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1.

Fast and cost-effective protocol to produce Paracoccidioides spp. antigens

Fernandes-Beraldo, Karolina Rosa; Freitas-Xavier, Roseli Santos de; Pardini-Vicentini, Adriana.

Biomédica (Bogotá) ; 43(Supl. 1)ago. 2023.

Article in English | LILACS-Express | LILACS | ID: biblio-1533900

ABSTRACT

Introduction. The existing methods for Paracoccidioides spp. antigen production are problematic in terms of standardization, specificity, stability, repeatability, and reproducibility. Objective. To optimize the methodology for Paracoccidioides spp. antigen production and evaluate its applicability in paracoccidioidomycosis immunodiagnosis. Materials and methods. The antigens were obtained from Paracoccidioides lutzii isolates (01, 66, and 8334), Paracoccidioides brasiliensis sensu stricto (113), and Paracoccidioides restripiensis (B-339). These fungi were grown at 36 °C ± 1 °C, on modified Fava-Netto agar, according to Freitas et al. (2018). Paracoccidioides lutzii antigens were obtained after 5, 10, and 20 days of culture, whereas P. brasiliensis and P. restripiensis antigens were obtained after 10 days. Antigens were evaluated in natura, 10 and 20 times concentrated. Antigenic capacity was evaluated using a double immunodiffusion assay against serum samples from patients with paracoccidioidomycosis, histoplasmosis, and aspergillosis, and random blood donors. Results. Cross-reactivity between Paracoccidioides spp. antigens was observed when P. brasiliensis, P. restrepiensis antigens, and P. lutzii antigens were evaluated with the polyclonal antibodies against P. lutzii and P. brasiliensis, respectively. No cross-reactivity was obtained for polyclonal antibodies against Histoplasma capsulatum, Aspergillus fumigatus, and random blood donors. The proposed protocol allowed stable, repeatable, and reproducible genus-specific antigen production at a low cost and in a short cultivation time. Conclusion. The proposed protocol allowed us to obtain genus-specific antigens that can be developed and reproduced in all laboratories in Brazil and South America, where paracoccidioidomycosis is a neglected disease, contributing to an early diagnosis, especially in endemic regions, regardless of the species.

Introducción. Los métodos existentes para la producción de los antígenos de Paracoccidioides spp. son problemáticos en su estandarización, especificidad, estabilidad, repetibilidad y reproducibilidad. Objetivo. Optimizar la metodología para la producción de antígenos de Paracoccidioides spp. y evaluar su aplicabilidad en el inmunodiagnóstico de la paracoccidioidomicosis. Materiales y métodos. Los antígenos se obtuvieron de aislamientos de P. lutzii (01, 66 y 8334), P. brasiliensis sensu stricto (113) y P. restripiensis (B-339). Estos hongos se cultivaron a 36 °C ± 1 °C en agar Fava-Netto modificado, según Freitas et al. (2018). Los antígenos de P. lutzii se obtuvieron a los 5, 10 y 20 días de cultivo y los antígenos de P. brasiliensis y P. restripiensis se obtuvieron a los 10 días. Los antígenos se evaluaron in natura, concentrados 10 y 20 veces. La capacidad antigénica se evaluó mediante un ensayo de inmunodifusión doble con muestras de suero de pacientes con paracoccidioidomicosis, histoplasmosis, aspergilosis y donantes de sangre aleatorios. Resultados. Se observó reacción cruzada con Paracoccidioides spp. cuando se evaluaron los antígenos de P. brasiliensis, P. restrepiensis y P. lutzii frente a los anticuerpos policlonales contra P. lutzii y P. brasiliensis, respectivamente. No hubo reactividad cruzada con los anticuerpos policlonales contra Histoplasma capsulatum y Aspergillus fumigatus, ni contra los donantes de sangre aleatorios. El protocolo propuesto permitió la producción estable, repetible y reproducible de antígenos dirigidos de un género específico (Paracoccidiodes) en un tiempo corto de cultivo y a un menor costo. Conclusión. El protocolo propuesto permitió obtener antígenos específicos de un género, que pueden ser desarrollados y reproducidos en todos los laboratorios de Antígenos de Paracoccidioides spp.: protocolo rápido Brasil y Surámerica donde la paracoccidioidomicosis es una enfermedad endémica y desatendida. Estos antígenos pueden contribuir al diagnóstico precoz de la infección, independientemente de la especie.

2.

Multiparametric assay of screening for the diagnosis of mycoses of interest in Public Health: standardization of methodology / Ensaio multiparamétrico de triagem para diagnóstico de micoses de interesse em Saúde Pública: padronização da metodologia

Kamikawa, Camila Mika; Vicentini, Adriana Pardini.

Rev. Inst. Adolfo Lutz ; 81: e37165, mar.1, 2022. ilus

Article in English | LILACS, CONASS, ColecionaSUS, SES-SP, VETINDEX, SESSP-ACVSES, SESSP-IALPROD, SES-SP, SESSP-IALACERVO | ID: biblio-1393020

ABSTRACT

The standardization and validation of a multiplex assay requires the combination of important parameters such as sensitivity and specificity, acceptable levels of performance, robustness, and reproducibility. We standardized a multiparametric Dot-blot aimed at the serological screening of paracoccidioidomycosis, histoplasmosis, and aspergillosis. A total of 148 serum were evaluated: 10 from healthy subjects, 36 from patients with paracoccidioidomycosis, 62 from patients with histoplasmosis, and 40 from patients with aspergillosis. It was found that the multiparametric Dot-blot showed a high percentage of cross-reactivity. However, when evaluated individually, in the serological screening of histoplasmosis, a good performance was observed when compared to the double immunodiffusion assay, considered the gold standard test, with 100% co-positivity and 83.3% co-negativity. The performance of serological screening for aspergillosis was not satisfactory when compared to double immunodiffusion, showing 71.4% co-positivity and 100% co-negativity. The evaluation of the stability of nitrocellulose membranes showed that membranes sensitized with H. capsulatum antigen remained stable for 90 days and those sensitized with A. fumigatus antigen for 30 days. We conclude that the use of crude antigens was not suitable for the standardization of the multiparametric Dot-blot assay, due to the high cross-reactivity, and that further tests should be performed with purified proteins (AU).

A padronização e validação de um ensaio multiplex requer a combinação de parâmetros importantes, como sensibilidade e especificidade, níveis aceitáveis de desempenho, robustez e reprodutibilidade. Este trabalho padronizou um Dot-blot multiparamétrico visando a triagem sorológica da paracoccidioidomicose, histoplasmose e aspergilose. Foram avaliadas 148 amostras de soro: 10 de indivíduos saudáveis, 36 de pacientes com paracoccidioidomicose, 62 de pacientes com histoplasmose e 40 de pacientes com aspergilose. Verificou-se que o Dot-blot multiparamétrico apresentou elevado percentual de reatividade cruzada. Entretanto, quando avaliado individualmente, na triagem sorológica da histoplasmose observou-se bom desempenho quando comparado ao ensaio de imunodifusão dupla, considerado o teste padrão ouro, com 100% de co-positividade e 83,3% de co-negatividade. O desempenho da triagem sorológica da aspergilose não foi satisfatório quando comparado a imunodifusão dupla, apresentando 71,4% de co-positividade e 100% de co-negatividade. A avaliação da estabilidade das membranas de nitrocelulose mostrou que membranas sensibilizadas com antígeno de H. capsulatum permaneceram estáveis por 90 dias e as sensibilizadas com antígeno de A. fumigatus, por 30 dias. Concluímos que o uso de antígenos brutos não foi adequado para a padronização do ensaio de Dot-blot multiparamétrico, devido ao alto índice de reatividade cruzada, e que novos testes devem ser realizados com proteínas purificadas (AU).

Subject(s)

Paracoccidioidomycosis , Aspergillosis , Reference Standards , Immunologic Tests , Public Health , Methodology as a Subject , Histoplasmosis , Mycoses/diagnosis

3.

Current status and research progress of microfluidic immunochips in medical detection / 中华检验医学杂志

Zhichen ZOU; Keguan SONG; Qiushi SONG; Fengnian ZHAO; Shixin JIN; Hongzhi WANG.

Chinese Journal of Laboratory Medicine ; (12): 87-92, 2022.

Article in Chinese | WPRIM | ID: wpr-934341

ABSTRACT

The traditional-immunological strategies for clinical laboratories often rely on large and expensive instruments and skilled operators, and the measurement time is also long. However, the sensitivity of these strategies is still unsatisfactory. It is urgent to research and develop the point-of-care testing (POCT) featured as a highly sensitive, accurate, and rapid/POCT diagnosis. The Microfluidic chips have multi-advantages that are suitable for the clinical POCT diagnosis: high sensitivity, throughput, and automation. Recently, the Microfluidic-immune chips developed based on the microfluidic technology combined with immune detection have considered not only hotspots in the related research but also benefit to the tumor marker detection, antigen and antibody detection of infectious diseases, autoantibody detection, hormone detection, and other fields. However, there are still many challenges to be overcome during the application of chips, such as more effective microfluidic manipulation, more sensitive collection, and analysis of reaction signals.

4.

Analysis of the spatio-temporal dynamics of incidence, mortality and test rates (rapid and RT-PCR) of COVID-19 in the state of Minas Gerais, Brazil / Análise da dinâmica espaço-temporal da incidência, mortalidade e taxas de testes (rápidos e moleculares) da COVID-19 no estado de Minas Gerais, Brasil / Análisis de la dinámica espacio-temporal de la incidencia, mortalidad y tasas de prueba (rápida e RT-PCR) de COVID-19 en el estado de Minas Gerais, Brasil

Silva-Júnior, Milton José da; Mendonça, Kaio Saramago; Lima, Caio Augusto de; Pires, Priscilla Larissa Silva; Calegari, Tatiany; Oliveira, Stefan Vilges de.

Rev. epidemiol. controle infecç ; 11(1): 32-39, jan.-mar. 2021. ilus

Article in English | LILACS | ID: biblio-1362159

ABSTRACT

Background and Objectives: A novel type of coronavirus, SARS-CoV-2, is responsible for an unprecedented pandemic with profound socioeconomic consequences. Owing to its recent discovery still represents a great unknown to researchers. Thus, this study aims to establish the spatio-temporal associations of the incidence, mortality, and the rate of both rapid and RT-PCR tests in Minas Gerais. Methods: This is a quantitative analysis of secondary data based on a cross-sectional research design. Incidence, mortality, date of the first notification of COVID-19 and number of rapid and RT-PCR tests were obtained from the sources: "GAL", "e-SUS VE" and "SES-MG". Pearson coefficient for correlation was calculated to establish the level of association between the relevant data. Descriptive statistical procedures were used to provide a comprehensive understanding of the distribution of incidence, mortality and test rates in the territory. Results: Positive correlations were found between the rate of rapid tests and incidence; rate of RT-PCR tests and incidence/mortality. At the municipal level, incidence, mortality, rate of rapid tests and RT-PCR revealed a negative correlation with days elapsed since the First Notified Case. The same effect occurs at the level of health macro-regions. Conclusion: The heterogeneity of the incidence and mortality of COVID-19 in the territory of Minas Gerais, as well as the rate of tests may be caused, in part, due to the different dates of introduction of the virus in the municipalities/macro-regions. It is speculated that this phenomenon occurs due to the dynamics of regional and inter-regional flows of people.(AU)

Justificativa e Objetivos: Um novo tipo de coronavírus, SARS-CoV-2, é responsável por uma pandemia sem precedentes com profundas consequências socioeconômicas. Devido à sua recente descoberta, o vírus surgido na cidade chinesa de Wuhan, em dezembro de 2019, ainda lança grandes incógnitas. Este estudo objetiva estabelecer as associações espaço-temporais da incidência; mortalidade; e taxas de testes rápidos e RT-PCR em Minas Gerais. Métodos: Trata-se de uma análise quantitativa de dados secundários a partir de um desenho de pesquisa transversal. Incidência, mortalidade, data da(s) primeira(s) notificações da doença, número de testes rápidos e de RT-PCR foram obtidos nas fontes: "Gerenciador de Ambiente Laboratorial", "e-sus VE" e SES-MG. O coeficiente de Pearson para correlação foi calculado para estabelecer o nível de associação entre os dados relevantes. Técnicas estatísticas descritivas foram empregadas para compreender a distribuição da incidência, mortalidade e taxas de testes no território. Resultados: Correlações positivas foram encontradas entre taxa de testes rápidos e incidência; taxa de testes RT-PCR e incidência/mortalidade. A nível municipal, incidência, mortalidade, taxa de testes rápidos e de RT-PCR têm correlação negativa com dias transcorridos desde o Primeiro Caso Notificado. O mesmo efeito ocorre, em diferentes intensidades, a nível das macrorregiões de saúde. Conclusão: A heterogeneidade da incidência e mortalidade da COVID-19 no território mineiro, assim como, das taxas de testes (rápidos e RT-PCR) pode ser causada, em parte, devido às diferentes datas de introdução do vírus nos municípios/macrorregiões de saúde. Especula-se que esse fenômeno se deve às dinâmicas dos fluxos regionais e inter-regionais de pessoas.(AU)

Justificación y Objetivos: El SARS-CoV-2 es responsable por una pandemia sin precedentes con profundas consecuencias socioeconómicas. Debido a su reciente descubrimiento, este vírus representa una gran incógnita para los investigadores. Así, este estudio tiene como objetivo establecer las asociaciones espacio-temporales de la incidencia, la mortalidad y la tasa de pruebas rápidas y RT-PCR en Minas Gerais. Métodos: Trata-se de un análisis cuantitativo de datos secundarios basado en un diseño de investigación transversal. Incidencia, mortalidad, fecha de la primera notificación de COVID-19 y número de pruebas rápidas y RT-PCR se obtuvieron de las fuentes: "GAL", "e-SUS VE" y "SES-MG". Se calculó el coeficiente de correlación de Pearson para establecer el nivel de asociación entre los datos relevantes. Se utilizaron procedimientos estadísticos descriptivos para proporcionar una comprensión integral de la distribución de la incidencia, la mortalidad y las tasas de prueba en el territorio. Resultados: Se encontraron correlaciones positivas entre la tasa de pruebas rápidas y la incidencia; tasa de pruebas de RT-PCR y incidencia/mortalidad. A nivel municipal, la incidencia, mortalidad, tasa de pruebas rápidas y RT-PCR revelaron una correlación negativa con los días transcurridos desde el Primer Caso Notificado. El mismo efecto ocorre a nivel de macrorregiones de salud. Conclusiones: La heterogeneidad de la incidencia y mortalidad de COVID-19 en el territorio de Minas Gerais, así como la tasa de pruebas puede deberse, en parte, a las diferentes fechas de introducción de la virus en los territorios. Se especula que este fenómeno ocurre debido a la dinámica de los flujos regionales e interregionales de personas.(AU)

Subject(s)

Humans , Immunologic Tests , Spatio-Temporal Analysis , SARS-CoV-2 , COVID-19/mortality , COVID-19/epidemiology

5.

Immunochromatography and laboratory serologies: an evaluation of immunodiagnoses in prenatal care / Inmunocromatográficos y serologías laboratoriales: evaluación de inmunodiagnósticos en el cuidado prenatal / Imunocromatográficos e sorologias laboratoriais: avaliação de imunodiagnósticos no cuidado pré-natal

Damiani, Pattrícia da Rosa; Backes, Marli Terezinha Stein; Stoco, Patrícia Hermes; Fernandes, Vanessa Martinhago Borges; Soares, Gustavo Lopes.

Rev. bras. enferm ; 74(2): e20200877, 2021. tab, graf

Article in English | LILACS-Express | LILACS, BDENF | ID: biblio-1251156

ABSTRACT

ABSTRACT Objectives: to describe the use of affinity chromatographies and laboratory serologies in the evaluation of immunodiagnoses during prenatal. Methods: quantitative study, characterized as a descriptive observational research. Data was collected from the records of 46 pregnant women who were in prenatal follow up in the Primary Health Care in a capital in the South of Brazil. The data found was codified and analyzed using descriptive statistics. Results: a mean of 43.1 days was found to take place between the request of laboratory serology and the evaluation by a professional. It was also found that 21.7% of pregnant women did not collect the serologies requested during the first prenatal consultation, and that the affinity chromatographies were only applied in 10.8% of the participants. Conclusions: in spite of the studies for the improvement of prenatal consultations, for the provision of new technologies and for the permanent education offered to the professionals, there are still questions that make the actual implementation of affinity chromatographies more difficult.

RESUMEN Objetivos: describir la utilización de los inmunocromatográficos y de las serologías laboratoriales en la evaluación de inmunodiagnósticos durante el prenatal. Métodos: estudio de abordaje cuantitativo, caracterizado como una investigación observacional del tipo descriptiva. Recogidos datos de los prontuarios de 46 gestantes que realizan acompañamiento prenatal en la Atención Primaria de Salud del Sur de Brasil. Datos obtenidos tuvieron su contenido codificado y analizados mediante estadística descriptiva. Resultados: identificada una mediana de 43,1 días desde la solicitud de las serologías laboratoriales hasta la evaluación profesional. Así, también se verificó que 21,7% de las gestantes no recogieron las serologías solicitadas durante la primera consulta prenatal y que aplicaron inmunocromatográficos en solo 10,8% de los participantes. Conclusiones: sin embargo los estudios para perfeccionamiento de consulta prenatal, provisión de nuevas tecnologías y educación permanente ofertada a los profesionales, aún persisten cuestiones que dificultan la concreta implementación de inmunocromatográficos.

RESUMO Objetivos: descrever a utilização dos testes imunocromatográficos e das sorologias laboratoriais na avaliação de imunodiagnósticos durante o pré-natal. Métodos: estudo de abordagem quantitativa, caracterizado como uma pesquisa observacional do tipo descritiva. Foram coletados dados dos prontuários de 46 gestantes que realizam acompanhamento pré-natal na Atenção Primária à Saúde de uma capital do Sul do Brasil. Os dados obtidos tiveram seu conteúdo codificado e analisados mediante estatística descritiva. Resultados: foi identificada uma média de 43,1 dias desde a solicitação das sorologias laboratoriais até a avalição profissional. Nesse sentido, também foi verificado que 21,7% das gestantes não coletaram as sorologias solicitadas durante a primeira consulta pré-natal e que foram aplicados testes imunocromatográficos em apenas 10,8% dos participantes. Conclusões: apesar dos estudos para o aprimoramento da consulta pré-natal, do fornecimento de novas tecnologias e da educação permanente ofertada aos profissionais, ainda persistem questões que dificultam a concreta implementação dos testes imunocromatográficos.

6.

Estandarización y utilidad de la contrainmunoelectroforesis para el diagnóstico de la bartonelosis / Standardization and utility of counterimmunoelectrophoresis for the diagnosis of bartonellosis

Acuña, Dante; Cornejo, William.

An. Fac. Med. (Perú) ; 81(3): 294-300, jul-set 2020. tab, graf

Article in Spanish | LILACS-Express | LILACS | ID: biblio-1285032

ABSTRACT

RESUMEN Introducción. La enfermedad de Carrión, causada por Bartonella bacilliformis, es una enfermedad reemergente en el Perú, que se diagnostica convencionalmente mediante el frotis sanguíneo y el cultivo, los cuales son métodos poco sensibles, necesitándose métodos diagnósticos alternativos. Objetivos. Determinar la sensibilidad y especificidad de la contrainmunoelectroforesis (CIEF) utilizando un antígeno sonicado obtenido de una cepa de Bartonella sp., para detectar anticuerpos contra la bacteria comparado con el cultivo como estándar de referencia. Métodos. El antígeno para la prueba se obtuvo por sonicación de un aislado de Bartonella sp., cultivado en un medio bifásico con y sin sangre de carnero. La reactividad del antígeno sonicado fue evaluada por la CIEF empleando 123 sueros de personas, de los cuales 60 fueron de pacientes con diagnóstico clínico y bacteriológico de enfermedad de Carrión, 54 de personas con otras infecciones y 9 de personas sanas. Para la estandarización de la prueba de CIEF se evaluaron el tamaño y la distancia entre los pocillos, así como la concentración del antígeno y los volúmenes de los reactivos usados. Resultados. La concentración óptima del antígeno fue de 0,64 mg/mL, la distancia entre los pocillos de 3 mm, el tamaño de los pocillos de 3 mm y el volumen de los reactivos de 12 μL. La CIEF estandarizada tuvo una sensibilidad de 43,3% y una especificidad de 98,4%. Conclusiones. Los resultados de la CIEF revelan una baja sensibilidad de la prueba, pudiéndose usar como una prueba confirmatoria dada su elevada especificidad, pero no puede ser utilizada como prueba de tamizaje serológico por su escasa sensibilidad.

ABSTRACT Introduction. Carrion's disease, caused by the bacterium Bartonella bacilliformis, is a reemerging disease in Perú, which is conventionally diagnosed by blood smear and culture, which are not very sensitive methods, requiring alternative diagnostic methods. Objectives. To determine the sensitivity and specificity of the counterimmunoelectrophoresis (CIEP) using a sonicated antigen obtained from a Bartonella sp. strain, to detect antibodies against the bacteria compared to the culture as reference standard. Methods. The test antigen was obtained by sonication of an isolate of Bartonella sp., grown in a biphasic medium with and without sheep blood. The reactivity of the sonic antigen was evaluated by the CIEP using 123 sera from people, of which 60 were from patients with a clinical and bacteriological diagnosis of Carrion's disease, 54 from people with other infections and 9 from healthy people. For the standardization of the CIEP test, the size and distance between the wells were evaluated, as well as the concentration of the antigen and the volumes of the reagents used. Results. The optimal concentration of the antigen was 0,64 mg/mL, the distance between the 3 mm wells, the size of the 3 mm wells and the volume of the reagents of 12 μL. The standardized CIEP had a sensitivity of 43,3% and a specificity of 98,4%. Conclusions. The results of the CIEP reveal a low sensitivity of the test, being able to be used as a confirmatory test given its high specificity but cannot be used as a serological screening test due to the low sensitivity referred to.

7.

COVID-19: clinical and laboratory manifestations in novel coronavirus infection / COVID-19: manifestações clínicas e laboratoriais na infecção pelo novo coronavírus

Xavier, Analucia R.; Silva, Jonadab S.; Almeida, João Paulo C. L.; Conceição, Johnatan Felipe F.; Lacerda, Gilmar S.; Kanaan, Salim.

J. Bras. Patol. Med. Lab. (Online) ; 56: e3232020, 2020. tab, graf

Article in English | LILACS-Express | LILACS | ID: biblio-1134631

ABSTRACT

ABSTRACT COVID-19 is a highly contagious disease caused by the coronavirus of severe acute respiratory syndrome 2 (SARS-CoV-2). In 2020, due to the outbreak, it was considered by the World Health Organization (WHO) as a pandemic. The infection caused by the novel coronavirus has high mortality in a small portion of the infected population, especially in elderly, immunosuppressed, diabetic, cardiac, and hypertensive individuals. Many infected are asymptomatic (and may be carriers) or present mild or moderate flu-like symptoms. The most severe clinical picture of COVID-19 is characterized by an inflammatory cytokine storm, with hematological changes and coagulation dysfunction, which can lead to tissue damage and death. Nonspecific laboratory biomarkers may be either increased or decreased as the course of the disease progresses and are often useful in predicting complications of the disease, such as the use of D-dimer and platelet/lymphocyte ratio. Specific laboratory diagnosis is based on the detection of viral ribonucleic acid (RNA) by real-time polymerase chain reaction (RT-PCR) of nasal and oropharyngeal swab samples; it is more effective when performed in the first days after symptom onset. Serological tests are useful in detecting the immune response, since both class M (IgM) and class G (IgG) immunoglobulin antibodies can be detected seven days after the onset of clinical symptoms, and may extend for more than 25 days, although not exempting the individual from remaining infectious, depending on their viral load and clinical presentation. The rational use of specific laboratory markers must respect the disease chronology, and the correct interpretation may provide subsidies for a better management of affected patients, as well as identifying asymptomatic carriers or those with mild symptoms.

RESUMEN La COVID-19 es una enfermedad altamente contagiosa causada por el coronavirus del síndrome respiratorio agudo grave (SARS-CoV-2). En 2002, a causa del brote, fue reconocida como una pandemia por la Organización Mundial de la Salud (OMS). La infección por el nuevo coronavirus provoca alta mortalidad en una pequeña parcela de la población infectada, especialmente en ancianos, pacientes inmunodeprimidos, diabéticos, cardiópatas e hipertensos. Muchos infectados son asintomáticos (y pueden ser portadores) o presentan síntomas leves a moderados, como en un estado gripal. El cuadro clínico de la COVID-19 en la forma más grave es caracterizado por una tormenta inflamatoria de citoquinas, con cambios hematológicos y de la coagulación que pueden llevar a daño tisular y muerte. Pruebas de laboratorio inespecíficas pueden presentar tasas más altas o bajas según el curso de la enfermedad, y muchas veces son útiles en la predicción de complicaciones, como el uso del dímero D y la ratio plaquetas/linfocitos. El diagnóstico de laboratorio específico se basa en la detección del ácido ribonucleico (ARN) viral por reacción en cadena de la polimerasa (PCR) en tiempo real de muestras de hisopado nasal y orofaríngeo; es más efectiva en los primeros días tras el inicio de los síntomas. Pruebas serológicas son útiles para detectar la respuesta inmune, pues tanto los anticuerpos de la inmunoglobulina M (IgM) como de la G (IgG) pueden se detectar siete días después del inicio de los síntomas clínicos, y pueden permanecer por más de 25 días, aunque no eximen al individuo de seguir infeccioso, dependiendo de su carga viral y presentación clínica. El uso racional de los marcadores de laboratorio específicos debe respetar la cronología de la enfermedad, y la interpretación correcta puede proporcionar recursos para un mejor manejo de los pacientes afectados, así como identificar portadores asintomáticos o con pocos síntomas.

RESUMO COVID-19 é uma doença altamente contagiosa provocada pelo coronavírus da síndrome respiratória aguda grave 2 (SARS-CoV-2). Em 2020, devido ao surto, foi caracterizada pela Organização Mundial da Saúde (OMS) como pandemia. A infecção causada pelo novo coronavírus tem alta mortalidade em uma pequena parcela da população infectada, especialmente em indivíduos idosos, imunodeprimidos, diabéticos, cardiopatas e hipertensos. Muitos infectados são assintomáticos (e podem ser portadores) ou apresentam sintomas leves a moderados, semelhantes ao estado gripal. O quadro clínico da COVID-19 na forma mais severa é caracterizado por uma tempestade inflamatória de citocinas, com alterações hematológicas e da coagulação que podem levar ao dano tecidual e morte. Exames laboratoriais inespecíficos podem apresentar-se mais elevados ou diminuídos conforme o curso da doença, e muitas vezes são úteis na predição de complicações, como o uso do D-dímero e a razão plaqueta/linfócitos. O diagnóstico laboratorial específico se baseia na detecção do ácido ribonucleico (RNA) viral por reação em cadeia da polimerase em tempo real (RT-PCR) de amostras de suabe nasal e orofaríngeo; é mais efetivo nos primeiros dias após o início dos sintomas. Testes sorológicos são úteis na detecção da resposta imune, pois tanto os anticorpos da imunoglobulina da classe M (IgM) quanto da classe G (IgG) podem ser detectados após sete dias do início dos sintomas clínicos, podendo se estender por mais de 25 dias, embora não isente o indivíduo de continuar infectante, dependendo de sua carga viral e apresentação clínica. O uso racional dos marcadores laboratoriais específicos deve respeitar a cronologia da doença, e a interpretação correta pode fornecer subsídios para um melhor manejo dos pacientes acometidos, bem como identificar portadores assintomáticos ou com pouco sintomas.

8.

Cut-off values of immunological tests to identify patients at high risk of severe lupus nephritis

Gargiulo, María De Los Ángeles; Khoury, Marina; Gómez, Graciela; Grimaudo, Sebastián; Suárez, Lorena; Collado, María Victoria; Sarano, Judith.

Medicina (B.Aires) ; 78(5): 329-335, oct. 2018. tab

Article in English | LILACS | ID: biblio-976121

ABSTRACT

Cut-off values for anti-dsDNA, anti-nucleosome and anti-C1q antibodies tests and for complement-mediated hemolytic activity (CH50) were explored to identify patients with high risk of developing severe lupus nephritis (LN). Forty-one patients with confirmed systemic lupus erythematosus (SLE) were identified; their levels for the three antibodies and complement had been measured on a same serum sample. These patients were classified based on the presence of renal involvem ent; sixteen had active proliferative LN. With the cut-off values accepted in the laboratory for SLE diagnosis (anti-dsDNA > 100 UI/ml, anti-nucleosome > 50 U/ ml or CH50 < 190 UCH50%) no significant differences were found between patients with and without LN. Anti-C1q > 40 U/ml showed a statistically significant association with LN and had 80% of specificity. Cut-off values for LN identified by Receiver Operating Characteristic curves (ROC) were higher for anti-dsDNA (> 455 IU/ml) and anti-nucleosome (>107 U/ml), lower for CH50 (< 150 UCH50%) and, for anti-C1q (> 41 U/ml) coincided with the cut-off values accepted for SLE. Anti-C1q > 134 U/ml had a 92% of specificity, 56% of sensibility and was associated with a fifteen-fold increased risk of LN. The simultaneous presence of anti-nucleosome > 107 U/ml and anti-C1q > 134 U/ml was associated with a 27-fold higher probability for LN. According to these results, the cut-off values used to detect SLE activity could be inadequate to identify patients at high risk of severe LN.

Se exploraron valores de corte para los ensayos de anti-ADNdc, anti-nucleosoma, anti-C1q y complemento hemolítico total (CH50) capaces de identificar los casos con mayor riesgo de nefritis lúpica (NL) grave. Se seleccionaron 41 pacientes ≥ 16 años con lupus eritematoso sistémico (LES) confirmado que tenían titulados los niveles de los tres anticuerpos y CH50, en una misma muestra de suero. Fueron clasificados según presencia de compromiso renal; 16 presentaron formas proliferativas de NL activa. Con los valores de corte aceptados por el laboratorio para el diagnóstico de LES (anti-ADNdc > 100 UI/ml, anti-nucleosoma > 50 U/ml o un CH50 < 190 UCH50%) no se encontraron diferencias significativas entre casos con y sin NL. Un anti-C1q > 40 U/ml tuvo una especificidad del 80% y mostró una asociación estadísticamente significativa con NL. Al aplicar curvas Receiver Operating Characteristic (ROC) para NL, se identificaron valores de corte más altos para anti-ADNdc (> 455 IU/ml) y anti-nucleosoma (> 107 U/ml), más bajo para CH50 (< 150 UCH50%) y para el anti-C1q (> 41 U/ml) coincidió con el aceptado para diagnóstico de LES. Un anti-C1q > 134 U/ml presentó una sensibilidad del 56%, una especificidad del 92% y se asoció con quince veces más riesgo de NL. La presencia simultánea de anti-C1q > 134 U/ml y anti-nucleosoma > 107 U/ml se asoció 27 veces más riesgo de NL. De acuerdo a estos resultados los valores de corte empleados para actividad en pacientes con LES podrían resultar inadecuados para identificar pacientes con mayor riesgo de NL grave.

Subject(s)

Humans , Male , Female , Infant , Child, Preschool , Child , Adolescent , Adult , Middle Aged , Young Adult , Immunologic Tests/standards , Lupus Nephritis/blood , Reference Standards , Severity of Illness Index , Immunologic Tests/methods , Lupus Nephritis/diagnosis , Nucleosomes/immunology , Biomarkers/blood , Complement C1q/immunology , Complement Hemolytic Activity Assay/methods , Complement Hemolytic Activity Assay/standards , Antibodies, Antinuclear/blood , Retrospective Studies , Risk Factors , Sensitivity and Specificity , Risk Assessment/methods , Lupus Erythematosus, Systemic/immunology , Lupus Erythematosus, Systemic/blood

9.

Sangue oculto nas fezes: uma comparação entre os métodos químico e imunoquímico / Fecal occult blood: a comparison of chemical and immunochemical tests

Borges, Luana Vilarinho; Mattar, Rejane; Silva, Joyce Matie Kinoshita da; Silva, Ana Luiza Werneck da; Carrilho, Flair José; Hashimoto, Cláudio Lyoiti.

Arq. gastroenterol ; 55(2): 128-132, Apr.-June 2018. tab, graf

Article in English | LILACS | ID: biblio-950517

ABSTRACT

ABSTRACT BACKGROUND: Colorectal bleeding is a warning sign that may be identified by fecal occult blood testing. A positive fecal occult blood test result requires a subsequent colonoscopy, a costly and invasive examination. Therefore, the use of diagnostic tests with optimal sensitivity and specificity is warranted. In this study, we evaluated four different fecal occult blood tests in 176 patients undergoing colonoscopy and compared their results. OBJECTIVE: To assess the sensitivity, specificity and predictive values of chemical and immunochemical fecal occult blood tests in patients undergoing colonoscopy and to evaluate the degree of concordance between the tests and colonoscopy. METHODS: Patients with indications for colonoscopy also underwent fecal occult blood testing by chemical (toluidine test) and immunochemical methods, employing three commercially available kits. Based on the endoscopic findings, the colonoscopy was rated as positive or negative for colorectal bleeding. The degree of concordance between the fecal occult blood tests and the colonoscopy was evaluated by the kappa index. RESULTS: Forty-four (25%) colonoscopies were categorized as positive for colorectal bleeding. The toluidine test presented lower concordance than the immunochemical tests, which showed moderate concordance with the colonoscopy. The toluidine test had the least sensitivity, specificity, and positive and negative predictive values. CONCLUSION: The immunochemical fecal occult blood tests showed greater sensitivity, specificity and predictive values in detecting colorectal bleeding. The immunochemical tests had superior indexes of agreement with colonoscopy compared to the toluidine test.

RESUMO CONTEXTO: O sangramento colorretal é considerado um sinal de alarme e não deve ser ignorado. O resultado positivo de um teste de pesquisa de sangue oculto nas fezes (PSOF) requer investigação complementar com colonoscopia, exame invasivo e de alto custo. Justifica-se, portanto, a aplicação de um teste diagnóstico mais sensível e específico. No presente estudo, foram avaliados quatro diferentes testes de PSOF em 176 pacientes submetidos à colonoscopia e seus resultados foram comparados. OBJETIVO: Avaliar a sensibilidade, a especificidade e os valores de predição dos testes químico e imunoquímico de PSOF em pacientes submetidos à colonoscopia e avaliar o grau de concordância entre os testes de PSOF e a colonoscopia. MÉTODOS: Pacientes com indicação de realizar colonoscopia foram submetidos também à PSOF pelo método químico (o-toluidina) e pelo método imunoquímico, empregando três kits comerciais disponíveis no mercado. Fundamentado nos achados endoscópicos, a colonoscopia foi categorizada em positiva ou negativa, de acordo com a possível fonte de sangramento colorretal. O grau de concordância entre os testes de PSOF foi avaliado pelo índice kappa. RESULTADOS: Quarenta e quatro (25%) colonoscopias foram categorizadas como positivas quanto à fonte de sangramento colorretal. O teste da o-toluidina mostrou menor concordância que os testes imunoquímicos, os quais apresentaram moderada concordância com a colonoscopia. O teste da o-toluidina revelou menor sensibilidade, especificidade, valor preditivo positivo e valor preditivo negativo. CONCLUSÃO: Os testes imunoquímicos revelaram maior sensibilidade, especificidade e valores de predição na detecção de sangramento colorretal. Os testes imunoquímicos apresentaram melhores índices de concordância com a colonoscopia, quando comparados ao teste da o-toluidina.

Subject(s)

Humans , Male , Female , Adolescent , Adult , Young Adult , Toluidines/analysis , Colorectal Neoplasms/diagnosis , Colonoscopy/standards , Feces/chemistry , Occult Blood , Immunohistochemistry , Mass Screening , Predictive Value of Tests , Sensitivity and Specificity , Early Detection of Cancer , Middle Aged

10.

Pacientes portadores de sífilis atendidos em uma unidade terciária em Fortaleza: perfil sociodemográfico / Patients with syphilis assisted in tertiary care unit in Fortaleza: sociodemographic profile

Silva, Zélia Firmino da; Teixeira, Kelly Sivocy Sampaio; Nascimento, Daniel Soares do.

Rev. bras. anal. clin ; 49(1): 105-109, jun.16, 2017. tab

Article in Portuguese | LILACS | ID: biblio-1151853

ABSTRACT

A sífilis é definida como uma doença sexualmente transmissível (DST), infecto-contagiosa, possui formas características de infecção, caracterizada em três fases: primária, secundária e terciária, sendo a congênita por sintomatologia mais específica. O presente trabalho teve por objetivo traçar o perfil sociodemográfico dos portadores de sífilis atendidos em um hospital de Fortaleza. A coleta de dados ocorreu no período de seis meses, entre os meses de janeiro a junho de 2015. Foi realizado um estudo descritivo de caráter exploratório e retrospectivo de pacientes atendidos no Hospital Geral César Cals. Foram realizados testes não treponêmicos, VDRL (Venereal Disease Research Laboratory) e/ou treponêmicos (Treponema Screen), onde os pacientes teriam que apresentar resultados reagentes para sífilis. Constatou-se que a população estudada foi composta de pacientes adultos e recémnascidos, no referido período de estudo, sendo identificados 166 pacientes reagentes a sífilis. A população adulta apresentou o mesmo perfil quanto à faixa etária (20-29 anos) e local de moradia, sendo que a população geral residia no município de Fortaleza, CE. Quanto ao grau de escolaridade, 43,0% das mulheres concluíram o fundamental e os homens (62,5%) concluíram o ensino médio. Setenta e oito por cento das mulheres haviam dado à luz até três filhos. Dentre os pacientes do referido estudo, foi possível determinar que a paciente do sexo feminino obteve maior predominância. A sífilis congênita se fez presente no referido estudo, evidenciando os casos de sífilis transmitida de mães para filhos. O diagnóstico laboratorial demonstrou sua importância para obtenção do perfil sorológico da população.

Syphilis is defined as a sexually transmitted disease (STD), contagious infectious, it has forms of infection characterized in three stages: Primary, Secondary and Tertiary, being the primary one, congenital by a more specific symptomatology. The present study aimed to outl in the sociodemographic profile of Syphilis carriers attended in a Hospital of Fortaleza city. The data collection occurred in the six months between January and June 2015. It was did a descriptive study of exploratory and retrospective character of patients treated at the General Hospital César Cals. It was performed nontreponemal test of VDRL (Venereal Disease Research Laboratory) treponemic and / or (Treponemic screen), in which patients should to show positive results to syphilis. The studied population was composed of adult and newborn patients. In the study period had been identified 166 syphilis positive patients. The adult population presented the same profile in the age range (20-29 years) and places of residence, in the way that the general population residing in the city of Fortaleza / CE. About the education level, 43.0% of the women completed the fundamental school and 62.5% of the men completed the high school. 78.0% of the women had given birth up to three sons. Among those patients in this study, it was possible to conclude that female patients had obtained more predominance. The congenital syphilis appeared in this study, evidenced by the cases in which syphilis was transmitted by mother to children. The laboratorial diagnostic has proven of key importance to obtain the population serological profile

Subject(s)

Humans , Male , Female , Infant, Newborn , Adult , Syphilis, Congenital , Immunologic Tests , Syphilis

11.

Validez de tres métodos de inmuno-diagnóstico de neurocisticercosis: revisión sistemática de la literatura con meta-análisis 1960-2014 / Validity of three methods for inmuno-diagnostic of neurocysticercosis: systematic review of the literature with meta-analysis 1960-2014

Cardona-Arias, Jaiberth Antonio; Carrasquilla-Agudelo, Yoneida Elena; Restrepo-Posada, Deisy Cristina.

Rev. chil. infectol ; 34(1): 33-44, feb. 2017. ilus, graf, tab

Article in Spanish | LILACS | ID: biblio-844442

ABSTRACT

Introduction: The screening of neurocysticercosis is complex and immunological methods have varying validity. Objective: To evaluate the validity of ELISA for antigen and antibody, and EITB for antibody in the screening of neurocysticercosis. Methods: Meta-analysis of diagnostic tests with an ex-ante protocol implemented in five databases with 15 search strategies, ensuring reproducibility in the selection and extraction of information. Sensitivity, specificity, likelihood ratios (LR), diagnostic odds ratio and ROC curve were estimated in MetaDiSc, and predictive values, and Youden index were estimated in Epidat. Results: EITB presented sensitivity of 85.7% (95% CI 83.5-87.7), specificity 93.9% (95% CI = 92.7-95.0), PLR 19.6 (95% CI = 8,6-44.6), NLR 0.16 (95% CI = 0.12-0.21), OR diagnostic 136.2 (95% CI = 54.7-342.6) and area under the curve 0.926. In ELISA for antibody sensitivity was 87.5% (95% CI = 86.1-88.8), specificity 92.2% (95% CI = 91.4-93.0), PLR 11.3 (95% CI = 8.45-15.11), NLR 0.15 (95% CI = 0.13-0.18), diagnostic OR 87.4 (95% CI = 60.1-127.1) and area under the curve 0.950. ELISA for antigen showed low diagnostic validity. No differences were found in these parameters by sample, antigen or antibody type. Conclusion: ELISA for antibodies and EITB have a similar diagnostic value, detection of serum and CSF showed a similar validity.

Introducción: La tamización de neurocisticercosis es compleja y los métodos inmunológicos presentan validez variable y generalmente bajos tamaños de muestra. Objetivo: Evaluar la validez de ELISA para detección de antígeno y anticuerpo, y EITB para detección de anticuerpo en la tamización de neurocisticercosis. Métodos: Meta-análisis de pruebas diagnósticas con un protocolo ex-ante aplicado en cinco bases de datos con 15 estrategias de búsqueda, garantizando reproducibilidad en la selección y extracción de la información. Se estimó sensibilidad, especificidad, cocientes de probabilidad (CP), razón de odds diagnósticas y curva ROC en MetaDiSC, y valores predictores, índice de Youden y exactitud en Epidat. Resultados: EITB presentó sensibilidad de 85,7% (IC 95% = 83,5-87,7), especificidad 93,9% (IC9 5% = 92,7-95,0), CPP 19,6 (IC 95% = 8,6-44,6), CPN 0,16 (IC 95% = 0,12-0,21), OR diagnóstica 136,2 (IC 95% = 54,7-342,6) y área bajo la curva 0,926. En ELISA para anticuerpos la sensibilidad fue 87,5% (IC 95% = 86,1-88,8), especificidad 92,2% (IC 95% = 91,4-93,0), CPP 11,3 (IC 95% = 8,45-15,11), CPN 0,15 (IC 95% = 0,13-0,18), OR diagnóstica 87,4 (IC 95% = 60,1-127,1) y área bajo la curva 0,950. ELISA para antígeno presentó baja validez diagnóstica. No se hallaron diferencias en estos parámetros según tipo de muestra, antígeno o anticuerpo. Conclusión: ELISA para anticuerpos y EITB presentan una utilidad diagnóstica similar, la detección de suero presentó una validez similar al líquido cefalorraquídeo.

Subject(s)

Humans , Taenia/immunology , Antibodies, Helminth/blood , Immunoenzyme Techniques/methods , Neurocysticercosis/diagnosis , Antigens, Helminth/immunology , Enzyme-Linked Immunosorbent Assay , Reproducibility of Results , ROC Curve , Sensitivity and Specificity

12.

Producción y evaluación del antígeno recombinante TES-30 de Toxocara canis para el inmunodiagnóstico de toxocariasis / Production and evaluation of the recombinant antigen TES-30 of Toxocara canis for the immunodiagnosis of toxocariasis

Olave, Ana M.; Mesa, Jairo A.; Botero, Jorge H.; Patiño, Edwin B.; García, Gisela M.; Alzate, Juan F..

Biomédica (Bogotá) ; 36(1): 39-51, ene.-mar. 2016. ilus, graf, tab

Article in Spanish | LILACS | ID: lil-779530

ABSTRACT

Introducción. Toxocara canis es un nematodo patógeno de cánidos que accidentalmente puede ser transmitido a los humanos. A pesar de la importancia de la serología para el diagnóstico de esta zoonosis, los kits diagnósticos usan antígenos crudos de excreción-secreción, en su mayoría glucoproteínas que no son específicas de especie, por lo cual pueden presentarse reacciones cruzadas con anticuerpos generados contra otros parásitos. Objetivos. Producir el antígeno recombinante TES-30 de T. canis y evaluarlo para el inmunodiagnóstico de la toxocariasis. Materiales y métodos. Se clonó el gen que codifica TES-30 en el vector de expresión pET28a (+), usando oligonucleótidos de cadena sencilla unidos mediante reacción en cadena de la polimerasa (PCR). La proteína rTES-30 se purificó por cromotografia de afinidad (Ni 2+ ). La reacción serológica de rTES-30 se evaluó mediante immunoblot . Teniendo en cuenta que no existe una prueba de referencia , se observó el comportamiento del antigeno en comparación con la prueba de rutina para el inmunodiagnóstico de la toxocariasis, es decir, la técnica ELISA convencional con antígenos de excreción-secreción. Resultados. El rTES-30 se produjo a partir de un cultivo de Escherichia coli LB, con un rendimiento de 2,25 mg/l y 95 % de pureza. La concordancia de la reacción entre el immunoblot rTES-30 y la ELISA convencional, fue de 73 % (46/63) y de 100 % con los 21 sueros no reactivos. De los 21 sueros con diagnóstico de otras parasitosis, 19 fueron reactivos con ELISA, mientras que tan solo siete fueron positivos con el immunoblot rTES-30. La concordancia entre la ELISA y el immunoblot fue moderada (índice kappa de 0,575; IC 95% 0,41-0,74). Conclusiones. Los datos presentados respaldan la utilidad del immunoblot r TES-3 0 para la confirmación de los posibles positivos por ELISA, no solo en los estudios epidemiológicos, sino también, como candidato para el desarrollo de pruebas diagnósticas de la toxocariasis ocular en Colombia.

Introduction: Toxocara canis is a pathogenic nematode of canines which can be accidentally transmitted to humans. Although serology is the most important diagnostic tool for this zoonosis, diagnostic kits use crude excretion/secretion antigens, most of them being glycoproteins which are not species-specific and may cross-react with antibodies generated against other parasites. Objectives: To produce the rTES-30 recombinant antigen of Toxocara canis and evaluate it in the immunodiagnosis of toxocariasis. Materials and methods: The gene that codes for TES-30 was cloned in the expression vector pET28a (+) using single-stranded oligonucleotides united by PCR. The protein rTES-30 was purified by Ni 2+ affinity chromotography. Seroreactivity of rTES-30 was evaluated by immunoblot. Given that there is no gold standard test, the behaviour of the antigen was compared with the method that is routinely used to immunodiagnose toxocariasis, i.e., the conventional ELISA technique using excretion/secretion antigens. Results: The rTES-30 was produced from an Escherichia coli LB culture which yielded 2.25 mg/L of the antigen with a purity of 95%. The results obtained showed 73% (46/63) concordance of reactivity between the rTES-30 immunoblot and the conventional ELISA, and 100% concordance with the non-reactive sera (21). Nineteen of the 21 sera positive for other parasitoses reacted with ELISA, while only seven of these were positive with the rTES-30 immunoblot. Concordance between the ELISA and the immunoblot was moderate (kappa coefficient: 0.575; 95% CI: 0.41- 0.74). Conclusions: The data presented show the potential of the rTES-30 inmunoblot for confirmation of possible ELISA positives, not only in epidemiological studies, but also as a candidate for the development of diagnostic tests for ocular toxocariasis in Colombia.

Subject(s)

Animals , Humans , Immunoblotting , Toxocariasis/diagnosis , Toxocara canis/immunology , Antigens, Helminth/blood , Peptide Fragments/isolation & purification , Peptide Fragments/analysis , Peptide Fragments/genetics , Peptide Fragments/immunology , Solubility , Recombinant Fusion Proteins/isolation & purification , Recombinant Fusion Proteins/analysis , Enzyme-Linked Immunosorbent Assay , Base Sequence , Toxocariasis/blood , Eye Infections, Parasitic/diagnosis , Chromatography, Affinity , Escherichia coli , Genes, Synthetic , Antigens, Helminth/isolation & purification , Antigens, Helminth/genetics

13.

Investigation and analysis of internal quality control on clinical chemistry, clinical immunology and clinical hematology of mutual recognition laboratories in 142 medical institutions in Beijing / 中华检验医学杂志

Rui ZHOU; Yanyan QIN; Jian GUO; Meiyi HE; Yanmin YANG; Rui ZHANG; Shunli ZHANG; Yuhong YUE; Zhixin SONG; Chunying WU; Hongyi YIN; Yufang LIANG; Tingting JIA; Qingtao WANG.

Chinese Journal of Laboratory Medicine ; (12): 922-929, 2016.

Article in Chinese | WPRIM | ID: wpr-508770

ABSTRACT

Objective To investigate the internal quality control ( IQC ) on clinical chemistry , clinical immunology and clinical hematology in mutual recognition laboratories in medical institutions in Beijing.Methods By means of questionnaire survey and on -site investigation, fresh frozen serum and whole blood samples with assigned values by reference method were measured to investigate the status of IQC on clinical chemistry , clinical immunology and clinical hematology in 142 mutual recognition laboratories in medical institutions of Beijing,and results were analyzed.Results 142 copies of questionnaireson clinical chemistry, clinical immunology and clinical hematology were send out and 120, 97, and 101 laboratories returned the questionnaires respectively .The information feedback rate was 84.5%, 68.3% and 71.1%respectively .All the questionnaires were effective .Questionnaires survey results showed that more than 50%laboratories set up quality control goals and the most of the goals were probability for error detection ( Ped) 95%, probability for false rejection(Pfr)5%;About 70% laboratories usecd the same quality control plan for different tests ;The most frequently used quality control rules are 12s/13s/22s.On-site investigation showed that ,take the results of clinical chemistry for example , based on the desirable biological variation and WS/T 403 -2012 , most of the tests can't meet the quality control goalsunder the existing quality controlcondition.Conclusion Clinical laboratories should consider their actual situations , assess their own qualitylevels that they can reach , set reasonable quality standards for themselves , and make appropriateindividualized quality control plan.

14.

Detecção de chlamydia trachomatis através de testes imunológicos em população feminina adolescente e adulta na grande Cuiabá, Mato Grosso / Detection of chlamydia trachomatis by immunological methods in adult and adolescent female population in Cuiabá, Mato Grosso

Matos, Marly Pinto de; Machado, Alexandre Paulo; Zavala, Arturo Ayala Zavala y; Silva, Zaíra Batista da; Barbosa, Dulce Aparecida.

DST j. bras. doenças sex. transm ; 27(1-2): 16-21, 2015. tab

Article in English | LILACS | ID: lil-768554

ABSTRACT

Mundialmente, a infecção por Chlamydia trachomatis continua sendo um importante problema de saúde pública, especialmente para adultos jovens sexualmente ativos. Objetivo: Investigar doença sexualmente transmissível por Chlamydia trachomatis em adolescentes e jovens do sexo feminino,na faixa etária de 15 a 25 anos de idade em Cuiabá e Várzea Grande, Mato Grosso, através dos métodos imunológicos de ELISA e imunofluorescência direta. Métodos: Estudo de corte transversal quantitativo de amostras endocervicais de 328 mulheres sexualmente ativas, não grávidas, que frequentaram as Unidades Básicas de Saúde. Amostras endocervicais foram coletadas, sendo a detecção dos antígenos de Chlamydia trachomatis realizada pelos métodos ELISA e imunofluorescência direta. Resultados: Foram obtidas 11 amostras positivas por meio do ELISA (3,4%) e 69 pela imunofluorescência direta(24,4%). Observou-se elevado número de casos entre 16 a 25 anos (24,39%). Conclusão: O índice de casos positivos observado foi representativo,assemelhando-se aos encontrados em outros estudos e denotando, portanto, uma circulação de cepas de clamídia na população estudada. A amplificação das medidas profiláticas, diagnósticas e terapêuticas nos serviços públicos de saúde será um passo importante para conter o avanço da doença sexualmente transmissível, inclusive a infecção genital por Chlamydia trachomatis na população feminina

Worldwide, Chlamydia trachomatis infection remains a major public health problem, especially for sexually active young adults.Objective: To investigate the sexually transmitted disease by Chlamydia trachomatis in adolescents and young women aged 15?25 years from Cuiabáand Várzea Grande, Mato Grosso, Brazil, through the ELISA and direct immunofluorescence methods. Methods: A cross-sectional quantitative study ofendocervical samples from 328 nonpregnant, sexually active women who received care in basic health units. Endocervical samples were collected andC. trachomatis antigens detected by ELISA and direct immunofluorescence methods. Results: A total of 11 positive samples were obtained with ELISA(3.4%) and 69 with direct immunofluorescence (24.4%). The largest number of cases occurred in the 16?25 years age group (24.39%). Conclusion: Therate of positive cases observed was representative, similarly to those found in other studies, and, therefore, indicating Chlamydia strains circulating inthe population studied. Amplification of prophylactic, diagnostic, and therapeutic measures in public health services will be an important step to counterthe spread of sexually transmitted diseases, including genital infection by C. trachomatis in the female population.

Subject(s)

Humans , Female , Adolescent , Adult , Chlamydia trachomatis , Immunologic Tests , Enzyme-Linked Immunosorbent Assay/methods , Sexually Transmitted Diseases/diagnosis , Cross-Sectional Studies , Fluorescent Antibody Technique, Direct

15.

Aspergilose invasiva em pacientes imunodeprimidos: comparação entre as provas de galactomanana, 1,3 betaD-glucana, dados tomográficos e desfecho clínico / Performance of galactomannan and 1,3 beta-glucan enzyme assays in the serum and bronchoalveolar lavage and comparison with computer tomography scan for the diagnosis of invasive aspergillosis in immunocompromised hosts

Batista, Marjorie Vieira.

São Paulo; s.n; 2015. [130] p. ilus, tab, graf.

Thesis in Portuguese | LILACS | ID: biblio-870751

ABSTRACT

A aspergilose invasiva (AI) é a infecção por fungos filamentosos mais comum em pacientes imunodeprimidos, especialmente em transplantes de células tronco hematopoiético e neoplasias hematológicas. Objetivo: Geral: Estabelecer a comparação entre a dosagem de Galactomanana (GM), 1,3betaD-glucana (BDG) e dados tomográficos no diagnóstico da AI bem como seu papel no desfecho clínico. Específicos: 1. Verificar a sensibilidade e especificidade dos ensaios de Galactomanana e de 1,3betaD-glucana no soro e lavado broncoalveolar. 2. Comparar os resultados da galatomanana e 1,3betaD-glucana com os dados de imagem em pacientes com suspeita de AI. 3. Verificar a relação entre a evolução dos níveis de GM e desfecho clínico (óbito e sobrevida). Casuística, Materiais e Métodos: Realizou-se um estudo tipo coorte prospectiva, incluindo 398 sujeitos das diversas enfermarias de pacientes imunodeprimidos do HCFMUSP, sendo incluídos dois grupos de pacientes: 202(51%) AI e 198(49%) controles. Resultados: Dos casos, 18 (8,8%) tinham aspergilose provada, 28 (13,7%) provável e 158 possível (77,5%), de acordo a classificação de 2002 EORTC/MSG (European Organization for Research and Treatment of Cancer / Mycoses Study Group). Os sujeitos submetidos ao TCTH eram 42,7%, com neoplasias hematológicas 37%, TOS 9% e outras doenças 11,3%. Os fatores de risco associados ao desenvolvimento da AI foram neutropenia, monocitopenia, uso de corticóide, presença de doença pelo citomegalovírus e rejeição ou doença do enxerto contra o hospedeiro. O fator de risco associado à evolução para o óbito foi a presença de AI. Foram observados bons desempenhos para a GM tanto no soro como no LBA com LR menores que os registrados na literatura. O melhor desempenho da GM no soro para aspergilose+provável ocorreu com LR de 0,35 com sensibilidade-S, especificidade-E, valor preditivo positivo- VPP), valor preditivo negativo-VPN) e área sob a curva-ASC de 54,4%, 73,4%, 50,8%, 76,2% e 0,64, sendo os valores superiores...

Invasive aspergillosis (IA) has become the leading infectious cause of death in immunocompromised hosts, particularly in subjects under SCTH and hematologic neoplasias. Objectives: General: To compare the performance of GM and BG tests in serum and bronchoalveolar lavage fluid (BAL) and computer tomography (CT) scans in the diagnosis of IA in immunocompromised hosts as well as their role in the patient outcome. Specific: 1. To analyse the sensitivity and specificity of Galactomannan and 1,3 betaD-glucan assays in the serum and bronchoalveolar lavage. 2. To compare the results of Galactomannan and 1,3betaD-glucan assays with CT scans in patients with invasive aspergilosis. 3. To analyse the relationship between the evolution of galactomannan levels and clinical outcome (death or survival). Patients, Materials and Methods: From December 2008 to March 2013, a prospective cohort of 398 patients from several wards of immunocompromised patients of Hospital das Clínicas, Faculdade de Medicina, University of São Paulo was included classified in two groups of patients: 202 (51%) with invasive aspergillosis (IA) and 198 (49%) control patients. Results: Considering 202 cases, 18(8.8%) were subjects with proven, 28(13.7%) with probable aspergillosis and 156(77.5%), with possible aspergillosis, according to 2002 EORTC/MSG (European Organization for Research and Treatment of Cancer/Mycoses Study Group) criteria. The most common underlying disease were: HSCT (42.7%), hematologic malignancy (37%), SOT (9%), or other diseases (11.3%). The main risk factors associated with IA were neutropenia, monocytopenia, patients under corticosterois, presence of CMV disease, and rejection or graft versus host disease. The risk factor associated with death was the presence of invasive aspergillosis. Good performances for serum and BAL GM were registered with lower cutoffs in the present workin relationship to those found in the literature. The best cutoff for proven + probable...

Subject(s)

Humans , Invasive Pulmonary Aspergillosis/microbiology , beta-Glucans , Febrile Neutropenia , Galactans/administration & dosage , Hematopoietic Stem Cell Transplantation , Immunocompromised Host , Immunologic Tests , Mycoses/microbiology , Tomography, X-Ray Computed , Transplantation

16.

Estandarización de la técnica de aglutinación directa para el inmunodiagnóstico de la enfermedad de Chagas / Standardization of a direct agglutination test for the immunodiagnosis of Chagas disease

Alviarez, Yenny; Lares, María; Viettri, Mercedes; Aguilar, Cruz M.; Herrera, Leidi; Ferrer, Elizabeth.

Biomédica (Bogotá) ; 34(2): 308-317, abr.-jun. 2014. ilus, tab

Article in Spanish | LILACS | ID: lil-712412

ABSTRACT

Introducción. La enfermedad de Chagas es causada por el parásito Trypanosoma cruzi y su diagnóstico inmunológico se basa principalmente en la detección de anticuerpos contra T. cruzi mediante pruebas tales como ELISA, inmunofluorescencia indirecta (IFI) y hemaglutinación indirecta (HAI). Esta última tiene el inconveniente de requerir la preparación de eritrocitos de carnero, difíciles de obtener y de poca duración. Sin embargo, existen pruebas alternativas, como la técnica de aglutinación directa. Objetivo. Estandarizar la técnica de aglutinación directa para el diagnóstico de la enfermedad de Chagas. Materiales y métodos. Se prepararon parásitos epimastigotes de T. cruzi mediante dos protocolos, con tratamiento con tripsina y sin él. Los parásitos se colorearon, y se determinaron las condiciones óptimas de concentración parasitaria y diluciones de suero. Se utilizaron sueros de pacientes con enfermedad de Chagas, de individuos sanos y con otras parasitosis. Resultados. La concentración parasitaria óptima fue de 500 x10 6 parásitos/ml, utilizando parásitos coloreados y sin tratamiento con tripsina. Las diluciones de suero óptimas fueron de 1/25, 1/50 y1/100, y el punto de corte, la dilución de 1/50. La técnica estandarizada mostró índices diagnósticos de sensibilidad de 94,3 % (IC 95% 79,5-99,0) y de especificidad de 96,3 % (IC 95% 88,8-99,0); se encontró reacción cruzada en tres sueros de individuos con leishmaniasis visceral, con valores pronósticos positivo y negativo de 91,7 % (IC 95% 76,4-97,8) y de 97,5 % (IC 95% 90,4-99,6), respectivamente. Se compararon los resultados con los obtenidos por HAI, ELISA e IFI y la concordancia fue de 96 % con un índice kappa de 0,90 (IC 95% 0,81-0,99). Conclusión. La técnica de aglutinación directa estandarizada podría ser útil para el inmunodiagnóstico de la enfermedad de Chagas.

Introduction: Chagas´ disease is caused by the parasite Trypanosoma cruzi and its immunological diagnosis is mainly based on the detection of antibodies against T. cruzi using tests such as the ELISA, the indirect fluorescence antibody test (IFAT) and the indirect hemagglutination test (IHAT). The main disadvantage of the IHAT is the need to prepare sheep erythrocytes, whose availability is limited and they have a short duration once prepared. However, there are alternative tests, such as the direct agglutination test (DAT). Objective: To standardize the direct agglutination test for the diagnosis of Chagas disease. Materials and methods: Trypanosoma cruzi epimastigotes were prepared using two protocols, with and without trypsin treatment. The parasites were stained and optimal conditions for parasitic concentration and serum dilutions were determined. We evaluated the technique using sera from patients with Chagas disease, from healthy individuals and from individuals with other parasitic diseases. Results: The optimal parasitic concentration was 500 x 10 6 parasites/ml using stained parasites without trypsin treatment. The optimal serum dilutions were 1/25, 1/50 y 1/100 and the cut-off point was the 1/50 dilution. The diagnostic indices for the standardized technique were as follows: Sensitivity, 94.3% (95% CI: 79.5-99.0) and specificity, 96.3% (95% CI: 88.8-99.0), with positive and negative predictive values ?? of 91.7% (95% CI: 76.4-97.8) and 97.5% (95% CI: 90.4-99.6), respectively. Cross-reaction was observed only in three sera from individuals with visceral leishmaniasis. The results were compared with those obtained by IHA, ELISA, and IFA, and the concordance rate was 96% and the kappa index, 0.90 (95% CI: 0.81-0.99). Conclusion: The standardized direct agglutination test could be useful for immunodiagnosis of Chagas disease.

Subject(s)

Humans , Antibodies, Protozoan/blood , Chagas Disease/diagnosis , Hemagglutination Tests/standards , Parasitemia/diagnosis , Trypanosoma cruzi/immunology , Antibody Specificity , Cross Reactions , Enzyme-Linked Immunosorbent Assay , False Negative Reactions , False Positive Reactions , Fluorescent Antibody Technique, Indirect , Leishmania donovani/immunology , Parasite Load , Predictive Value of Tests , Parasitic Diseases/diagnosis , Retrospective Studies , Sensitivity and Specificity

17.

Cisteínoproteasas Catepsinas L de Taenia solium: Rol biológico en la infección y potencial uso para el inmunodiagnóstico de la neurocisticercosis / Cathepsin L Cysteine Protease from Taenia solium: Its biological role in the infection and potential use for the immunodiagnosis of neurocysticercosis

León, Nancy; Padilla, Carlos; Pajuelo, Mónica; Sheen, Patricia; Zimic, Mirko.

Rev. peru. med. exp. salud publica ; 30(3): 446-454, jul.-sep. 2013. ilus, graf, tab

Article in Spanish | LILACS, LIPECS | ID: lil-688045

ABSTRACT

Taenia solium es un helminto aplanado responsable de la teniosis y de la cisticercosis humana, siendo esta última producida por el consumo de huevos infectivos. Los cisticercos pueden desarrollarse en diferentes tejidos del hombre, frecuentemente en el sistema nervioso central causando la neurocisticercosis (NCC). Para el diagnóstico de la NCC se requiere de una adecuada interpretación de datos clínicos, resultados de neuroimagen y pruebas serológicas. Sin embargo, las pruebas serológicas podrían mejorarse con el desarrollo de antígenos candidatos capaces de incrementar su sensibilidad y especificidad. En los últimos años se han descrito una serie de proteínas de superficie y de secreción de T. solium esenciales para la interacción parásito-hospedero. Una de estas familias son las cisteínoproteasas catepsinas L, las cuales cumplen un rol preponderante para el desarrollo y supervivencia del parásito, participando en la invasión tisular, la evasión de la respuesta inmune, el desenquistamiento y enquistamiento del cisticerco. Son consideradas como antígenos potenciales para el inmunodiagnóstico de la neurocisticercosis.

Taenia solium is a plane helminth responsible for taeniasis and human cysticercosis, the latter being the result of the consumption of infective eggs. Cysticerci can develop in different human tissues, often in the central nervous system, causing neurocysticercosis (NCC). For the diagnosis of NCC, an adequate interpretation of clinical data, neuroimaging results and serological tests are required. However, serological tests could be improved by developing candidate antigens able to increase their sensibility and specificity. In the last years, a series of surface and secretory proteins of T. solium essential for the parasite-host interaction have been described. One of these families is cathepsin L cysteine proteases, which have a predominant role in the development and survival of the parasite. They take part in the tissue invasion, immune response evasion, excystation and encystment of cysticercus. They are considered potential antigens for the immunodiagnosis of neurocysticercosis.

Subject(s)

Animals , Humans , Cathepsin L/physiology , Neurocysticercosis/diagnosis , Neurocysticercosis/immunology , Taenia solium/pathogenicity , Cathepsin L/analysis , Immunologic Tests , Taenia solium/enzymology , Taenia solium/immunology

18.

Recent applications of basophil activation tests in the diagnosis of drug hypersensitivity

Woo-Jung SONG; Yoon-Seok CHANG.

Asia Pacific Allergy ; (4): 266-280, 2013.

Article in English | WPRIM | ID: wpr-749959

ABSTRACT

Immediate-type drug hypersensitivity is an increasingly significant clinical issue; however, the diagnosis is frequently hindered due to lack of safe and precise diagnostic tests. Flow cytometry-assisted basophil activation test is a safe in vitro diagnostic tool for assessing basophil activation upon allergen stimulation. In this review, we have summarized current literature on the diagnostic utilities, new indications, and methodological aspects of the basophil activation test for the diagnosis of drug hypersensitivity.

Subject(s)

Basophils , Diagnosis , Diagnostic Tests, Routine , Drug Hypersensitivity , Immunologic Tests , In Vitro Techniques

19.

The trend of development of clinical immunology in laboratory medicine / 中华检验医学杂志

Lanlan WANG.

Chinese Journal of Laboratory Medicine ; (12): 29-31, 2013.

Article in Chinese | WPRIM | ID: wpr-432413

ABSTRACT

With the rapid development of the individual medical care in the 21st century,based on the quick advancement of the preclinical immunology as well as the relevant bioscience technology,the application of clinical immunological diagnostic inspection has been involved in multiple diseases,including the investigation of the pathology,diagnosis,selection of the treatment regime and the evaluation of the therapy efficacy.Along with the further research,novel means of the treatment and the inspection technology have been to be utilized or explored.The focus should be concentrated on the utilization of the new technologies,new ways of the clinical immunological inspection,improving the fabric of the knowledge and the application ability of the professionals in this major,in order to provide effective service to the clinical medical care and the health of the patients.

20.

The expression and significance of P57KIP2 in hydatidifotrm mole / 中国基层医药

Yuan YANG.

Chinese Journal of Primary Medicine and Pharmacy ; (12): 1331-1332, 2012.

Article in Chinese | WPRIM | ID: wpr-426215

ABSTRACT

Objective To study the expression and significance of P57KIP2 in complete mole(CM ) and partial mole(PM).Methods The expression of P57KIP2 in histology unequivocal 45 cases of CM and 30 cases of PM was detected by immunohistochemistry method.Results In the PMs,expression of P57kip2 was strongly and continuously(30/34),in the CMs,it was absent or weak expressed (5/45).The difference of P57K1P2 expression between PMs and CMs was statistically significant( P ＜ 0.05 ).Conclusion P57KIP2 immunostaining is a sensitive sign of partial moleand in differential diagnosis of PM from CM and it is deserving of clinical application.

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