Discovery of Quinazoline-Based Fluorescent Probes to α1-Adrenergic Receptors

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Functional differences between wild‐type and mutant‐type BRCA1‐associated protein 1 tumor suppressor against malignant mesothelioma cells

Malignant mesothelioma (MM) shows inactivation of the BRCA1‐associated protein 1 (BAP1) gene. In this study, we found BAP1 mutations in 5 (26%) of the 19 cell lines that we established from Japanese MM patients, and examined functional differences between the WT and mutant BAP1. First, we studied the subcellular localization of BAP1, demonstrating that the WT primarily resides in the nucleus and that the mutant BAP1 is found in the cytoplasm of the cells. Transduction of the WT BAP1 vector into MM cells with homozygous deletion at the BAP1 3′ side resulted in both inhibition of cell proliferation and anchorage‐independent cell growth, whereas BAP1 mutants of a missense or C‐terminal truncated form showed impaired growth inhibitory effects. Next, we studied how BAP1 is involved in MM cell survival after irradiation (IR), which causes DNA damage. After IR, we found that both WT and mutant BAP1 were similarly phosphorylated and phospho‐BAP1 localized mainly in the nucleus. Interestingly, BRCA1 proteins were decreased in the MM cells with BAP1 deletion, and transduction of the mutants as well as WT BAP1 increased BRCA1 proteins, suggesting that BAP1 may promote DNA repair partly through stabilizing BRCA1. Furthermore, using the MM cells with BAP1 deletion, we found that WT BAP1, and even a missense mutant, conferred a higher survival rate after IR compared to the control vector. Our results suggested that, whereas WT BAP1 suppresses MM cell proliferation and restores cell survival after IR damage, some mutant BAP1 may also moderately retain these functions.     

Altered intracellular region of MUC1 and disrupted correlation of polarity‐related molecules in breast cancer subtypes

MUC1 glycoprotein is overexpressed and its intracellular localization altered during breast carcinoma tumorigenesis. The present study aimed to clarify the relationship of cytoplasmic localization of MUC1 with the breast cancer subtype and the correlation of 10 molecules associated with cell polarity in breast cancer subtypes. We immunostained 131 formalin-fixed and paraffin-embedded breast cancer specimens with an anti-MUC1 antibody (MUC1/CORE). For 48 of the 131 tumor specimens, laser-assisted microdissection and real-time quantitative RT-PCR were performed to analyze mRNA levels of MUC1 and 10 molecules, β-catenin, E-cadherin, claudin 3, claudin 4, claudin 7, RhoA, cdc42, Rac1, Par3 and Par6. Localization of MUC1 protein varied among breast cancer subtypes, that is, both the apical domain and cytoplasm in luminal A-like tumors (P < 0.01) and both the cytoplasm and cell membrane in luminal B-like (growth factor receptor 2 [HER2]+) tumors (P < 0.05), and no expression was found in triple negative tumors (P < 0.001). Estrogen receptor (ER)+ breast cancers showed higher MUC1 mRNA levels than ER− breast cancers (P < 0.01). The incidence of mutual correlations of expression levels between two of the 10 molecules (55 combinations) was 54.5% in normal breast tissue and 38.2% in luminal A-like specimens, 16.4% in luminal B-like (HER2+), 3.6% in HER2 and 18.2% in triple negative specimens. In conclusion, each breast cancer subtype has characteristic cytoplasmic localization patterns of MUC1 and different degrees of disrupted correlation of the expression levels between the 10 examined molecules in comparison with normal breast tissue.     

Comparative biodistribution in mice of cyanine dyes loaded in lipid nanoparticles

Two near infrared cyanine dyes, DiD (1,1′-dioctadecyl-3,3,3′,3′-tetramethylindotricarbocyanine perchlorate) and ICG (Indocyanine Green) were loaded in lipid nanoparticles (LNP). DiD-LNP and ICG-LNP presented similar physicochemical characteristics (hydrodynamic diameter, polydispersity, zeta potential), encapsulation efficiency, and colloidal stability when stored in PBS buffer. However, whereas DiD had similar biodistribution than cholesteryl-1-¹⁴C-oleate ([¹⁴C]CHO, a constituent of the nanoparticle used as a reference radiotracer), ICG displayed a different biodistribution pattern, similar to that of the free dye, indicative of its immediate leakage from the nanovector after blood injection. NMR spectroscopy using Proton NOE (Nuclear Overhauser Effect) measurements showed that the localization of the dye in the lipid nanoparticles was slightly different: ICG, more amphiphilic than DiD, was found both inside the lipid core and at particle interface, whereas DiD, more hydrophobic, appeared exclusively located inside the particle core. The ICG release rate from the particles was 7% per 1 month under storage conditions (4 °C, dark, 10% of lipids), whereas no leakage could be detected for DiD. ICG leakage increased considerably in the presence of BSA 40 g/L (45% leakage in 24 h at 100 mg/mL of lipids), because of the high affinity of the fluorophore for plasma proteins. On the contrary, no DiD leakage was observed, until high dilution of the nanoparticles which triggered their dissociation (45% leakage in 24 h at 1 mg/mL of lipids). Altogether, the subtle difference in dye localization into the nanoparticles, the partial dissociation of the LNP in diluted media, and more importantly the high ICG affinity for plasma proteins, accounted for the differences observed in the fluorescence biodistribution after tail vein injection of the dye-loaded nanoparticles.     

P50 Suppression and Its Neural Generators in Antipsychotic-Na?ve First-Episode Schizophrenia Before and After 6 Months of Quetiapine Treatment

Background: Numerous studies have demonstrated sensory gating deficits in schizophrenia. However, only a few longitudinal studies report on the effects of antipsychotic treatment on sensory gating deficits and their results are inconsistent. In the present study, P50 suppression and its neural generators were investigated in antipsychotic-naïve first-episode patients with schizophrenia before and after 6 months of treatment with quetiapine. Methods: Thirty-four antipsychotic-naïve first-episode schizophrenia patients and age and gender matched healthy controls were tested in an auditory sensory gating paradigm at baseline and after 6 months. During this period, the patients were treated with quetiapine, while controls received no treatment. Sixteen patients completed the study. Results: Patients showed significant reduced P50 suppression compared with controls at baseline but not at follow-up. Furthermore, a significant positive correlation between baseline P50 suppression and dose of quetiapine at follow-up was found. P50 suppression in patients receiving above median dosages of quetiapine increased significantly from baseline to follow-up. At baseline, a frontocentral source was significantly more active in patients than in controls at the time of the testing stimulus. Conclusions: The present findings suggest that P50 suppression deficits are already present at an early stage of schizophrenia. Furthermore, particularly those patients with more severe gating deficits appeared to need higher dosages of quetiapine, although their clinical symptoms did not seem to indicate this. Quetiapine treatment significantly improved these gating deficits. Furthermore, a frontocentral source in the brain appeared to be involved in the deficient P50 gating of the patients.     

眼内异物的CT诊断和定位

目的 探讨CT在眼内异物定位中的使用价值。方法 参阅CT横扫序列片将异物按照测量的结果标画在CT眼内异物定位图上。结果 40例可疑眼内异物患者有16例查出为眼内异物或球壁异物(其中6例普通x线不显影)，采用此法定位，迅速、准确地作出了诊断和定位。结论 利用CT诊断和定位眼内异物，简便易行、迅速准确，值得推广。     

Ventral and dorsal visual pathways support auditory motion processing in the blind: evidence from electrical neuroimaging

Blindness induces processes of neural plasticity, resulting in recruitment of the deafferentated visual areas for non‐visual sensory functions. These processes are related to superior abilities of blind compared with sighted individuals for specific auditory and tactile tasks. Recently, an exceptional performance of the blind has been demonstrated for auditory motion perception, with a minimum audible movement angle that was half that of sighted controls (J. Lewald (2013) Neuropsychologia, 51 , 181–186). The present study revealed an electrophysiological correlate of this finding by analysing the so‐called motion‐onset response, a prominent auditory‐evoked potential to the onset of motion. The cN1 component of this response, appearing about 170 ms after motion onset, was two times higher in amplitude for blind compared with matched sighted control subjects. At the time of the cN1, electrical neuroimaging using sLORETA revealed stronger activation in blind than sighted subjects primarily in ventral visual areas (V1v, V2v, VP, V4v) of the right occipital lobe. Activation was also obtained in middle temporal area V5. These findings suggest that blindness results in stronger involvement of both non‐motion areas of the ventral visual stream and motion areas of the dorsal visual stream in processing of auditory motion at the same point in time after motion onset. This argues against the view that visual motion areas, such as area V5, are preferentially recruited for auditory motion analysis in the blind. Rather, cross‐modal reorganization of cortical areas induced by blindness seems to be largely independent of the specific visual functions of the same areas in sighted persons.     

不同分子亚型乳腺癌细胞系中RUNX3蛋白表达及定位研究

目的:检测人类Runt相关转录因子3(RUNX3)在不同分子亚型乳腺癌细胞系中的表达及其亚细胞定位情况,为进一步揭示RUNX3的失活机制和发现新的治疗靶点提供理论依据。方法:在5种乳腺癌细胞(MCF-7、T47D、SKBR-3、MDA-MB-231和BT-549)及正常乳腺上皮细胞(MCF-10A)中,通过Western blot和免疫荧光实验检测RUNX3的蛋白表达和亚细胞定位情况;采用来普霉素B(Leptomycin B)抑制RUNX3的出核,利用CCK-8法检测细胞活力的改变,EdU染色检测细胞增殖情况,Western blot和免疫荧光实验检测RUNX3的蛋白表达和亚细胞定位的改变。结果:与MCF-10A细胞相比,5种乳腺癌细胞系中RUNX3的核定位减少、胞浆定位增多。经Leptomycin B处理后,CCK-8实验结果显示5种乳腺癌细胞的活力明显减弱,EdU染色显示5种乳腺癌细胞增殖能力明显降低,Western blot和免疫荧光实验显示5种乳腺癌细胞胞浆中的RUNX3蛋白表达量明显降低、胞核中的RUNX3蛋白表达量明显增多(P0.05)。结论:不同分子亚型乳腺癌细胞中均存在RUNX3的胞浆转位失活现象,针对性地逆转RUNX3的出核过程可以明显降低肿瘤细胞的活力和增殖能力,可能成为乳腺癌潜在的治疗靶点。