Search results for "cryopreservation"

showing 10 items of 148 documents

A new technique for analysis of human sperm morphology in unstained cells from raw semen

2014

Sperm morphology analysis is a fundamental component of semen analysis, but its real significance has been clouded by the plethora of techniques used for its evaluation. Most involve different fixation and staining procedures that induce artefacts. Herein we describe Trumorph (Proiser R+D, Paterna, Spain), a new method for sperm morphology analysis based on examination of wet preparations of spermatozoa immobilised, after a short 60°C shock, in narrow chambers and examined by negative phase contrast microscopy. A range of morphological forms was observed, similar to those found using conventional fixed and stained preparations, but other forms were also found, distinguishable only by the o…

Male0301 basic medicineReproductive immunologySemenReproductive technologySemen analysisBiologyCryopreservationTeratozoospermia03 medical and health sciences0302 clinical medicineEndocrinologySemenMicroscopyGeneticsmedicineHumansMicroscopy Phase-ContrastCell ShapeMolecular Biology030219 obstetrics & reproductive medicinemedicine.diagnostic_testurogenital systemAnatomySpermatozoaStainingSemen Analysis030104 developmental biologyReproductive MedicineBiochemistryCase-Control StudiesAnimal Science and ZoologySpermatogenesisDevelopmental BiologyBiotechnologyReproduction, Fertility and Development
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Methodological Approach to Use Fresh and Cryopreserved Vessels as Tools to Analyze Pharmacological Modulation of the Angiogenic Growth

2016

The sprouting of new vessels is greatly influenced by the procedure chosen. We sought to optimize the experimental conditions of the angiogenic growth of fresh and cryopreserved vessels cultured in Matrigel with the aim to use this system to analyze the pharmacological modulation of the process. Segments of second-order branches of rat mesenteric resistance arteries, thoracic aorta of rat or mouse, and cryopreserved rat aorta and human femoral arteries were cultured in Matrigel for 7-21 days in different mediums, as well as in the absence of endothelial or adventitia layer. Quantification of the angiogenic growth was performed by either direct measurement of the mean length of the neovessel…

Male0301 basic medicinemedicine.medical_treatmentNeovascularization PhysiologicAorta Thoracic030204 cardiovascular system & hematologycryopreservationFibroblast growth factorhuman vesselsNeovascularizationAndrologyangiogenesisMice03 medical and health scienceschemistry.chemical_compoundOrgan Culture Techniques0302 clinical medicinemedicine.arteryAdventitiamatrigelmedicineAnimalsHumansThoracic aortaRats WistarCryopreservationPharmacologyAortaMatrigelGrowth factorarterial ring assayRatsVascular endothelial growth factorDrug Combinations030104 developmental biologymedicine.anatomical_structurechemistryAdrenergic alpha-1 Receptor Antagonistscardiovascular systemProteoglycansAdrenergic alpha-1 Receptor AgonistsCollagenLamininmedicine.symptomCardiology and Cardiovascular MedicineJournal of Cardiovascular Pharmacology
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Viability, attachment efficiency, and xenobiotic metabolizing enzyme activities are well maintained in EDTA isolated rat liver parenchymal cells afte…

1995

Rat liver parenchymal cells were isolated by EDTA perfusion and were subsequently purified by Percoll centrifugation. The freshly isolated liver cells had a mean viability of 95% as judged by trypan blue exclusion. Isolated liver parenchymal cells were then stored at 0°C for up to 1 wk in University of Wisconsin solution (UW). During this hypothermic preservation, the viability was only slightly reduced to 92% after 1 d and to 85% after 3 d at 0°C. Thereafter, the viability decreased rapidly. After cold storage for up to 3 d, it was possible to use the parenchymal liver cells either in short-term suspension or in cell culture. The attachment efficiency in cell culture was the same for fresh…

MaleAdenosineCell SurvivalAllopurinolOrgan Preservation SolutionsCold storageBiologyXenobioticsRats Sprague-Dawleychemistry.chemical_compoundCryoprotective AgentsRaffinoseCell AdhesionAnimalsInsulinViaspanCentrifugationCells CulturedEdetic AcidCryopreservationCell BiologyGeneral MedicineGlutathioneMolecular biologyIn vitroEnzymesRatsLiverBiochemistrychemistryCell cultureTrypan blueStem cellPercollDevelopmental BiologyIn Vitro Cellular & Developmental Biology - Animal
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Cultures with cryopreserved hepatocytes: applicability for studies of enzyme induction

2000

The use of hepatocyte cultures is well established for the study of drug-drug interactions. However, the major hindrance for the use of human hepatocyte cultures is that human hepatocytes are only occasionally available. This problem could be overcome by cryopreservation. Although cryopreserved hepatocytes have been recommended for short term applications in suspension, studies on induction of enzyme activity, requiring a more prolonged maintenance of cryopreserved hepatocytes in culture, represent a new field of research. In the present study, we established a technique that allows preparation of rat hepatocyte co-cultures, using cryopreserved hepatocytes. After incubation with phenobarbit…

MaleCell SurvivalMetaboliteBiologyToxicologyCryopreservationRats Sprague-DawleyHydroxylationchemistry.chemical_compoundCytochrome P-450 Enzyme SystemIn vivoCell AdhesionCytochrome P-450 CYP1A1medicineAnimalsEnzyme inducerCells CulturedGlutathione TransferaseCryopreservationCytochrome P450General MedicineCoculture TechniquesEnzyme assayRatsmedicine.anatomical_structureLiverchemistryBiochemistryEnzyme InductionPhenobarbitalHepatocyteCytochrome P-450 CYP2B1biology.proteinHydroxytestosteronesInstitut für ErnährungswissenschaftMethylcholanthreneChemico-Biological Interactions
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A Method for the Cryopreservation of Liver Parenchymal Cells for Studies of Xenobiotics

1993

Abstract An optimized computer-controlled freezing protocol for the cryopreservation of rat liver parenchymal cells was developed. The best survival rates were obtained when a slow cooling rate was used and when the supercooling was interrupted with a shock cooling to initiate ice nucleation. Ten percent dimethyl sulfoxide was added and removed gradually for best results. Thawed rat liver parenchymal cells had a viability, as judged by trypan blue exclusion, of 69% (SD = 6) versus 82% (SD = 7) for freshly isolated cells. The content and activities of the xenobiotic metabolizing enzymes, cytochrome P450. UDP-glucuronosyl transferase, and microsomal and cytosolic epoxide hydrolase, were not a…

MaleCryobiologyCell SurvivalGuinea PigsIn Vitro TechniquesBiologyGeneral Biochemistry Genetics and Molecular BiologyCryopreservationXenobioticsRats Sprague-Dawleychemistry.chemical_compoundDogsSpecies SpecificityCricetinaeBenzo(a)pyrenemedicineAnimalsHumansDimethyl SulfoxideEpoxide hydrolaseCryopreservationGeneral MedicineMolecular biologyRatsmedicine.anatomical_structureLiverBiochemistrychemistryEvaluation Studies as TopicHepatocyteMicrosomeTrypan blueGeneral Agricultural and Biological SciencesPercollDrug metabolismCryobiology
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Derivation and characterization of three new Spanish human embryonic stem cell lines (VAL −3 −4 −5) on human feeder and in serum-free conditions

2006

A total of 184 human embryos, frozen for >5 years, were donated; informed consent was obtained according to Spanish law 45/2003. Survival rate was 40% and three out of 24 blastocysts (12.5%) developed into putative hESC lines, named VAL-3, VAL-4, and VAL-5. The derivation process was performed on microbiologically tested and irradiated human foreskin fibroblasts and designed to minimize contact with xeno-components in knockout DMEM supplemented with knockout serum replacement, and basic fibroblast growth factor. Fingerprinting and HLA typing of the cell lines allowed their identification and traceability. Karyotype was normal for VAL-3 (46XY), VAL-4 (46XX) and VAL-5 (46XX). All three hESC l…

MaleHomeobox protein NANOGCellular differentiationTransplantation HeterologousCell Culture TechniquesGene ExpressionMice SCIDGerm layerBiologyCriptoCulture Media Serum-FreeCell LineMiceSOX2Mice Inbred NODmedicineAnimalsHumansEmbryonic Stem CellsDNA PrimersCryopreservationGeneticsBase SequenceObstetrics and GynecologyCell DifferentiationFibroblastsEmbryonic stem cellMolecular biologyCoculture TechniquesTransplantationmedicine.anatomical_structureReproductive MedicineSpainKaryotypingembryonic structuresFemaleEndodermBiomarkersStem Cell TransplantationDevelopmental BiologyReproductive BioMedicine Online
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Cryopreservation of rat, dog and human hepatocytes: influence of preculture and cryoprotectants on recovery, cytochrome P450 activities and induction…

2006

Several cryopreservation protocols for hepatocytes have been proposed over the past few years, but their effectiveness varies greatly as a function of the characteristics of the method used. One factor in the success of cryopreservation is the quality of cells before freezing. The results suggest that the cryopreservation of hepatocytes in a medium containing polyvinylpyrrolidone (PVP), in addition to DMSO, constitutes a convenient means of long-term storage of hepatocytes for preparing primary cultures to be used in drug metabolism studies. The combined use of the two cryoprotectants is particularly critical for low-viability cell suspensions. An interesting alternative to increase cell vi…

MaleHot TemperatureCryoprotectantHealth Toxicology and MutagenesisCellCombined useDrug Evaluation PreclinicalToxicologyBiochemistryCryopreservationRats Sprague-DawleyCryoprotective AgentsDogsCytochrome P-450 Enzyme SystemmedicineAnimalsHumansDimethyl SulfoxideViability assayCells CulturedCryopreservationPharmacologybiologyPovidoneCytochrome P450General MedicineRatsCell biologyEnzyme Activationmedicine.anatomical_structureBiochemistryHepatocytesbiology.proteinDrug metabolismXenobiotica
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The effect of cancer on sperm DNA fragmentation as measured by the sperm chromatin dispersion test

2008

The percentage of spermatozoa with fragmented DNA from cancer patients before surgery, chemotherapy, or radiotherapy treatments was compared with infertile male patients in an assisted reproduction program and with sperm donors of proven fertility. The percentages of DNA fragmentation were 34.3% in cancer patients, 30.9% in infertile men whose partners did not become pregnant, 28.8% in men who partners became pregnant, and 10.8% in fertile sperm donors. The DNA fragmentation of sperm donors was statistically significantly lower compared the other groups. No statistically significant differences were found in the levels of DNA fragmentation when comparing cancer types, including those of tes…

MaleInfertilityendocrine systemPregnancy Ratemedia_common.quotation_subjectPilot ProjectsFertilitySemenDNA FragmentationBiologyAndrologyPregnancyNeoplasmsmedicineHumansSperm Injections IntracytoplasmicFragmentation (cell biology)Infertility Malereproductive and urinary physiologySperm motilitymedia_commonCryopreservationSperm Counturogenital systemObstetrics and GynecologyCancermedicine.diseaseSpermatozoaSpermChromatinTreatment OutcomeReproductive MedicineSperm MotilityDNA fragmentationFemaleSemen PreservationFertility and Sterility
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Neonatal Livers: A Source for the Isolation of Good-Performing Hepatocytes for Cell Transplantation

2014

Hepatocyte transplantation is an alternative therapy to orthotopic liver transplantation for the treatment of liver diseases. However, the supply of hepatocytes is limited given the shortage of organs available to isolate good-functioning quality cells. Neonatal livers may be a potential source alternative to adult livers to obtain good-performing hepatic cells for hepatocyte transplantation, which has not yet been explored profoundly. High-yield preparations of viable hepatocytes were isolated from 1- to 23-day-old liver donors, cryopreserved, and banked. Cell integrity and functional quality assessment were performed after thawing. Neonatal hepatocytes showed better postthawing recovery …

MaleLiver cytologyCellBiomedical Engineeringlcsh:MedicineCell SeparationBiologyCryopreservationAndrologymedicineHumansProgenitor cellCells CulturedCryopreservationTransplantationlcsh:RInfant NewbornCell BiologyLiver TransplantationTransplantationmedicine.anatomical_structureLiverApoptosisHepatocyteHepatocytesHepatic stellate cellFemaleCell Transplantation
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Computer assisted sperm morphometry in mammals: a review.

2014

Computer-assisted sperm morphometry analysis (CASMA or ASMA) systems were developed to reduce the subjectivity of sperm morphology assessement. This review focuses on a complete description of the CASMA technique, including recent developments, factors of variation, results in the different species and possible applications. Techniques to study sperm morphometry include light microscopy, phase-contrast microscopy and, more recently, fluorescence microscopy. Most published studies on sperm morphometry have been centered on the whole sperm heads, although some of them also measured other parts of the sperm structure, such as the nucleus, acrosome, midpiece or flagellum. The independent study …

MaleMammalsendocrine systemurogenital systemmedia_common.quotation_subjectSample processingFertilitySemenGeneral MedicineBiologySemen cryopreservationSpermSpermatozoaAndrologySemen AnalysisEndocrinologyFood AnimalsSperm morphologyImage Processing Computer-AssistedAnimalsAnimal Science and ZoologySperm qualityAcrosomereproductive and urinary physiologymedia_commonAnimal reproduction science
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