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5. From Gene to Protein in Hours not Days

Author

Zaiss, K., primary, Fernholz, E., additional, Metzler, T., additional, Buchberger, B., additional, Wizemann, S., additional, Watzele, M., additional, Nemetz, C., additional, Schels, H., additional, Mutter, W., additional, and Röder, A., additional

Published
2000
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7. Constraining the brachial plexus does not compromise regional control in oropharyngeal carcinoma.

Author

Robert, Mutter W., Lok, Benjamin H., Dutta, Pinaki R., Riaz, Nadeem, Setton, Jeremy, Berry, Sean L., Goenka, Anuj, Zhigang Zhang, Rao, Shyam S., Wolden, Suzanne L., Lee, Nancy Y., Mutter, Robert W, and Zhang, Zhigang

Subjects
*BRACHIAL plexus, *OROPHARYNGEAL cancer, *HEAD & neck cancer treatment, *RADIOTHERAPY complications, *HUMAN dissection, *COMPUTERS in medicine, *BRACHIAL plexus neuropathies, *RETROSPECTIVE studies, *RADIATION doses, *RADIOTHERAPY, *RADIATION injuries, *SQUAMOUS cell carcinoma
Abstract

Background: Accumulating evidence suggests that brachial plexopathy following head and neck cancer radiotherapy may be underreported and that this toxicity is associated with a dose-response. Our purpose was to determine whether the dose to the brachial plexus (BP) can be constrained, without compromising regional control.Methods: The radiation plans of 324 patients with oropharyngeal carcinoma (OPC) treated with intensity-modulated radiation therapy (IMRT) were reviewed. We identified 42 patients (13%) with gross nodal disease <1 cm from the BP. Normal tissue constraints included a maximum dose of 66 Gy and a D05 of 60 Gy for the BP. These criteria took precedence over planning target volume (PTV) coverage of nodal disease near the BP.Results: There was only one regional failure in the vicinity of the BP, salvaged with neck dissection (ND) and regional re-irradiation. There have been no reported episodes of brachial plexopathy to date.Conclusions: In combined-modality therapy, including ND as salvage, regional control did not appear to be compromised by constraining the dose to the BP. This approach may improve the therapeutic ratio by reducing the long-term risk of brachial plexopathy. [ABSTRACT FROM AUTHOR]

Published
2013
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9. Adoptive immunotherapy of murine cytomegalovirus adrenalitis in the immunocompromised host: CD4-helper-independent antiviral function of CD8-positive memory T lymphocytes derived from latently infected donors

Author

Reddehase, M J, Jonjic, S, Weiland, F, Mutter, W, and Koszinowski, U H

Abstract

The ability of memory T lymphocytes derived from latently infected mice to control murine cytomegalovirus disease in the immunocompromised host was studied by adoptive transfer experiments. At a stage of pathogenesis when virus had already colonized target tissues, a therapeutic antiviral function could be ascribed to the CD8+ subset. This in vivo function was not restricted to sites in which intravenously infused lymphocytes usually are trapped or home in, such as the lungs or the spleen, respectively, but was also evident in the adrenal glands, a site to which antiviral effector cells have to specifically migrate. Specific infiltration of adrenal gland cortical tissue by donor-derived CD8+ memory T lymphocytes was demonstrated. CD4+ memory T lymphocytes had no antiviral effect by themselves and also were not required for the function of the CD8+ effector cells in this short-term immunotherapy model. These findings should help settle the debate about which subset of T lymphocytes comprises the effector cells that can directly control cytomegalovirus infection in the murine model system.

Published
1988
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10. CD8-positive T lymphocytes specific for murine cytomegalovirus immediate-early antigens mediate protective immunity

Author

Reddehase, M J, Mutter, W, Münch, K, Bühring, H J, and Koszinowski, U H

Abstract

We have shown in a murine model system for acute, lethal cytomegalovirus (CMV) disease in the immunocompromised natural host that control of virus multiplication in tissues, protection from virus-caused tissue destruction, and survival are mediated by virus-specific CD8+ CD4-T lymphocytes. Protection from a lethal course of disease did not result in a rapid establishment of virus latency, but led to a long-lasting, persistent state of infection. The CD8- CD4+ subset of T lymphocytes was not effective by itself in controlling murine CMV (MCMV) multiplication in tissue or essential for the protective function of the CD8+ CD4- effector cells. The antiviral efficacy of the purified CD8+ CD4- subset was not impaired by preincubation with fibroblasts that presented viral structural antigens, but was significantly reduced after depletion of effector cells specific for the nonstructural immediate-early antigens of MCMV, which are specified by the first among a multitude of viral genes expressed during MCMV replication in permissive cells. Thus, MCMV disease provides the first example of a role for nonstructural herpesvirus immediate-early antigens in protective immunity.

Published
1987
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11. Failure in generating hemopoietic stem cells is the primary cause of death from cytomegalovirus disease in the immunocompromised host.

Author

Mutter, W, Reddehase, M J, Busch, F W, Bühring, H J, and Koszinowski, U H

Abstract

We have shown in a murine model system for cytomegalovirus (CMV) disease in the immunocompromised host that CMV infection interferes with the earliest detectable step in hemopoiesis, the generation of the stem cell CFU-S-I, and thereby prevents the autoreconstitution of bone marrow after sublethal irradiation. The antihemopoietic effect could not be ascribed to a direct infection of stem cells. The failure in hemopoiesis was prevented by adoptive transfer of antiviral CD8+ T lymphocytes and could be overcome by syngeneic bone marrow transplantation. CD8+ T lymphocytes and bone marrow cells both mediated survival, although only CD8+ T lymphocytes were able to limit virus multiplication in host tissues. We concluded that not the cytopathic effect of virus replication in host tissues, but the failure in hemopoiesis, is the primary cause of death in murine CMV disease.

Published
1988
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12. Site-restricted persistent cytomegalovirus infection after selective long-term depletion of CD4+ T lymphocytes.

Author

Jonjić, S, Mutter, W, Weiland, F, Reddehase, M J, and Koszinowski, U H

Abstract

We have established a murine model system for exploring the ability of a CD4 subset-deficient host to cope with cytomegalovirus infection, and reported three findings. First, an antiviral response of the CD8 subset of T lymphocytes could be not only initiated but also maintained for a long period of time despite a continued absence of the CD4 subset, whereas the production of antiviral antibody proved strictly dependent upon help provided by the CD4 subset. Second, no function in the defense against infection could be ascribed as yet to CD4-CD8- T lymphocytes, which were seen to accumulate to a new subset as a result of depletion of the CD4 subset. This newly arising subset did not substitute for CD4+ T lymphocytes in providing help to B lymphocytes, and was also not effective in controlling the spread of virus in host tissues. As long as a function of these cells in the generation and maintenance of a CD8 subset-mediated response is not disproved, caution is indicated with concern to an autonomy of the CD8 subset. Third, even though with delay, the CD8+ effector cells raised in the CD4 subset-deficient host were able of clear vital tissues from productive infection and to restrict asymptomatic, persistent infection to acinar glandular epithelial cells in salivary gland tissue.

Published
1989
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13. In vivo application of recombinant interleukin 2 in the immunotherapy of established cytomegalovirus infection.

Author

Reddehase, M J, Mutter, W, and Koszinowski, U H

Abstract

We have shown in a murine model system for cytomegalovirus (CMV) disease in the immunocompromised host that in vivo application of recombinant human IL-2 (rhIL-2) can enhance the antiviral effect of a limited number of CD8+T lymphocytes, not only in prophylaxis, but also in therapy, when virus has already colonized host tissues. The observed net effect of IL-2 was consistent with the assumption of daily effector population doublings. The prospects for IL-2-supported immunotherapy of established CMV infection depend upon the tissues involved in disease. It appears that the prospects for controlling established CMV adrenalitis are less promising than for a therapy of interstitial CMV pneumonia.

Published
1987
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15. Optimising grinding processes in planetary ball mills.

Author

Scholl R., Mutter W., Wegerle R., Scholl R., Mutter W., and Wegerle R.

Abstract

During grinding, the heat generated by the impact between balls can cause ignition and result in gas reactions or thermal effects such as mechanical alloying. With the newly developed GTM (Gas pressure-Temperature-Measurement) system, such effects can be utilised to optimise the grinding process. Experiments were conducted in two planetary mills with varying numbers of Cr-Ni steel grinding balls of 10-15 mm diameter, using 5.1 g of titanium and 1.82 g of silicon in argon to investigate the effect of the spontaneous synthesis of Ti and Si powder to Ti5Si3. By recording the exact length of time from the start of grinding to spontaneous synthesis, direct comparisons could be made between mills or different process variables. It was found that more intensive grinding could be achieved in both mills when twenty 15 mm balls were used rather than fifty 10 mm balls. Increasing the number of balls from 50 to 250 showed an optimum of about 160 for fast, intensive grinding., During grinding, the heat generated by the impact between balls can cause ignition and result in gas reactions or thermal effects such as mechanical alloying. With the newly developed GTM (Gas pressure-Temperature-Measurement) system, such effects can be utilised to optimise the grinding process. Experiments were conducted in two planetary mills with varying numbers of Cr-Ni steel grinding balls of 10-15 mm diameter, using 5.1 g of titanium and 1.82 g of silicon in argon to investigate the effect of the spontaneous synthesis of Ti and Si powder to Ti5Si3. By recording the exact length of time from the start of grinding to spontaneous synthesis, direct comparisons could be made between mills or different process variables. It was found that more intensive grinding could be achieved in both mills when twenty 15 mm balls were used rather than fifty 10 mm balls. Increasing the number of balls from 50 to 250 showed an optimum of about 160 for fast, intensive grinding.

22. Filter clotting with continuous renal replacement therapy in COVID-19.

Author

Endres P, Rosovsky R, Zhao S, Krinsky S, Percy S, Kamal O, Roberts RJ, Lopez N, Sise ME, Steele DJR, Lundquist AL, Rhee EP, Hibbert KA, Hardin CC, Mc Causland FR, Czarnecki PG, Mutter W, Tolkoff-Rubin N, and Allegretti AS

Subjects
Anticoagulants administration & dosage, Anticoagulants adverse effects, Blood Coagulation drug effects, Clinical Protocols, Dose-Response Relationship, Drug, Equipment Failure Analysis, Factor Xa analysis, Female, Humans, Male, Middle Aged, SARS-CoV-2, Biomarkers, Pharmacological analysis, COVID-19 blood, COVID-19 physiopathology, COVID-19 therapy, Continuous Renal Replacement Therapy adverse effects, Continuous Renal Replacement Therapy methods, Critical Illness therapy, Drug Monitoring methods, Heparin administration & dosage, Heparin adverse effects, Micropore Filters adverse effects
Abstract

Coronavirus disease 2019 (COVID-19) appears to be associated with increased arterial and venous thromboembolic disease. These presumed abnormalities in hemostasis have been associated with filter clotting during continuous renal replacement therapy (CRRT). We aimed to characterize the burden of CRRT filter clotting in COVID-19 infection and to describe a CRRT anticoagulation protocol that used anti-factor Xa levels for systemic heparin dosing. Multi-center study of consecutive patients with COVID-19 receiving CRRT. Primary outcome was CRRT filter loss. Sixty-five patients were analyzed, including 17 using an anti-factor Xa protocol to guide systemic heparin dosing. Fifty-four out of 65 patients (83%) lost at least one filter. Median first filter survival time was 6.5 [2.5, 33.5] h. There was no difference in first or second filter loss between the anti-Xa protocol and standard of care anticoagulation groups, however fewer patients lost their third filter in the protocolized group (55% vs. 93%) resulting in a longer median third filter survival time (24 [15.1, 54.2] vs. 17.3 [9.5, 35.1] h, p = 0.04). The rate of CRRT filter loss is high in COVID-19 infection. An anticoagulation protocol using systemic unfractionated heparin, dosed by anti-factor Xa levels is reasonable approach to anticoagulation in this population.

Published
2021
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23. The Recombinant Bacteriophage Endolysin HY-133 Exhibits In Vitro Activity against Different African Clonal Lineages of the Staphylococcus aureus Complex, Including Staphylococcus schweitzeri.

Author

Idelevich EA, Schaumburg F, Knaack D, Scherzinger AS, Mutter W, Peters G, Peschel A, and Becker K

Subjects
Africa, Anti-Bacterial Agents biosynthesis, Cephalosporins pharmacology, Endopeptidases biosynthesis, Endopeptidases genetics, Humans, Methicillin Resistance genetics, Microbial Sensitivity Tests, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Staphylococcal Infections microbiology, Staphylococcus growth & development, Staphylococcus isolation & purification, Staphylococcus aureus growth & development, Staphylococcus aureus isolation & purification, beta-Lactam Resistance genetics, Ceftaroline, Anti-Bacterial Agents pharmacology, Endopeptidases pharmacology, Recombinant Proteins pharmacology, Staphylococcus drug effects, Staphylococcus Phages metabolism, Staphylococcus aureus drug effects
Abstract

HY-133 is a recombinant bacteriophage endolysin with bactericidal activity againstStaphylococcus aureus Here, HY-133 showedin vitroactivity against major African methicillin-susceptible and methicillin-resistantS. aureuslineages and ceftaroline/ceftobiprole- and borderline oxacillin-resistant isolates. HY-133 was also active againstStaphylococcus schweitzeri, a recently described species of theS. aureuscomplex. The activity of HY-133 on the tested isolates (MIC50, 0.25 μg/ml; MIC90, 0.5 μg/ml; range, 0.125 to 0.5 μg/ml) was independent of the species and strain background or antibiotic resistance., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published
2016
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24. Approaching clinical proteomics: current state and future fields of application in cellular proteomics.

Author

Apweiler R, Aslanidis C, Deufel T, Gerstner A, Hansen J, Hochstrasser D, Kellner R, Kubicek M, Lottspeich F, Maser E, Mewes HW, Meyer HE, Müllner S, Mutter W, Neumaier M, Nollau P, Nothwang HG, Ponten F, Radbruch A, Reinert K, Rothe G, Stockinger H, Tárnok A, Taussig MJ, Thiel A, Thiery J, Ueffing M, Valet G, Vandekerckhove J, Wagener C, Wagner O, and Schmitz G

Subjects
Analytic Sample Preparation Methods, Computational Biology, Humans, Proteomics standards, Statistics as Topic, Cells metabolism, Proteomics methods, Proteomics trends
Abstract

Recent developments in proteomics technology offer new opportunities for clinical applications in hospital or specialized laboratories including the identification of novel biomarkers, monitoring of disease, detecting adverse effects of drugs, and environmental hazards. Advanced spectrometry technologies and the development of new protein array formats have brought these analyses to a standard, which now has the potential to be used in clinical diagnostics. Besides standardization of methodologies and distribution of proteomic data into public databases, the nature of the human body fluid proteome with its high dynamic range in protein concentrations, its quantitation problems, and its extreme complexity present enormous challenges. Molecular cell biology (cytomics) with its link to proteomics is a new fast moving scientific field, which addresses functional cell analysis and bioinformatic approaches to search for novel cellular proteomic biomarkers or their release products into body fluids that provide better insight into the enormous biocomplexity of disease processes and are suitable for patient stratification, therapeutic monitoring, and prediction of prognosis. Experience from studies of in vitro diagnostics and especially in clinical chemistry showed that the majority of errors occurs in the preanalytical phase and the setup of the diagnostic strategy. This is also true for clinical proteomics where similar preanalytical variables such as inter- and intra-assay variability due to biological variations or proteolytical activities in the sample will most likely also influence the results of proteomics studies. However, before complex proteomic analysis can be introduced at a broader level into the clinic, standardization of the preanalytical phase including patient preparation, sample collection, sample preparation, sample storage, measurement, and data analysis is another issue which has to be improved. In this report, we discuss the recent advances and applications that fulfill the criteria for clinical proteomics with the focus on cellular proteomics (cytoproteomics) as related to preanalytical and analytical standardization and to quality control measures required for effective implementation of these technologies and analytes into routine laboratory testing to generate novel actionable health information. It will then be crucial to design and carry out clinical studies that can eventually identify novel clinical diagnostic strategies based on these techniques and validate their impact on clinical decision making.

Published
2009
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25. Approaching clinical proteomics: current state and future fields of application in fluid proteomics.

Author

Apweiler R, Aslanidis C, Deufel T, Gerstner A, Hansen J, Hochstrasser D, Kellner R, Kubicek M, Lottspeich F, Maser E, Mewes HW, Meyer HE, Müllner S, Mutter W, Neumaier M, Nollau P, Nothwang HG, Ponten F, Radbruch A, Reinert K, Rothe G, Stockinger H, Tarnok A, Taussig MJ, Thiel A, Thiery J, Ueffing M, Valet G, Vandekerckhove J, Verhuven W, Wagener C, Wagner O, and Schmitz G

Subjects
Biomarkers analysis, Clinical Medicine standards, Clinical Medicine trends, Proteomics standards, Proteomics trends, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Body Fluids chemistry, Clinical Medicine methods, Proteins analysis, Proteomics methods
Abstract

The field of clinical proteomics offers opportunities to identify new disease biomarkers in body fluids, cells and tissues. These biomarkers can be used in clinical applications for diagnosis, stratification of patients for specific treatment, or therapy monitoring. New protein array formats and improved spectrometry technologies have brought these analyses to a level with potential for use in clinical diagnostics. The nature of the human body fluid proteome with its large dynamic range of protein concentrations presents problems with quantitation. The extreme complexity of the proteome in body fluids presents enormous challenges and requires the establishment of standard operating procedures for handling of specimens, increasing sensitivity for detection and bioinformatical tools for distribution of proteomic data into the public domain. From studies of in vitro diagnostics, especially in clinical chemistry, it is evident that most errors occur in the preanalytical phase and during implementation of the diagnostic strategy. This is also true for clinical proteomics, and especially for fluid proteomics because of the multiple pretreatment processes. These processes include depletion of high-abundance proteins from plasma or enrichment processes for urine where biological variation or differences in proteolytic activities in the sample along with preanalytical variables such as inter- and intra-assay variability will likely influence the results of proteomics studies. However, before proteomic analysis can be introduced at a broader level into the clinical setting, standardization of the preanalytical phase including patient preparation, sample collection, sample preparation, sample storage, measurement and data analysis needs to be improved. In this review, we discuss the recent technological advances and applications that fulfil the criteria for clinical proteomics, with the focus on fluid proteomics. These advances relate to preanalytical factors, analytical standardization and quality-control measures required for effective implementation into routine laboratory testing in order to generate clinically useful information. With new disease biomarker candidates, it will be crucial to design and perform clinical studies that can identify novel diagnostic strategies based on these techniques, and to validate their impact on clinical decision-making.

Published
2009
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26. Twin pregnancy and the risk of preeclampsia: bigger placenta or relative ischemia?

Author

Bdolah Y, Lam C, Rajakumar A, Shivalingappa V, Mutter W, Sachs BP, Lim KH, Bdolah-Abram T, Epstein FH, and Karumanchi SA

Subjects
Adult, Diseases in Twins, Enzyme-Linked Immunosorbent Assay, Female, Gene Expression, Humans, Incidence, Ischemia blood, Neovascularization, Pathologic blood, Placenta blood supply, Placenta Growth Factor, Polymerase Chain Reaction, Pre-Eclampsia etiology, Pre-Eclampsia physiopathology, Pregnancy, Risk Factors, Twins, Up-Regulation, Ischemia physiopathology, Placenta pathology, Pre-Eclampsia epidemiology, Pregnancy Proteins blood, Receptor, Fibroblast Growth Factor, Type 1 blood, Vascular Endothelial Growth Factor A blood
Abstract

Objective: Twin pregnancies are a risk factor for preeclampsia with a reported incidence of 2-3 times higher than singleton pregnancies. Soluble fms-like tyrosine kinase 1 (sFlt1), which is a circulating antiangiogenic molecule of placental origin, plays a central role in preeclampsia by antagonizing placental growth factor (PlGF) and vascular endothelial growth factor signaling in the maternal vasculature. Increased sFlt1 and the ratio sFlt1/free PlGF have been shown to antedate clinical signs in preeclampsia. Although the cause of the upregulated sFlt1 in preeclampsia still is not understood clearly, placental ischemia with accompanying hypoxia is thought to play an important role. We therefore hypothesized that the higher risk of preeclampsia in twin pregnancies results from high sFlt1 (or sFlt1/PlGF) and that the sFlt1 upregulation was due to either relative placental hypoxia and/or increased placental mass., Study Design: Maternal serum samples and placentas from third-trimester twin and singleton pregnancies without preeclampsia were used. Serum samples were analyzed for levels of sFlt1 and free PlGF by enzyme-linked immunosorbent assay and reported as means (in nanograms per milliliter and picograms per milliliter, respectively). Placentas were weighed and examined for content of sFlt1 and PlGF messenger RNA (mRNA) by quantitative polymerase chain reaction and hypoxia inducible factor-1alpha (HIF-1alpha) protein by Western blot., Results: Soluble Flt1 concentrations in twin pregnancy maternal serum were 2.2 times higher than those that were measured in singleton pregnancy maternal serum samples (30.98 +/- 9.78 ng/mL vs 14.14 +/- 9.35 ng/mL, respectively; P = .001). Free PlGF concentrations were not significantly different between twin and singleton maternal serum samples, but the mean sFlt1/PlGF ratio of twin pregnancy maternal serum samples was 2.2 times higher than the equivalent ratio in singleton pregnancy samples (197.58 +/- 126.86 ng/mL vs 89.91 +/- 70.63 ng/mL, respectively; P = .029). Quantitative polymerase chain reaction for sFlt1 and PlGF mRNA revealed no significant differences between the 2 study groups. Western blot analysis of placental samples for HIF-1alpha revealed a mean ratio HIF-1alpha/actin of 0.53 vs 0.87, for the twins vs singletons placental samples respectively (twins showed lower HIF-1alpha, not higher). The mean weights of twin and singleton placentas were 1246 vs 716 g, respectively (P < .001). Importantly, the placental weights correlated very well with the circulating sFlt1 levels (R(2) = .75)., Conclusion: In twin pregnancies, circulating sFlt1 levels and sFlt1/PlGF ratios were twice as high as those in singleton pregnancies. The increased serum sFlt1 levels in twin pregnancies were not accompanied by any changes in the levels of sFlt1 mRNA and HIF-1alpha protein in the twin placentas but were correlated with increased placental weight. These findings suggest that the increased risk of preeclampsia in twin pregnancies may be due to increased placental mass that leads to increased circulating levels of sFlt1.

Published
2008
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27. Protease activity of urokinase and tumor progression in a syngeneic mammary cancer model.

Author

Merchan JR, Tang J, Hu G, Lin Y, Mutter W, Tong C, Karumanchi SA, Russell SJ, and Sukhatme VP

Subjects
Animals, Blotting, Northern, Cell Proliferation, Clone Cells, Disease Progression, Enzyme-Linked Immunosorbent Assay, Female, Gene Expression Regulation, Neoplastic, Immunohistochemistry, Lung Neoplasms metabolism, Lung Neoplasms secondary, Mice, Mice, Inbred BALB C, Peptide Hydrolases metabolism, Platelet Endothelial Cell Adhesion Molecule-1 analysis, Proliferating Cell Nuclear Antigen analysis, Survival Analysis, Tissue Plasminogen Activator genetics, Transfection, Transplantation, Isogeneic, Tumor Cells, Cultured, Up-Regulation, Urokinase-Type Plasminogen Activator genetics, Mammary Neoplasms, Experimental metabolism, Mammary Neoplasms, Experimental pathology, Mutation, Tissue Plasminogen Activator metabolism, Urokinase-Type Plasminogen Activator metabolism
Abstract

Background: We and others have previously shown that plasminogen activators generate endogenous angiogenesis inhibitors and induce antiangiogenic activity. Here we assessed the effects of plasminogen activator overexpression on tumor progression in a syngeneic mammary cancer model., Methods: Genes encoding murine tissue plasminogen activator (tPA), urokinase (uPA), and vector controls were stably transfected into 4T1 murine mammary cancer cells, and cell proliferation in vitro was analyzed. Cells were also implanted into female BALB/c mice (n = 12 per group), and tumor growth, lung metastases, and survival were compared. Tumor cell proliferation and microvessel formation were analyzed by immunohistochemistry using antibodies to proliferating cell nuclear antigen and CD31, respectively. 4T1 cells transfected with proteolytically inactive uPA mutants (A and B) were assayed for proliferation in vitro and tumor growth in vivo by using the same syngeneic model (eight to 10 mice per group). All statistical tests were two-sided., Results: In vitro growth of uPA- and tPA-overexpressing and control 4T1 cells was similar. In vivo, however, inhibition of tumor growth and lung metastasis were inhibited in the mice carrying tPA- and uPA-overexpressing tumors, compared with controls (tumor weight at day 34: control, mean = 1760 mg, 95% confidence interval [CI] = 1434 to 2087 mg; tPA, mean = 921, 95% CI = 624 to 1217 mg; P < .001; uPA, mean = 395 mg, 95% CI = 161 to 629 mg; P < .001; number of lung metastases at day 34: control, mean = 117, 95% CI = 74 to 159; tPA, mean = 33, 95% CI = 13 to 52; uPA, mean = 15, 95% CI = 4 to 25; P < .001). Median survival was 42 (95% CI = 36 to 44), 55 (95% CI = 48 to 61), and 73 (95% CI = 51 to 86) days in the control, tPA, and uPA groups, respectively (P < .001). uPA- and tPA-expressing tumors had reduced angiogenesis and cell proliferation compared with controls. Tumors overexpressing uPA mutants grew faster than tumors expressing wild-type uPA (tumor volume at day 30: wild-type uPA, mean = 203, 95% CI = 121 to 285 mm3; control, mean = 534, 95% CI = 460 to 608 mm3; P < .001; mutant A, mean = 600, 95% CI = 520 to 679 mm3; P < .001; and mutant B, mean = 435, 95% CI = 358.9 to 511 mm3; P = .005)., Conclusions: In this mouse model, uPA expression delayed tumor progression and had antiangiogenic and antiproliferative effects that may be mediated by uPA's protease activity. These results challenge the current dogma of proteases being exclusively tumor promoting and provide further rationale for exploring plasminogen activators as antitumor agents.

Published
2006
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28. High-yield, in vitro protein expression using a continuous-exchange, coupled transcription/ translation system.

Author

Martin GA, Kawaguchi R, Lam Y, DeGiovanni A, Fukushima M, and Mutter W

Subjects
3T3 Cells, Animals, Chloramphenicol O-Acetyltransferase biosynthesis, Chloramphenicol O-Acetyltransferase genetics, Chloramphenicol O-Acetyltransferase isolation & purification, Cloning, Molecular, Escherichia coli genetics, Gene Expression, Green Fluorescent Proteins, In Vitro Techniques, Interleukin-2 biosynthesis, Interleukin-2 genetics, Interleukin-2 isolation & purification, Killer Cells, Lymphokine-Activated immunology, Luminescent Proteins biosynthesis, Luminescent Proteins genetics, Luminescent Proteins isolation & purification, Mice, Proteins isolation & purification, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Biotechnology instrumentation, Protein Biosynthesis, Proteins genetics, Transcription, Genetic
Abstract

The Rapid Translation System (RTS 500) (Roche Molecular Biochemicals) is a high-yield protein expression system that utilizes an enhanced E. coli lysate for an in vitro transcription/translation reaction. In contrast to conventional transcription/translation, this system allows protein expression to continue for more than 24 h. We demonstrated the utility of the RTS 500 by expressing different soluble and active proteins that generally pose problems in cell-based expression systems. We first expressed GFP-lunasin, a fusion protein that, because of its toxicity, has been impossible to produce in whole cells. The second protein we expressed, human interleukin-2 (IL-2), is generally difficult to produce, either as the native molecule or as a GSTfusion protein, in a soluble form in bacteria. Finally, we demonstrated the capacity of the RTS 500 to co-express proteins, by the simultaneous production of GFP and CAT in a single reaction. This new technology appears to be particularly usefulfor the convenient production of preparative amounts (100-900 microg) of proteins that are toxic or insoluble in cell-based systems.

Published
2001
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29. Molecular analysis of herpesviral gene products recognized by protective cytolytic T lymphocytes.

Author

Koszinowski UH, Reddehase MJ, Keil GM, Volkmer H, Jonjic S, Messerle M, del Val M, Mutter W, Münch K, and Bühler B

Subjects
Animals, Antigens, Viral genetics, Antigens, Viral immunology, Cytomegalovirus genetics, Genes, Viral, Mice, Vaccinia virus genetics, Vaccinia virus immunology, Viral Proteins genetics, Viral Vaccines immunology, Cytomegalovirus immunology, T-Lymphocytes, Cytotoxic immunology, Viral Proteins immunology
Abstract

The infection of the mouse with murine cytomegalovirus (MCMV) served as a model system to understand the biology of human CMV infection. The contribution of cytolytic T lymphocytes (CTL) to the recovery from infection was studied. Protection against lethal MCMV disease could be conferred on immunodepleted hosts by adoptive transfer of lymphocytes. The antiviral effect was mediated by specifically sensitized T lymphocytes of the CD8+ subset. These cells limited viral spread, prevented tissue destruction by viral cytopathic effects, and protected from lethal disease. Transferred cells have protective therapeutic function even when the virus has already colonized host tissues. CD8+ cells do not require the contribution of CD4+ cells for in vivo function. Selective expression of immediate-early (IE) phase genes in target cells allowed the detection of the immunodominant IE antigen recognized by CTL. The major IE gene ieI encodes a non-structural viral phosphoprotein, pp89, which resides in the nucleus of infected cells where it acts as transcriptional regulator. Expression of gene ieI is under temporal control, and membrane presentation of the protein domain detected by CTL is down-regulated by MCMV early-phase products. A recombinant vaccinia virus expressing gene ieI induced immunity that protected mice against a subsequent challenge with a lethal dose of MCMV. The protective effect was entirely mediated by CD8+ T lymphocytes. Thus, an experimental vaccine expressing a single nonstructural herpesvirus protein can induce a protective cellular immune response.

Published
1987
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30. The role of Cu(I)-thiolate clusters during the proteolysis of Cu-thionein.

Author

Weser U, Mutter W, and Hartmann HJ

Subjects
Animals, Carrier Proteins, Endopeptidase K, Endopeptidases metabolism, Kinetics, Liver metabolism, Lysosomes enzymology, Male, Oxidation-Reduction, Rats, Rats, Inbred Strains, Saccharomyces cerevisiae metabolism, Streptomyces griseus enzymology, Thermolysin metabolism, Copper metabolism, Metallothionein metabolism, Organometallic Compounds metabolism, Peptide Hydrolases metabolism
Abstract

Rat liver Cu,Zn-[35S]thionein and yeast Cu-thionein were subjected to proteolysis in vitro using equilibrium dialysis. The partially copper-loaded vertebrate thionein (2-7 Cu/mol) was affected by different proteases including thermolysin, proteinase K, protease from Streptomyces griseus and lysosomal enzymes. Unlike the 2Cu-thionein the respective 7Cu-thiolate-centred metallothionein was hardly proteolytically digested. In contrast to fully copper-loaded native yeast Cu-thionein both the H2O2-oxidized and the metal-free protein were effectively cleaved in the presence of proteinase K. It is important to realize that the native Cu(I)-thiolate chromophore survives the proteolytic attack. When the copper-sulphur bonding is broken and the same amount of copper is unspecifically bound to the thionein portion, proteolysis proceeds identically with respect to the rate observed in the presence of the apoprotein. The unsuccessful proteolysis of native Cu-thionein is not attributable to a simple copper-dependent inhibition of the proteinases. It is suggested that prior to proteolysis the copper-sulphur clusters must be destroyed.

Published
1986
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