Search results for "Lysine"

showing 10 items of 170 documents

Mobility of Acetylated Histones in Sodium Dodecyl Sulfate–Polyacrylamide Gel Electrophoresis

1999

Abstract We describe an altered mobility for acetylated histone isoforms in sodium dodecyl sulfate–polyacrylamide gel electrophoresis. Isoforms of histones H3 and H4 with a higher acetylation degree have a slightly faster electrophoretic mobility. Since acetylation neutralizes the positive charge of the e-amino group of lysine, without significantly changing the molecular mass of the protein, the acetylation-dependent mobility shift could be explained by the increase of the net negative charge of the SDS–histone complexes. A possible consequence of this differential mobility for the acetylation site determination by protein microsequencing from SDS gels is discussed.

ErythrocytesSodiumLysineBiophysicschemistry.chemical_elementBiochemistryHistoneschemistry.chemical_compoundElectrochemistryAnimalsSodium dodecyl sulfateMolecular BiologyPolyacrylamide gel electrophoresisGel electrophoresisChromatographyMolecular massReproducibility of ResultsSodium Dodecyl SulfateAcetylationCell BiologyBlood Protein ElectrophoresisElectrophoresischemistryBiochemistryAcetylationElectrophoresis Polyacrylamide GelChickensAnalytical Biochemistry
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The pioneering role of PRDM9 indel mutations in tarsier evolution

2016

PRDM9 is currently the sole speciation gene found in vertebrates causing hybrid sterility probably due to incompatible alleles. Its role in defining the double strand break loci during the meiotic prophase I is crucial for proper chromosome segregation. Therefore, the rapid turnover of the loci determining zinc finger array seems to be causative for incompatibilities. We here investigated the zinc finger domain-containing exon of PRDM9 in 23 tarsiers. Tarsiers, the most basal extant haplorhine primates, exhibit two frameshifting indels at the 5'-end of the array. The first mutation event interrupts the reading frame and function while the second compensates both. The fixation of this allele…

Evolution MolecularINDEL MutationProtein DomainsTarsiidaeAnimalsZinc FingersHistone-Lysine N-MethyltransferaseArticle570 Biowissenschaften570 Life sciencesScientific Reports
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Fluorometric determination of chemically available lysine: adaptation, validation and application to different milk products.

2004

A spectrophotometric method based on the reaction between available lysine and ortho-phthaldialdehyde (OPA) was adapted and validated for fluorometric determination of the chemically available lysine contents in milk matrices (UHT and conventional in-bottle sterilized cow milk, milk-based infant formulas and infant formula ingredients). The values of the analytical parameters show its usefulness as a routine method (linearity, r = 0.9992; detection limit, 0.0066 mg/mL assay; accuracy, 99-108%; precision, intra-day 2.1-5.9% and inter-day 3.5 10.2%). No statistically significant differences (p < 0.05) were found between the values obtained with the adapted method and those obtained applying t…

Food HandlingLysineFluorescence spectrometryPasteurizationBiological AvailabilitySensitivity and Specificitylaw.inventionCow milkMilk productslawAnimalsHumansFluorometryFood scienceDetection limitChromatographyChemistryLysineSterilized milkInfant Newbornfood and beveragesInfantReproducibility of ResultsMilkInfant formulaCalibrationInfant FoodFood ScienceDie Nahrung
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Risk Assessment of "Other Substances" – L-lysine

2020

The Norwegian Scientific Committee for Food Safety (Vitenskapskomiteen for mattrygghet, VKM) has, at the request of the Norwegian Food Safety Authority (Mattilsynet; NFSA), assessed the risk of "other substances" in food supplements and energy drinks sold in Norway. VKM has assessed the risk of doses given by NFSA. These risk assessments will provide NFSA with the scientific basis while regulating "other substances" in food supplements.&#x0D; "Other substances" are described in the food supplement directive 2002/46/EC as substances other than vitamins or minerals that have a nutritional and/ or physiological effect. It is added mainly to food supplements, but also to energy drinks and other…

Food supplementbusiness.industryAdverse health effectEnvironmental healthLysineMedicinebusinessRisk assessmentEuropean Journal of Nutrition &amp; Food Safety
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Transcriptional regulation of theNε-fructoselysine metabolism inEscherichia coliby global and substrate-specific cues

2020

AbstractThermally processed food is an important part of the human diet. Heat-treatment, however, promotes the formation of so-called Amadori rearrangement products (ARPs), such as fructoselysine. The gut microbiota includingEscherichia colican utilize these compounds as a nutrient source. While the degradation route for fructoselysine is well described, regulation of the corresponding pathway genesfrlABCDremained poorly understood. Here we use bioinformatics combined with molecular and biochemical analyses and show that inE. coli, fructoselysine metabolism is tightly controlled at the transcriptional level. The global regulator Crp (CAP), as well as the alternative sigma factor σ32 (RpoH) …

FructoselysineChemistrySigma factorAmadori rearrangementTranscriptional regulationmedicineRegulatorRepressormedicine.disease_causeGeneEscherichia coliCell biology
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Rapid PCR-based test for identifying Candida albicans by using primers derived from the pH-regulated KER1 gene.

2006

A PCR-based method in combination with a simple, reliable and inexpensive DNA extraction procedure for rapid detection of Candida albicans clinical isolates is described here. The extraction protocol is based on a combination of chemical (NaOH and detergents) and physical (boiling) treatments, thus avoiding many of the problems inherent in the currently available DNA extraction protocols (basically the use of expensive and/or toxic chemical reagents), and may be useful for daily clinical routine. The PCR-based system described here uses a single pair of primers (SC1F and SC1R) deduced from the C. albicans-specific KER1 gene sequence. These primers amplify a 670-bp fragment of the KER1 gene.…

Fungal proteinbiologyInverse polymerase chain reactionLysineGenes FungalMultiple displacement amplificationGlutamic AcidMembrane ProteinsGeneral MedicineAmpliconHydrogen-Ion Concentrationbiology.organism_classificationApplied Microbiology and BiotechnologyMicrobiologyDNA extractionMolecular biologyPolymerase Chain ReactionCorpus albicanslaw.inventionFungal ProteinslawCandida albicansCandida albicansPolymerase chain reactionDNA PrimersFEMS yeast research
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Promoter-Targeted Histone Acetylation of Chromatinized Parvoviral Genome Is Essential for the Progress of Infection

2015

ABSTRACT The association of host histones with parvoviral DNA is poorly understood. We analyzed the chromatinization and histone acetylation of canine parvovirus DNA during infection by confocal imaging and in situ proximity ligation assay combined with chromatin immunoprecipitation and high-throughput sequencing. We found that during late infection, parvovirus replication bodies were rich in histones bearing modifications characteristic of transcriptionally active chromatin, i.e., histone H3 lysine 27 acetylation (H3K27ac). H3K27ac, in particular, was located in close proximity to the viral DNA-binding protein NS1. Importantly, our results show for the first time that in the chromatinized …

Gene Expression Regulation Viral0301 basic medicineParvovirus CanineVirus IntegrationvirusesImmunologyGenome ViralMicrobiologyCell LineEpigenesis Geneticviral DNAHistonesParvoviridae Infections03 medical and health sciencesHistone H3VirologyAnimalsHistone codeNucleosomePromoter Regions GeneticEpigenomicsMicroscopy ConfocalbiologyLysinecanine parvovirushistone acetylationAcetylationHistone acetyltransferaseVirologyChromatinchromatinizationVirus-Cell Interactions3. Good healthChromatin030104 developmental biologyHistoneInsect ScienceDNA ViralCatsbiology.proteinChromatin immunoprecipitationJournal of Virology
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Human cationic amino acid transporter gene hCAT-2 is assigned to 8p22 but is not the causative gene in lysinuric protein intolerance

1997

Lysinuric protein intolerance (LPI) is a recessively inherited amino acid disorder characterized by defective efflux of cationic amino acids at the basolateral membrane of the intestinal and renal tubular epithelium. Recently, cDNAs encoding the related proteins hCAT-2A and hCAT-2B have been cloned. These two carrier proteins are most likely the product of the same gene, hCAT-2. Using the hCAT-2B cDNA, we assigned the hCAT-2 gene to chromosome 8p22. Furthermore, by linkage analysis in Finnish LPI families, we ruled out that hCAT-2B is involved in LPI disease.

Genetic LinkageBiologyGene mappingGenetic linkageComplementary DNAGeneticsmedicineHumansAmino acid transporterAmino Acid Metabolism Inborn ErrorsGeneGenetics (clinical)chemistry.chemical_classificationLysineChromosome MappingMembrane Proteinsmedicine.diseaseLysinuric protein intoleranceAmino acidchemistryBiochemistryAmino Acid Transport Systems BasicEffluxCarrier ProteinsChromosomes Human Pair 8Microsatellite RepeatsHuman Genetics
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Lysine synthesis control in Corynebacterium glutamicum RC 115 in mixed substrate (glucose-acetate) medium.

2003

The effect of acetate as a glucose co-substrate on growth, lysine synthesis and experimental lysine yield from carbon substrates by Corynebacterium glutamicum RC 115 was investigated. It was found that low amounts of acetate, injected with a glucose-acetate pulse into the steady-state continuous culture in bioreactor, caused a slight decrease in the specific rates of glucose uptake and bacterial growth, but a significant increase in the cell specific rate of lysine synthesis and an increase in lysine yield. In contrast, acetate injected in high amounts was followed by a drastic decrease in the values of these parameters. A strong increase in experimental lysine yield under the latter condit…

Glucose uptakeLysineCell Culture TechniquesBioengineeringBacterial growthBiologyAcetatesCorynebacteriumcomplex mixturesApplied Microbiology and BiotechnologyCorynebacterium glutamicumFeedbackchemistry.chemical_compoundBioreactorsBiosynthesisBioreactorHomeostasisLysineSubstrate (chemistry)General MedicineAdaptation PhysiologicalGlucoseBiochemistrychemistryYield (chemistry)Flow Injection AnalysisbacteriaCell DivisionBiotechnologyJournal of biotechnology
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Differential specificity of substrate-attached lectins stimulating spreading of GH3-cells under serum-free, hormone-supplemented culture conditions

1982

Most mammalian cells are capable of growth in culture only when they are supplied with an appropriate substrate to which they can adhere and spread. To prepare suitable substrates different lectins were attached onto polystyrene tissue-culture dishes after coating with polylysine. GH3-cells (a pituitary-tumor-cell line) were seeded into the culture dishes containing serum-free, hormone-supplemented medium. When succinylated Concanavalin A (s-Con A), which binds specifically to mannose residues, is attached to the surface an extraordinary spreading of GH3-cells is induced within 15 to 20 min after seeding. Other lectins with a different sugar-binding specificity are less effective in inducin…

HistologyCellMannosePituitary neoplasmBiologyCell LinePathology and Forensic MedicineStructure-Activity Relationshipchemistry.chemical_compoundCell MovementLectinsCell AdhesionConcanavalin AmedicineAnimalsPituitary NeoplasmsCell adhesionSubstrate (chemistry)Cell BiologyHormonesCulture MediaKineticsmedicine.anatomical_structurechemistryBiochemistryCell cultureConcanavalin APolylysinebiology.proteinMannoseCell and Tissue Research
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