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Start Over Author "Ulrich Sack" Journal cytometry. part a : the journal of the international society for analytical cytology
10 results on '"Ulrich Sack"'

1. A comparative study of two separation methods to isolate monocytes

Author

Ronald Weiss, Anja Grahnert, Wilhelm Gerdes, Rommy Berthold, Franziska Leonhardt, and Ulrich Sack

Subjects
0301 basic medicine, Histology, medicine.drug_class, Cell Culture Techniques, Cell Separation, Monoclonal antibody, Monocytes, Pathology and Forensic Medicine, 03 medical and health sciences, 0302 clinical medicine, Immune system, Affinity chromatography, Antigens, CD, medicine, Humans, Cells, Cultured, Whole blood, Magnetic-activated cell sorting, Chemistry, Immunomagnetic Separation, Monocyte, Cell Differentiation, Cell Biology, Dendritic Cells, Flow Cytometry, Cell biology, 030104 developmental biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Separation method, Cytometry
Abstract

Separation of specific blood cells is necessary for a deeper insight into their role in health and disease. To obtain such cells, efficient and robust isolation methods are needed. We compare here the Fab-based Traceless Affinity Cell Selection (TACS®) technology and the Magnetic Activated Cell Sorting (MACS®) technology to isolate human monocytes from whole blood and buffy coats as well as the differentiation of the isolated monocytes to dendritic cells (DCs). TACS® is a positive selection technology using immune affinity chromatography based on CD-specific low affinity Fab-fragments for the reversible capture and release of target cells. The positive selection by MACS® is based on magnetic beads coated with specific high affinity monoclonal antibodies to catch the target cells. The target cells separated by TACS® are "label-free" while cells positively isolated by MACS® will carry the cell specific label. Our data show that the separation methods described here are well suited to obtain functional monocytes of high quality and purity. A differentiation of the cells into DCs leads to comparable results with the exception that CD1a expression levels on immature and mature DCs are elevated when monocytes are isolated using the TACS® technology. Taken together, our results suggest that the TACS® method may be of advantage when preparing monocytes and monocyte-derived DCs for functional analyses, while the MACS® method seems to be capable of higher monocyte recoveries. © 2018 International Society for Advancement of Cytometry.

Published
2018

3. Attenuation of graft-versus-host-disease in NOD scid IL-2Rγ(-/-) (NSG) mice by ex vivo modulation of human CD4(+) T cells

Author

Nadja, Hilger, Jakob, Glaser, Claudia, Müller, Christoph, Halbich, Anne, Müller, Ulla, Schwertassek, Jörg, Lehmann, Peter, Ruschpler, Franziska, Lange, Andreas, Boldt, Lilly, Stahl, Ulrich, Sack, Christopher, Oelkrug, Frank, Emmrich, and Stephan, Fricke

Subjects
CD4-Positive T-Lymphocytes, Mice, Knockout, Disease Models, Animal, Mice, Hematopoietic Stem Cell Transplantation, Leukocytes, Mononuclear, Animals, Graft vs Host Disease, Humans, Antibodies, Interleukin Receptor Common gamma Subunit
Abstract

NOD.Cg-Prkdc(scid) IL-2rg(tm1Wjl) /SzJ (NSG) mice are a valuable tool for studying Graft-versus-Host-Disease (GvHD) induced by human immune cells. We used a model of acute GvHD by transfer of human peripheral blood mononuclear cells (PBMCs) into NSG mice. The severity of GvHD was reflected by weight loss and was associated with engraftment of human cells and the expansion of leukocytes, particularly granulocytes and monocytes. Pre-treatment of PBMCs with the anti-human CD4 antibody MAX.16H5 IgG1 or IgG4 attenuated GvHD. The transplantation of 2 × 10(7) PBMCs without anti-human CD4 pre-treatment induced a severe GvHD (0% survival). In animals receiving 2 × 10(7) PBMCs pre-incubated with MAX.16H5 IgG1 or IgG4, GvHD development was reduced and survival was increased. Immune reconstitution was measured by flow cytometry and confirmed for human leukocytes (CD45), CD3(+) /CD8(+) cytotoxic T cells and CD3(+) /CD4(+) T helper cells. Human B cells (CD19) and monocytes (CD14) could not be detected. Histopathological analysis (TUNEL assay) of the gut of recipient animals showed significantly less apoptotic crypt cells in animals receiving a MAX.16H5 IgG1 pre-incubated graft. These findings indicate that pre-incubation of an allogeneic graft with an anti-human CD4 antibody may decrease the frequency and severity of GvHD after hematopoietic stem cell transplantation (HSCT) and the need of conventional immunosuppressive drugs. Moreover, this approach most probably provides a safer HSCT that must be confirmed in appropriate clinical trials in the future. © 2016 International Society for Advancement of Cytometry.

Published
2016

4. Clinical Cell Cycle Analysis Revisited

Author

Ulrich Sack and Attila Tárnok

Subjects
Cell cycle analysis, Histology, Cell cycle genetics, Cell Cycle, MEDLINE, Humans, Cell Biology, Biology, Bioinformatics, Pathology and Forensic Medicine, Introductory Journal Article
Published
2015

5. Assessment of modulated cytostatic drug resistance by automated γH2AX analysis

Author

Annika, Reddig, Sebastian, Lorenz, Rico, Hiemann, Karina, Guttek, Roland, Hartig, Lisa, Heiserich, Caroline, Eberle, Vanessa, Peters, Peter, Schierack, Ulrich, Sack, Dirk, Roggenbuck, and Dirk, Reinhold

Subjects
Adult, Male, Sirolimus, DNA, Cytostatic Agents, Drug Resistance, Multiple, Histones, Young Adult, Microscopy, Fluorescence, Cyclosporine, Leukocytes, Mononuclear, Humans, DNA Breaks, Double-Stranded, Female, Etoposide
Abstract

The efficacy of many chemotherapeutic agents relies on the preferential destruction of rapidly dividing cancer cells by inducing various kinds of DNA damage. The most deleterious type of DNA lesions are DNA double-strand breaks (DSB), which can be detected by immunofluorescence staining of phosphorylated histone protein H2AX (γH2AX). Furthermore, γH2AX has been suggested as clinical pharmacodynamic biomarker in chemotherapeutic cancer treatment. A great challenge in treating neoplastic diseases is the varying response behavior among cancer patients. Thus, intrinsic or drug-induced overexpression of efflux pumps often leads to multiple drug resistance (MDR) and treatment failure. In particular, inter-individual differences in expression levels of efflux pumps, such as the permeability glycoprotein (P-gp), were shown to correlate with cancer progression. Several efficient cytostatic drugs, including the DSB-inducing agent etoposide (ETP) are known P-gp substrates. In this respect, modulation of MDR by P-gp inhibitors, like the immunosuppressives cyclosporine A (CsA) and rapamycin (Rapa) have been described. Here, we investigated the application of γH2AX focus assay to monitor the impact of CsA and Rapa on ETP-induced cytotoxicity in human peripheral blood mononuclear cells. Evaluation of γH2AX foci was performed by the automated fluorescence microscopy and interpretation system AKLIDES. Compared to ETP treatment alone, our results revealed a significant rise in γH2AX focus number and percentage of DSB-positive cells after cells have been treated with ETP in the presence of either CsA or Rapa. In contrast, DSB levels of cells incubated with CsA or Rapa alone were comparable to focus number of untreated cells. Our results successfully demonstrated how automated γH2AX analysis can be used as fast and reliable approach to monitor drug resistance and the impact of MDR modulators during treatment with DSB-inducing cytostatics..

Published
2015

6. Fully automated analysis of chemically induced γH2AX foci in human peripheral blood mononuclear cells by indirect immunofluorescence

Author

Annika, Willitzki, Sebastian, Lorenz, Rico, Hiemann, Karina, Guttek, Alexander, Goihl, Roland, Hartig, Karsten, Conrad, Eugen, Feist, Ulrich, Sack, Peter, Schierack, Lisa, Heiserich, Caroline, Eberle, Vanessa, Peters, Dirk, Roggenbuck, and Dirk, Reinhold

Subjects
Histones, Leukocytes, Mononuclear, Humans, DNA Breaks, Double-Stranded, Fluorescent Antibody Technique, Indirect, DNA Damage, Etoposide
Abstract

Analysis of phosphorylated histone protein H2AX (γH2AX) foci is currently the most sensitive method to detect DNA double-strand breaks (DSB). This protein modification has the potential to become an individual biomarker of cellular stress, especially in the diagnosis and monitoring of neoplastic diseases. To make γH2AX foci analysis available as a routine screening method, different software approaches for automated immunofluorescence pattern evaluation have recently been developed. In this study, we used novel pattern recognition algorithms on the AKLIDES® platform to automatically analyze immunofluorescence images of γH2AX foci and compared the results with visual assessments. Dose- and time-dependent γH2AX foci formation was investigated in human peripheral blood mononuclear cells (PBMCs) treated with the chemotherapeutic drug etoposide (ETP). Moreover, the AKLIDES system was used to analyze the impact of different immunomodulatory reagents on γH2AX foci formation in PBMCs. Apart from γH2AX foci counting the use of novel pattern recognition algorithms allowed the measurement of their fluorescence intensity and size, as well as the analysis of overlapping γH2AX foci. The comparison of automated and manual foci quantification showed overall a good correlation. After ETP exposure, a clear dose-dependent increase of γH2AX foci formation was evident using the AKLIDES as well as Western blot analysis. Kinetic experiments on PBMCs incubated with 5 μM ETP demonstrated a peak in γH2AX foci formation after 4 to 8 h, while a removal of ETP resulted in a strong reduction of γH2AX foci after 1 to 4 h. In summary, this study demonstrated that the AKLIDES system can be used as an efficient automatic screening tool for γH2AX foci analysis by providing new evaluation features and facilitating the identification of drugs which induce or modulate DNA damage.

Published
2013

7. Multiplex assessment of non-organ-specific autoantibodies with a novel microbead-based immunoassay

Author

Christian Schröder, Karsten Conrad, Dirk Roggenbuck, Kai Grossmann, Ulrich Sack, and Peter Schierack

Subjects
Adult, Male, Histology, Population, Enzyme-Linked Immunosorbent Assay, Biology, Immunofluorescence, Sensitivity and Specificity, Pathology and Forensic Medicine, Antibody Specificity, Rheumatic Diseases, medicine, Humans, Multiplex, Serologic Tests, education, Fluorescent Antibody Technique, Indirect, Autoantibodies, Immunoassay, education.field_of_study, medicine.diagnostic_test, Autoantibody, IIf, Antigens, Nuclear, Cell Biology, Microbead (research), DNA, Middle Aged, Molecular biology, Primary and secondary antibodies, Microspheres, Microscopy, Fluorescence, Multiphoton, Antibodies, Antinuclear, Immunoglobulin G, biology.protein, Female
Abstract

Advances in immunofluorescence assay development paved the way for the simultaneous detection of several antibodies in one sample, for the serological diagnosis of systemic rheumatic diseases. Standardized automated screening of such antibodies can be achieved by HEp-2 cell-based indirect immunofluorescence (IIF) using a multicolor fluorescence imaging technical platform. To create a common platform for both screening and specific antibody assessment, multiplex measurement of antibodies using fluorescence-coded immobilized microbeads was employed on the same platform. The multicolor fluorescence detection system VideoScan (AKLIDES 1 ) was used for the fluorescence analysis of a multiplex microbead-based immunoassay (MIA). First, immunoglobulin G (IgG) was covalently coupled to one microbead population in duplicate and in three independent experiments. The coupled IgG was detected by a Cy TM 5-conjugated secondary antibody. Thus, intra- and interassay coefficients of variation (CV) were obtained. Second, a multiplex determination of antinuclear autoantibodies (ANA) to Scl-70, Sm, dsDNA, SS-A (Ro60), CENP-B, and La/SS-B by solid-phase MIA was investigated, using 72 sera from patients with autoimmune diseases such as systemic lupus erythematosus and systemic sclerosis (SS). The reproducibility study revealed intra-assay CVs ranging from 3.2% to 9.9%, and interassay CVs ranging from 9.6% to 14.7%. The detection of Scl-70-, Sm-, CENP-B-, and La/SS-B-ANA with MIA showed very good agreement with the ELISA results (kappa 5 1.0). The resulting relative sensitivities and specificities for Scl-70-, Sm-, CENP-B-, dsDNA-, and La/SS-B-ANA were 100%, respectively, with the exception of dsDNA (specificity 97%). Multiplex detection by immobilized fluorescence-coded microbeads using multicolor fluorescence is a reliable method for the assessment of rheumatic-disease-specific antibodies. Multicolor fluorescence analyses with pattern detection algorithms provide a common platform technique for both the screening of ANA by cell-based IIF and specific antibody assessment by multiplex detection. ' 2011 International Society for Advancement of Cytometry

Published
2010

8. Objective quality evaluation of fluorescence images to optimize automatic image acquisition

Author

Martin Weigert, Nadja Hilger, Ulrich Sack, Rico Hiemann, and Publica

Subjects
Histology, Indoles, genetic structures, Test data generation, Computer science, media_common.quotation_subject, Image processing, Pathology and Forensic Medicine, Image (mathematics), Optics, Cell Line, Tumor, medicine, Image Processing, Computer-Assisted, Humans, Quality (business), Computer vision, Image sensor, media_common, Data collection, business.industry, Data Collection, Reproducibility of Results, Cell Biology, Object (computer science), medicine.anatomical_structure, Microscopy, Fluorescence, Visual Perception, Human eye, Artificial intelligence, business
Abstract

Background Because different spectral sensitivities of human eye and image sensor lead to different perception of fluorescence signals, data generation is an important step in image analysis, because following work steps depend on it. Methods We developed a method to determine image parameters allowing an objective appraisal of quality of image data as well as a separation of object and background. Results Calculated parameters can be used for an automated adjustment of camera parameters in image analysis systems. Discussion Our approach for objective adjusted data generation achieves an improvement of analysis quality. © 2006 International Society for Analytical Cytology

Published
2006

9. Multiplex analysis of cytokines in exhaled breath condensate

Author

Robert Scheibe, Gerard Hoheisel, Ulrich Sack, Christian Gessner, Michael Wötzel, Hubert Wirtz, Hartmut Kuhn, Stefan Hammerschmidt, Frank Emmrich, and Publica

Subjects
Adult, Male, Histology, Low protein, medicine.medical_treatment, Lung injury, Pathology and Forensic Medicine, Medicine, Humans, In patient, Exhaled breath condensate, Multiplex, Aged, Respiratory Distress Syndrome, Lung, business.industry, Interleukin-6, Tumor Necrosis Factor-alpha, Interleukin-8, Smoking, Interleukin, Reproducibility of Results, Cell Biology, Pneumonia, Middle Aged, Flow Cytometry, Interleukin-12, Respiration, Artificial, respiratory tract diseases, Interleukin-10, Cytokine, medicine.anatomical_structure, Breath Tests, Immunology, Cytokines, Female, business, Interleukin-1
Abstract

Background: To improve monitoring of lung diseases, we analyzed cytokines in exhaled breath condensate (EBC). The main challenge in measurement of cytokines in EBC is the low protein content, which requires concentration steps that conflict with the need for excessive fluid required by most commonly used kits. Methods: Here, a multiplex bead array for the detection of interleukins (IL) -1b, -6, -8, -10, TNF-a, and IL-12p70 was modified and validated for analysis in EBC samples. Furthermore, 33 healthy volunteers and 11 patients with acute lung injury were investigated. Results: In patients with inflammatory lung diseases, cytokine levels for all investigated cytokines were higher in comparison to healthy smokers or healthy volunteers. Discussion: Multiplexed immunoassays in highly sensitive approaches allow for cytokine detection in EBC. We found significant differences between patients and controls for all investigated cytokines. q 2006 International Society for Analytical Cytology

Published
2006

10. Sequential photobleaching of fluorochromes for polychromatic slide-based cytometry

Author

Anja Mittag, Ulrich Sack, Dominik Lenz, Attila Tárnok, Andreas O. H. Gerstner, Jozsef Bocsi, and Publica

Subjects
Histology, Photobleaching, CD3 Complex, business.industry, Antigens, CD19, Cell Biology, Biology, Cellular level, CD5 Antigens, Information density, Pathology and Forensic Medicine, Laser Scanning Cytometry, Slide based cytometry, Optics, Biophysics, Leukocytes, Humans, business, Cytometry, Merge (version control), Fluorescent Dyes
Abstract

Background Slide-based cytometry is a key technology for polychromatic cytomic investigations. Here we exploit the relocalization and merge feature of Laser Scanning Cytometry for distinguishing fluorochromes of comparable emission spectra but different photostabilities. Methods Blood specimens were stained with the fluorochrome pairs: FITC/ALEXA488, PE/ALEXA532, or APC/ALEXA633. Bleaching was performed by repeated laser excitation. Results Since ALEXA dyes are photostable as compared to the conventional fluorochromes FITC, PE, and APC, a differentiation within one fluorochrome pair is possible. Conclusion The sequential photobleaching method results in an increased information density on a single cell level and represents an important component to perform polychromatic cytometry. © 2006 International Society for Analytical Cytology

Published
2006

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