14 results on '"Harald, Klüter"'
Search Results
2. Atmospheric pressure plasma assisted immobilization of hyaluronic acid on tissue engineering PLA-based scaffolds and its effect on primary human macrophages
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Julia Kzhyshkowska, Harald Klüter, K.S. Stankevich, Victor D. Filimonov, Sergei I. Tverdokhlebov, Alexandu Gudima, Vladimir Riabov, E.N. Bolbasov, Gennady E. Remnev, Anna Malashicheva, M. V. Zhuravlev, Tengfei Liu, Elina Kibler, Valeriya L. Kudryavtseva, and Yuri M. Zhukov
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0301 basic medicine ,chemistry.chemical_classification ,Tube formation ,Scaffold ,Materials science ,Biocompatibility ,Mechanical Engineering ,02 engineering and technology ,Polymer ,Matrix metalloproteinase ,021001 nanoscience & nanotechnology ,03 medical and health sciences ,chemistry.chemical_compound ,030104 developmental biology ,chemistry ,Polylactic acid ,Tissue engineering ,Mechanics of Materials ,Hyaluronic acid ,lcsh:TA401-492 ,Biophysics ,lcsh:Materials of engineering and construction. Mechanics of materials ,General Materials Science ,0210 nano-technology ,Biomedical engineering - Abstract
Bioactive polylactic acid based (PLA) scaffolds with hyaluronic acid immobilized on their surface by atmospheric pressure plasma assisted modification method were developed. By using X-ray photoelectron spectroscopy and wettability measurements it was shown that atmospheric pressure plasma treatment leads to the changes in surface chemical composition of the PLA-based scaffolds that resulted in an increased long-term hydrophilicity of the scaffolds surface. Scanning electron microscopy and mechanical studies revealed that the use of plasma for surface activation allows for the non-destructive immobilization of bioactive compounds like hyaluronic acid. The modified PLA-based scaffolds effect on the release of cytokines and matrix metalloproteinases by primary human monocyte-derived macrophages was investigated. The macrophages reaction to the scaffolds was donor-specific, however, the two best materials from immunological point of view were identified - plasma treated PLA-based scaffold and PLA-based scaffold with the least amount of immobilized hyaluronic acid. Both hyaluronic acid attachment and atmospheric pressure plasma treatment enhance PLA-based scaffolds biocompatibility. It was found that supernatants collected after the macrophages coculture with modified PLA-based scaffolds stimulate HUVECs' tube formation. The modified PLA-based scaffolds possess pro-angiogenic activity. Thus, our research offers a high-performing method for the creation of polymer-based tissue engineering scaffolds with modified bioactive surface. Keywords: Polylactic acid (PLA), Hyaluronic acid (HA), Tissue engineering scaffold (TES), Plasma, Macrophages, Cytokines
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- 2017
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3. Retinal pigment epithelial phenotype induced in human adipose tissue-derived mesenchymal stromal cells
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Harald Klüter, Karen Bieback, Jost B. Jonas, Hermann-Josef Thierse, Urs Vossmerbaeumer, Sandra Kuehl, Stefanie Ohnesorge, and Minna Haapalahti
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cis-trans-Isomerases ,Cancer Research ,Cell type ,Pathology ,medicine.medical_specialty ,Stromal cell ,Swine ,Cellular differentiation ,Immunology ,Vasoactive intestinal peptide ,Retinal Pigment Epithelium ,Biology ,chemistry.chemical_compound ,Chloride Channels ,medicine ,Animals ,Humans ,Immunology and Allergy ,Melanocyte-Stimulating Hormones ,Bestrophins ,Eye Proteins ,Genetics (clinical) ,Melanins ,Transplantation ,Retinal pigment epithelium ,Keratin-18 ,Keratin-8 ,Mesenchymal stem cell ,Cell Differentiation ,Mesenchymal Stem Cells ,Retinal ,Cell Biology ,Antigens, Differentiation ,eye diseases ,Cell biology ,medicine.anatomical_structure ,Adipose Tissue ,Oncology ,chemistry ,Culture Media, Conditioned ,Cis-trans-Isomerases ,sense organs ,Stromal Cells ,Carrier Proteins ,Vasoactive Intestinal Peptide - Abstract
Background aims The non-exudative form of age-related macular degeneration (ARMD) is characterized by a progressive decay of retinal pigment epithelium cells at the posterior pole of the eye. As mesenchymal stromal cells (MSC) have been shown to differentiate into various cell types from the mesodermal and ectodermal lineages, we investigated whether we can induce a phenotype displaying retinal pigment epithelium (RPE) characteristics. Methods The differentiation of human lipo-aspirate-derived MSC toward the RPE lineage was triggered by exposure to conditioned medium from either human or porcine RPE cells. In a second approach we tested whether adding vasoactive intestinal peptide (VIP) is capable of further modifying differentiation processes. Resulting cell populations were assessed for expression of RPE-specific markers by immunofluorescence, quantitative real time (RT)-polymerase chain reaction (PCR) and Western blotting. The potential for pigment synthesis was assessed by the response to melanocyte-stimulating hormone (MSH). Results Following culture of undifferentiated MSC with RPE-conditioned medium and/or VIP, expression of typical RPE markers bestrophin, cytokeratins 8 and 18 and RPE 65 was induced. MSH induced the formation of pigmented granula in differentiated MSC. Conclusions MSC are shown to express RPE markers upon induction with either RPE-conditioned medium and/or VIP. The gain of basic functional features of RPE cells was indicated by melanin synthesis. This alludes to a differentiation potential of MSC into the neuroectodermal lineage, yielding cells with phenotypic characteristics of RPE cells.
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- 2009
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4. Cultivation and differentiation characteristics of human limbal progenitor cells
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Urs Vossmerbaeumer, Jost B. Jonas, Sandra Kuehl, Harald Klüter, and Karen Bieback
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Pathology ,medicine.medical_specialty ,Cell Culture Techniques ,Mitosis ,Limbus Corneae ,Corneal limbus ,chemistry.chemical_compound ,Phagocytosis ,medicine ,Humans ,Progenitor cell ,Pigment Epithelium of Eye ,Fluorescein isothiocyanate ,Cells, Cultured ,Progenitor ,Neurons ,Retinal pigment epithelium ,biology ,Stem Cells ,Cell Differentiation ,Cell Biology ,General Medicine ,Nestin ,eye diseases ,Cell biology ,medicine.anatomical_structure ,Bestrophin 1 ,chemistry ,Cell culture ,biology.protein ,sense organs ,Neuroglia ,Biomarkers ,Developmental Biology - Abstract
Background The aim of this study was to investigate whether limbal progenitor cells can be cultured, expanded and differentiated in vitro not only to enter corneal differentiation but also towards RPE (retinal pigment epithelium) characteristics. Methods A 3 mm broad strip of human corneoscleral limbal tissue was digested enzymatically and cells were set into cell culture. Differentiation status and characteristics, proliferation and phagocytotic activity were assessed by immunocytochemical staining in combination with digital and confocal microscopy. Results Immunocytological analysis revealed expression of Nestin and p63 marker suggesting progenitor cell properties. Mitotic activity was demonstrated by BrdU (bromodesoxyuridine) uptake. Upon consecutive passages, corneal differentiation markers were predominantly expressed. Phagocytotic activity was demonstrated via uptake of FITC (fluorescein isothiocyanate) labelled latex beads. RPE markers Bestrophin and Cytokeratin 8/18 as well as glial marker GFAP and neuronal marker MAP with respective controls were negative indicating no differentiation towards characteristics of retinal pigment epithelium or neural and glial lineage. Conclusions The results suggest that isolation and cultivation of proliferating and phagocytotic cells from the human corneal limbus was achieved which showed characteristics of both progenitor and differentiated corneal cells. No evidence was found for the hypothesis of spontaneous differentiation potential towards RPE lineage or neuronal characteristics, providing evidence of the inherent directional capacity of limbal progenitor cells.
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- 2008
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5. Effects of alimentary lipemia and inflammation on platelet CD40-ligand
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Harald Klüter, Xuan Duc Nguyen, Elif Elmas, H. Leweling, Stefan Kralev, Thorsten Kälsch, Carl-Erik Dempfle, and Martin Borggrefe
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Adult ,Blood Platelets ,Lipopolysaccharides ,Male ,medicine.medical_specialty ,CD40 Ligand ,Hypercholesterolemia ,Hyperlipidemias ,Inflammation ,Stimulation ,Thromboplastin ,chemistry.chemical_compound ,Internal medicine ,medicine ,Humans ,Platelet ,CD40 Antigens ,L-Selectin ,Aged ,Whole blood ,Triglyceride ,Monocyte ,hemic and immune systems ,Hematology ,Middle Aged ,Postprandial Period ,medicine.anatomical_structure ,Postprandial ,Endocrinology ,Gene Expression Regulation ,chemistry ,Female ,medicine.symptom ,Lipoprotein - Abstract
Introduction In patients with chronic hypercholesterolemia, the CD40–CD40L dyad is upregulated, contributing to the initiation and progression of atherosclerosis. Our aim was to describe the role of postprandial lipemia and inflammatory stimulation on platelet and monocyte activation and CD40-ligand (CD40L) levels. Methods and results Before and 2 h after consumption of a defined fatty meal, whole blood samples of 31 healthy subjects were incubated with endotoxin (LPS). CD40-ligand and CD62P expression on platelets, tissue-factor expression on monocytes and platelet-monocyte aggregates were measured with flow cytometry. Soluble CD40-ligand plasma levels were measured with an ELISA. After the meal, serum triglyceride levels increased from 137.6 ± 60.5 mg/dl to 201.5 ± 75.0 mg/dl. Expression of CD40L and CD62P on platelets and plasma levels of soluble CD40L were significantly decreased. No significant changes after the meal were observed concerning tissue factor expression on monocytes and platelet-monocyte aggregates. Addition of LPS showed no significant effect concerning CD40L or CD62P expression on platelets, whereas the amount of platelet-monocyte aggregates significantly increased under LPS stimulation after the fatty meal. Conclusions Acute alimenatry lipemia leads to a decreased expression of CD40L on platelets and a reduced plasma level of sCD40L, suggesting an increased turnover in the CD40L system. Condensed abstract Before and after a fatty meal, blood samples of 31 healthy subjects were incubated with LPS. After the meal, expression of CD40L and CD62P on platelets and plasma levels of soluble CD40L were significantly decreased. Addition of LPS showed no effect concerning CD40L or CD62P expression, whereas the amount of platelet-monocyte aggregates significantly increased under LPS stimulation after the fatty meal.
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- 2007
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6. Coagulation activation and expression of CD40 ligand on platelets upon in vitro lipopolysaccharide-challenge in patients with unstable angina
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Nadine Grebert, Carl-Erik Dempfle, Thorsten Kälsch, Harald Klüter, Elif Elmas, Martin Borggrefe, Xuan Duc Nguyen, and Tim Süselbeck
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Blood Platelets ,Lipopolysaccharides ,Male ,medicine.medical_specialty ,CD40 Ligand ,Coronary Disease ,Coronary thrombosis ,Internal medicine ,medicine ,Humans ,Platelet ,Angina, Unstable ,Myocardial infarction ,Blood Coagulation ,Aged ,Whole blood ,Triazines ,Unstable angina ,business.industry ,Middle Aged ,Flow Cytometry ,medicine.disease ,Coagulation ,Circulatory system ,Prothrombin Time ,Cardiology ,Female ,Cardiology and Cardiovascular Medicine ,business ,Platelet factor 4 - Abstract
Background Elevated markers of inflammation and coagulation are found in patients with coronary heart disease. A role of inflammatory stimulation on coagulation time and expression of CD40 ligand on platelets in acute coronary syndromes has not been described yet. Methods and results Whole blood samples of 9 patients with coronary heart disease and stable angina, 10 patients with unstable angina, 7 patients with acute myocardial infarction and 7 patients without coronary heart disease were incubated with lipopolysaccharide (LPS). Coagulation time was measured in arterial and coronary blood with the ReoRox®, a viscometric whole blood coagulometer. CD40L and CD62P expression on platelets and platelet–monocyte aggregates were measured by flow cytometry. Without LPS, patients with unstable angina showed a significantly decreased coagulation time in arterial and coronary blood compared to patients without coronary heart disease. After incubation with LPS, in patients with unstable angina, a significantly decreased coagulation time in coronary blood was observed compared to patients with stable angina or patients without coronary heart disease. CD40L expression on platelets in patients with unstable angina was significantly higher in arterial and coronary blood compared to patients with stable angina. No significant differences between the patient groups were observed concerning CD62P expression on platelets, tissue factor binding on monocytes, platelet–monocyte aggregates and plasma levels of platelet factor 4. Conclusions Patients with unstable angina show an enhanced coagulation activation and an upregulation of CD40L on platelets. This may be of importance in the understanding of coronary plaque rupture and formation of coronary thrombosis.
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- 2006
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7. Enhanced expression of platelet CD40-ligand by in vitro lipopolysaccharide-challenge in patients with ventricular fibrillation complicating acute myocardial infarction
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Christian Wolpert, Karl K. Haase, Xuan Duc Nguyen, Elif Elmas, Martin Borggrefe, Thorsten Kälsch, Carl-Erik Dempfle, and Harald Klüter
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Lipopolysaccharides ,Male ,medicine.medical_specialty ,Heart disease ,CD40 Ligand ,Myocardial Infarction ,In Vitro Techniques ,Tissue factor ,Internal medicine ,medicine ,Humans ,Platelet ,cardiovascular diseases ,Platelet activation ,Myocardial infarction ,Retrospective Studies ,Whole blood ,business.industry ,Middle Aged ,medicine.disease ,Cross-Sectional Studies ,Case-Control Studies ,Ventricular Fibrillation ,Circulatory system ,Ventricular fibrillation ,Cardiology ,Female ,Cardiology and Cardiovascular Medicine ,business ,Biomarkers - Abstract
Background Acute myocardial infarction can be complicated by ventricular arrhythmias due to electrophysiological changes in the ischemic myocardium, but the exact predisposing factors causing ventricular fibrillation during myocardial infarction still remain unclear. A role of inflammatory stimulation on platelets as a potential risk factor for ventricular fibrillation during acute myocardial infarction has not been described yet. Methods and results Whole blood samples of 21 patients with a history of acute myocardial infarction (AMI) and ventricular fibrillation (VF) were incubated with lipopolysaccharide (LPS). As a control group, we studied 19 patients without VF during AMI. CD40-ligand and CD62P expression on platelets and tissue factor binding on monocytes were measured by flow cytometry. Platelet–monocyte aggregates were measured by CD41 expression on platelets adherent to monocytes. Soluble CD40-ligand plasma levels were measured with an ELISA. Without LPS, no significant difference between the patient groups concerning CD40L expression on platelets was observed, but plasma levels of soluble CD40L were significantly higher in patients with a history of AMI with VF. After LPS stimulation, patients with a history of VF showed a significantly increased expression of CD40L in comparison to the patients without ventricular fibrillation, based on a significantly higher increase of CD40L expression. CD62P expression on platelets was significantly increased in patients with a history of VF. Conclusions Patients with a history of VF complicating AMI show an enhanced expression of CD40L on platelets after in vitro lipopolysaccharide-challenge with an enhanced platelet activation.
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- 2006
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8. Introduction of a validation concept for a PCR-based Mycoplasma detection assay
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E. Pirkl, M. Stoermer, I. Bruchmüller, Peter Bugert, R. Herrmann, Harald Klüter, and Hermann Eichler
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DNA, Bacterial ,Cancer Research ,Transplantation ,Oligonucleotide ,Immunology ,Pcr assay ,Reproducibility of Results ,Cell Biology ,Mycoplasma ,Biology ,medicine.disease_cause ,16S ribosomal RNA ,Polymerase Chain Reaction ,Sensitivity and Specificity ,Microbiology ,Oncology ,Research Design ,RNA, Ribosomal, 16S ,medicine ,Humans ,Immunology and Allergy ,Self-Sustained Sequence Replication ,Genetics (clinical) ,Mycoplasma contamination - Abstract
Mycoplasma contamination is amongst the most frequently occurring problems associated with cell cultures. In order to meet the legal requirements (European Pharmacopoeia and FDA) for Mycoplasma testing of cell lines and therapeutics, we have developed a PCR-based method to detect mycoplasms and introduce a validation concept.The PCR assay specifically amplifies a 280-bp DNA fragment of the gene coding for the 16S rDNA. Simultaneous amplification of an artificial oligonucleotide containing primer-binding sites allowed control of the efficacy of the PCR. The validation of the PCR assay was performed with two Mycoplasma reference strains, M. orale and M. pneumoniae. The validation concept included (i) cultivation of M. orale and M. pneumoniae in medium with an indicator for bacterial metabolism, (ii) determination of the color-changing units (CCU) in repeated dilution experiments and (iii) correlation of the PCR results with CCU values.The detection range was found to include all Mycoplasma species most commonly found in cell cultures. The analytical sensitivity of the PCR was the CCU equivalent of 100 for M. orale and M. pneumoniae. Probit analysis revealed a detection probability of 9% for a mean concentration of 1222 (935-1844) CCU/mL for M. pneumoniae and 2547 (1584-10,352) CCU/mL for M. orale.The validation of the Mycoplasma detection assay supported PCR as an attractive diagnostic tool that will help manage the important issue of Mycoplasma contamination of cell cultures.
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- 2006
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9. Diseased vein grafts express elevated inflammatory cytokine levels compared with atherosclerotic coronary arteries
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Hans H. Sievers, J.F. Matthias Bechtel, Harald Klüter, Claus Bartels, Uwe Schönbeck, D. Hartwig, and Jan Felix Christiansen
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Male ,Reoperation ,Pulmonary and Respiratory Medicine ,Pathology ,medicine.medical_specialty ,Coronary Artery Disease ,Veins ,Proinflammatory cytokine ,Coronary Restenosis ,medicine ,Humans ,Saphenous Vein ,Vein ,Aged ,Interleukin-6 ,Reverse Transcriptase Polymerase Chain Reaction ,Tumor Necrosis Factor-alpha ,business.industry ,Vascular disease ,Interleukin-8 ,Arteriosclerosis ,Middle Aged ,medicine.disease ,Coronary Vessels ,Immunohistochemistry ,Coronary arteries ,C-Reactive Protein ,medicine.anatomical_structure ,Circulatory system ,Cytokines ,Female ,Surgery ,Inflammation Mediators ,Cardiology and Cardiovascular Medicine ,Vein graft disease ,business ,Interleukin-1 ,Blood vessel - Abstract
The pathologic modifications characterizing vein graft disease resemble those observed in native arteriosclerosis, but in accelerated form. Although both disorders are considered to be inflammatory diseases, it remains to be determined whether diseased vein grafts and atherosclerotic coronary arteries differentially express inflammatory mediators. Therefore, we examined whether differences in the expression of proinflammatory cytokines by these two distinct vascular pathologies favor the accelerated inflammation within diseased vein grafts.The messengerRNA expression of various cytokines (interleukin-1 beta [IL-1 beta], IL-6, IL-8, tumor necrosis factor-alpha [TNF-alpha], interferon-gamma [IFN-gamma]) was quantified using real-time reverse transcriptase-polymerase chain reaction (RT-PCR) in tissue samples of native saphenous veins (NSV, n = 5), diseased coronary arteries (CAD, n = 25), and diseased vein grafts (VG, n = 13).Native saphenous veins did not contain any detectable transcripts except for IFN-gamma. As expected, CAD was characterized by the expression of IL-1 beta, IL-6, IL-8, IFN-gamma, and TNF-alpha mRNA. Interestingly VG also expressed these mediators, but at markedly higher levels. Quantification by RT-PCR revealed that, compared with specimens from the CAD group, VG specimens contained 5.8 +/- 1.2 times, 286 +/- 22 times, and 29 +/- 7.3 times as many transcripts for the cytokines IL-1 beta, IL-6 and TNF-alpha, respectively, as well as 25 +/- 8.3 times more transcripts for the chemokine IL-8. In contrast, the expression of IFN-gamma transcripts did not differ among the groups.The elevated expression of proinflammatory cytokine transcripts supports the hypothesis that diseased vein grafts, compared with atherosclerotic coronary arteries, are characterized by enhanced inflammatory activity that might accelerate atherosclerotic modifications. This may implicate new therapeutic strategies for the prevention of vein graft disease.
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- 2004
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10. Prenatal HLA genotyping of uncultured amniotic fluid samples contaminated with maternal blood
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Andrea B. Lese, W. Zieger, Peter Bugert, Hermann Eichler, Harald Klüter, and Jessica Meckies
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Amniotic fluid ,Genotype ,Oligonucleotides ,Human leukocyte antigen ,Polymerase Chain Reaction ,Umbilical cord ,law.invention ,Andrology ,Fetus ,HLA Antigens ,Pregnancy ,law ,medicine ,Humans ,Typing ,Polymerase chain reaction ,medicine.diagnostic_test ,business.industry ,Obstetrics and Gynecology ,Amniotic Fluid ,Blood ,medicine.anatomical_structure ,HLA-B Antigens ,Molecular Probes ,Cord blood ,Immunology ,Amniocentesis ,Female ,business ,Forecasting - Abstract
Objective: Allogenic transplantation of umbilical cord blood (UCB) from HLA-identical siblings is a therapeutic concept of increasing importance. Prenatal HLA typing results can provide important information as to whether the UCB should be collected. Therefore, we tested the suitability of two methods based on polymerase chain reaction (PCR) for low-resolution HLA genotyping of uncultured amniocytes contaminated with maternal blood. Study Design: Amniotic fluid samples (~10 mL, n=4) were collected and divided into 5 equal sized portions. Subsequently, maternal blood was added to produce a series of varying degrees of artificial contamination ranging from 0% to 5% (vol/vol). Corresponding maternal blood and cord blood samples were collected and served as reference material. After DNA preparation, all samples were subjected to both PCR-SSP (sequence-specific primers) and PCR-SSO (sequence-specific oligonucleotides) typing procedures, designed for low-resolution typing of the highly polymorphic HLA-B locus. Results: Both PCR tests were able to accurately predict the fetal HLA-B type when pure amniotic fluid was used in all cases. The PCR-SSP method could still determine the fetal HLA type at 0.1% contamination but not at levels above this; in contrast, PCR-SSO failed if any degree of contamination was present. Conclusion: Fetal cells from amniotic fluid represent a reasonable source for prenatal testing of the fetal HLA genotype with either the PCR-SSP or the PCR-SSO method. Low levels of contamination with maternal blood in the amniotic fluid are tolerated by the more robust PCR-SSP method. In contrast, the PCR-SSO procedure is more sensitive to any degree of contamination, but it is the method of choice if the amount of DNA is limited because of the very low volume of specimens of amniotic fluid available. (Am J Obstet Gynecol 2002;186:1366-71.)
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- 2002
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11. Anti-HLA class I antibodies and pulmonary homograft function after the Ross procedure
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J.F. Matthias Bechtel, Claus Bartels, Michael Müller-Steinhardt, Wim Skibba, Hans-Hinrich Sievers, Harald Klüter, and Claudia Schmidtke
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Adult ,Graft Rejection ,Male ,Pulmonary and Respiratory Medicine ,Aortic valve ,medicine.medical_specialty ,medicine.medical_treatment ,Human leukocyte antigen ,Gastroenterology ,Antibody Specificity ,Isoantibodies ,Internal medicine ,medicine ,Humans ,Pulmonary Valve ,biology ,business.industry ,Ross procedure ,Histocompatibility Antigens Class I ,Middle Aged ,Pathophysiology ,Echocardiography, Doppler, Color ,Surgery ,medicine.anatomical_structure ,Ventricle ,Aortic Valve ,Pulmonary valve ,biology.protein ,Female ,Antibody ,Cardiology and Cardiovascular Medicine ,Complication ,business ,Blood Flow Velocity ,Follow-Up Studies - Abstract
Background . The Ross procedure provides excellent long-term results in the majority of patients. However, degeneration of the pulmonary homograft in some patients remains an unresolved problem that may be related to immunologic factors. Therefore, we studied the prevalence of antihuman leukocyte antigen (HLA) class I antibodies and echocardiographic results of homograft function at rest. Methods . Forty-seven patients (37 men, 10 women; 47 ± 15 years) were seen for echocardiography 1.1 to 63.9 months (median, 27 months) postoperatively. The presence of anti-HLA antibodies was tested against a panel of lymphocytes of 50 donors. Results . Twenty-seven (57%) of the patients produced anti-HLA class I antibodies. No difference in the maximal or mean transhomograft pressure gradient, or in the frequency of homograft regurgitation according to the presence or absence of anti-HLA antibodies was found. However, the right ventricle was slightly but significantly larger in antibody-positive patients (26.3 ± 4.2 versus 30.7 ± 3.5 mm; p = 0.001). Conclusions . In the first years after the Ross procedure, we could not detect significant evidence of an association between anti-HLA class I antibodies and echocardiographic results of homograft function at rest in adults.
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- 2001
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12. Ex vivo induction of cytokine mRNA expression in human blood samples
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Harald Klüter, Gregor Bein, Christoph Härtel, and Michael Müller-Steinhardt
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Blood Cells ,Lymphocyte ,medicine.medical_treatment ,Immunology ,Cell Culture Techniques ,Blood flow ,Biology ,Molecular biology ,Peripheral blood mononuclear cell ,medicine.anatomical_structure ,Cytokine ,Gene Expression Regulation ,In vivo ,medicine ,Cytokines ,Humans ,Immunology and Allergy ,RNA, Messenger ,Ex vivo ,Blood sampling ,Whole blood - Abstract
The interest in the quantitative analysis of cytokine mRNA profiles has increased substantially in recent years. This is based on the potential use of basal cytokine mRNA expression as sensitive markers for in vivo lymphocyte activation in a variety of clinical settings. However, it is less well known to what extent differences in blood collection and preparation techniques may cause ex vivo alteration of quantitative cytokine mRNA levels. We therefore evaluated the effect of blood sampling and the impact of cell separation on interleukin (IL)-2, IL-4, interferon (IFN)-gamma and tumour necrosis factor (TNF)-alpha mRNA expression in an intraindividual study design (n=8). Two different blood sampling procedures were applied. A whole blood sample 1 was collected by constant moderate blood flow into a blood collection tube containing lithium-heparin. Moreover, a second sample from the same donor was collected by a 5-fold acceleration of blood flow. Furthermore, peripheral blood mononuclear cell (PBMC) were isolated from the first whole blood sample by density separation over Ficoll-Hypaque. The quantification of cytokine mRNA expression was performed by real-time PCR in native whole blood/PBMC samples or unstimulated cultures. We found a significant increase of IL-2, IL-4 and TNF-alpha mRNA expression (P=0.018, P=0.028, P=0.018) in whole blood samples collected by rapid sampling. The isolation of PBMC by density gradient separation prompted on upregulation of the mRNA levels of IL-2, IL-4 and TNF-alpha 5-9-fold (P=0.018, P=0.018, P=0.018). In contrast, IFN-gamma mRNA expression was not significantly influenced by differences in blood sample preparation. Our data clearly demonstrate that differences in the blood sampling technique or cell separation should be considered as important factors for non-physiological ex vivo induction of cytokine mRNA expression. The current data emphasize the need for data on the impact of ex vivo variation in order to extract reliable and consistent information, particularly when cytokine mRNA expression data from healthy blood donors are included in clinical studies.
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- 2001
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13. Effects of amantadine treatment on in vitro production of interleukin-2 in de-novo patients with idiopathic Parkinson's disease
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Peter Vieregge, Marion Peters, Harald Klüter, Klaus P Wandinger, Matthias Rothermundt, and Johann Hagenah
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Adult ,Male ,Interleukin 2 ,Parkinson's disease ,T-Lymphocytes ,medicine.medical_treatment ,Dopamine Agents ,Immunology ,Pharmacology ,Interferon-gamma ,Amantadine ,medicine ,Humans ,Immunology and Allergy ,Lymphocyte Count ,Prospective Studies ,Neuropharmacology ,Aged ,Whole blood ,Aged, 80 and over ,business.industry ,Neurodegeneration ,Parkinson Disease ,Middle Aged ,medicine.disease ,Lymphocyte Subsets ,Interleukin-10 ,Cytokine ,Neurology ,Interleukin-2 ,Major depressive disorder ,Female ,Neurology (clinical) ,business ,medicine.drug - Abstract
An involvement of immunological events in the process of neurodegeneration has frequently been reported. We investigated the cytokine producing capacity for interleukin-2 (IL-2), interferon-gamma (IFN-gamma) and interleukin-10 (IL-10) in whole blood cultures of de-novo patients with idiopathic Parkinson's disease (PD) at the time of first diagnosis and after oral amantadine treatment. Before treatment, productions of IL-2 and IFN-gamma were markedly decreased in PD patients compared to patients with major depressive disorder and healthy controls. After amantadine treatment, the in vitro IL-2 secretion defect was corrected to normal levels in half of the patients, and the increase in IL-2 production was correlated with an increase in IFN-gamma secretion. Our findings suggest that immunological abnormalities occur in the course of PD and that a formerly unappreciated therapeutic potential of amantadine may arise from its immunomodulatory effects on altered T cell function in patients with PD.
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- 1999
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14. Clinical and molecular findings in multiple sclerosis patients with type 1 diabetes mellitus
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P. Trillenberg, K. Wessel, Klaus-Peter Wandinger, Harald Klüter, and Holger Kirchner
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Type 1 diabetes ,medicine.medical_specialty ,endocrine system diseases ,business.industry ,Multiple sclerosis ,Haplotype ,General Medicine ,medicine.disease ,Neurology ,Physiology (medical) ,Internal medicine ,Immunopathology ,Diabetes mellitus ,Immunology ,HLA-DQ ,medicine ,Genetic predisposition ,Surgery ,Neurology (clinical) ,business ,Progressive disease - Abstract
The clinical and molecular findings in three patients with multiple sclerosis (MS) and additional type 1 diabetes mellitus are described. These patients all presented with a severe and progressive disease course of MS. Molecular testing for HLA class II genes demonstrated the presence of the haplotype DRB1 ∗ 0401, DQB1 ∗ 0302 in all patients. This haplotype is closely linked to type 1 diabetes mellitus and is increased among patients with the primary progressive subtype of MS. We conclude that the immunogenetic background in patients with diabetes mellitus may determine the severity and clinical course of MS in these individuals.
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- 1999
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