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1. Analytical comparison of ELISA and mass spectrometry for quantification of serum hepcidin in critically ill patients

Author

Delaby, C, Vialaret, J, Hirtz, C, Lefebvre, T, Herkert, M, Puy, H, Lasocki, S, and Lehmann, S

Subjects
ELISA, hepcidin, anemia, mass spectrometry
Abstract

Aim: To compare methods of quantifying serum hepcidin (based on MS and ELISA) and their ability to diagnose true iron deficiency anemia in critically ill patients. Materials & methods: Serum hepcidin was measured in 119 critically ill patients included in the HEPCIDANE clinical trial, using either an ultra-sensitive ELISA kit (from DRG) or two different MS methods. Results: The results show a good correlation between the different methods studied. The Bland-Altman analysis and the Kappa test for clinical groups show a good or very good agreement between the different tests. Conclusion: ELISA or MS show a satisfactory commutability to quantify serum hepcidin. This is of great importance for the determination of therapeutic strategies in iron deficiency.

Published
2021
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3. Toward Worldwide Hepcidin Assay Harmonization: Identification of a Commutable Secondary Reference Material

Author

Vorm, L.N. van der, Hendriks, J.C.M., Laarakkers, C.M., Klaver, S., Armitage, A.E., Bamberg, A., Geurts-Moespot, A.J., Girelli, D., Herkert, M., Itkonen, O., Konrad, R.J., Tomosugi, N., Westerman, M., Bansal, S.S., Campostrini, N., Drakesmith, H., Fillet, M., Olbina, G., Pasricha, S.R., Pitts, K.R., Sloan, J.H., Tagliaro, F., Weykamp, C.W., Swinkels, D.W., Vorm, L.N. van der, Hendriks, J.C.M., Laarakkers, C.M., Klaver, S., Armitage, A.E., Bamberg, A., Geurts-Moespot, A.J., Girelli, D., Herkert, M., Itkonen, O., Konrad, R.J., Tomosugi, N., Westerman, M., Bansal, S.S., Campostrini, N., Drakesmith, H., Fillet, M., Olbina, G., Pasricha, S.R., Pitts, K.R., Sloan, J.H., Tagliaro, F., Weykamp, C.W., and Swinkels, D.W.

Abstract

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Published
2016

12. Analytical comparison of ELISA and mass spectrometry for quantification of serum hepcidin in critically ill patients.

Author

Delaby C, Vialaret J, Hirtz C, Lefebvre T, Herkert M, Puy H, Lasocki S, and Lehmann S

Subjects
Anemia, Iron-Deficiency blood, Anemia, Iron-Deficiency diagnosis, Critical Illness, Humans, Protein Isoforms blood, Reagent Kits, Diagnostic, Anemia, Iron-Deficiency etiology, Enzyme-Linked Immunosorbent Assay methods, Hepcidins blood, Mass Spectrometry methods
Abstract

Aim: To compare methods of quantifying serum hepcidin (based on MS and ELISA) and their ability to diagnose true iron deficiency anemia in critically ill patients. Materials & methods: Serum hepcidin was measured in 119 critically ill patients included in the HEPCIDANE clinical trial, using either an ultra-sensitive ELISA kit (from DRG) or two different MS methods. Results: The results show a good correlation between the different methods studied. The Bland-Altman analysis and the Kappa test for clinical groups show a good or very good agreement between the different tests. Conclusion: ELISA or MS show a satisfactory commutability to quantify serum hepcidin. This is of great importance for the determination of therapeutic strategies in iron deficiency.

Published
2021
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13. Optimizing hepcidin measurement with a proficiency test framework and standardization improvement.

Author

Aune ET, Diepeveen LE, Laarakkers CM, Klaver S, Armitage AE, Bansal S, Chen M, Fillet M, Han H, Herkert M, Itkonen O, van de Kerkhof D, Krygier A, Lefebvre T, Neyer P, Rieke M, Tomosugi N, Weykamp CW, and Swinkels DW

Subjects
Accreditation, Blood Specimen Collection, Calibration, Chromatography, High Pressure Liquid, Enzyme-Linked Immunosorbent Assay, Humans, Laboratories standards, Quality Assurance, Health Care standards, Quality Control, Reference Standards, Tandem Mass Spectrometry, Hepcidins blood
Abstract

Objectives: Hepcidin measurement advances insights in pathophysiology, diagnosis, and treatment of iron disorders, but requires analytically sound and standardized measurement procedures (MPs). Recent development of a two-level secondary reference material (sRM) for hepcidin assays allows worldwide standardization. However, no proficiency testing (PT) schemes to ensure external quality assurance (EQA) exist and the absence of a high calibrator in the sRM set precludes optimal standardization., Methods: We developed a pilot PT together with the Dutch EQA organization Stichting Kwaliteitsbewaking Medische Laboratoriumdiagnostiek (SKML) that included 16 international hepcidin MPs. The design included 12 human serum samples that allowed us to evaluate accuracy, linearity, precision and standardization potential. We manufactured, value-assigned, and validated a high-level calibrator in a similar manner to the existing low- and middle-level sRM., Results: The pilot PT confirmed logistical feasibility of an annual scheme. Most MPs demonstrated linearity (R2>0.99) and precision (duplicate CV>12.2%), although the need for EQA was shown by large variability in accuracy. The high-level calibrator proved effective, reducing the inter-assay CV from 42.0% (unstandardized) to 14.0%, compared to 17.6% with the two-leveled set. The calibrator passed international homogeneity criteria and was assigned a value of 9.07±0.24 nmol/L., Conclusions: We established a framework for future PT to enable laboratory accreditation, which is essential to ensure quality of hepcidin measurement and its use in patient care. Additionally, we showed optimized standardization is possible by extending the current sRM with a third high calibrator, although international implementation of the sRM is a prerequisite for its success.

Published
2020
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14. Provisional standardization of hepcidin assays: creating a traceability chain with a primary reference material, candidate reference method and a commutable secondary reference material.

Author

Diepeveen LE, Laarakkers CMM, Martos G, Pawlak ME, Uğuz FF, Verberne KESA, van Swelm RPL, Klaver S, de Haan AFJ, Pitts KR, Bansal SS, Abbas IM, Fillet M, Lefebvre T, Geurts-Moespot AJ, Girelli D, Castagna A, Herkert M, Itkonen O, Olbina G, Tomosugi N, Westerman ME, Delatour V, Weykamp CW, and Swinkels DW

Subjects
Calibration, Chromatography, High Pressure Liquid standards, Enzyme-Linked Immunosorbent Assay standards, Hepcidins standards, Humans, Isotope Labeling, Reference Standards, Enzyme-Linked Immunosorbent Assay methods, Hepcidins blood, Tandem Mass Spectrometry standards
Abstract

Background Hepcidin concentrations measured by various methods differ considerably, complicating interpretation. Here, a previously identified plasma-based candidate secondary reference material (csRM) was modified into a serum-based two-leveled sRM. We validated its functionality to increase the equivalence between methods for international standardization. Methods We applied technical procedures developed by the International Consortium for Harmonization of Clinical Laboratory Results. The sRM, consisting of lyophilized serum with cryolyoprotectant, appeared commutable among nine different measurement procedures using 16 native human serum samples in a first round robin (RR1). Harmonization potential of the sRM was simulated in RR1 and evaluated in practice in RR2 among 11 measurement procedures using three native human plasma samples. Comprehensive purity analysis of a candidate primary RM (cpRM) was performed by state of the art procedures. The sRM was value assigned with an isotope dilution mass spectrometry-based candidate reference method calibrated using the certified pRM. Results The inter-assay CV without harmonization was 42.1% and 52.8% in RR1 and RR2, respectively. In RR1, simulation of harmonization with sRM resulted in an inter-assay CV of 11.0%, whereas in RR2 calibration with the material resulted in an inter-assay CV of 19.1%. Both the sRM and pRM passed international homogeneity criteria and showed long-term stability. We assigned values to the low (0.95±0.11 nmol/L) and middle concentration (3.75±0.17 nmol/L) calibrators of the sRM. Conclusions Standardization of hepcidin is possible with our sRM, which value is assigned by a pRM. We propose the implementation of this material as an international calibrator for hepcidin.

Published
2019
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15. Toward Worldwide Hepcidin Assay Harmonization: Identification of a Commutable Secondary Reference Material.

Author

van der Vorm LN, Hendriks JC, Laarakkers CM, Klaver S, Armitage AE, Bamberg A, Geurts-Moespot AJ, Girelli D, Herkert M, Itkonen O, Konrad RJ, Tomosugi N, Westerman M, Bansal SS, Campostrini N, Drakesmith H, Fillet M, Olbina G, Pasricha SR, Pitts KR, Sloan JH, Tagliaro F, Weykamp CW, and Swinkels DW

Subjects
Humans, Immunochemistry, Linear Models, Reference Standards, Clinical Laboratory Services standards, Hepcidins blood, International Cooperation
Abstract

Background: Absolute plasma hepcidin concentrations measured by various procedures differ substantially, complicating interpretation of results and rendering reference intervals method dependent. We investigated the degree of equivalence achievable by harmonization and the identification of a commutable secondary reference material to accomplish this goal., Methods: We applied technical procedures to achieve harmonization developed by the Consortium for Harmonization of Clinical Laboratory Results. Eleven plasma hepcidin measurement procedures (5 mass spectrometry based and 6 immunochemical based) quantified native individual plasma samples (n = 32) and native plasma pools (n = 8) to assess analytical performance and current and achievable equivalence. In addition, 8 types of candidate reference materials (3 concentrations each, n = 24) were assessed for their suitability, most notably in terms of commutability, to serve as secondary reference material., Results: Absolute hepcidin values and reproducibility (intrameasurement procedure CVs 2.9%-8.7%) differed substantially between measurement procedures, but all were linear and correlated well. The current equivalence (intermeasurement procedure CV 28.6%) between the methods was mainly attributable to differences in calibration and could thus be improved by harmonization with a common calibrator. Linear regression analysis and standardized residuals showed that a candidate reference material consisting of native lyophilized plasma with cryolyoprotectant was commutable for all measurement procedures. Mathematically simulated harmonization with this calibrator resulted in a maximum achievable equivalence of 7.7%., Conclusions: The secondary reference material identified in this study has the potential to substantially improve equivalence between hepcidin measurement procedures and contributes to the establishment of a traceability chain that will ultimately allow standardization of hepcidin measurement results., (© 2016 American Association for Clinical Chemistry.)

Published
2016
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16. Serum hepcidin measured with an improved ELISA correlates with parameters of iron metabolism in patients with myelodysplastic syndrome.

Author

Zipperer E, Post JG, Herkert M, Kündgen A, Fox F, Haas R, Gattermann N, and Germing U

Subjects
Aged, Biomarkers blood, Biomarkers metabolism, Enzyme-Linked Immunosorbent Assay methods, Female, Humans, Iron metabolism, Male, Myelodysplastic Syndromes mortality, Registries, Survival Rate trends, Hepcidins blood, Iron blood, Myelodysplastic Syndromes blood, Myelodysplastic Syndromes diagnosis
Abstract

Patients with myelodysplastic syndromes (MDS) often show elevated serum ferritin levels at diagnosis, probably caused by increased intestinal iron uptake attributable to ineffective erythropoiesis. Many patients also develop transfusional iron overload. Hepcidin, a pivotal regulator of iron homeostasis, controls iron uptake in the duodenum as well as iron release from macrophages and is potentially involved in iron distribution to different organs. We measured serum hepcidin, together with other laboratory parameters related to iron metabolism and hematopoiesis (ferritin, transferrin, transferrin saturation, soluble transferrin receptor, erythropoietin, and hemoglobin), and C-reactive protein as marker of inflammation, in 89 MDS patients. Hepcidin levels were measured with two different competitive ELISAs: (a) EIA-4705 as described by Schwarz et al. (J Gastroenterol 46:648-656; 2011) and (b) Hepcidin 25 bioactive ELISA (EIA-5258), which was develop by DRG Diagnostics, Marburg, in 2012. Median hepcidin levels with EIA-5258 were as follows: entire cohort 17.5 ng/ml (n = 89), RA/RARS 5.9 ng/ml (n = 5), RCMD 17.8 ng/ml (n = 38), RS-RCMD 8.7 ng/ml (n = 7), RAEB I/II 29.1 ng/ml (n = 22), CMML I/II 16.9 ng/ml (n = 10), and MDS with del(5q) 26.3 ng/ml (n = 7). Hepcidin levels of the RA/RARS patients were significantly lower than in the other groups except RS-RCMD. RS-RCMD had significantly lower levels than RAEB and 5q- patients. There was a positive correlation between hepcidin levels and serum ferritin and transferrin saturation, and a negative correlation between hepcidin and hemoglobin and transferrin. Malcovati et al. (Blood 112:2676a, 2008), Santini et al. (PLoS One 6:e23109, 2011), and Ambaglio et al. (Haematologica 98:420-423, 2013), using mass spectrometry, reported similar results. We further assessed transfusional status and could show that patients who had been transfused have significantly higher hepcidin levels (median 33.3 versus 8.8 ng/ml (p < 0.001)). A dichotomized hepcidin level correlated with worse survival. EIA-4705 as described by Schwarz showed no correlation with markers of iron metabolism. Measurement of serum hepcidin with an improved ELISA yield results that correlate with other parameters of iron metabolism as well as survival and transfusion needs.

Published
2013
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20. Evaluation of an ELISA for p16INK4a as a screening test for cervical cancer.

Author

Balasubramanian A, Hughes J, Mao C, Ridder R, Herkert M, Kiviat NB, and Koutsky LA

Subjects
Adolescent, Adult, DNA, Viral analysis, DNA, Viral genetics, Female, Humans, Male, Middle Aged, Papillomaviridae isolation & purification, Polymerase Chain Reaction, Prognosis, Uterine Cervical Neoplasms virology, Vaginal Smears, Young Adult, Biomarkers, Tumor analysis, Cyclin-Dependent Kinase Inhibitor p16 analysis, Enzyme-Linked Immunosorbent Assay methods, Mass Screening, Uterine Cervical Neoplasms chemistry
Abstract

Background: The low sensitivity of cytology and low specificity of human papillomavirus testing prompts searching for more accurate cervical cancer screening strategies. Our goal was to evaluate an ELISA-based test for p16(INK4a)., Methods: 1,781 women undergoing routine screening provided cervical specimens for p16(INK4a) ELISA (original and enhanced versions of a prototype), liquid-based cytology, and Hybrid Capture II (hc2) testing. All women with a positive result and a random sample of those with negative results on all tests were referred for histologic diagnosis. Cervical intraepithelial neoplasia grade >or=3 (>or=CIN3) was the main outcome. The original analysis included all >or=CIN3 outcomes (n = 28). The a posteriori analysis was used to represent clinically relevant results with >or=CIN3 as outcomes only when detected after a positive screening test (n = 27)., Results: Participants had a median age of 23 years. The prevalence of high-risk human papillomavirus DNA was 30.6%. In a posteriori analyses, the sensitivity and specificity for p16(INK4a) ELISA (>or=8 pg/mL cut-point), cytology, and hc2 were 50.9%, 58.1%, and 100.0%, respectively, and 90.4%, 89.3%, and 69.2%, respectively. Referral to colposcopy of women with positive results for hc2 and p16(INK4a) (enhanced ELISA, >or=6 pg/mL cut-point) had a sensitivity of 91.8% (95% confidence interval, 79.1-100.0%) and specificity of 86.0% (95% confidence interval, 82.0-89.0%). Results of the original analyses had similar specificity but substantially lower sensitivity due to the strong influence of the single CIN3 case with completely negative screening results., Conclusions: An enhanced version of this prototypic p16(INK4a) ELISA showed promise in screening, particularly when combined with hc2.

Published
2009
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21. Evaluation of a new p16(INK4A) ELISA test and a high-risk HPV DNA test for cervical cancer screening: results from proof-of-concept study.

Author

Mao C, Balasubramanian A, Yu M, Kiviat N, Ridder R, Reichert A, Herkert M, von Knebel Doeberitz M, and Koutsky LA

Subjects
Adolescent, Adult, Biomarkers, Tumor, Feasibility Studies, Female, Humans, Middle Aged, Sensitivity and Specificity, Cyclin-Dependent Kinase Inhibitor p16 analysis, DNA, Viral analysis, Enzyme-Linked Immunosorbent Assay methods, Papillomaviridae genetics, Uterine Cervical Neoplasms diagnosis
Abstract

p16(INK4a), a cell cycle regulation protein, accumulates in abnormal epithelial cells infected with high-risk human papilloma virus (HPV). In immunostaining studies, p16(INK4a) has shown potential as a marker of high grade cervical intraepithelial neoplasia (CIN) and invasive cervical cancer. To evaluate its potential use in cervical cancer screening, we conducted a feasibility study to compare the performance of a new enzyme linked immunosorbant assay (ELISA) for p16(INK4a) (mtm laboratories, Heidelberg, Germany) to that of the Hybrid Capture 2 (hc2) test for high-risk HPV DNA for the detection of CIN3. Three hundred and nineteen women were referred from Western Washington Planned Parenthood clinics for colposcopy examination and cervical biopsy because of abnormal Pap test results. Cervical samples were obtained from study participants for p16(INK4a) ELISA, liquid-based cytology and hc2. The order (first and second) for obtaining samples for cervical cytology and p16(INK4a) ELISA changed with every other subject. Concentrations of p16(INK4a) protein were higher when the sample was taken before the cytology. The sensitivity of p16(INK4a) ELISA (concentration > or = 8 units/ml) taken as first sample was 90.0% for CIN3, and the sensitivity of HC2 taken as a second sample was 85%. In the same group, the specificity of p16(INK4a) ELISA (46.9%) was slightly better than hc2 (35.4%) Results from this proof-of-concept study suggest that p16(INK4a) ELISA has a similar sensitivity and slightly better specificity for CIN3 compared to hc2. These findings support proceeding with a larger study with samples from a population of women presenting for routine cytology screening.

Published
2007
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22. Identification of high-grade cervical dysplasia by the detection of p16INK4a in cell lysates obtained from cervical samples.

Author

Wentzensen N, Hampl M, Herkert M, Reichert A, Trunk MJ, Poremba C, Ridder R, and von Knebel Doeberitz M

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Enzyme-Linked Immunosorbent Assay, Female, Humans, Middle Aged, Predictive Value of Tests, ROC Curve, Up-Regulation, Cervix Uteri pathology, Cyclin-Dependent Kinase Inhibitor p16 analysis, Uterine Cervical Dysplasia diagnosis, Vaginal Smears
Abstract

Background: Current cervical cancer screening approaches are based on cytology supplemented by human papillomavirus (HPV) testing in some settings. Whereas cytology is laborious and depends on the cytologists' experience, HPV testing has limited specificity when it is used to detect high-grade lesions. A dichotomous test to identify high-grade lesions with greater specificity may be a useful tool for cervical cancer screening. p16(INK4a) is a cell-cycle regulator that has demonstrated strong overexpression in cervical precancer cells and cervical cancer induced by the deregulated expression of HPV oncogenes., Methods: The authors used a sandwich enzyme-linked immunosorbent assay (ELISA) to quantify the amount of solubilized p16(INK4a) protein in lysates that were prepared from cervical samples to detect high-grade cervical lesions. In total, 187 specimens that were obtained after sampling for conventional cytology in women who attended a cervical colposcopy clinic were analyzed. Seventy-six women underwent a biopsy, and 45 of those women showed histologically confirmed, high-grade cervical intraepithelial neoplasia., Results: For 76 women with biopsy-proven diagnoses, receiver operating characteristic (ROC) analysis of different cutoff values showed an area under the ROC curve of 0.89 for the detection of high-grade cervical dysplasia. At a cutoff value of 8 U/mL, the sensitivity of the p16(INK4a) ELISA for detecting high-grade dysplastic cervical lesions was 96%., Conclusions: The data obtained in this study suggested that ELISA-based quantification of solubilized p16(INK4a) protein may have high sensitivity for detecting cervical precancer. Further population-based studies will be necessary to analyze the specificity and predictive values of p16(INK4a) protein quantification in cervical samples., ((c) 2006 American Cancer Society.)

Published
2006
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23. Formation of molecular complexes by N-methyl-D-aspartate receptor subunit NR2B and ryanodine receptor 2 in neonatal rat myocard.

Author

Seeber S, Humeny A, Herkert M, Rau T, Eschenhagen T, and Becker CM

Subjects
Amino Acid Sequence, Animals, Animals, Newborn, Base Sequence, Cells, Cultured, Central Nervous System metabolism, DNA Primers, In Vitro Techniques, Models, Molecular, Molecular Sequence Data, Peptide Fragments chemistry, Protein Conformation, Protein Subunits chemistry, Protein Subunits genetics, Protein Subunits metabolism, Rats, Receptors, N-Methyl-D-Aspartate genetics, Receptors, N-Methyl-D-Aspartate metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Ryanodine Receptor Calcium Release Channel genetics, Ryanodine Receptor Calcium Release Channel metabolism, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Myocardium metabolism, Receptors, N-Methyl-D-Aspartate chemistry, Ryanodine Receptor Calcium Release Channel chemistry
Abstract

The N-methyl-d-aspartate (NMDA) receptor is a glutamate gated cation channel prevalent in the postsynaptic membranes of central nervous system neurons. The neurotransmitter receptor complex is thought to represent a tetramer where variable NR2 or NR3 polypeptides form heteromeric assemblies with an obligatory NR1 subunit. Recently, we showed that cardiac myocytes from perinatal rats transiently express the NMDA receptor subunit NR2B, the function of which in heart is unknown. To characterize the cardiac NR2B protein, we determined its subcellular distribution and specific molecular interaction partners. By immunostaining of rat heart tissue slices and acutely dissociated cardiac myocytes, the NR2B antigen was localized at the sarcomeric Z-bands. Using immunoprecipitation of detergent-solubilized NR2B protein and subsequent analysis employing matrix-assisted laser desorption/ionization time of flight mass spectrometry, ryanodine receptor 2 was identified as a molecular interaction partner of the cardiac NR2B polypeptide. Differences in antibody recognition indicate that the cardiac NR2B polypeptide carries a structurally altered C terminus as compared with the NR2B variant prevalent in central nervous system. Based on its localization and protein interaction, the function of cardiac NR2B protein may relate to mechanosensitivity or play a role in the regulation of the contractile apparatus of neonatal heart.

Published
2004
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24. Induction by beta-bungarotoxin of apoptosis in cultured hippocampal neurons is mediated by Ca(2+)-dependent formation of reactive oxygen species.

Author

Shakhman O, Herkert M, Rose C, Humeny A, and Becker CM

Subjects
Animals, Antioxidants pharmacology, Apoptosis drug effects, Hippocampus cytology, Hippocampus embryology, Lipid Peroxidation drug effects, Neurons cytology, Neurotoxins pharmacology, Oxidants pharmacology, Rats, Rats, Wistar, Signal Transduction drug effects, Apoptosis physiology, Bungarotoxins pharmacology, Calcium metabolism, Neurons drug effects, Reactive Oxygen Species metabolism
Abstract

The component of the venom of the Taiwanese banded krait Bungarus multicinctus, beta-bungarotoxin (beta-BuTx), acts as an extremely potent inducer of neuronal apoptosis when applied to rat hippocampal cultures. While induction of cell death is dependent on toxin binding to voltage-activated K+ channels and subsequent internalization, the pro-apoptotic signals triggered by picomolar concentrations of beta-BuTx are not understood. Following toxin binding, a dramatic increase in intracellular Ca2+ became detectable after 30 min, and in reactive oxygen species (ROS) after 3-4 h. Conversely, Ca2+ chelators, radical quenchers and antioxidants efficiently antagonized beta-BuTx induced apoptosis. As shown for the antioxidant 2,3-dihydroxybenzoic acid, analysis by matrix assisted laser desorbtion-time of flight (MALDI-TOF) mass spectrometry excluded the protective effects to be due to reductive cleavage of the toxic beta-BuTx dimer. Inhibitors of the intracellular antioxidant defence system enhanced neuronal susceptibility to beta-BuTx, supporting the essential role of ROS in beta-BuTx-initiated apoptosis. Cell damage was accompanied by an accumulation of markers of oxidative cell stress, phospholipid hydroxyperoxides and the lipid peroxidation product, malonyl dialdehyde. These observations indicate that beta-BuTx-induced cell death resulted from an intracellular signalling cascade involving subsequent stages of a dramatic rise in free Ca2+, the accumulation of ROS, membrane lipid peroxidation and, finally, apoptosis.

Published
2003
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25. Beta-bungarotoxin is a potent inducer of apoptosis in cultured rat neurons by receptor-mediated internalization.

Author

Herkert M, Shakhman O, Schweins E, and Becker CM

Subjects
Animals, Annexin A5 analysis, Calpain antagonists & inhibitors, Calpain metabolism, Caspase Inhibitors, Caspases metabolism, Cells, Cultured, Cysteine Proteinase Inhibitors pharmacology, Dipeptides pharmacology, Dose-Response Relationship, Drug, Elapid Venoms pharmacology, Female, Hippocampus cytology, In Situ Nick-End Labeling, Neurons chemistry, Neurons metabolism, Neurotoxins pharmacology, Phospholipases A metabolism, Pregnancy, Rats, Rats, Wistar, Signal Transduction physiology, Apoptosis drug effects, Bungarotoxins pharmacokinetics, Neurons cytology, Receptors, Cell Surface metabolism
Abstract

The neurotoxic phospholipase A(2), beta-bungarotoxin (beta-BuTx), is a component of the snake venom from the Taiwanese banded krait Bungarus multicinctus. beta-BuTx affects presynaptic nerve terminal function of the neuromuscular junction and induces widespread neuronal cell death throughout the mammalian and avian CNS. To analyse the initial events of beta-BuTx-mediated cell death, the toxin was applied to cultured rat hippocampal neurons where it induced neuronal cell death in a concentration-dependent manner (EC(50) approximately equal to 5 x 10(-13) M) within 24 h. Fluorescence labelled beta-BuTx was completely incorporated by neurons within < 10 min. Binding and uptake of beta-BuTx, as well as induction of cell death, were efficiently antagonized by preincubation with dendrotoxin I, a blocker of voltage-gated potassium channels devoid of phospholipase activity. Binding of beta-BuTx was selective for neurofilament-positive cells. As evident from intense annexin-V and TUNEL stainings, application of beta-BuTx induced apoptotic cell death exclusively in neurons, leaving astrocytes unaffected. No evidence was obtained for any contribution of either caspases or calpains to beta-BuTx-induced apoptosis, consistent with the inability of the inhibitors Z-Asp-DCB and calpeptin, respectively, to protect neurons from beta-BuTx-induced cell death. These observations indicate that induction of cell death by beta-BuTx comprises several successive phases: (i) binding to neuronal potassium channels is the initial event, followed by (ii) internalization and (iii) induction of apoptotic cell death via a caspase-independent pathway.

Published
2001
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26. Transient expression of NMDA receptor subunit NR2B in the developing rat heart.

Author

Seeber S, Becker K, Rau T, Eschenhagen T, Becker CM, and Herkert M

Subjects
Animals, Antibodies isolation & purification, Antibodies metabolism, Antibody Specificity, Blotting, Western, Cells, Cultured, Glycine metabolism, Glycine pharmacology, Heart drug effects, Immunohistochemistry, Membrane Potentials drug effects, Myocardium cytology, N-Methylaspartate metabolism, N-Methylaspartate pharmacology, Patch-Clamp Techniques, RNA, Messenger analysis, RNA, Messenger metabolism, Rats, Rats, Wistar, Receptors, N-Methyl-D-Aspartate analysis, Receptors, N-Methyl-D-Aspartate genetics, Heart embryology, Heart growth & development, Myocardium metabolism, Receptors, N-Methyl-D-Aspartate biosynthesis
Abstract

NMDA receptors represent a subtype of the ionotropic glutamate receptor family, comprising three classes of subunits (NR1, NR2A-D, NR3), which exhibit distinct patterns of regional and developmental expression in the CNS. Recently, some NMDA receptor subunits have also been described in adult extraneuronal tissues and keratinocytes. However, their developmental expression patterns are currently unknown. With use of RT-PCR and western blot analysis, the expression of NMDA receptor subunit NR2B was investigated in the developing rat heart. NR2B mRNA and protein were detected in heart tissue of rats from embryonic day 14 until postnatal day 21 but disappeared 10 weeks after birth. In contrast, no NMDA receptor subunit NR1, alpha-amino-3-hydroxy-5-methylisoxazole-4-propionic acid receptor subunit GluR2, or anchoring postsynaptic density protein-95 could be detected in rat heart at any developmental stage. Confocal microscopy of cultured cardiac myocytes (CMs) from neonatal rats revealed distinct NR2B staining mainly of intracellular structures. However, no functional NMDA receptor could be detected on CMs by whole-cell recordings. In conclusion, high concentrations of NR2B protein can be detected in early rat heart development, but its function still remains elusive.

Published
2000
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27. The NMDA receptor subunit NR2B of neonatal rat brain: complex formation and enrichment in axonal growth cones.

Author

Herkert M, Röttger S, and Becker CM

Subjects
Amino Acid Sequence, Animals, Animals, Newborn, Antibody Specificity, Antigens analysis, Axons ultrastructure, Cell Division physiology, Cells, Cultured, Cerebral Cortex growth & development, Molecular Sequence Data, Neuronal Plasticity physiology, Rats, Rats, Wistar, Solubility, Subcellular Fractions chemistry, Water chemistry, Axons physiology, Cerebral Cortex chemistry, Receptors, N-Methyl-D-Aspartate chemistry
Abstract

The N-methyl-D-aspartate (NMDA) subtype of ionotropic glutamate receptors comprises a family of highly homologous subunits which assemble into oligomeric protein complexes. Alterations in subunit composition are developmentally regulated, leading to functionally distinct receptor populations. Here, the contribution of the subunit NR2B to NMDA receptor complex formation was analysed in neonatal rat brain, employing polyclonal antibodies raised against NR2B-specific synthetic peptides. By hydrodynamic size fractionation of the solubilized receptor protein and chemical cross-linking, NR2B antigen was found to be associated with several protein species of up to 690 kDa molecular weight. These observations show NR2B to be part of a multimeric receptor complex. Fractionation of cortex homogenates from E18 rat embryos on sucrose density gradients revealed NR2B polypeptide to be highly enriched in axonal growth cones. A similar distribution was found by fluorescence microscopy of immature hippocampal neurons, showing a preferential accumulation of NR2B antigen in axonal growth cones and varicosities. In mature cells, NR2B antigen displayed a punctated distribution pattern with redistribution to somato-dendritic spheres. The association of NR2B with axonal growth cones and processes of immature neurons suggests a role of NMDA receptors in the regulation of neurite outgrowth and migration.

Published
1998
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