Quantitative changes of nicotinic receptors in the hippocampus of dystrophin-deficient mice

Lack of dystrophin in Duchenne muscle dystrophy (DMD) and in the mutant mdx mouse results in progressive muscle degeneration, structural changes at the neuromuscular junction, and destabilization of the nicotinic acetylcholine receptors (nAChRs). One-third of DMD patients also present non-progressive cognitive impairments. Considering the role of the cholinergic system in cognitive functions, the number of nAChR binding sites and the mRNA levels of alpha 4, beta 2, and alpha 7 subunits were determined in brain regions normally enriched in dystrophin (cortex, hippocampus and cerebellum) of mdx mice using specific ligands and reverse-transcription polymerase chain reaction assays, respectively. Membrane preparations of these brain regions were obtained from male control and mdx mice at 4 and 12 months of age. the number of [H-3]-cytisine (alpha 4 beta 2) and [I-125]-alpha-bungarotoxin ([I-125]-alpha BGT, alpha 7) binding sites in the cortex and cerebellum was not altered with age or among age-matched control and mdx mice. A significant reduction in [H-3]-cytisine (48%) and [I-125]-alpha BGT (37%) binding sites was detected in the hippocampus of mdx mice at 12 months of age. When compared with the age-matched control groups, the mdx mice did not have significantly altered [H-3]-cytisine binding in the hippocampus, but [I-125]-alpha BGT binding in the same brain region was 52% higher at 4 months and 20% lower at 12 months. mRNA transcripts for the nAChR alpha 4, beta 2, and alpha 7 subunits were not significantly altered in the same brain regions of all animal groups. These results suggest a potential alteration of the nicotinic cholinergic function in the hippocampus of dystrophin-deficient mice, which might contribute to the impairments in cognitive functions, such as learning and memory, that have been reported in the dystrophic murine model and DMD patients. (C) 2012 Elsevier B.V. All rights reserved.Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)Universidade Federal de São Paulo, Escola Paulista Med, Sect Nat Prod, Dept Pharmacol, São Paulo, BrazilUniversidade Federal de São Paulo, Escola Paulista Med, Sect Expt Endocrinol, Dept Pharmacol, São Paulo, BrazilUniv Fed Santa Catarina, Dept Pharmacol, Neuropharmacol Lab, Florianopolis, SC, BrazilAmazon Biotechnol Ctr, Lab Pharmacol & Toxicol, Manaus, AM, BrazilUniversidade Federal de São Paulo, Escola Paulista Med, Sect Nat Prod, Dept Pharmacol, São Paulo, BrazilUniversidade Federal de São Paulo, Escola Paulista Med, Sect Expt Endocrinol, Dept Pharmacol, São Paulo, BrazilWeb of Scienc

Social inequalities in the prevalence of self-reported chronic non-communicable diseases in Brazil: national health survey 2013

Considering the high socioeconomic inequalities in Brazil related to occurrence of morbidity and premature mortality, the objective of this study was to analyze inequalities in self-reported prevalence of Non-Communicable Diseases (NCD) and in the physical limitations caused by these diseases, among the Brazilian adult population, according to sociodemographic variables. This was a population-based cross-sectional study that analyzed information on 60,202 individuals who formed a representative sample of Brazilian adults interviewed for the National Health Survey 2013. Disparities by schooling levels and possession of private health insurance were assessed by calculating the prevalence (P) and prevalence ratio (PR) of each of the 13 NCDs and any associated limitations, while controlling for other socioeconomic and demographic variables. 45 % of the Brazilian adult population reported having at least one NCD. The prevalence ratio was greater among women (1.24 CI 1.21-1.28), individuals over 55 years of age, individuals with low schooling levels (illiterate and incomplete elementary education) (1.08 CI 1.02-1.14) and people living in the Southeast (1.10 CI 1.04-1.16), South (1.26 CI 1.19-1.34) and Central-West (1.11 CI 1.05-1.18) regions of the country. Diseases such as diabetes (1.42 CI 1.13-1.47), hypertension (1.17 CI 1.06-1.28), stroke (2.52 CI 1.74-3.66), arthritis (1.4 CI 1.11-1.77), spinal problems (1.39 CI .1.25-1.56), and chronic renal failure (1.65 CI 1.10.2.46), were more prevalent among adults with low education. For most NCDs, greater reports of limitations were associated with lower schooling levels and lack of private health insurance. Populations with lower schooling levels and lack of private health insurance present higher prevalence of various NCD and greater degrees of limitation due to these diseases. Results reveal the extent of social inequalities that persist with regard to occurrence and the impact of NCDs in Brazil.15153CONSELHO NACIONAL DE DESENVOLVIMENTO CIENTÍFICO E TECNOLÓGICO - CNPQ307865/2014-

Intersubunit Interactions at Putative Sites of Ethanol Action in the M3 and M4 Domains of the NMDA Receptor GluN1 and GluN2B Subunits

Background and Purpose: The N-methyl-D-aspartate (NMDA) receptor is an important target of alcohol action in the brain. Recent studies in this laboratory have demonstrated that alcohol-sensitive positions in the intersubunit interfaces of the M3 and M4 domains of GluN1 and GluN2A subunits interact with respect to ethanol sensitivity and receptor kinetics, and that alcohol-sensitive positions in the M domains of GluN2A and GluN2B subunits differ. In this study we tested for interactions among alcohol-sensitive positions at the M domain intersubunit interfaces in GluN1/GluN2B NMDA receptors. Experimental Approach: We used whole-cell patch-clamp recording in tsA201 cells expressing tryptophan substitution mutants at ethanol-sensitive positions in the GluN1 and GluN2B NMDA receptor subunits to test for interactions among positions. Key Results: Six pairs of positions in GluN1/GluN2B significantly interacted to regulate ethanol inhibition: Gly638/Met824, Gly638/Leu825, Phe639/Leu825, Phe639/Gly826, Met818/Phe637 and Val820/Phe637. Tryptophan substitution at Met824 or Leu825 in GluN2B did not alter ethanol sensitivity but interacted with positions in the GluN1 M3 domain to regulate ethanol action, whereas tryptophan substitution at Gly638, which is the cognate of an ethanol-sensitive position in GluN2A, did not alter ethanol sensitivity or interact with positions in GluN1. Two and three pairs of positions interacted to regulate glutamate steady-state and peak current EC50, respectively, and one pair interacted with respect to macroscopic desensitization. Conclusions: Despite highly-conserved M domain sequences and similar ethanol sensitivity in the GluN2A and GluN2B subunits, the manner in which these subunits interact with the GluN1 subunit to regulate ethanol sensitivity and receptor kinetics differs

Consensus statement on natural orifice transluminal endoscopic surgery and single-incision laparoscopic surgery: heralding a new era in urology?

[Excerpt] For decades, urologists have implemented technologies that provide effective treatment while limiting morbidity. In many instances, this has been achieved by operating via natural body openings (eg, cystoscopy, transurethral resection, and ureteroscopy) [1,2]. Urologists have also pioneered novel techniques to address clinical situations where access through natural body openings was impossible, such as percutaneous stone surgery, laparoscopy, and robotics [3–5].[...

Convergent evidences from human and animal studies implicate angiotensin I-converting enzyme activity in cognitive performance in schizophrenia

In schizophrenia (SCZ), higher angiotensin I-converting enzyme (ACE) levels have been reported in patient's blood and cerebrospinal fluid (CSF). Hereby, we propose to explore whether the ACE activity levels are associated to cognitive performance in SCZ. Seventy-two patients with SCZ or schizoaffective disorder diagnosis, and 69 healthy controls (HCs) underwent a cognitive battery with parallel collection of peripheral blood samples to measure ACE activity. Significant higher ACE activity levels were confirmed in the plasma of SCZ patients compared with HCs (Student's t=−5.216; P<0.001). ACE activity significantly correlated to Hopkins delayed recall measures (r=−0.247; P=0.004) and Hopkins total (r=−0.214; P=0.012). Subjects grouped as high ACE activity (above average) had worse performance compared with low ACE activity level group for Hopkins delayed recall measure, even after correction for clinical condition, age, gender and years of education (P=0.029). The adjusted R squared for this final model was 0.343. This result was evident only comparing extreme groups for ACE activity, when splitting the sample in three groups with similar number of subjects. To clarify this finding, we performed an evaluation of the cognitive performance of transgenic mice with three copies of ACE gene in novel object recognition (NOR) test, which showed that such animals presented impairment in NOR (P<0.05) compared with two copies of wild-type animals. The results observed in SCZ patients and animal model suggest both the association of ACE to cognitive deficits in SCZ. This finding may support the evaluation of novel treatment protocols and/or of innovative drugs for specific intervention of cognitive deficits in SCZ envisioning concomitant ACE activity and behavior evaluations

Kinetic characterization of gyroxin, a serine protease from Crotalus durissus terrificus venom

This work describes for the first time the characterization of the enzymatic features of gyroxin, a serine protease from Crotalus durissus terrificus venom, capable to induce barrel rotation syndrome in rodents. Measuring the hydrolysis of the substrate ZFR-MCA, the optimal pH for proteolytic cleavage of gyroxin was found to be at pH 8.4. Increases in the hydrolytic activity were observed at temperatures from 25 degrees C to 45 degrees C, and increases of NaCl concentration up to 1 M led to activity decreases. the preference of gyroxin for Arg residues at the substrate P1 position was also demonstrated. Taken together, this work describes the characterization of substrate specificity of gyroxin, as well as the effects of salt and pH on its enzymatic activity. (C) 2012 Elsevier Masson SAS. All rights reserved.Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)Universidade Federal de São Paulo, Dept Farmacol, BR-04044020 São Paulo, BrazilUniversidade Federal de São Paulo, Dept Biofis, BR-04044020 São Paulo, BrazilInst Ciencias Mar UFC, BR-60165081 Fortaleza, Ceara, BrazilUniv Estado Amazonas, Escola Super Ciencias Saude INCT, BR-69065001 Manaus, Amazonas, BrazilUniversidade Federal de São Paulo, Dept Farmacol, BR-04044020 São Paulo, BrazilUniversidade Federal de São Paulo, Dept Biofis, BR-04044020 São Paulo, BrazilWeb of Scienc

Different Sites of Alcohol Action in the NMDA Receptor GluN2A and GluN2B Subunits

The NMDA receptor is a major target of alcohol action in the CNS, and recent behavioral and cellular studies have pointed to the importance of the GluN2B subunit in alcohol action. We and others have previously characterized four amino acid positions in the third and fourth membrane-associated (M) domains of the NMDA receptor GluN2A subunit that influence both ion channel gating and alcohol sensitivity. In this study, we found that substitution mutations at two of the four corresponding positions in the GluN2B subunit, F637 and G826, influence ethanol sensitivity and ion channel gating. Because position 826 contains a glycine residue in the native protein, we focused our attention on GluN2B(F637). Substitution mutations at GluN2B(F637) significantly altered ethanol IC50 values, glutamate EC50 values for peak (Ip) and steady-state (Iss) current, and steady-state to peak current ratios (Iss:Ip). Changes in apparent glutamate affinity were not due to agonist trapping in desensitized states, as glutamate Iss EC50 values were not correlated with Iss:Ip values. Ethanol sensitivity was correlated with values of both Ip and Iss glutamate EC50, but not with Iss:Ip. Values of ethanol IC50, glutamate EC50, and Iss:Ip for mutants at GluN2B(F637) were highly correlated with the corresponding values for mutants at GluN2A(F636), consistent with similar functional roles of this position in both subunits. These results demonstrate that GluN2B(Phe637) regulates ethanol action and ion channel function of NMDA receptors. However, despite highly conserved M domain sequences, ethanol\u27s actions on GluN2A and GluN2B subunits differ

Expression of immunohistochemical biomarkers in equine melanocytic neoplasms using tissue microarray

O objetivo deste estudo foi verificar o comportamento morfológico e a expressão das proteínas S-100, Melan-A, HMB-45, Ki-67, PCNA e p53, em 25 neoplasias melanocíticas de equinos. Informações clínicas (gênero, raça, pelagem, idade e localização da lesão) e morfológicas (características celulares, pigmentares, nucleares, de nucléolo, de melanófagos, presença de invasão e necrose) dos animais foram coletadas. Para a expressão das proteínas por imunoistoquímica foi confeccionado um bloco de microarranjo de tecidos das amostras teciduais, juntamente com os controles positivos das reações. A avaliação da expressão das proteínas S100, HMB-45 e Melan-A foi baseada em um escore, e a das proteínas Ki-67, PCNA e p53 foi feita por contagem de células. Animais SRD (16/25, 64%), de raça Lusitana (6/25, 24%), Árabe (2/25, 8%) e Sueca (1/25, 4%) fizeram parte deste estudo, todos tordilhos e a maioria machos (18/25, 72%). A idade dos animais variou de 4 a 24 anos (média de 13 anos). A região perianal (13/25, 52%) foi a que mais apresentou neoplasias. Na análise morfológica houve predomínio de neoplasias com celularidade moderada (52%) e intensa (40%), distribuição difusa e em feixes (52%), ausência de figuras de mitose (96,0%) e predomínio de células epitelióides e fusiformes no mesmo tumor (80%). A atipia nuclear era discreta (48%) e moderada (44%), com núcleos de formato arredondado e alongado em um mesmo tumor (76%) e cromatina dispersa (60%). Os nucléolos eram múltiplos e, em sua maioria, proeminentes (88%). Observou-se predomínio de células tumorais de pigmentação intensa (68%), distribuição difusa e localização em derme (100%). A maioria dos casos apresentou alta celularidade de macrógafos (64%) e distribuição difusa (96%). Quanto à expressão de proteínas para melanócitos por imunoistoquímica, 44% dos casos apresentaram expressão moderada a forte de S100, 56% apresentaram expressão fraca de HMB-45 e 64% apresentaram expressão negativa de Melan-A. Houve positividade de 72% dos casos para pelo menos dois dos anticorpos citados acima. Os anticorpos de proliferação celular Ki-67 e PCNA tiveram média de acima. Os anticorpos de proliferação celular Ki-67 e PCNA tiveram média de positividade de 0,0005% e 15,7%, respectivamente. A análise da expressão de p53 teve média de 6,1% de positividade. Houve associação estatisticamente positiva entre a celularidade dos macrófagos com S100 e com p53. Em conclusão: 1. os dados clínicos obtidos reproduzem o comportamento biológico das neoplasias melanocíticas em equinos, exceto pela idade dos animais; 2. as neoplasias equinas se assemelham a nevos azuis celulares em humanos e melanocitomas em cães; 3. o microarranjo de tecidos mostrou-se uma maneira econômica, rápida e com menos variáveis técnicas; 4. a utilização de um painel de anticorpos de melanócitos é pertinente na diferenciação entre tumores melanocíticos e não melanocíticos, reproduzindo o painel diagnóstico utilizado em literatura humana e canina; 5. o índice de proliferação celular encontrado sugere que os dois anticorpos (Ki-67 e PCNA) podem ser usados na contagem de células em atividade mitótica e 6. a proteína p53 tem maior relação com a parada do ciclo celular que a observada em outros estudos em equinos, podendo indicar um comportamento biológico diferente do apresentado em cães e humanos.The aim of this study was to evaluate the morphological behavior, and expression of the following proteins: S-100, Melan-A, HMB-45, Ki-67, PCNA and p53, in 25 equine melanocytic neoplasms. Clinical (gender, breed, coat color, age and lesions location) and morphological (cellular, pigment, nuclear, nucleoli, melanophages, invasion and necrosis) data were collected. A tissue microarray block, embedded in paraffin, with equine tissue samples and positive controls, was elaborated for protein expression through immunohistochemistry. The evaluation of S100, HMB-45 and Melan-A was based on a score, and for Ki-67, PCNA and p53 it was based on cellular count. Breeds were: Mixed breed (16/25, 64%), Lusitano (6/25, 24%), Arab (2/25, 8%) and Swedich (1/25, 4%). All animals were gray and the majority males (18/25, 72%). Age varied from 4 to 24 years old (mean=13 years). The perianal region (13/25, 52%) was the most common location. Morphological analysis have shown neoplasms with predominantly moderate (52%) and intense (40%) cellularity, diffuse and fascicles distribution (52%), no mitoses figures (96%) and predominance of epithelioid and spindle cells in the same tumor (80%). There was discrete (48%) and moderate (44%) nuclear atypia, round and elongated nucleus in the same tumor (76%), and disperse chromatin (60%). Nucleoli were multiple and prominent in the majority of cases (88%). Tumor cells with diffuse and intense pigmentation, with dermal location (100%) were predominant. High cellularity of macrophages (64%) with diffuse distribution (96%) was mostly seen. The protein expression for melanocytes have shown 44% of moderate to strong expression for S100 protein, 56% of weak expression for HMB-45 protein and 64% of negative expression for Melan-A protein. It was found positivity for more than two antibodies in 72% of equine melanocytic neoplasms. The proliferation antibodies Ki-67 and PCNA had mean positivity of 0,0005% and 15,7%, respectively. The p53 expression had mean positivity of 6,1%. Macrophages cellularity was statistically associated with S100 and p53. In conclusion: 1. clinical data obtain reproduce the biological behavior of equine Macrophages celllularity was statistically associated with S100 and p53. In conclusion: 1. clinical data obtain reproduce the biological behavior of equine melanocytic neoplasms, excepting the animals age; 2. equine melanocytic neoplasms assemble to human cellular blue nevi and dogs melanocytoma; 3. the tissue microarray was shown to be an economic, rapid and less variable technique; 4. using a panel for antibodies for melanocytes is relevant to differentiate melanocytic and not melanocytic tumors, reproducing the diagnosis panel used in human and canine literature; 5. the proliferation index found suggests that both antibodies (Ki-67 and PCNA) could be used in mitotic activity cell count; and 6. p53 protein has more relation with cellular cycle stop than in other equine studies, probably indicating a different biological behavior than the presented in humans and dogs