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4. Upregulation of Aldo-Keto-Reductase 1C1 and 1C3 (AKR1C1, AKR1C3) is Associated with Poor Prognosis in Oropharyngeal Squamous Cell Carcinomas (OPSCC) Independent of Human Papillomavirus (HPV) Status

Author

Speel, E. J. M., Verhees, F. S., Poluschkin, L., Olthof, N. S., Kolligs, J., Siefer, O. G., Henfling, M. S., Ramaekers, F. C. S., Preuss, S. F., Beutner, D., Seehawer, J., Drebber, U., Lam, W. L., Vucic, E. A., Kremer, B. S., Klussmann, J. P., Huebbers, C. U., Speel, E. J. M., Verhees, F. S., Poluschkin, L., Olthof, N. S., Kolligs, J., Siefer, O. G., Henfling, M. S., Ramaekers, F. C. S., Preuss, S. F., Beutner, D., Seehawer, J., Drebber, U., Lam, W. L., Vucic, E. A., Kremer, B. S., Klussmann, J. P., and Huebbers, C. U.

Published
2018

6. Transient expression of phosphatidylserine at cell-cell contact areas is required for myotube formation

Author

van den Eijnde, S. M., van den Hoff, M. J., Reutelingsperger, C. P., van Heerde, W. L., Henfling, M. E., Vermeij-Keers, C., Schutte, B., Borgers, M., Ramaekers, F. C., and Other departments

Abstract

Cell surface exposure of phosphatidylserine (PS) is shown to be part of normal physiology of skeletal muscle development and to mediate myotube formation. A transient exposure of PS was observed on mouse embryonic myotubes at E13, at a stage of development when primary myotubes are formed. The study of this process in cell cultures of differentiating C2C12 and H9C2 myoblasts also reveals a transient expression of PS at the cell surface. This exposure of PS locates mainly at cell-cell contact areas and takes place at a stage when the structural organization of the sarcomeric protein titin is initiated, prior to actual fusion of individual myoblast into multinucleated myotubes. Myotube formation in vitro can be inhibited by the PS binding protein annexin V, in contrast to its mutant M1234, which lacks the ability to bind to PS. Although apoptotic myoblasts also expose PS, differentiating muscle cells show neither loss of mitochondrial membrane potential nor detectable levels of active caspase-3 protein. Moreover, myotube formation and exposure of PS cannot be blocked by the caspase inhibitor zVAD(OMe)-fmk. Our findings indicate that different mechanisms regulate PS exposure during apoptosis and muscle cell differentiation, and that surface exposed PS plays a crucial role in the process of myotube formation

Published
2001

11. Transient expression of phosphatidylserine at cell-cell contact areas is required for myotube formation.

Author

M, van den Eijnde S, J, van den Hoff M, P, Reutelingsperger C, L, van Heerde W, E, Henfling M, C, Vermeij-Keers, B, Schutte, M, Borgers, and C, Ramaekers F

Abstract

Cell surface exposure of phosphatidylserine (PS) is shown to be part of normal physiology of skeletal muscle development and to mediate myotube formation. A transient exposure of PS was observed on mouse embryonic myotubes at E13, at a stage of development when primary myotubes are formed. The study of this process in cell cultures of differentiating C2C12 and H9C2 myoblasts also reveals a transient expression of PS at the cell surface. This exposure of PS locates mainly at cell-cell contact areas and takes place at a stage when the structural organization of the sarcomeric protein titin is initiated, prior to actual fusion of individual myoblast into multinucleated myotubes. Myotube formation in vitro can be inhibited by the PS binding protein annexin V, in contrast to its mutant M1234, which lacks the ability to bind to PS. Although apoptotic myoblasts also expose PS, differentiating muscle cells show neither loss of mitochondrial membrane potential nor detectable levels of active caspase-3 protein. Moreover, myotube formation and exposure of PS cannot be blocked by the caspase inhibitor zVAD(OMe)-fmk. Our findings indicate that different mechanisms regulate PS exposure during apoptosis and muscle cell differentiation, and that surface exposed PS plays a crucial role in the process of myotube formation.

Published
2001

12. Onderzoek naar de interne structuur van waterafdunbare dispersie-verfsystemen: met behulp van permeabiliteitsmetingen en transmissiespectroscopie

Author

Henfling, M. (author) and Henfling, M. (author)

Abstract

Gedurende dit afstudeerproject is gepoogd om een meetmethode te ontwikkelen om de verouderingsgraad van waterafdunbare dispersie verfsystemen te bepalen. Hiervoor is gebruik gemaakt van twee meetmethodes, namelijk; (1.)- permeabiliteitsmetingen; (2.)- transmissiespectrummetingen; Bij de eerste methode is uitgegaan van het principe, dat de diffusie van een waterige oplossing door een latexfilm langzamer zou verlopen, naarmate de film ouder zou zijn. De verkregen resultaten waren echter niet reproduceerbaar, waardoor het ook onmogelijk was om met behulp van deze methode een relatie te leggen tussen de diffusie van een vloeistof door een film en de verouderingsgraad van deze film. Bij de tweede methode werd gebruik gemaakt van het feit, dat een vloeistof een film indringt door diffusie (vanwege polaire aantrekkingskrachten) indien deze film in deze vloeistof wordt ondergedompeld. De vloeistof verdeelt zich hierbij over de inclusies, die tussen de latexdeeltjes aanwezig zijn. Vanwege brekingsindex-verschillen tussen polymeerfase en waterfase is het dan mogelijk om de verstrooiing van invallend licht op deze inclusies te bepalen. Met behulp van de intensiteit van deze verstrooiing kan de grootte van deze inclusie worden bepaald. Om de gehele structuur van inclusies te vereenvoudigen zijn twee modellen ontwikkeld. Een model bleek bruikbaar te zijn bij de bepaling van de grootte van de inclusies. Door ook het aantal inclusies te berekenen is een parameter ontwikkeld, die zeer waarschijnlijk toepasbaar is om de verouderingsgraad van een latexfilm te bepalen., Applied Sciences, Scheikundige Technologie en der Materiaalkunde, Technologie van Macromoleculaire Stoffen

Published
1989

13. Genome-Wide Expression Profiling Reveals Downregulation of OTP and CD44 and Upregulation of RET as Indicators of Poor Prognosis in Lung Carcinoids.

Author

Swarts, D., Van Neste, L., Henfling, M., Van Suylen, R. J., Volante, M., Ramaekers, F., Van Criekinge, W., Van Engeland, M., and Speel, E. J.

Subjects
LUNG cancer, CARCINOID, CHROMAFFIN cell tumors, NEUROENDOCRINE tumors, CANCER invasiveness, IMMUNOHISTOCHEMISTRY
Abstract

Introduction: Lung carcinoids comprise a heterogeneous group of neuroendocrine tumors. Only few parameters have been identified that correlated with poor disease outcome, including 11q22-q25 deletions. New biomarkers are required to further improve diagnosis and prediction of prognosis. Aim(s): To identify differentially expressed genes between carcinoids with a favorable and poor outcome using high resolution gene-expression profiling, and to test their value as prognostic markers. Materials and methods: mRNA of five tumors with a favorable (>5yr survival) and five with a poor (distant metastasis / deceased) disease outcome was labeled and hybridized to 4x44k Agilent arrays, with a human pool expressing 70-80% of genes as a control. Results were validated by qRT-PCR and immunohistochemistry on an independent series of lung carcinoids. Results: Expression profiling revealed amongst others overexpression of the RET oncogene and repression of the homeobox gene OTP and CD44 in the poor prognosis group. In 54 frozen cases, low CD44 (p<0.0001) and OTP (p=0.0013), and high RET (p=0.0035) expression were significantly associated with decreased 15-year survival, outperforming WHO classification. Downregulation of CD44 and OTP expression was confirmed in tumors with a poor prognosis by immunohistochemistry. Conclusion: High resolution expression profiling unmasked new lung carcinoid candidate genes, of which CD44, OTP, and RET efficiently predict poor outcome. [ABSTRACT FROM AUTHOR]

Published
2012

15. Upregulation of AKR1C1 and AKR1C3 expression in OPSCC with integrated HPV16 and HPV-negative tumors is an indicator of poor prognosis.

Author

Huebbers CU, Verhees F, Poluschkin L, Olthof NC, Kolligs J, Siefer OG, Henfling M, Ramaekers FCS, Preuss SF, Beutner D, Seehawer J, Drebber U, Korkmaz Y, Lam WL, Vucic EA, Kremer B, Klussmann JP, and Speel EM

Subjects
Carcinoma, Squamous Cell pathology, Carcinoma, Squamous Cell virology, DNA, Viral genetics, Female, Genes, Viral genetics, Humans, Male, Metabolic Networks and Pathways genetics, Middle Aged, Oropharyngeal Neoplasms pathology, Oropharyngeal Neoplasms virology, Papillomavirus Infections genetics, Papillomavirus Infections pathology, Papillomavirus Infections virology, Prognosis, Survival Rate, 20-Hydroxysteroid Dehydrogenases genetics, Aldo-Keto Reductase Family 1 Member C3 genetics, Carcinoma, Squamous Cell genetics, Human papillomavirus 16 genetics, Oropharyngeal Neoplasms genetics, Up-Regulation genetics, Virus Integration genetics
Abstract

Different studies have shown that HPV16-positive OPSCC can be subdivided based on integration status (integrated, episomal and mixed forms). Because we showed that integration neither affects the levels of viral genes, nor those of virally disrupted human genes, a genome-wide screen was performed to identify human genes which expression is influenced by viral integration and have clinical relevance. Thirty-three fresh-frozen HPV-16 positive OPSCC samples with known integration status were analyzed by mRNA expression profiling. Among the genes of interest, Aldo-keto-reductases 1C1 and 1C3 (AKR1C1, AKR1C3) were upregulated in tumors with viral integration. Additionally, 141 OPSCC, including 48 HPV-positive cases, were used to validate protein expression by immunohistochemistry. Results were correlated with clinical and histopathological data. Non-hierarchical clustering resulted in two main groups differing in mRNA expression patterns, which interestingly corresponded with viral integration status. In OPSCC with integrated viral DNA, often metabolic pathways were deregulated with frequent upregulation of AKR1C1 and AKR1C3 transcripts. Survival analysis of 141 additionally immunostained OPSCC showed unfavorable survival rates for tumors with upregulation of AKR1C1 or AKR1C3 (both p <0.0001), both in HPV-positive (p ≤0.001) and -negative (p ≤0.017) tumors. OPSCC with integrated HPV16 show upregulation of AKR1C1 and AKR1C3 expression, which strongly correlates with poor survival rates. Also in HPV-negative tumors, upregulation of these proteins correlates with unfavorable outcome. Deregulated AKR1C expression has also been observed in other tumors, making these genes promising candidates to indicate prognosis. In addition, the availability of inhibitors of these gene products may be utilized for drug treatment., (© 2018 UICC.)

Published
2019
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16. The IGF pathway is activated in insulinomas but downregulated in metastatic disease.

Author

Henfling M, Perren A, Schmitt AM, Saddig CM, Starke AA, Riedl RG, Versleijen-Jonkers YMH, Sprij-Mooij DM, Ramaekers FCS, Hofland L, and Speel EM

Abstract

Clinical and molecular studies have implicated epidermal growth factor receptor (EGFR), insulin-like growth factor (IGF) and target of rapamycin (mTOR) signaling pathways in the regulation of pancreatic neuroendocrine tumor (PanNET) growth. Interpretation and comparison of these studies is complex due to clinical and molecular tumor heterogeneity. We therefore focused in this study on insulinomas, which we examined for mRNA and protein expression of EGFR, IGF and mTOR signaling pathway components by quantitative real-time PCR (n=48) and immunohistochemistry (n=86). Findings were compared with normal pancreatic islets and correlated with histopathological data and clinical outcome. Insulinomas showed low EGFR and high IGF2 expression. IGFBP2, IGFBP3 and IGFBP6 mRNA levels were 2-4 folds higher than in islets. High protein expression of IGF2, IGF1R and INSR (in 51-92% of the tumors) and low to moderate expression of mTORC1 pathway proteins p-PS6k and p-4EBP1 (7-28% of the tumors) were observed. Correlations were found between 1) ERK1 mRNA expression and that of numerous IGF pathway genes, 2) p-ERK and IGF1R protein expression and 3) decrease of IGF pathway components and both metastatic disease and shorter 10 years disease free survival. In conclusion, our observations suggest that high expression of IGF signaling pathway components is a hallmark of insulinomas, but does not necessarily lead to increased mTOR signaling. Reduced expression of IGF pathway components may be an adverse prognostic factor in insulinomas.

Published
2018
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17. Comprehensive analysis of HPV16 integration in OSCC reveals no significant impact of physical status on viral oncogene and virally disrupted human gene expression.

Author

Olthof NC, Speel EJ, Kolligs J, Haesevoets A, Henfling M, Ramaekers FC, Preuss SF, Drebber U, Wieland U, Silling S, Lam WL, Vucic EA, Kremer B, Klussmann JP, and Huebbers CU

Subjects
Adult, Aged, Aged, 80 and over, Carcinoma, Squamous Cell genetics, DNA, Viral genetics, Female, Genes, Viral genetics, Humans, Male, Middle Aged, Papillomavirus E7 Proteins genetics, RNA, Messenger genetics, RNA, Viral genetics, Gene Expression genetics, Human papillomavirus 16 genetics, Oncogene Proteins, Viral genetics, Oropharyngeal Neoplasms genetics, Papillomavirus Infections genetics, Virus Integration genetics
Abstract

Infection with high-risk human papillomavirus (HPV) type 16 is an independent risk factor for the development of oropharyngeal squamous cell carcinomas (OSCC). However, it is unclear whether viral integration is an essential hallmark in the carcinogenic process of OSCC and whether HPV integration correlates with the level of viral gene transcription and influences the expression of disrupted host genes. We analyzed 75 patients with OSCC. HPV16-positivity was proven by p16(INK4A) immunohistochemistry, PCR and FISH. Viral integration was examined using DIPS- as well as APOT-PCR. Viral E2, E6 and E7 gene expression levels were quantified by quantitative reverse transcriptase (RT-q)PCR. Expression levels of 7 human genes disrupted by the virus were extracted from mRNA expression profiling data of 32 OSCCs. Viral copy numbers were assessed by qPCR in 73 tumors. We identified 37 HPV16-human fusion products indicating viral integration in 29 (39%) OSCC. In the remaining tumors (61%) only episome-derived PCR products were detected. When comparing OSCC with or without an integration-derived fusion product, we did not find significant differences in the mean RNA expression of viral genes E2, E6 and E7 or the viral copy numbers per cell, nor did the RNA expression of the HPV-disrupted genes differ from either group of OSCC. In conclusion, our data do not support the hypothesis that integration affects the levels of viral and/or HPV-disrupted human gene transcripts. Thus constitutive, rather than a high level, of expression of oncogene transcripts appears to be required in HPV-related OSCC.

Published
2014
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18. The caspase-9 derived C-terminal fragment of cytokeratin 18 modulates topoisomerase action.

Author

Schutte B, Henfling ME, Verheyen FK, Li G, Tolstonog GV, and Ramaekers FC

Subjects
Cell Line, Tumor, Cell Nucleolus metabolism, Cell Nucleolus pathology, Chromatin Assembly and Disassembly physiology, DNA Fragmentation, Electrophoretic Mobility Shift Assay, Humans, Microscopy, Electron, Transmission, Transcription, Genetic physiology, Apoptosis physiology, Caspase 9 metabolism, DNA Topoisomerases, Type I metabolism, Keratin-18 metabolism, Peptide Fragments metabolism
Abstract

During early apoptosis the 33 amino acid C-terminal cytokeratin 18 (CK18) fragment is released by caspase-9 cleavage at the 393DALD/S site. This basic peptide relocates from the cytoskeleton to the nucleoplasm as shown by confocal laser scanning. It is shown that the C-terminal peptide modulates topoisomerase activity as measured by relaxation of plasmid DNA. In an in vitro assay recombinant caspase-induced chromatin condensation is inhibited by the peptide and at the electron microscopical level a clear inhibition of nucleolar breakdown was observed in its presence. We hypothesize that the C-terminal CK18 fragment exerts an effect in the nucleolus by stimulating rRNA transcription and processing via modulation of enzymatic activity of topoisomerase I. This leads to preservation of general transcriptional activity required to exert active steps during early stages of programmed cell death.

Published
2009
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19. DEDD association with cytokeratin filaments correlates with sensitivity to apoptosis.

Author

Schutte B, Henfling M, and Ramaekers FC

Subjects
Caco-2 Cells, Drug Resistance, Neoplasm, Gene Expression, HCT116 Cells, HT29 Cells, HeLa Cells, Humans, Protein Binding physiology, Tissue Distribution, Ubiquitin metabolism, Apoptosis drug effects, DNA-Binding Proteins metabolism, DNA-Binding Proteins physiology, Death Domain Receptor Signaling Adaptor Proteins metabolism, Death Domain Receptor Signaling Adaptor Proteins physiology, Keratins metabolism
Abstract

The cytokeratin 8/18 (CK8/18) cytoskeleton network is an early target for caspase cleavage during apoptosis. Recent reports suggest that the highly conserved and ubiquitous death effector domain containing DNA binding protein (DEDD) plays a role in the recruitment of procaspase-9 and -3 at this CK8/18 scaffold. DEDD interacts with both the CK8/18 intermediate filament network and procaspase-3 and -9. It is suggested that the CK8/18 fibrils may provide a scaffold for the proximity-induced autocleavage and activation of procaspase-9 in close association with caspase-3.We addressed this issue by investigating DEDD staining patterns in various cell lines and by correlating these expression patterns with the sensitivity of these cell lines for roscovitine-induced apoptosis. We showed that in some cell lines DEDD revealed a bright filamentous staining pattern in others DEDD staining was weak and diffusely distributed in the cytoplasm of the cells. The difference in staining patterns was irrespective of the phosphorylation status of the cytokeratin filaments. In cells showing a filamentous staining pattern, DEDD was strongly associated with the CK8/18 cytokeratin filaments as evidenced by double immunofluorescence and its resistance to extraction with Triton X-100. Subcellular fractionation indicates that DEDD co-purifies with CK18, which corroborates a strong association of DEDD and the cytokeratin network. DEDD was either mono- or diubiquinated. Cells showing a filamentous DEDD distribution are more apoptosis-prone as evidenced by the rapid appearance of M30 CytoDeath-positive cells after induction of apoptosis. The sensitivity towards apoptosis is irrespective of the procaspase-3 content of the cells. Our data support the notion that DEDD-mediated accumulation of procaspases at the cytokeratin scaffold leads to an increase in the local concentration, which renders cells more apoptosis-prone.

Published
2006
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20. Keratin 8/18 breakdown and reorganization during apoptosis.

Author

Schutte B, Henfling M, Kölgen W, Bouman M, Meex S, Leers MP, Nap M, Björklund V, Björklund P, Björklund B, Lane EB, Omary MB, Jörnvall H, and Ramaekers FC

Subjects
Caspase 3, Caspase 7, Caspase 9, Catalytic Domain physiology, Cell Line, Tumor, Humans, Keratin-18, Keratin-8, Phosphorylation, Protein Structure, Tertiary physiology, Apoptosis physiology, Caspases metabolism, Cell Membrane metabolism, Cytoskeleton metabolism, Keratins metabolism
Abstract

Monoclonal antibodies that specifically recognize caspase cleaved K18 fragments or specific (phospho)epitopes on intact K8 and K18 were used for a detailed investigation of the temporal and causal relationship of proteolysis and phosphorylation in the collapse of the keratin cytoskeleton during apoptosis. Caspases involved in the specific proteolysis of keratins were analyzed biochemically using recombinant caspases and specific caspase inhibitors. Finally, the fate of the keratin aggregates was analyzed using the M30-ApoptoSense trade mark Elisa kit to measure shedding of caspase cleaved fragments into the supernatant of apoptotic cell cultures. From our studies, we conclude that C-terminal K18 cleavage at the (393)DALD/S site is an early event during apoptosis for which caspase 9 is responsible, both directly and indirectly by activating downstream caspases 3 and 7. Cleavage of the L1-2 linker region of the central alpha-helical rod domain is responsible for the final collapse of the keratin scaffold into large aggregates. Phosphorylation facilitates formation of these aggregates, but is not crucial. K8 and K18 remain associated in heteropolymeric aggregates during apoptosis. At later stages of the apoptotic process, that is, when the integrity of the cytoplasmic membrane becomes compromised, keratin aggregates are shed from the cells.

Published
2004
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21. Inhibition of the cell cycle and induction of apoptosis by Noclosan and Loxat in cell lines irrespective of their origin.

Author

Schutte B, Harmsa M, Costongs G, Henfling M, Ummelen M, Dignef W, and Ramaekers F

Subjects
Dose-Response Relationship, Drug, Drug Synergism, Endothelium, Vascular metabolism, Endothelium, Vascular pathology, Female, Humans, JNK Mitogen-Activated Protein Kinases metabolism, MAP Kinase Kinase 4, Mitogen-Activated Protein Kinase Kinases metabolism, Mitogen-Activated Protein Kinases metabolism, Neoplasms metabolism, Tumor Cells, Cultured, Apoptosis drug effects, Cell Division drug effects, G2 Phase drug effects, Neoplasms pathology, Plant Extracts pharmacology, Solanum tuberosum chemistry
Abstract

The effects of Noclosan and Loxat, extracts from the potato tuber, on cancer cell lines and human endothelial cells in culture were examined with respect to cell cycle inhibition and apoptosis induction. Both components effect the cell cycle of the cancer cell lines, most likely by inhibition of the M to G1-phase transition. Furthermore, both compounds very effectively induced apoptosis in a dose-dependent manner. Strikingly, combination of both compounds revealed a synergistic effect, that can be explained by the observation that induction of apoptosis occurs through both the mitochondrial and the non-mitochondrial route. Preliminary studies suggest that the components affect the SAPK/JNK cell signaling pathway.

Published
2004

22. Transient expression of phosphatidylserine at cell-cell contact areas is required for myotube formation.

Author

van den Eijnde SM, van den Hoff MJ, Reutelingsperger CP, van Heerde WL, Henfling ME, Vermeij-Keers C, Schutte B, Borgers M, and Ramaekers FC

Subjects
Animals, Annexin A5 metabolism, Apoptosis, Cell Adhesion physiology, Cell Differentiation, Cell Line, Connectin, Enzyme Inhibitors metabolism, Fluorescent Dyes metabolism, Humans, Intercellular Junctions chemistry, Membrane Proteins metabolism, Mice, Microscopy, Fluorescence, Muscle Proteins metabolism, Muscle, Skeletal metabolism, Myocardium cytology, Myocardium metabolism, Protein Kinases metabolism, Recombinant Proteins metabolism, Cell Fusion, Intercellular Junctions metabolism, Muscle Development, Muscle, Skeletal cytology, Muscle, Skeletal embryology, Phosphatidylserines metabolism
Abstract

Cell surface exposure of phosphatidylserine (PS) is shown to be part of normal physiology of skeletal muscle development and to mediate myotube formation. A transient exposure of PS was observed on mouse embryonic myotubes at E13, at a stage of development when primary myotubes are formed. The study of this process in cell cultures of differentiating C2C12 and H9C2 myoblasts also reveals a transient expression of PS at the cell surface. This exposure of PS locates mainly at cell-cell contact areas and takes place at a stage when the structural organization of the sarcomeric protein titin is initiated, prior to actual fusion of individual myoblast into multinucleated myotubes. Myotube formation in vitro can be inhibited by the PS binding protein annexin V, in contrast to its mutant M1234, which lacks the ability to bind to PS. Although apoptotic myoblasts also expose PS, differentiating muscle cells show neither loss of mitochondrial membrane potential nor detectable levels of active caspase-3 protein. Moreover, myotube formation and exposure of PS cannot be blocked by the caspase inhibitor zVAD(OMe)-fmk. Our findings indicate that different mechanisms regulate PS exposure during apoptosis and muscle cell differentiation, and that surface exposed PS plays a crucial role in the process of myotube formation.

Published
2001
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23. The effect of the cyclin-dependent kinase inhibitor olomoucine on cell cycle kinetics.

Author

Schutte B, Nieland L, van Engeland M, Henfling ME, Meijer L, and Ramaekers FC

Subjects
Antimetabolites pharmacology, Apoptosis drug effects, Bromodeoxyuridine pharmacology, CDC2 Protein Kinase metabolism, Carcinoma, Non-Small-Cell Lung, Cell Cycle drug effects, Cyclin-Dependent Kinases metabolism, Dose-Response Relationship, Drug, Flow Cytometry, G2 Phase drug effects, G2 Phase physiology, Humans, Kinetin, Lung Neoplasms, Mitosis drug effects, Mitosis physiology, Neuroblastoma, Roscovitine, S Phase drug effects, S Phase physiology, Tumor Cells, Cultured cytology, Tumor Cells, Cultured drug effects, Tumor Cells, Cultured enzymology, Cell Cycle physiology, Cyclin-Dependent Kinases antagonists & inhibitors, Enzyme Inhibitors pharmacology, Purines pharmacology
Abstract

The effect of the cyclin-dependent (CDK) inhibitors olomoucine and roscovitine on cell kinetics was studied. To this end, nonsmall cell lung cancer (NSCLC) cell line MR65 and neuroblastoma cell line CHP-212 were pulse labeled with bromodeoxyuridine (BrdUrd) and chased in culture medium, to which various concentrations of olomoucine or roscovitine were added. A dose-dependent inhibition of the G1/S-phase and G2/ M-/G1 transitions was observed. Furthermore, S-phase progression was also inhibited in a dose-dependent manner. Similarly, roscovitine, another CDK inhibitor with a 10-fold higher efficiency for both CDK1 and CDK2 as compared to olomoucine, showed the same effects at a 10-fold lower concentration. At the highest tested doses both olomoucine (200 microM) and roscovitine (40 microM) induced a complete cell cycle block in both cell lines, paralleled by the appearance of apoptotic figures. In these cultures a decrease in CDK1 protein level was found as shown by Western blotting. Bivariate CDK1/DNA analysis confirmed these observations and showed that a subpopulation of cells with characteristics of apoptosis became CDK1 negative. The presented data suggest that cyclins and CDKs are involved at an important nodal point shared by pathways regulating cellular proliferation and apoptosis.

Published
1997
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24. Detailed analysis of cell cycle kinetics upon proteasome inhibition.

Author

Machiels BM, Henfling ME, Gerards WL, Broers JL, Bloemendal H, Ramaekers FC, and Schutte B

Subjects
Animals, Bromodeoxyuridine metabolism, Calpain antagonists & inhibitors, Cysteine Proteinase Inhibitors pharmacology, Glycoproteins pharmacology, Humans, Kinetics, Leupeptins chemistry, Leupeptins pharmacology, Microscopy, Phase-Contrast, Oligopeptides pharmacology, Protease Inhibitors pharmacology, Proteasome Endopeptidase Complex, Tumor Cells, Cultured, Cell Cycle drug effects, Cysteine Endopeptidases metabolism, Enzyme Inhibitors pharmacology, Multienzyme Complexes metabolism
Abstract

We have studied specific effects of proteasome inhibition on cell cycle progression. To this end, the protease inhibitors MG115, calpain inhibitor I, and calpain inhibitor II, which display differential inhibitory effects on proteasomes, were used. Cell kinetic studies using bromodeoxyuridine pulse labeling revealed a complete block of G1/S and metaphase transitions and a delayed progression through S phase in cell cultures treated with 54 microM of MG115. Calpain inhibitor I in similar concentrations displayed a fivefold lower effect on cell cycle kinetics. Calpain inhibitor II and MG2M, which is a structural analogue of MG115, had no effect on the cell cycle. The inhibitory effect of MG115 treatment was reversible, because the cell cycle was immediately resumed when the MG115-containing culture medium was replaced by fresh culture medium. Because ubiquitinated proteins accumulated after MG115 treatment, it was confirmed that ubiquitin-dependent protein degradation, and thus proteasomal activity were blocked. By comparison of biochemical and in vitro proteasome inhibition experiments, it was hypothesized that chymotrypsin-like activity of proteasomes may play an important role in cell cycle kinetics.

Published
1997

25. Subcellular localization of proteasomes in apoptotic lung tumor cells and persistence as compared to intermediate filaments.

Author

Machiels BM, Henfling ME, Schutte B, van Engeland M, Broers JL, and Ramaekers FC

Subjects
Blotting, Western, Carcinoma, Squamous Cell, Endopeptidases analysis, Flow Cytometry, Fluorescent Antibody Technique, Lung Neoplasms, Subcellular Fractions chemistry, Tumor Cells, Cultured cytology, Tumor Cells, Cultured enzymology, Tumor Cells, Cultured ultrastructure, Apoptosis physiology, Endopeptidases metabolism, Intermediate Filaments metabolism, Multienzyme Complexes analysis
Abstract

We have studied the subcellular localization and expression levels of proteasomes during apoptosis in a lung cancer cell line. Apoptosis was induced by exposing the cells to 200 microM olomoucine, a specific cyclin-dependent kinase inhibitor. The morphological changes characteristic for apoptotic cells were visible: the cells reduced in size, the chromatin condensed and the membranes became convoluted. As the process continued, the nuclei became fragmented, and the cells broke up into cytoplasmic vesicles and apoptotic bodies. Immunocytochemically, apoptotic cells were detected by the ability to bind annexin V at their surface. During the initial stages of apoptosis, proteasomes were present in the nucleus as well as in the cytoplasm. Upon increased chromatin condensation, nuclear proteasomes were found predominantly surrounding the chromatin, while the chromatin itself remained devoid of staining. That the proteasomes persisted relatively long in the apoptotic cells was shown by immunoblotting of non-denaturing gels, which indicated that both 20S and 26S proteasomes were present in apoptotic cells. In immunofluoresence microscopy the proteasome fluorescence intensity of apoptotic cells seemed higher than that of non-apoptotic cells. These differences in intensity were even more pronounced after Triton X-100 extraction. Flow cytometry revealed that the absolute levels of proteasome staining in cells were decreased after Triton X-100 extraction. However, no differences in staining levels were detected between apoptotic and non-apoptotic cells. A relative increase of proteasome concentration through cell shrinkage or a concentration in certain cell compartments may be the origin of the apparently increased signal that was seen in immunofluorescence microscopy. Furthermore, proteasomes were clearly detectable in the apoptotic bodies and cytoplasmic vesicles at the time immunocytochemical reactivity for cytokeratins and lamins had diminished to a large extent. Immunoblotting of denaturing polyacrylamide gels confirmed the results obtained by flow cytometry. The proteasome content was retained only partially in the cells after Triton X-100 extraction, while the intermediate filaments were not detectable anymore in the apoptotic cells.

Published
1996

26. Changes in immunocytochemical detectability of proteasome epitopes depending on cell growth and fixation conditions of lung cancer cell lines.

Author

Machiels BM, Henfling ME, Broers JL, Hendil KB, and Ramaekers FC

Subjects
Blotting, Western, Carcinoma, Small Cell immunology, Carcinoma, Squamous Cell immunology, Cell Adhesion, Cell Compartmentation, Cell Division, Cysteine Endopeptidases immunology, Desmosomes, Epitopes, Flow Cytometry, Lung Neoplasms immunology, Multienzyme Complexes immunology, Proteasome Endopeptidase Complex, Tissue Fixation methods, Tumor Cells, Cultured, Carcinoma, Small Cell ultrastructure, Carcinoma, Squamous Cell ultrastructure, Cysteine Endopeptidases ultrastructure, Fluorescent Antibody Technique, Lung Neoplasms ultrastructure, Multienzyme Complexes ultrastructure
Abstract

The localization of proteasome epitopes in the lung cancer cell lines NCI-H82, derived from a small cell lung cancer, and MR65, derived from a squamous cell lung carcinoma, was studied in relation to cell growth conditions. For this purpose the proteasome monoclonal antibodies MCP34 and MCP20 were applied to the cells growing under different nutritional conditions, resulting in different proliferative states. Using indirect immunofluorescence microscopy with brief fixation in methanol (5 sec, -20 degrees C) followed by three dips in acetone (5 sec at room temperature), it became obvious that the intracellular detectability of the proteasomes changes depending on the nutritional and proliferative status of the tumor cells. Two types of experiments were carried out: (1) cells were grown for two days at different cell densities, with an excess of culture medium, and (2) cells were seeded in a low cell density and monitored for 6 days without change of medium. In cells grown at low density, the proteasomes can be detected mainly in the nuclei, while the nucleoli are almost devoid of staining, and the cytoplasm is only slightly stained. In cells grown at high density, the staining pattern changes with a much less pronounced nuclear staining than in the cells at low density, while the cytoplasm remains slightly stained. In the nutrient depletion experiment similar changes were seen. In cells growing under favorable conditions (1 or 2 days in fresh medium) proteasomes are detected mainly in the nuclei, whereas when the medium becomes depleted of nutrients (4 or 5-day-old medium) the staining pattern changes to one with a much less pronounced nuclear staining. However, in immunofluorescence studies on cells grown under similar conditions but fixed in ethanol (-20 degrees C) for 15 min, the changes in proteasome localization pattern were not detected during medium depletion. Using this fixation protocol the proteasomes are detected mainly in the nuclei at all stages of the medium exhaustion experiment. These apparently contrasting results suggest that upon nutrient depletion the proteasome epitopes become less accessible to the antibodies used. Apparently, the epitopes can regain accessibility if an extended ethanol fixation is used. This hypothesis was confirmed by flow cytometry and immunoblotting experiments. In flow cytometry of ethanol-fixed cells the fluorescence intensity of only a minor part of the cell population decreases to some extent with medium depletion, but in the majority of the cells fluorescence remains at its initial level. The immunoblotting experiments show no quantitative changes in proteasome content of the tumor cells at the different growth conditions.

Published
1995

27. Accessory cell function of thoracic duct nonlymphoid cells, dendritic cells, and splenic adherent cells in the Brown-Norway rat.

Author

Nagelkerken L, Henfling M, and van Breda Vriesman P

Subjects
Animals, Cell Adhesion, Concanavalin A pharmacology, Lymphocyte Activation drug effects, Macrophages immunology, Male, Rats, Rats, Inbred BN, Rats, Inbred Lew, Antigen-Presenting Cells physiology, Lymphoid Tissue cytology, Spleen cytology, Thoracic Duct cytology
Abstract

Thoracic duct lymph of lymphadenectomized Brown-Norway (BN) rats is highly enriched for nonlymphoid cells (NLC) which share several characteristics with splenic dendritic cells (DC), e.g., the binding of monoclonal antibody OX2. The accessory cell activity of NLC was analyzed by comparing these cells with DC and splenic adherent cells (SAC). In concanavalin A (Con A)-induced T-cell proliferation NLC, like DC, were very effective accessory cells at low cell numbers, as a consequence of an efficient induction of interleukin 2 (IL-2) production and IL-2 responsiveness. Responses in the presence of SAC were poor, even after the addition of excess IL-2. A fourfold enhancement of accessory cell activity of SAC was achieved by the depletion of FcR-positive cells, which were responsible for suppression of the Con A response. Low responsiveness of BN rats with respect to Lewis rats can in part be explained by a higher suppressive activity of macrophages in the BN rat.

Published
1985
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