Search results for "label"

showing 10 items of 797 documents

Inhibition of ubiquitin-dependent proteolysis by a synthetic glycine-alanine repeat peptide that mimics an inhibitory viral sequence.

2002

AbstractThe glycine–alanine repeat (GAr) of the Epstein–Barr virus nuclear antigen-1 is a cis-acting transferable element that inhibits ubiquitin/proteasome-dependent proteolysis in vitro and in vivo. We have here examined the effect of a synthetic 20-mer GAr oligopeptide on the degradation of iodinated or biotin labeled lysozyme in a rabbit reticulocyte lysates in vitro assay. Micromolar concentrations of the GA-20 peptide inhibited the hydrolysis of lysozyme without significant effect on ubiquitination. Addition of the peptide did not inhibit the hydrolysis of fluorogenic substrate by purified proteasomes and did not affect the ubiquitination of lysozyme. An excess of the peptide failed t…

Herpesvirus 4 HumanProteasome Endopeptidase ComplexGly–Ala repeatPolymersProteolysisMolecular Sequence DataBiophysicsGlycineBiotinPeptideBiochemistryIodine Radioisotopeschemistry.chemical_compoundS5aUbiquitinStructural BiologyMultienzyme ComplexesGeneticsmedicineAnimalsAmino Acid SequenceEnzyme InhibitorsMolecular BiologyPeptide sequenceUbiquitinsEpstein–Barr virus nuclear antigen-1Alaninechemistry.chemical_classificationOligopeptideAlaninebiologymedicine.diagnostic_testProteasomeMolecular MimicryUbiquitinationCell BiologyCysteine EndopeptidasesBiochemistryProteasomechemistryEpstein-Barr Virus Nuclear AntigensIsotope Labelingbiology.proteinMuramidaseRabbitsLysozymeCarrier ProteinsPeptidesOligopeptidesFEBS letters
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Unusual basement layer in the midgut of gammaridean Niphargus virei Chevreux (Crustacea, Amphipoda).

1988

The basement membrane of the midgut and posterior caeca epithelium in the gammaridean amphipod Niphargus virei Chevreux, 1896 is made of an unusual structure. This basal lamina, properly called “basal layer”, shows a dense sheet formed by a system of dense hexagonal plates connected by thin filaments. Histochemical studies and enzymatic reactions lead to the conclusion that these structures are proteinaceous, without collagenous protein, and embedded in a neutral polysaccharide matrix. The possible mechanical significance of these mesenteric structures is discussed.

HistologyAmphipodaMatrix (biology)Basement MembraneCrustaceamedicineAnimalsMolecular BiologyBasement membranebiologyStaining and LabelingHistocytochemistryProteinsMidgutCell BiologyGeneral MedicineAnatomybiology.organism_classificationCrustaceanEpitheliumMedical Laboratory TechnologyMicroscopy Electronmedicine.anatomical_structureBasal laminaCollagenAnatomyGeneral Agricultural and Biological SciencesLayer (electronics)Digestive SystemHistochemistry
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Supravital Uptake of Methylene Blue by Dendritic Cells within Stratified Squamous Epithelia: a Light and Electron Microscope Study

1996

Electron microscopic data on methylene blue staining of dendritic cells in the epithelia of the soft palate and skin of the mouse after supravital dye injection are presented. The ultra-structural details were compared with corresponding light microscopic findings. Methylene blue stained tissue was fixed by immersion in a paraformaldehyde-glutaraldehyde solution containing phosphomolybdic acid. The ensuing dye precipitate was stabilized by ammonium heptamolybdate. The light microscopic investigation revealed that selective staining of dendritic cells depended on the presence of ambient oxygen. In addition, delicate morphological characteristics, like spinous structures of the dendrites, wer…

HistologyConnective tissueEpitheliumlaw.inventionMicechemistry.chemical_compoundlawOrganellemedicineAnimalsColoring AgentsSkinParaffin EmbeddingStaining and LabelingEpithelial CellsDendritic CellsGeneral MedicineEpitheliumStainingMethylene BlueMicroscopy ElectronMedical Laboratory Technologymedicine.anatomical_structureVital stainchemistryBiochemistryCytoplasmBiophysicsPalate SoftElectron microscopeMethylene blueBiotechnic & Histochemistry
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Differential staining of mucin granules from epoxy resin sections by a phosphotungstic acid-methyl green procedure.

1991

After treatment of epoxy resin semithin sections from glutaraldehyde fixed rat large intestine with 5% aqueous phosphotungstic acid (PTA), staining with unpurified 0.2% solutions of methyl green at 60 C for 5 min produces a color differentiation between mucin granules of goblet cells. Some mucin granules and the glycocalyx appear deep green while the remaining granules, luminal mucin and collagen fibers are pink. The known contamination of unpurified methyl green with crystal violet seems to be responsible for the pink staining reaction of the latter structures, which also present an orange-red fluorescence under green exciting light. Electron microscopic observations show selective contras…

HistologyCytoplasmic Granuleslaw.inventionGlycocalyxchemistry.chemical_compoundMethyl GreenlawAnimalsPhosphotungstic acidCrystal violetIntestine LargeStaining and LabelingDifferential stainingEpoxy ResinsGastric MucinsMucinRats Inbred StrainsGeneral MedicinePhosphotungstic AcidStainingRatsMedical Laboratory TechnologyMicroscopy ElectronchemistryBiochemistryGentian VioletGlutaraldehydeElectron microscopeNuclear chemistryBiotechnichistochemistry : official publication of the Biological Stain Commission
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My life in Wittekind's lab.

2007

HistologyHistoryStaining and LabelingHistocytochemistryMEDLINEHistorical ArticleBiographyGeneral MedicineHistory 20th CenturyHistory 21st CenturyMedical Laboratory TechnologyLeadershipGermanyClassicsBiotechnichistochemistry : official publication of the Biological Stain Commission
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Zinc-positive boutons in the cerebral cortex of lizards show glutamate immunoreactivity

1991

Zinc-positive boutons, originating in the medial cortex of lizards, exhibit glutamate immunoreactivity. This finding supports the presumed homology between lizard zinc-positive boutons and the hippocampal mossy fibres of mammals, which are also glutamate-immunoreactive and zinc-positive. Zinc-positive boutons of lizards contain a chelatable pool of zinc located in the hippocampal mossy fibres of mammals. These synaptic systems also contain glutamate, which indicates a possible simultaneous action of zinc and glutamate during synaptic transmission.

HistologyMedial cortexCentral nervous systemHippocampal formationHippocampusPodarcis hispanicaSynaptic vesicleGlutamatesbiology.animalmental disordersparasitic diseasesmedicineAnimalsCerebral CortexStaining and LabelingbiologyLizardGeneral NeurosciencefungiGlutamate receptorAntibodies MonoclonalLizardsCell BiologyAnatomybiology.organism_classificationZincmedicine.anatomical_structurenervous systemCerebral cortexSynapsesSynaptic Vesiclessense organsAnatomyJournal of Neurocytology
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Estimation of Microbial Viability Using Flow Cytometry.

2020

For microorganisms in particular, viability is a term that is difficult to define and a state consequently difficult to measure. The traditional (and gold standard) usage equates viability and culturability (i.e., the ability to multiply) but the process of determining culturability is often too slow. Flow cytometry provides the opportunity to make rapid and quantitative measurements of dye uptake in large numbers of cells and we can therefore exploit the flow cytometric approach to evaluate so-called viability stains and to develop protocols for more routine assessments of microbial viability. This article provides a commentary and several protocols have been included to ensure that users …

HistologyMicrobial ViabilityMicrobial Viabilitymedicine.diagnostic_testStaining and LabelingComputer scienceGeneral MedicineFlow CytometryFluoresceinsBiochemistryFluorescenceFlow cytometryMedical Laboratory TechnologyDye uptakeCalibrationmedicineBiochemical engineeringFluorescent DyesCurrent protocols in cytometryLITERATURE CITED
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Timm-staining intensity is correlated with the density of Timm-positive presynaptic structures in the cerebral cortex of lizards

1987

In cortical areas of the lizard, Podarcis hispanica, Timm staining reveals a distinct pattern of lamination. At the electron-microscope level, virtually all of the reaction product is located in the synaptic vesicles of Timm-positive boutons. Using linear-regression analysis, the area density of Timm-positive bouton profiles as well as the numerical and volume density of stained vesicles were found to be closely correlated with the light-microscopic densitometric values obtained for each Timm-positive cortical zone. We discuss the possibility of estimating stereological electron-microscopic data parameters from densitometric measurements at the light-microscope level.

HistologyPodarcis hispanicaSynaptic vesicleTimm stainingmedicineAnimalsMolecular BiologyCerebral CortexStaining and LabelingbiologyVesicleLizardsCell BiologyGeneral MedicineAnatomybiology.organism_classificationIntensity (physics)Reaction productMicroscopy ElectronMedical Laboratory Technologymedicine.anatomical_structureCerebral cortexUltrastructureRegression AnalysisSynaptic VesiclesAnatomyGeneral Agricultural and Biological SciencesDensitometryHistochemistry
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Immunohistochemical localization of polysialic acid in tissue sections: differential binding to polynucleotides and DNA of a murine IgG and a human I…

1990

For immunolocalization of alpha(2-8)-linked polysialic acid, which forms part of the neural cell adhesion molecule (N-CAM), two monoclonal antibodies, MAb735 and IgMNOV, were employed. Both antibodies have previously been shown to bind the extremely low immunogenic capsular polysaccharide of group B meningococci, which also consists of alpha(2-8) polysialic acid, but not to other, even closely related forms of polysialic acid. Despite the identical polysaccharide specificity of these two MAb, we observed marked differences of the staining pattern in tissue sections. We showed that these differences in immunostaining were due to the crossreactivity of IgMNOV with polynucleotides and DNA. MA…

Histologymedicine.drug_classCell Adhesion Molecules NeuronalPolynucleotidesAntibody AffinityEnzyme-Linked Immunosorbent AssayMonoclonal antibodyBinding CompetitiveImmunoglobulin Gchemistry.chemical_compoundMiceAntigenmedicineAnimalsHumansAntigensBrain ChemistrybiologyStaining and LabelingPolysialic acidBacterial polysaccharideAntibodies MonoclonalDNAMolecular biologyImmunohistochemistrySialic acidBiochemistrychemistryLiverImmunoglobulin Gbiology.proteinSialic AcidsNeural cell adhesion moleculeAnatomyDNA ProbesImmunostainingThe journal of histochemistry and cytochemistry : official journal of the Histochemistry Society
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Magnetic Resonance Microscopy Contribution to Interpret High-Resolution Magic Angle Spinning Metabolomic Data of Human Tumor Tissue

2010

[EN] HRMAS NMR is considered a valuable technique to obtain detailed metabolic profile of unprocessed tissues. To properly interpret the HRMAS metabolomic results, detailed information of the actual state of the sample inside the rotor is needed. MRM (Magnetic Resonance Microscopy) was applied for obtaining structural and spatially localized metabolic information of the samples inside the HRMAS rotors. The tissue was observed stuck to the rotor wall under the effect of HRMAS spinning. MRM spectroscopy showed a transference of metabolites from the tissue to the medium. The sample shape and the metabolite transfer after HRMAS indicated that tissue had undergone alterations and it can not be s…

Hrmas nmrMagnetic Resonance SpectroscopyProteomelcsh:BiotechnologyHealth Toxicology and Mutagenesislcsh:MedicineHigh resolutionNuclear magnetic resonanceMetabolomicslcsh:TP248.13-248.65Tumor Cells CulturedGeneticsMagic angle spinningHumansTissue DistributionMolecular BiologyMethodology ReportBrain NeoplasmsMagnetic resonance microscopyChemistrylcsh:RGliomaGeneral MedicineNuclear magnetic resonance spectroscopyMagnetic Resonance ImagingHuman tumorBiochemistryMetabolomeMolecular MedicineSpin LabelsMetabolic profileBiotechnologyJournal of Biomedicine and Biotechnology
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