TY - JOUR A1 - Sturm, Julia B. A1 - Hess, Michael A1 - Weibel, Stephanie A1 - Chen, Nanhei G. A1 - Yu, Yong A. A1 - Zhang, Quian A1 - Donat, Ulrike A1 - Reiss, Cora A1 - Gambaryan, Stepan A1 - Krohne, Georg A1 - Stritzker, Jochen A1 - Szalay, Aladar A. T1 - Functional hyper-IL-6 from vaccinia virus-colonized tumors triggers platelet formation and helps to alleviate toxicity of mitomycin C enhanced virus therapy N2 - Background: Combination of oncolytic vaccinia virus therapy with conventional chemotherapy has shown promise for tumor therapy. However, side effects of chemotherapy including thrombocytopenia, still remain problematic. Methods: Here, we describe a novel approach to optimize combination therapy of oncolytic virus and chemotherapy utilizing virus-encoding hyper-IL-6, GLV-1h90, to reduce chemotherapy-associated side effects. Results: We showed that the hyper-IL-6 cytokine was successfully produced by GLV-1h90 and was functional both in cell culture as well as in tumor-bearing animals, in which the cytokine-producing vaccinia virus strain was well tolerated. When combined with the chemotherapeutic mitomycin C, the anti-tumor effect of the oncolytic virotherapy was significantly enhanced. Moreover, hyper-IL-6 expression greatly reduced the time interval during which the mice suffered from chemotherapy-induced thrombocytopenia. Conclusion: Therefore, future clinical application would benefit from careful investigation of additional cytokine treatment to reduce chemotherapy-induced side effects. KW - Biologie KW - vaccinia virus KW - cancer KW - cytokine KW - hyper-IL-6 KW - oncolysis KW - chemotherapy Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-75224 ER - TY - JOUR A1 - Hailer, Amelie A1 - Grunewald, Thomas G. P. A1 - Orth, Martin A1 - Reiss, Cora A1 - Kneitz, Burkhard A1 - Spahn, Martin A1 - Butt, Elke T1 - Loss of tumor suppressor mir-203 mediates overexpression of LIM and SH3 Protein 1 (LASP1) in high-risk prostate cancer thereby increasing cell proliferation and migration JF - Oncotarget N2 - Several studies have linked overexpression of the LIM and SH3 domain protein 1 (LASP1) to progression of breast, colon, liver, and bladder cancer. However, its expression pattern and role in human prostate cancer (PCa) remained largely undefined. Analysis of published microarray data revealed a significant overexpression of LASP1 in PCa metastases compared to parental primary tumors and normal prostate epithelial cells. Subsequent gene-set enrichment analysis comparing LASP1-high and -low PCa identified an association of LASP1 with genes involved in locomotory behavior and chemokine signaling. These bioinformatic predictions were confirmed in vitro as the inducible short hairpin RNA-mediated LASP1 knockdown impaired migration and proliferation in LNCaP prostate cancer cells. By immunohistochemical staining and semi-quantitative image analysis of whole tissue sections we found an enhanced expression of LASP1 in primary PCa and lymph node metastases over benign prostatic hyperplasia. Strong cytosolic and nuclear LASP1 immunoreactivity correlated with PSA progression. Conversely, qRT-PCR analyses for mir-203, which is a known translational suppressor of LASP1 in matched RNA samples revealed an inverse correlation of LASP1 protein and mir-203 expression. Collectively, our results suggest that loss of mir-203 expression and thus uncontrolled LASP1 overexpression might drive progression of PCa. KW - mir-203 KW - PSA KW - LNCaP KW - LASP1 KW - prostate cancer Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120540 SN - 1949-2553 VL - 5 IS - 12 ER - TY - THES A1 - Reiß, Cora T1 - Einfluss von Defekten des Mismatch Reparatur Proteins MLH1 (Mut L Homolog 1) auf Fertilität und Tumorgenese im Mausmodell T1 - Impact of defects of the mismatch repair protein MLH1 (Mut L Homolog 1) on fertility and tumogenesis in mice N2 - Mutationen im humanen DNA Mismatch-Reparatur (MMR) Gens Mlh1 sind mit dem erblichen, nicht-polypösen Kolonkarzinom (Lynch Syndrom, HNPCC) und einem signifikanten Anteil sporadischer kolorektaler Tumore assoziiert. Zudem konnten MMR Defekte in sporadischen und erblichen Lymphom Erkrankungen beschrieben werden. In Zellen resultiert die Inaktivierung des Mlh1 Gens in der Akkumulation von somatischen Mutationen im Genom und einer erhöhten Resistenz gegenüber den genotoxischen Effekten einer Vielzahl von DNA schädigenden Agenzien. Mäuse, die ein Null Allel für das MMR Gen Mlh1 tragen zeigen einen starken Tumorprädispositions Phänotyp. Sie entwickeln vorrangig B- und T-Zell Lymphome und mit geringerer Haufigkeit gastrointestinale Tumore. Zusätzlich sind Mlh1-/- Mäuse durch einen meiotischen Phänotyp charakterisiert, der zu Sterilitäten in beiden Geschlechtern führt. Um die Effekte von Mlh1 missense Mutationen auf die Tumoranfälligkeit zu untersuchen, erzeugten wir eine Mauslinie, die die häufig in HNPCC Patienten beschriebene MLH1G67R Mutation tragen, die in einer der ATP Bindungs-Domänen von MLH1 lokalisiert ist. Auch wenn die MLH1G67R Mutation in homozygot mutanten Mäusen in einer DNA Reparatur Defizienz resultierte hatte sie keinen Effekt auf die MMR vermittelte zelluläre Antwort auf DNA Schäden. Hierzu gehörte die apoptotische Antwort von Epithelzellen der intestinalen Mucosa auf Cisplatin, die in Mlh1-/- Mäusen defektiv jedoch in Mlh1G67R/G67R Mäusen normal ausfiel. Mlh1G67R/G67R mutante Mäuse zeigten wie Mlh1-/- Tiere einen starken Tumorprädispositions Phänotyp. Sie entwickelten jedoch im Vergleich zu Mlh1-/- Tieren signifikant weniger gastrointestinale Tumore, was darauf hinweist, dass Mlh1 missense Mutationen die Tumor supprimierende MMR Funktion in einer Gewebs-spezifischen Weise beeinflussen können. Darüber hinaus sind Mlh1G67R/G67R Mäuse, aufgrund der fehlenden Bindungsfähigkeit des MLH1G67R Proteins an die meiotischen Chromosomen im Pachytän Stadium, steril. Dies zeigt, dass die ATPase Aktivität von MLH1 für die Fertilität in Säugern essentiell ist. Diese Untersuchungen belegen, dass die Mlh1G67R Mutation die biologischen MLH1 Funktionen differentiell mit einem eindeutigen Phänotyp beeinflusst. Um die Rolle von MLH1 für die Lymphomagenese detaillierter untersuchen zu können, generierten wir ein neues Mausmodell mit einem konditionellen Mlh1 Allel (Mlh1flox/flox). Das Einkreuzen von transgenen EIIa-Cre Mausen in die Mlh1flox/flox Mauslinie führte zur konstitutiven Inaktivierung von MLH1. Die resultierende Mlh1Δex4/Δex4 Mauslinie zeichnete sich durch MMR Defizienz und einen zu Mlh1-/- Tieren vergleichbaren Tumorprädispositions Phänotyp aus. Zur T-Zell spezifischen MMR Inaktivierung kombinierten wir das Mlh1flox/flox Allel mit dem Lck-Cre Transgen. In den resultierenden Mlh1TΔex4/TΔex4 Mäusen ist die MLH1 Inaktivierung auf doppelt positive und einzel positive Thymozyten und naïve periphere TZellen beschränkt. Die Entwicklung von T-Zell Lymphomen in Mlh1TΔex4/TΔex4 Mäusen ist im Vergleich zu Mlh1-/- Mäusen signifikant reduziert, was eine wichtige, Lymphom supprimierende MMR Funktion in frühen Stadien der T-Zell Entwicklung oder in lymphoiden Vorläuferzellen impliziert. N2 - Mutations in the human DNA mismatch repair (MMR) gene Mlh1 are associated with hereditary nonpolyposis colorectal cancer (Lynch syndrome, HNPCC) and a significant proportion of sporadic colorectal cancer. Furthermore, MMR defects have also been observed in sporadic and hereditary lymphoid malignancies. In cells the inactivation of MLH1 results in the accumulation of somatic mutations in the genome and an increased resistance to the genotoxic effects of a variety of DNA damaging agents. Mice carrying a null allele for the MMR gene Mlh1 show a strong tumor predisposition phenotype. They are preferentially prone to the development of lymphomas of B- and T-cell origin and to a lesser extent gastrointestinal tumors. Additionally Mlh1-/- mice are characterized by a meiotic phenotype leading to male and female sterility. To study the effect of Mlh1 missense mutations on cancer susceptibility, we generated a mouse line carrying the recurrent MLH1G67R mutation that is located in one of the ATP-binding domains of MLH1. Although the MLH1G67R mutation resulted in DNA repair deficiency in homozygous mutant mice, it did not affect the MMR-mediated cellular response to DNA damage, including the apoptotic response of epithelial cells in the intestinal mucosa to cisplatin, which was defective in Mlh1-/- mice but remained normal in Mlh1G67R/G67R mice. Similar to Mlh1-/- mice, Mlh1G67R/G67R mutant mice displayed a strong cancer predisposition phenotype. However, in contrast to Mlh1-/- mice, Mlh1G67R/G67R mutant mice developed significantly fewer intestinal tumors, indicating that Mlh1 missense mutations can affect MMR tumor suppressor functions in a tissue-specific manner. In addition, Mlh1G67R/G67R mice were sterile because of the inability of the mutant Mlh1G67R protein to interact with meiotic chromosomes at pachynema, demonstrating that the ATPase activity of MLH1 is essential for fertility in mammals. These studies demonstrate that the Mlh1G67R mutation differentially affects the biological functions associated with MLH1 with distinct phenotypic effects. To study the role of MLH1 for lymphomagenesis in more detail, we generated a new mouse model carrying a conditional Mlh1 allele (Mlh1flox/flox). Mating of these mice with EIIa-Cre recombinase transgenic mice allowed the constitutive inactivation of MLH1 and the resulting Mlh1Δex4/Δex4 mouse line displays complete MMR deficiency and a cancer predisposition phenotype similar to Mlh1-/- mice. For T-cell specific MMR inactivation we combined the Mlh1flox/flox allele with the Lck-Cre Transgene. In the resulting Mlh1TΔex4/TΔex4 mice, MLH1 inactivation is limited to double positive and single positive thymocytes and naïve peripheral Tcells. The development of T-cell lymphomas in Mlh1TΔex4/TΔex4 mice is significantly reduced compared to Mlh1-/- mice implicating that MMR functions either at very early stages during Tcell development or even earlier in lymphoid precursor cells to suppress lymphomagenesis. KW - Colonkrebs KW - Genmutation KW - DNS-Reparatur KW - MLH1 KW - HNPCC KW - Mutation KW - Mausmodell KW - Tumor KW - MLH1 KW - HNPCC KW - mutation KW - mousemodell Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-53626 ER - TY - JOUR A1 - Ardelt, Peter U. A1 - Ebbing, Jan A1 - Adams, Fabian A1 - Reiss, Cora A1 - Arap, Wadih A1 - Pasqualini, Renata A1 - Bachmann, Alexander A1 - Wetterauer, Ulrich A1 - Riedmiller, Hubertus A1 - Kneitz, Burkard T1 - An anti-ubiquitin antibody response in transitional cell carcinoma of the urinary bladder JF - PLoS ONE N2 - Background To use combinatorial epitope mapping ("fingerprinting") of the antibody response to identify targets of the humoral immune response in patients with transitional cell carcinoma (TCC) of the bladder. Methods A combinatorial random peptide library was screened on the circulating pool of immunoglobulins purified from an index patient with a high risk TCC (pTa high grade plus carcinoma in situ) to identify corresponding target antigens. A patient cohort was investigated for antibody titers against ubiquitin. Results We selected, isolated, and validated an immunogenic peptide motif from ubiquitin as a dominant epitope of the humoral response. Patients with TCC had significantly higher antibody titers against ubiquitin than healthy donors (p<0.007), prostate cancer patients (p<0.0007), and all patients without TCC taken together (p<0.0001). Titers from superficial tumors were not significantly different from muscle invasive tumors (p = 0.0929). For antibody response against ubiquitin, sensitivity for detection of TCC was 0.44, specificity 0.96, positive predictive value 0.96 and negative predictive value 0.41. No significant titer changes were observed during the standard BCG induction immunotherapy. Conclusions This is the first report to demonstrate an anti-ubiquitin antibody response in patients with TCC. Although sensitivity of antibody production was low, a high specificity and positive predictive value make ubiquitin an interesting candidate for further diagnostic and possibly immune modulating studies. KW - Bacillus-Calmette-Guerin KW - immune response KW - ubiquitin KW - protein biomarkers KW - system bcg KW - tumor cells KW - immunotherapy KW - cancer surveillance Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143711 VL - 10 IS - 3 ER - TY - JOUR A1 - Gambaryan, Stepan A1 - Subramanian, Hariharan A1 - Kehrer, Linda A1 - Mindukshev, Igor A1 - Sudnitsyna, Julia A1 - Reiss, Cora A1 - Rukoyatkina, Natalia A1 - Friebe, Andreas A1 - Sharina, Iraida A1 - Martin, Emil A1 - Walter, Ulrich T1 - Erythrocytes do not activate purified and platelet soluble guanylate cyclases even in conditions favourable for NO synthesis JF - Cell Communication and Signaling N2 - Background Direct interaction between Red blood cells (RBCs) and platelets is known for a long time. The bleeding time is prolonged in anemic patients independent of their platelet count and could be corrected by transfusion of RBCs, which indicates that RBCs play an important role in hemostasis and platelet activation. However, in the last few years, opposing mechanisms of platelet inhibition by RBCs derived nitric oxide (NO) were proposed. The aim of our study was to identify whether RBCs could produce NO and activate soluble guanylate cyclase (sGC) in platelets. Methods To test whether RBCs could activate sGC under different conditions (whole blood, under hypoxia, or even loaded with NO), we used our well-established and highly sensitive models of NO-dependent sGC activation in platelets and activation of purified sGC. The activation of sGC was monitored by detecting the phosphorylation of Vasodilator Stimulated Phosphoprotein (VASPS239) by flow cytometry and Western blot. ANOVA followed by Bonferroni’s test and Student’s t-test were used as appropriate. Results We show that in the whole blood, RBCs prevent NO-mediated inhibition of ADP and TRAP6-induced platelet activation. Likewise, coincubation of RBCs with platelets results in strong inhibition of NO-induced sGC activation. Under hypoxic conditions, incubation of RBCs with NO donor leads to Hb-NO formation which inhibits sGC activation in platelets. Similarly, RBCs inhibit activation of purified sGC, even under conditions optimal for RBC-mediated generation of NO from nitrite. Conclusions All our experiments demonstrate that RBCs act as strong NO scavengers and prevent NO-mediated inhibition of activated platelets. In all tested conditions, RBCs were not able to activate platelet or purified sGC. KW - hemoglobin KW - erythrocytes KW - nitric oxide KW - soluble guanylate cyclase KW - platelets Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-161223 VL - 14 IS - 16 ER -