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Both oncogenic and tumor suppressor functions have been described for junction plakoglobin (JUP), also known as γ‐catenin. To clarify the role of JUP in prostate cancer, JUP protein expression was immunohistochemically detected in a tissue microarray containing 11 267 individual prostatectomy specimens. Considering all patients, high JUP expression was associated with adverse tumor stage (P = 0.0002), high Gleason grade (P < 0.0001), and lymph node metastases (P = 0.011). These associations were driven mainly by the subset without TMPRSS2:ERG fusion, in which high JUP expression was an independent predictor of poor prognosis (multivariate analyses, P = 0.0054) and early biochemical recurrence (P = 0.0003). High JUP expression was further linked to strong androgen receptor expression (P < 0.0001), high cell proliferation, and PTEN and FOXP1 deletion (P < 0.0001). In the ERG‐negative subset, high JUP expression was additionally linked to MAP3K7 (P = 0.0007) and CHD1 deletion (P = 0.0021). Contrasting the overall prognostic effect of JUP, low JUP expression indicated poor prognosis in the fraction of CHD1‐deleted patients (P = 0.039). In this subset, the association of high JUP and high cell proliferation was specifically absent. In conclusion, the controversial biological roles of JUP are reflected by antagonistic prognostic effects in distinct prostate cancer patient subsets.  相似文献   
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Background: Following pig to primate kidney transplantation, endothelial cell activation and xenogenic activation of the coagulation (XAC) system of the recipient eventually leading to organ dysfunction and disseminated intravascular coagulation (DIC) can be observed (1). In this study we examined the effect of a TNF‐Receptor‐Fusionprotein (TNF‐RFP) on XAC and endothelial cell activation utilizing an appropriate ex‐vivo perfusion system. Methods: Using an ex‐vivo perfusion circuit based on C1‐Inhibitor (C1‐Inh) and low dose heparin administration, we have analysed XAC following contact of human blood with porcine endothelium. Porcine kidneys were recovered following in situ cold perfusion with HTK organ preservation solution and were immediately connected to a perfusion circuit utilizing freshly drawn pooled porcine or human AB blood. The experiments were performed in three individual groups: autologous perfusion (n = 5), xenogenic perfusion without any further pharmacological intervention (n = 10) or with addition of TNF‐RFP (n = 5). After perfusion tissue samples were obtained for QPCR and immunohistological analyses. Endothelial cell activation was assessed by measuring the expression levels of E‐Selectin, ICAM‐1 and VCAM‐1 in QPCR. Results: Kidney survival during organ perfusion with human blood, CI‐Inh, heparin but without any further pharmacological intervention was 126 ± 78 min. XAC was observed with significantly elevated concentrations of d‐Dimer, thrombin antithrombin complex (TAT), resulting in formation of multiple microthrombi. Endothelial cell activation was pronounced, as shown by increased expression of E‐Selectin and VCAM‐1. In contrast, pharmacological intervention with TNF‐RFP reduced the consumption of antithrombin and fibrinogen and prolonged organ survival to 240 min (±0). Additionally, formation of microtrombi was reduced compared to the xenogenic control without pharmacological intervention. Remarkably, also endothelial cell activation was significantly reduced in the TNF‐RFP group. Conclusions: We conclude that TNF‐RFP can interfere with XAC and is able to suppress endothelial cell activation in this ex vivo perfusion model, thus representing a potential candidate as an adjuvant immunosuppressive drug. Reference: 1. BÜhler L, Basker M, Alwayn IPet al. Coagulation and thrombotic disorders associated with pig organ and hematopoietic cell transplantation in nonhuman primates. Transplantation 2000; 9: 1323–1331.  相似文献   
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Journal of Neurology - To approach the clinical value of MRI with vessel wall imaging (VWI) in patients with central nervous system vasculitis (CNSV), we analyzed patterns of VWI findings both at...  相似文献   
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