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Esse artigo objetiva fazer um panorama do financiamento da política de assistência social, apresentando as mudanças normativas, o aporte orçamentário e as perspectivas. Como metodologia, acessou-se o levantamento da produção normativa do órgão gestor da política, que pode ser solicitado aos autores, e a análise descritiva dos dados extraídos do Painel de Orçamento Federal, do atual Ministério da Economia1 , que são oriundos do Sistema Integrado de Administração Financeira do Governo Federal (SIAFI), sistema que realiza toda a execução orçamentária e financeira do governo federal. Os resultados apontam para mudanças, com base nas orientações da Política Nacional de Assistência Social (PNAS) e da Norma Operacional Básica (NOBs/SUAS), que propiciaram um novo padrão de financiamento, com adensamento da institucionalidade, maior abrangência territorial e populacional e ampliação do escopo protetivo da política. O trajeto orçamentário foi ascendente, saindo de um patamar de 0,9% do Produto Interno Bruto (PIB), em 2006, para 1,3%, em 2018. As perspectivas, porém, não são nada animadoras, tendo em vista o cenário de congelamento, em termos reais, da despesa primária da União e um fortalecimento da concepção de assistência social como caridade e benemerência.
This article aims to give an overview of the financing of social assistance policy, presenting the normative changes, the budget contribution, and the perspectives. As a methodology, it was accessed the survey of the normative production of the policy management body, which can be requested from the authors, and the descriptive analysis of the data extracted from the Federal Budget Panel of the current Ministry of Economy, which come from the Integrated System of Financial Administration of the Federal Government (SIAFI), system that performs all the budgetary and financial execution of the federal government. The results point to changes, based on the guidelines of the National Social Assistance Policy (PNAS) and the Basic Operational Standard (NOBs / SUAS), which provided a new standard of financing, with a broader institutional and territorial scope and expansion of the policy's protective scope. The budget line went up from 0.9% of gross domestic product (GDP) in 2006 to 1.3% in 2018. The outlook, however, is not encouraging, considering the scenario of freezing the Union's primary expenditure in real terms and strengthening the concept of social assistance as charity and benevolence.
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Serviço Social , Política PúblicaRESUMO
<p><b>OBJECTIVE</b>To explore the role of eukaryotic translation elongation factor 1A1 (eEF1A1) in regulating the invasion and metastasis of hepatocellular carcinoma (HCC) cells and the possible mechanism.</p><p><b>METHODS</b>qRT-PCR and Western blotting were used to detect the mRNA and protein expression of eEF1A1 and NOB1 in different HCC cell lines and normal liver cells. The invasion and migration abilities of HCC cells with eEF1A1 knockdown or overexpression were examined using Transwell chamber assay and RTCA assay, and the changes in NOB1 mRNA and protein expressions in the cells were detected. The effects of increasing NOB1 expression in HCCLM3-sheEF1A1 cells and decreasing NOB1 expression in eEF1A1-overexpressing MHCC97h cells on eEF1A1 expression and cell invasion and migration abilities were analyzed using Western blotting, Transwell chamber assay and RTCA assay.</p><p><b>RESULTS</b>The expressions of eEF1A1 and NOB1 were significantly increased in positive correlation in HCC cells as compared with normal hepatocytes. Knockdown of eEF1A1 significantly decreased the invasion and migration of HCC cells and reduced the mRNA and protein expression of NOB1 ( < 0.01). Overexpression of eEF1A1 significantly enhanced invasion and migration of HCC cells and increased NOB1 mRNA and protein expressions ( < 0.01). Increasing NOB1 expression in HCCLM3-sheEF1A1 cells led to the restoration of NOB1 expression and cell invasion and migration abilities ( < 0.01), whereas decreasing NOB1 in MHCC97h-eEF1A1 cells resulted in inhibition of NOB1 expression and cell invasion and migration ( < 0.01).</p><p><b>CONCLUSIONS</b>eEF1A1 positively regulates the expression of NOB1 to promote the invasion and migration of HCC cells .</p>
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Objective; To screen the genes may be regulated by NOB1 by using gene microarray technique, and to clarify the regulatory effect of NOB1 on the expression of osteosarcoma cell-related genes. Methods: The U20S cells were treated with lentivirus-mediated RNA interference and to establish the osteosarcoma cells Lv-shN0Bl-U20S. Lv-shCon-U20S group and Lv-shN0Bl-U20S group were set up. The mRNA expressions of those cells were detected using expression pattern analysis. Gene Oncology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) were used to predict the global functions of NOB1, including biological processes, cellular components, molecular functions, and signaling pathways. Results; After NOB1 interference in the U20S cells, there were 792 genes with up-regulated mRNA expression level and 1 059 genes with down-regulated mRNA expression level, with a total variation of 1 851 genes. The GO analysis results showed that from the enrichment degree of cell location entries, the differentially encoded product proteins were mainly distributed on the cell membrane as 56. 9% of the total difference genes, 39. 4% of the totally differential genes distributed in the extracellular region, and 20% of the totally differential genes in the extracellular space; from the enrichment degrees of the molecular function items, the main function of the differentially encoded product proteins was calciu mion binding-related function (22% of the totally differential genes), the second function was transporter activity (9. 2% of the totally differenital genes), and the third function was actin binding activity (8. 7% of the totally differential genes). In terms of the enrichment of biochemical process entries, the main participation process of differentially encoded product proteins was 18. 7% of the totally differential genes of signal transduction, the second involved process was 15. 6% of the totally differential genes produced by multiple organelles, and the third process was the cell adhesion process accounted for 10. 2% of the totally differential genes. The KEGG analysis results showed that their encoding proteins were involved in plasma membrane, calcium ion binding activity and signal transduction. Conclusion; Knockout of NOB1 can affect the expressions of osteosarcoma cell-related genes in an all-round way.
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Abstract Currently, nitrogen has become the main element of water pollution, causing riverine, lacustrine and coastal eutrophication. The continuous contamination of aquifers and the absence of planned water resource utilization, boost its scarcity, and has been the only way in which our societies become aware of the urgent need to process the generated wastewater. The objective of this research was to evaluate the nitrifying capacity of different autochthonous bacterial isolates from soils from nearby sources of domestic wastewater drainage. For this, bacteria were isolated from Pirro River, contaminated with nitrogen of domestic sewage. Nitrifying bacteria were counted by serial dilution and agar plates, and were isolated until obtaining axenic colonies. These were identified by biochemical batteries or genetic sequencing, and the quantification of their nitrifying capacity was obtained by the methods 4500- NH4 + -F and 4500-NO-2-B, all between September 26, 2011 and March 16, 2014. A total of seven strains of nitrifying microorganisms were isolated and purified, including four Streptomyces sp., one Pseudomonas putida, one Sphingomonas sp. and one Aeromonas sp. We found that there were 2.23 x 105 UFC/g of soil of ammonium oxidizing bacteria and 2.2 x 104 CFU/g of soil of nitrite oxidizing bacteria in the samples. The quantification of the nitrifying capacity of the strains by colorimetric methods, determined that the maximum ammonium removal capacity was 0.050 mg N/L/day and 0.903 mg N/L/day of nitrite. The collection of few strains of nitrifying organisms and a low CFU count, can be attributed to the technique used, since this only recovers 1 % of the microorganisms present in a sample, which, however, is acceptable for studies which main purpose is to obtain cultivable microorganisms. Future research should consider removal tests with higher ammonium and nitrite levels, to find the maximum capacity of the isolated microorganisms, and evaluate their potential use in wastewater treatment systems.
Resumen El suelo es la matriz fundamental donde suceden las reacciones químicas y biológicas que permiten el desarrollo de la vida en la tierra, y donde ocurren procesos fundamentales como la mineralización de los elementos y la fijación del nitrógeno. Hoy en día el nitrógeno se ha transformado en uno de los principales elementos contaminantes de los cuerpos de agua, causando consecuencias como la eutrofización de ríos, lago y costas. En los ambientes acuáticos, el nitrógeno puede ser encontrado en forma de amonio N-NH4 +, nitritos N-NO2 -o nitratos N-NO3 -, los cuales pueden ser utilizados por las bacterias nitrificantes amonio y nitrito oxidantes y desnitrificantes para su crecimiento y consecuente remoción. Esta investigación se planteó como objetivo evaluar la capacidad nitrificante de diferentes aislamientos bacterianos autóctonos, aislados de suelos cercanos a fuentes de vertido de aguas residuales de tipo doméstico para su potencial uso en sistemas de tratamiento de aguas residuales. Se realizó el recuento de bacterias nitrificantes por la técnica de dilución seriada y siembra en placas de agar mínimo mineral, su aislamiento por repique en placa hasta obtener colonias axénicas, su identificación por medio de baterías bioquímicas o secuenciación genética y la cuantificación de su capacidad nitrificante por los métodos 4500- NH4 +-F y 4500- NO- 2-B, entre el 26/09/2011 y 16/03/2014; las bacterias fueron aisladas de un punto del río Pirro contaminado con nitrógeno de aguas residuales de tipo doméstico. Se lograron aislar y purificar siete cepas de microorganismos nitrificantes entre las que se encuentran cuatro de Streptomyces sp., una de Pseudomonas putida, una de Sphingomonas sp. y una de Aeromonas sp. Se encontró que existen 2.23 x105 UFC/g de suelo de bacterias amonio oxidantes y 2.2 x104 UFC/g de suelo de las nitrito oxidantes. La cuantificación de la capacidad nitrificante de las cepas por medio de los métodos colorimétricos determinó que la capacidad máxima de remoción de amonio es de 0.050 mg N/L/día y la de nitrito en 0.903 mg N/L/día. La obtención de pocas cepas de organismos nitrificantes y un bajo recuento de UFC se puede atribuir a la técnica empleada, ya que esta solo recupera un 1 % de los microorganismos presentes en una muestras, lo cual sin embargo, es aceptable para estudios que tienen como objetivo la obtención de microorganismos cultivables. Se recomienda realizar ensayos de remoción con niveles de amonio y nitrito más altos para hallar la capacidad máxima de los microorganismos aislados.
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NOB1 is a newly found gene regulating the function of the 26S proteasome, cell cycle and gene transcription. NOB1 contains a zinc ribbon domain and a PIN domain. Recent studies have indicated that the PIN domain is related to gene transcription and the zinc ribbon domain plays an important role in regulating cell cycle. It has also been found that NOB1 is closely associated with development and progression of gastric, esophageal, and ovarian cancer. The paper reviews the role of NOB1 in the development and progression of tumors.
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One factor at a time design and first order exponential model were applied to investigate the effects of the four major factors(temperature,ionic strength,pH and osmo-regulator) in the preservation process of nitrite oxidization bacteria(NOB),and a first order decay kinetics was introduced.The result showed that the anoxic decay rate of nitrifying bacteria reduced from 0.25 to 0.015,the half life was extend to 53d at 4℃,pH7.60,ionic strength 0.035mol/kg.The protecting effect of glycerin showed obviously better than that of other cryoprotectants at 4℃.
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O presente trabalho consiste numa revisão da legislação que instituiu e vem modelando o Sistema Único de Saúde (SUS) no Brasil. Seu principal objetivo á analisar o percurso das politicas de saúde e as mudanças ocorridas nas leis desde a implantação do SUS até os dias atuais. O objeto deste trabalho foi uma análise crítica da legislação, além da experiência pessoal do outor na área de gestão.
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Legislação como Assunto , Política de Saúde , Sistema Único de Saúde , Atenção à Saúde , Diretrizes para o Planejamento em Saúde , Serviços de SaúdeRESUMO
Behcet's disease (BD) has been known to be strongly associated with the human leukocyte antigen (HLA) B51. This B51 association has been confirmed in many different ethnic groups between the Middle East and Japan, and it has been proposed that BD is prevalent in those ethnic groups along the old Silk Route. The hypothesis could be made that B51 molecules are primarily involved in BD development through specific antigen presentation. However, polymorphic analyses of the TNFB gene and Tau-a microsatellite between the HLA-B and TNF genes indicate that the pathogenic gene of BD is not the HLA-B51 gene itself but another gene located around the HLA-B gene. HLA-C genotyping by the PCR-SSP method also suggests that the BD pathogenic gene is not the HLA-C gene itself but other gene located near the HLA-B gene. Recently we sequenced a single contig of 236,822 bp from the MICA gene (58.2 kb centromeric of HLA-B) to 90.8 kb telomeric of HLA-C and identified 8 novel genes designated NOB1-8 (NOB: new organization associated with HLA-B). During the course of the genomic sequence analysis we clarified the genetic structure of the MICA (MHC class I chain-related gene A) gene and found a triplet repeat microsatellite polymorphism of (GCT/AGC)n in the transmebrane (TM) region. Furthermore, the microsatellite allele consisting of 6 repetitions of GCT/AGC (MICA A6 allele) was present at a significantly higher frequency in the BD patient group than in the control group and a significant fraction of B51-negative patients were positive for this MICA A6 allele. These results suggest the possibility of a primary association of BD with MICA rather than HLA-B.
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Humanos , Camundongos , Animais , Síndrome de Behçet/genética , Genótipo , Antígenos HLA-B/genética , Antígenos HLA-C/genética , Antígenos de Histocompatibilidade Classe I/genética , Camundongos Transgênicos , Repetições de Microssatélites , Reação em Cadeia da Polimerase , Polimorfismo GenéticoRESUMO
Objetivo. Describir la prevalencia de maracadores serológicos de los virus de la hepatitis en una población de embarazadas. Material y métodos. Se estudiaron 1 500 sueros de embarazadas en los que se determinaron: anticuerpos IgG contra el virus de la hepatitis A (anti-VHA); anticuerpos IgG contra el antígeno central del virus de la hepatitis B (ant-HB-c), y su antígeno de superficie (AgsHB); así como anticuerpos contra el virus de la hepatitis C (anti-VHC). En los casos positivos al AgsHB se buscaron anticuerpos contra el virus de la hepatitis D (anti-VHD) y el antígeno e del virus de la hepatitis B (AgeHB). Todas las determinaciones se realizaron por la técnica de ELISA. Resultados. El 93.3 por ciento de los sueros estudiados tuvo anti-VHA IgG positivos. La prevalencia del AgsHB fue del 0.26 por ciento y de anti-VHC del 0.53 por ciento. No hubo pacientes con positividad para anti-VHD ni para el AgeHB. Conclusiones. Se encontró una prevalencia del AgsHB superior a la de otros estudios en embarazadas mexicanas. Consideramos que el escrutinio del AgsHB debe formar parte de los exámenes de control prenatal
Objective. To determine the seroprevalence of hepatitis A, B, C and D virus infection among pregnant women attending a perinatal care hospital. Material and methods. A prospective study was carried out to determine the seroprevalence of hepatitis A virus IgG antibodies (anti-HAV), hepatitis B virus markers (anti-HBcAg and HBsAg) and hepatitis C virus antibodies (anti-HCV) in pregnant women. In HBsAg positive cases, HBeAg and hepatitis D virus antibodies (anti-HDV) were investigated. All analyses were performed with the ELISA technique. Results. Of the 1500 pregnant women studied, 93.3% were positive for anti-HAV IgG. The HBsAg seroprevalence was 0.26% and anti-HCV seroprevalence was 0.53%. There were no patients with HBeAg or antiHDV. Conclusions. A higher seroprevalence of HBsAg was found in this study than in other studies of pregnant Mexican women. We propose that HBsAg screening become a routine prenatal test.