyes, or relatively slow, in the case of specific genetically encoded markers based on proteins directed either to the membrane of the vacuole (tonoplast) or to the vacuole lumen. Any of these approaches provides useful information about the morphology and physiology of the vacuole.

Published

2018

31. Flow Cytometry and Fluorescence Microscopy as Tools for Structural and Functional Analysis of Vacuoles Isolated from Yeast and Plant Cells.

Author

Rodrigues JMP, Pereira CS, Fontes N, Gerós H, and Côrte-Real M

Subjects

Acridine Orange analysis, Aniline Compounds analysis, Barbiturates analysis, Calcium analysis, Calcium metabolism, Fluorescent Dyes analysis, Isoxazoles analysis, Neutral Red analysis, Pyridinium Compounds analysis, Quaternary Ammonium Compounds analysis, Staining and Labeling methods, Vacuolar Proton-Translocating ATPases analysis, Vacuolar Proton-Translocating ATPases metabolism, Vacuoles chemistry, Vacuoles enzymology, Vitis chemistry, Vitis enzymology, Vitis metabolism, Xanthenes analysis, Yeasts chemistry, Yeasts enzymology, Yeasts metabolism, Cell Fractionation methods, Flow Cytometry methods, Microscopy, Fluorescence methods, Vacuoles metabolism, Vacuoles ultrastructure, Vitis cytology, Yeasts cytology

Abstract

A series of optimized protocols to isolate vacuoles from both yeast and plant cells, and to characterize the purified organelles at a functional and structural level, are described. For this purpose, we took advantage of the combined use of cell fractionation techniques with different fluorescence-based approaches namely flow cytometry, fluorescence microscopy and spectrofluorimetry. These protocols altogether constitute valuable tools for the study of vacuole structure and function, as well as for the high-throughput screening of drug libraries to identify new molecules that target the vacuole.

Published

2018

32. Functional Screening of Core Promoter Activity.

Author

Even DY, Kedmi A, Ideses D, and Juven-Gershon T

Subjects

Animals, Cell Line, DNA genetics, Escherichia coli genetics, Flow Cytometry methods, Fluorescent Dyes metabolism, Genes, erbB-1, Genetic Engineering methods, Green Fluorescent Proteins genetics, Humans, Optical Imaging methods, Plasmids genetics, Real-Time Polymerase Chain Reaction methods, Transcriptional Activation, Transfection methods, Fluorescent Dyes analysis, Genes, Reporter, Green Fluorescent Proteins analysis, Promoter Regions, Genetic

Abstract

The core promoter is the DNA sequence that recruits the basal transcription machinery and directs accurate initiation of transcription. It is an active contributor to gene expression that can be rationally designed to manipulate the levels of expression. Core promoter function can be analyzed using different experimental approaches. Here, we describe the qualitative and quantitative analysis of engineered core promoter functions using the EGFP reporter gene that is driven by distinct core promoters. Expression plasmids are transfected into different mammalian cell lines, and the resulting fluorescence is monitored by live cell imaging , as well as by flow cytometry. In order to verify that the transcriptional activity of the examined core promoters is indeed a function of their activity, as opposed to differences in DNA uptake, real-time quantitative PCR analysis is performed. Importantly, the described methodology for functional screening of core promoter activity has enabled the analysis of engineered potent core promoters for extended time periods.

Published

2017

33. High-Throughput N-Glycan Analysis with Rapid Magnetic Bead-Based Sample Preparation.

Author

Szigeti M and Guttman A

Subjects

Fluorescence, Fluorescent Dyes analysis, Glycosylation, High-Throughput Screening Assays methods, Humans, Magnetics methods, Magnets chemistry, Pyrenes analysis, Specimen Handling, Electrophoresis, Capillary methods, Glycoproteins chemistry, Immunoglobulin G chemistry, Polysaccharides analysis

Abstract

N-glycan profiling of therapeutic glycoproteins is essential to ensure the activity and efficacy of these promising new-generation drugs. The N-linked glycan moieties of these entities highly affect circulation half-life, immunogenicity and receptor-binding activity as well as physicochemical and thermal stability properties. In addition, more than half of the biopharmaceuticals are glycoproteins representing multibillion dollar worldwide business, further emphasizing the importance of their analysis. In the biomedical field, on the other hand, revealing disease-related glycan structure alterations holds the promise of the discovery of new biomarkers for early diagnostics. Therefore, there is a great demand for widely applicable, high-throughput sample preparation and analysis methods for N-glycan profiling of glycoproteins. One of the newest exciting developments of the field is the magnetic bead based glycoprotein sample preparation technique. A detailed protocol of this method is given in this chapter in conjunction with rapid capillary electrophoresis analysis of the prepared samples by laser induced fluorescence detection (CE-LIF). N-glycans are digested by the endoglycosidase PNGase F and the released carbohydrates are labeled with the charged fluorophore dye of aminopyrenetrisulfonate (APTS). Effective glycan capture by magnetic microparticles enabled fast, easily automated sample preparation both in individual (single vial) and 96-well plate formats, including excess dye removal. Rapid separation of APTS labeled IgG glycans is also shown utilizing an optimized CE-LIF protocol.

Published

2017

34. Cell In Situ Zymography: Imaging Enzyme-Substrate Interactions.

Author

Chhabra A and Rani V

Subjects

Animals, Caseins analysis, Caseins metabolism, Cell Culture Techniques methods, Cell Line, Enzyme Assays methods, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Humans, Image Processing, Computer-Assisted methods, Matrix Metalloproteinases analysis, Rats, Substrate Specificity, Matrix Metalloproteinases metabolism, Microscopy, Fluorescence methods, Myoblasts, Cardiac metabolism

Abstract

Zymography has long been used for the detection of substrate-specific enzyme activity. In situ zymography (ISZ), an adaptation from the conventional substrate zymography, is a widely employed technique useful for the detection, localization, and estimation of enzyme-substrate interactions in tissues. Here, we describe a protocol to detect 'in position' matrix metalloproteinase (MMP) activity in cells utilizing H9c2 cardiomyoblasts as a model. This technique is primarily adopted from the method used for histological sections and is termed as 'Cell in situ Zymography'. It is a simple, sensitive, and quantifiable methodology to assess the functional activity of an enzyme 'on site/in position' in cell culture.

Published

2017

35. Monitoring Promoter Activity by Flow Cytometry.

Author

Taher TEI

Subjects

Animals, Fluorescent Dyes metabolism, Green Fluorescent Proteins genetics, Humans, Transfection methods, Flow Cytometry methods, Fluorescent Dyes analysis, Genes, Reporter, Green Fluorescent Proteins analysis, Promoter Regions, Genetic

Abstract

Genetic reporters have become invaluable tools for indirectly monitoring promoter activities. The quantitative measurement of promoter activities using reporter gene systems is fundamental for pharmaceutical, biomedical, and molecular biology research. Genetic reporters are used not only for measuring promoter activities but also for understanding the mechanisms controlling gene transcription and in the identification, and characterization of cis-acting regulatory elements. Fluorescent reporter proteins including enhanced green fluorescent protein (EGFP ) are reliable for monitoring quantitative underlying differences in promoter activities. The emitted fluorescence intensity of the expressed reporter is measured at the single-cell level by flow cytometry and represents a readout for the promoter activities. In this chapter, the protocol for measurement and analyzing of transfected cells expressing the reporter gene EGFP is thoroughly described and fully illustrated.

Published

2017

36. Zymography Principles.

Author

Wilkesman J and Kurz L

Subjects

Animals, Biocatalysis, Fluorescent Dyes analysis, Humans, Indicators and Reagents, Oxidation-Reduction, Proteomics methods, Electrophoresis, Polyacrylamide Gel methods, Enzyme Assays methods

Abstract

Zymography, the detection, identification, and even quantification of enzyme activity fractionated by gel electrophoresis, has received increasing attention in the last years, as revealed by the number of articles published. A number of enzymes are routinely detected by zymography, especially with clinical interest. This introductory chapter reviews the major principles behind zymography. New advances of this method are basically focused towards two-dimensional zymography and transfer zymography as will be explained in the rest of the chapters. Some general considerations when performing the experiments are outlined as well as the major troubleshooting and safety issues necessary for correct development of the electrophoresis.

Published

2017

37. Ratiometric Fluorescence Live Imaging Analysis of Membrane Lipid Order in Arabidopsis Mitotic Cells Using a Lipid Order-Sensitive Probe.

Author

Gerbeau-Pissot P, Der C, Grebe M, and Stanislas T

Subjects

Arabidopsis ultrastructure, Cell Culture Techniques, Membrane Microdomains ultrastructure, Optical Imaging methods, Plant Roots cytology, Plant Roots ultrastructure, Arabidopsis cytology, Fluorescent Dyes analysis, Membrane Lipids analysis, Microscopy, Fluorescence methods, Mitosis, Pyridinium Compounds analysis

Abstract

Eukaryotic cells contain membranes exhibiting different levels of lipid order mostly related to their relative amount of sterol-rich domains, thought to mediate temporal and spatial organization of cellular processes. We previously provided evidence in Arabidopsis thaliana that sterols are crucial for execution of cytokinesis, the last stage of cell division. Recently, we used di-4-ANEPPDHQ, a fluorescent probe sensitive to order of lipid phases, to quantify the level of membrane order of the cell plate, the membrane structure separating daughter cells during somatic cytokinesis of higher plant cells. By employing quantitative, ratiometric fluorescence microscopy for mapping localized lipid order levels, we revealed that the Arabidopsis cell plate represents a high-lipid-order domain of the plasma membrane. Here, we describe step-by-step protocols and troubleshooting for ratiometric live imaging procedures employing the di-4-ANEPPDHQ fluorescent probe for quantification of membrane lipid order during plant cell division in suspension cell cultures and roots of Arabidopsis thaliana.

Published

2016

38. Before In Vivo Imaging: Evaluation of Fluorescent Probes Using Fluorescence Microscopy, Multiplate Reader, and Cytotoxicity Assays.

Author

Zhang S

Subjects

Fluorescent Dyes pharmacokinetics, Fluorescent Dyes toxicity, Microscopy, Fluorescence, Quantum Theory, Toxicity Tests, Fluorescent Dyes analysis, Molecular Imaging methods

Abstract

Fluorescent probes are widely utilized for noninvasive fluorescence imaging. Continuing efforts have been made in developing novel fluorescent probes with improved fluorescence quantum yield, enhanced target-specificity, and lower cytotoxicity. Before such probes are administrated into a living system, it is essential to evaluate the subcellular uptake, targeting specificity, and cytotoxicity in vitro. In this chapter, we briefly outline common methods used to evaluate fluorescent probes using fluorescence microscopy, multiplate reader, and cytotoxicity assay.

Published

2016

39. Imaging Nuclear Morphology and Organization in Cleared Plant Tissues Treated with Cell Cycle Inhibitors.

Author

de Souza Junior JD, de Sa MF, Engler G, and Engler Jde A

Subjects

Arabidopsis drug effects, Cell Culture Techniques methods, Cell Nucleus drug effects, DNA, Plant analysis, Fluorescent Dyes analysis, Indoles analysis, Mitosis, Optical Imaging methods, Plant Roots cytology, Plant Roots drug effects, Plant Roots ultrastructure, Staining and Labeling methods, Arabidopsis cytology, Arabidopsis ultrastructure, Cell Cycle drug effects, Cell Nucleus ultrastructure, Microscopy, Confocal methods

Abstract

Synchronization of root cells through chemical treatment can generate a large number of cells blocked in specific cell cycle phases. In plants, this approach can be employed for cell suspension cultures and plant seedlings. To identify plant cells in the course of the cell cycle, especially during mitosis in meristematic tissues, chemical inhibitors can be used to block cell cycle progression. Herein, we present a simplified and easy-to-apply protocol to visualize mitotic figures, nuclei morphology, and organization in whole Arabidopsis root apexes. The procedure is based on tissue clearing, and fluorescent staining of nuclear DNA with DAPI. The protocol allows carrying out bulk analysis of nuclei and cell cycle phases in root cells and will be valuable to investigate mutants like overexpressing lines of genes disturbing the plant cell cycle.

Published

2016

40. Application of Fluorescence Polarization in HTS Assays.

Author

Huang X and Aulabaugh A

Subjects

Animals, Anisotropy, Binding, Competitive, Fluorescent Dyes metabolism, Humans, Enzyme Assays methods, Fluorescence Polarization methods, Fluorescent Dyes analysis, High-Throughput Screening Assays methods

Abstract

Steady-state measurements of fluorescence polarization have been widely adopted in the field of high-throughput screening for the study of biomolecular interactions. This chapter reviews the basic theory of fluorescence polarization, the underlying principle for using fluorescence polarization to study interactions between small-molecule fluorophores and macromolecular targets, and representative applications of fluorescence polarization in high-throughput screening.

Published

2016

41. Characterization of Cytokinetic Mutants Using Small Fluorescent Probes.

Author

Smertenko A, Moschou P, Zhang L, Fahy D, and Bozhkov P

Subjects

Arabidopsis genetics, Arabidopsis ultrastructure, Cell Wall genetics, Cell Wall ultrastructure, DNA, Plant genetics, Indoles analysis, Microscopy, Fluorescence methods, Mutation, Propidium analysis, Pyridinium Compounds analysis, Quaternary Ammonium Compounds analysis, Arabidopsis cytology, Cytokinesis, DNA, Plant analysis, Fluorescent Dyes analysis, Staining and Labeling methods

Abstract

Cytokinesis is a powerful paradigm for addressing fundamental questions of plant biology including molecular mechanisms of development, cell division, cell signaling, membrane trafficking, cell wall synthesis, and cytoskeletal dynamics. Genetics was instrumental in identification of proteins regulating cytokinesis. Characterization of mutant lines generated using forward or reverse genetics includes microscopic analysis for defects in cell division. Typically, failure of cytokinesis results in appearance of multinucleate cells, formation of cell wall stubs, and isotropic cell expansion in the root elongation zone. Small fluorescent probes served as a very effective tool for the detection of cytokinetic defects. Such probes stain living or formaldehyde-fixed specimens avoiding complex preparatory steps. Although resolution of the fluorescence probes is inferior to electron microscopy, the procedure is fast, easy, and does not require expensive materials or equipment. This chapter describes techniques for staining DNA with the probes DAPI and SYTO82, for staining membranes with FM4-64, and for staining cell wall with propidium iodide.

Published

2016

42. Preparation and Fluorescent Analysis of Plant Metaphase Chromosomes.

Author

Schwarzacher T

Subjects

Fluorescent Dyes analysis, Indoles analysis, Plant Cells metabolism, Polyploidy, Staining and Labeling methods, Tissue Fixation methods, Chromosomes, Plant, Metaphase, Microscopy, Fluorescence methods, Plants genetics

Abstract

Good preparations are essential for informative analysis of both somatic and meiotic chromosomes, cytogenetics, and cell divisions. Fluorescent chromosome staining allows even small chromosomes to be visualized and counted, showing their morphology. Aneuploidies and polyploidies can be established for species, populations, or individuals while changes occurring in breeding lines during hybridization or tissue culture and transformation protocols can be assessed. The process of division can be followed during mitosis and meiosis including pairing and chiasma distribution, as well as DNA organization and structure during the evolution of chromosomes can be studied. This chapter presents protocols for pretreatment and fixation of material, including tips of how to grow plants to get good and healthy meristem with many divisions. The chromosome preparation technique is described using proteolytic enzymes, but acids can be used instead. Chromosome slide preparations are suitable for fluorochrome staining for fast screening (described in the chapter) or fluorescent in situ hybridization (see Schwarzacher and Heslop-Harrison, In situ hybridization. BIOS Scientific Publishers, Oxford, 2000).

Published

2016

43. Accurate Assessment of Cell Death by Imaging Flow Cytometry.

Author

Rieger AM and Barreda DR

Subjects

Animals, Annexin A5 analysis, Fluorescent Dyes analysis, Humans, Software, Cell Death, Flow Cytometry methods, Image Cytometry methods

Abstract

The number of investigators using cell death analysis applications has greatly expanded since the introduction of flow cytometry. The Annexin V/propidium iodide (PI) method is among the most commonly used procedures and allows users to determine if cells are viable, apoptotic, or necrotic, based on changes in membrane lipid composition, integrity, and permeability. Unfortunately, PI can intercalate into RNA, in addition to DNA, which contributes to a large number of events showing PI staining within the cytoplasmic compartment. We show that this occurs across a broad range of animal primary cells and commonly used cell lines, and is most prevalent in large cells (nuclear:cytoplasmic ratio <0.5). Any cellular system where RNA levels change throughout an experiment will be particularly affected, such as those that utilize virally infected cells. As two examples, we highlight our recent work on cells infected with vesicular stomatitis virus (VSV), an RNA virus, and herpes simplex virus-1 (HSV-1), a DNA virus. Similarly, these issues are relevant to experimental systems where cells have increased RNA content such as during genotoxic stress, following exposure to cell cycle arrest drugs such as thymidine or hydroxyurea, or where developmental progression promotes discrete changes in cellular RNA synthesis. This chapter outlines a modified Annexin V/PI method that addresses cytoplasmic RNA staining issues to allow for accurate assessment of cell death. This protocol takes advantage of an additional cellular permeability caused by fixation to promote RNase A entry into the cell. Based on our observations, cell morphological parameters are well maintained and less than 5 % of total cellular events exhibit cytoplasmic PI staining under this protocol.

Published

2016

44. Isolation of Plant Nuclei at Defined Cell Cycle Stages Using EdU Labeling and Flow Cytometry.

Author

Wear EE, Concia L, Brooks AM, Markham EA, Lee TJ, Allen GC, Thompson WF, and Hanley-Bowdoin L

Subjects

Cell Cycle, Click Chemistry methods, DNA Replication, DNA, Plant analysis, DNA, Plant genetics, Deoxyuridine analogs & derivatives, Deoxyuridine analysis, Fluorescent Dyes analysis, Arabidopsis cytology, Arabidopsis genetics, Cell Fractionation methods, Cell Nucleus genetics, Flow Cytometry methods, Zea mays cytology, Zea mays genetics

Abstract

5-Ethynyl-2'-deoxyuridine (EdU) is a nucleoside analog of thymidine that can be rapidly incorporated into replicating DNA in vivo and, subsequently, detected by using "click" chemistry to couple its terminal alkyne group to fluorescent azides such as Alexa Fluor 488. Recently, EdU incorporation followed by coupling with a fluorophore has been used to visualize newly synthesized DNA in a wide range of plant species. One particularly useful application is in flow cytometry, where two-parameter sorting can be employed to analyze different phases of the cell cycle, as defined both by total DNA content and the amount of EdU pulse-labeled DNA. This approach allows analysis of the cell cycle without the need for synchronous cell populations, which can be difficult to obtain in many plant systems. The approach presented here, which was developed for fixed, EdU-labeled nuclei, can be used to prepare analytical profiles as well as to make highly purified preparations of G1, S, or G2/M phase nuclei for molecular or biochemical analysis. We present protocols for EdU pulse labeling, tissue fixation and harvesting, nuclei preparation, and flow sorting. Although developed for Arabidopsis suspension cells and maize root tips, these protocols should be modifiable to many other plant systems.

Published

2016

45. A Fluorescence-Based High-Throughput Screening Assay to Identify Growth Inhibitors of the Pathogenic Fungus Aspergillus fumigatus.

Author

Smith TM, Richie DL, and Tao J

Subjects

Aspergillosis microbiology, Aspergillus fumigatus growth & development, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Humans, Oxazines analysis, Oxazines metabolism, Xanthenes analysis, Xanthenes metabolism, Antifungal Agents pharmacology, Aspergillosis drug therapy, Aspergillus fumigatus drug effects, Growth Inhibitors pharmacology, High-Throughput Screening Assays methods, Microbial Sensitivity Tests methods

Abstract

Due to the advancements in modern medicine that have resulted in an increased number of immunocompromised individuals, the incidences and the associated mortality of invasive aspergillosis have continued to rise over the past three decades despite appropriate treatment. As a result, invasive aspergillosis has emerged as a leading cause of infection-related mortality in immunocompromised individuals. Utilizing the resazurin to resorufin conversion fluorescence readout to monitor cell viability, herein, we outline a high-throughput screening method amenable to profiling a large pharmaceutical library against the clinically relevant but less frequently screened fungal pathogen Aspergillus fumigatus. This enables the user to conduct high-throughput screening using a disease-relevant fungal growth assay and identify novel antifungal chemotypes as drug leads.

Published

2016

46. Perihematomal Cellular Injury Is Reduced by Trans-sodium Crocetinate in a Model of Intracerebral Hemorrhage.

Author

Wang Y, Schretter C, Clarke R, and Lee KS

Subjects

Animals, Carotenoids, Caudate Nucleus drug effects, Caudate Nucleus pathology, Cell Count, Cerebral Hemorrhage chemically induced, Cerebral Hemorrhage complications, Cerebral Hemorrhage pathology, Collagenases toxicity, Drug Evaluation, Preclinical, Fluoresceins analysis, Fluorescent Dyes analysis, Hematoma complications, Hematoma pathology, Male, Nerve Degeneration etiology, Nerve Degeneration pathology, Nerve Degeneration prevention & control, Neurons drug effects, Neurons pathology, Putamen drug effects, Putamen pathology, Rabbits, Rats, Rats, Sprague-Dawley, Vitamin A therapeutic use, Cerebral Hemorrhage drug therapy, Hematoma drug therapy, Neuroprotective Agents therapeutic use, Vitamin A analogs & derivatives

Abstract

The carotenoid compound trans-sodium crocetinate (TSC) has been shown to increase oxygenation in various tissues, including the brain. Notably, TSC can enhance oxygenation under conditions of reduced blood flow, thus attenuating the depth of an ischemic challenge. This study examined the impact of TSC on neuronal loss in an animal model of intracerebral hemorrhage (ICH). Utilizing a rat model of collagenase injection, TSC was shown to reduce perihematomal cellular loss after ICH, as assessed by Fluoro-Jade B staining in tissue sections. This is the first evidence demonstrating that TSC is capable of limiting hemorrhagic injury to neurons in the brain. The finding supports the concept that TSC may represent a candidate therapeutic for early intervention regardless of whether a stroke is hemorrhagic or ischemic in nature.

Published

2015

47. Isolation of murine bone marrow scavenging sinusoidal endothelial cells.

Author

McCourt PA, Oteiza A, Cao B, and Nilsson SK

Subjects

Animals, Flow Cytometry methods, Fluorescein-5-isothiocyanate analysis, Fluorescent Dyes analysis, Glycation End Products, Advanced analysis, Immunomagnetic Separation methods, Mice, Mice, Inbred C57BL, Spectrophotometry, Ultraviolet methods, Bone Marrow Cells cytology, Cell Separation methods, Endothelial Cells cytology

Abstract

The bone marrow (BM) is permeated with sinusoidal vessels lined with sinusoidal endothelial cells (SEC), which are crucial for BM physiology and hemopoietic stem cell (HSC) renewal. However, little is known about the characteristics or functional capacity of bone marrow sinusoidal endothelial cells (BMSEC). One significant barrier to the study of BMSEC is the lack of specific cell surface markers that can be used to isolate these cells. Nevertheless, BMSEC possess one exceptional property, namely, the ability to scavenge large amounts of soluble waste molecules such as advanced glycation end-products (AGE) and we have utilized this to label BMSEC for cell sorting and isolation. We describe the means to produce and fluorescently label AGE, its use as a functional in vivo marker of BMSEC and the isolation of these cells from murine BM using fluorescent activated cell separation (FACS).

Published

2015

48. Probing plasmodesmata function with biochemical inhibitors.

Author

White RG

Subjects

Actins antagonists & inhibitors, Actins genetics, Actins metabolism, Arabidopsis drug effects, Arabidopsis ultrastructure, Biological Transport, Bridged Bicyclo Compounds, Heterocyclic pharmacology, Cytochalasin B pharmacology, Depsipeptides pharmacology, Fixatives chemistry, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Gene Expression, Green Fluorescent Proteins analysis, Green Fluorescent Proteins genetics, Microinjections, Microscopy, Electron, Transmission, Microscopy, Fluorescence, Microtomy, Phalloidine pharmacology, Plant Roots drug effects, Plant Roots ultrastructure, Plasmodesmata drug effects, Plasmodesmata ultrastructure, Profilins pharmacology, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins genetics, Thiazolidines pharmacology, Tissue Fixation, Tradescantia drug effects, Tradescantia ultrastructure, Arabidopsis physiology, Cytotoxins pharmacology, Image Processing, Computer-Assisted methods, Plant Roots physiology, Plasmodesmata physiology, Tradescantia physiology

Abstract

To investigate plasmodesmata (PD) function, a useful technique is to monitor the effect on cell-to-cell transport of applying an inhibitor of a physiological process, protein, or other cell component of interest. Changes in PD transport can then be monitored in one of several ways, most commonly by measuring the cell-to-cell movement of fluorescent tracer dyes or of free fluorescent proteins. Effects on PD structure can be detected in thin sections of embedded tissue observed using an electron microscope, most commonly a Transmission Electron Microscope (TEM). This chapter outlines commonly used inhibitors, methods for treating different tissues, how to detect altered cell-to-cell transport and PD structure, and important caveats.

Published

2015

49. Visualization of epigenetic modifications in preimplantation embryos.

Author

Kimura H and Yamagata K

Subjects

Animals, Cells, Cultured, Female, Fluorescent Dyes analysis, Fluorescent Dyes chemistry, HeLa Cells, Humans, Image Processing, Computer-Assisted, Immunoglobulin Fab Fragments metabolism, Mice, Mice, Inbred Strains, Microinjections, Blastocyst physiology, Cytological Techniques methods, Epigenesis, Genetic

Abstract

Epigenetic modifications such as DNA methylation and posttranslational histone modifications change drastically during embryonic development. To visualize histone modifications in living embryos, a Fab-based live endogenous modification labeling (FabLEM) technique has been developed. Here we describe the methods required for FabLEM experiments, including Fab preparation from IgG, its conjugation with a fluorescent dye, loading into cultured cells or mouse embryos, and imaging.

Published

2015

50. Smartphone-based fluorescence detector for mHealth.

Author

Balsam J, Bruck HA, and Rasooly A

Subjects

Cell Phone, Developing Countries, Global Health, Humans, Image Processing, Computer-Assisted, Limit of Detection, Microtechnology, Optical Devices economics, Point-of-Care Systems, Telemedicine, Fluorescein analysis, Fluorescent Dyes analysis, Microfluidic Analytical Techniques instrumentation

Abstract

We describe here a compact smartphone-based fluorescence detector for mHealth. A key element to achieving high sensitivity using low sensitivity phone cameras is a capillary array, which increases sensitivity by 100×. The capillary array was combined with a white LED illumination system to enable wide spectra fluorescent excitation in the range of 450-740 nm. The detector utilizes an orthographic projection system to form parallel light projection images from the capillaries at a close distance via an object-space telecentric lens configuration that reduces the total lens-to-object distance while maintaining uniformity in measurement between capillaries. To further increase the limit of detection (LOD), a computational image processing approach was employed to decrease the level of noise. This enables an additional 5-10× decrease in LOD. This smartphone-based detector was used to measure serial dilutions of fluorescein with a LOD of 1 nM with image stacking and 10 nM without image stacking, similar to the LOD obtained with a commercial plate reader. Moreover, the capillary array required a sample volume of less than 10 μl, which is an order of magnitude less than the 100 μl required for the plate reader.As fluorescence detection is widely used in sensitive biomedical assays, the approach described here has the potential to increase mHealth clinical utility, especially for telemedicine and for resource-poor settings in global health applications.

Published

2015