Estudo comparativo entre teste rápido imunológico (LID-NDO) e PCR tempo real de raspado dérmico em álcool e em papel-filtro na hanseníase / Comparative study between immunological rapid test (LID-NDO) and real-time PCR of dermal smear in alcohol and filter paper in leprosy

Silva, Gabriela Pagano de Oliveira Gonçalves da

13 March 2017

A hanseníase é uma doença infecciosa que acomete pele e nervos periféricos. Seu diagnóstico é baseado eminentemente nos seus aspectos clínicos variáveis e poucos são os exames complementares que auxiliam no diagnóstico, como baciloscopia do raspado intradérmico, histopatologia, ELISA anti- PGL1 (APGL1) e anti-LID, geralmente positivos nas formas multibacilares, dificultando o diagnóstico das formas paucibacilares. Busca-se comparar os resultados obtidos com o teste rápido imunológico (LID-NDO) Orange Life® com os resultados da PCR tempo real realizada nas amostras de raspado intradérmico e os resultados do ELISA APGL1 coletadas durante a ação por demanda espontânea (Hanseníase Brasília 2014), além de comparar eficiência entre dois métodos diferentes de conservação destas amostras (papel-filtro x álcool). Foram coletadas 277 amostras de raspado dérmico de 50 pacientes clinicamente diagnosticados com hanseníase durante a ação. Na mesma ocasião, os indivíduos diagnosticados foram submetidos à coleta de sangue periférico para teste rápido sorológico (Orange Life®) e ELISA APGL1. A extração de DNA do raspado intradérmico, armazenado no álcool e no papel-filtro, foi realizada no Laboratório de Dermatologia do HC-FMRP-USP. A PCR em tempo real foi realizada usando par de primers específicos RLEP, e o master mix sybr greenPromega. Dos 50 pacientes diagnosticados clinicamente, 90% são multibacilares. Todos os testes, tanto o teste rápido sorológico como a PCR, apresentaram maior positividade nos pacientes multibacilares. O teste rápido sorológico foi positivo em 64,44% dos pacientes multibacilares e em 40% dos paucibacilares. A PCR nas amostras armazenadas no álcool foi positiva em 19,05% dos pacientes multibacilares e a PCR do papel-filtro em 17,78%; nenhuma PCR foi positiva em pacientes paucibacilares. O ELISA APGL foi positivo em 56% dos pacientes diagnosticados. Na PCR das amostras armazenadas no papel-filtro, o sítio de coleta com maior positividade foram os cotovelos (75%). A concordância entre o teste rápido sorológico e a PCR e a concordância entre o teste rápido e o ELISA APGL1 foram fair (suave). Já a concordância entre a PCR das amostras armazenadas no álcool e a PCR das amostras armazenadas no papel-filtro foi perfeita. Concluímos que o exame clínico é ainda essencial para o diagnóstico da hanseníase, principalmente das formas paucibacilares. Os métodos de armazenamento do material coletado por raspado intradérmico (papel-filtro x álcool) não interferiram no resultado final da PCR, portanto o armazenamento no papel-filtro pode ser feito preferencialmente, pois apresenta menor custo para a extração de DNA. O teste rápido sorológico e o ELISA anti-PGL1 têm baixa especificidade, porém podem ter outras aplicações, diferentes do diagnóstico da hanseníase. / Leprosy is an infectious disease that affects skin and peripheral nerves. Leprosy diagnosis is mainly based on its variable clinical aspects and few complementary tests that aid in the diagnosis, such as bacilloscopy, histopathology, besides the antiPGL1 ELISA (APGL1) and anti-LID, all of which are generally positive in multibacillary forms, confirming the difficulty in diagnosis of paucibacillary patients. The aim of this study was to compare the results obtained with the Orange Life® Immunological Rapid Test (LID-NDO) with the real-time PCR results obtained in the intradermal scraping samples and the results of the ELISA APGL1, collected during the \"Hanseníase\" action in Brasília in January 2014, in addition to comparing efficiency between two different methods of preservation of these samples (filter paper x alcohol). A total of 277 dermal smear samples were collected from 50 patients clinically diagnosed with leprosy during the procedure. At the same time, the individuals diagnosed were submitted to peripheral blood collection for serological rapid test (Orange Life®) and ELISA APGL1. The extraction of DNA from intradermal scrapings, stored in alcohol and filter paper, was carried out at the Dermatology Laboratory of HC-FMRP-USP. Real-time PCR was performed using a pair of primers specific for the RLEP gene, and the master sybr green-Promega. From 50 patients diagnosed clinically, 90% are multibacillary. All tests, both the serological rapid test and the PCR, were more positive in multibacillary patients. The rapid serological test was positive in 64.44% of the multibacillary patients, and in 40% of the paucibacillary. The PCR in the samples stored in the alcohol was positive in 19.05% of the multibacillary patients and the PCR of the filter paper in 17.78%; PCR weren\'t positive in paucibacillary patients. ELISA APGL was positive in 56% (28) of the diagnosed patients. In the PCR of the samples stored in the filter paper, the collection site with the highest positivity was the elbows (75%). The agreement between the rapid serological test and the PCR and the agreement between the rapid test and the ELISA APGL1 were fair. The agreement between the PCR of the samples stored in the alcohol and the PCR of the samples stored on the filter paper was perfect. We conclude that the clinical examination is still essential for the diagnosis of leprosy, especially in paucibacillary forms. We also concluded that the methods of storing the material collected by intradermal scraping (filter paper x alcohol) do not interfere in the final result of the PCR, therefore the storage in the filter paper can be done preferentially because it presents a lower cost for the extraction of DNA. Rapid serological test and the anti-PGL1 ELISA have low specificity, but may have other different applications than the diagnosis of leprosy.

anti-PGL1 ELISA

Diagnosis

Diagnóstico

ELISA antiPGL1

Hanseníase

Leprosy

PCR

PCR

Serological test

Teste sorológico

Estudo comparativo entre teste rápido imunológico (LID-NDO) e PCR tempo real de raspado dérmico em álcool e em papel-filtro na hanseníase / Comparative study between immunological rapid test (LID-NDO) and real-time PCR of dermal smear in alcohol and filter paper in leprosy

Gabriela Pagano de Oliveira Gonçalves da Silva

13 March 2017

A hanseníase é uma doença infecciosa que acomete pele e nervos periféricos. Seu diagnóstico é baseado eminentemente nos seus aspectos clínicos variáveis e poucos são os exames complementares que auxiliam no diagnóstico, como baciloscopia do raspado intradérmico, histopatologia, ELISA anti- PGL1 (APGL1) e anti-LID, geralmente positivos nas formas multibacilares, dificultando o diagnóstico das formas paucibacilares. Busca-se comparar os resultados obtidos com o teste rápido imunológico (LID-NDO) Orange Life® com os resultados da PCR tempo real realizada nas amostras de raspado intradérmico e os resultados do ELISA APGL1 coletadas durante a ação por demanda espontânea (Hanseníase Brasília 2014), além de comparar eficiência entre dois métodos diferentes de conservação destas amostras (papel-filtro x álcool). Foram coletadas 277 amostras de raspado dérmico de 50 pacientes clinicamente diagnosticados com hanseníase durante a ação. Na mesma ocasião, os indivíduos diagnosticados foram submetidos à coleta de sangue periférico para teste rápido sorológico (Orange Life®) e ELISA APGL1. A extração de DNA do raspado intradérmico, armazenado no álcool e no papel-filtro, foi realizada no Laboratório de Dermatologia do HC-FMRP-USP. A PCR em tempo real foi realizada usando par de primers específicos RLEP, e o master mix sybr greenPromega. Dos 50 pacientes diagnosticados clinicamente, 90% são multibacilares. Todos os testes, tanto o teste rápido sorológico como a PCR, apresentaram maior positividade nos pacientes multibacilares. O teste rápido sorológico foi positivo em 64,44% dos pacientes multibacilares e em 40% dos paucibacilares. A PCR nas amostras armazenadas no álcool foi positiva em 19,05% dos pacientes multibacilares e a PCR do papel-filtro em 17,78%; nenhuma PCR foi positiva em pacientes paucibacilares. O ELISA APGL foi positivo em 56% dos pacientes diagnosticados. Na PCR das amostras armazenadas no papel-filtro, o sítio de coleta com maior positividade foram os cotovelos (75%). A concordância entre o teste rápido sorológico e a PCR e a concordância entre o teste rápido e o ELISA APGL1 foram fair (suave). Já a concordância entre a PCR das amostras armazenadas no álcool e a PCR das amostras armazenadas no papel-filtro foi perfeita. Concluímos que o exame clínico é ainda essencial para o diagnóstico da hanseníase, principalmente das formas paucibacilares. Os métodos de armazenamento do material coletado por raspado intradérmico (papel-filtro x álcool) não interferiram no resultado final da PCR, portanto o armazenamento no papel-filtro pode ser feito preferencialmente, pois apresenta menor custo para a extração de DNA. O teste rápido sorológico e o ELISA anti-PGL1 têm baixa especificidade, porém podem ter outras aplicações, diferentes do diagnóstico da hanseníase. / Leprosy is an infectious disease that affects skin and peripheral nerves. Leprosy diagnosis is mainly based on its variable clinical aspects and few complementary tests that aid in the diagnosis, such as bacilloscopy, histopathology, besides the antiPGL1 ELISA (APGL1) and anti-LID, all of which are generally positive in multibacillary forms, confirming the difficulty in diagnosis of paucibacillary patients. The aim of this study was to compare the results obtained with the Orange Life® Immunological Rapid Test (LID-NDO) with the real-time PCR results obtained in the intradermal scraping samples and the results of the ELISA APGL1, collected during the \"Hanseníase\" action in Brasília in January 2014, in addition to comparing efficiency between two different methods of preservation of these samples (filter paper x alcohol). A total of 277 dermal smear samples were collected from 50 patients clinically diagnosed with leprosy during the procedure. At the same time, the individuals diagnosed were submitted to peripheral blood collection for serological rapid test (Orange Life®) and ELISA APGL1. The extraction of DNA from intradermal scrapings, stored in alcohol and filter paper, was carried out at the Dermatology Laboratory of HC-FMRP-USP. Real-time PCR was performed using a pair of primers specific for the RLEP gene, and the master sybr green-Promega. From 50 patients diagnosed clinically, 90% are multibacillary. All tests, both the serological rapid test and the PCR, were more positive in multibacillary patients. The rapid serological test was positive in 64.44% of the multibacillary patients, and in 40% of the paucibacillary. The PCR in the samples stored in the alcohol was positive in 19.05% of the multibacillary patients and the PCR of the filter paper in 17.78%; PCR weren\'t positive in paucibacillary patients. ELISA APGL was positive in 56% (28) of the diagnosed patients. In the PCR of the samples stored in the filter paper, the collection site with the highest positivity was the elbows (75%). The agreement between the rapid serological test and the PCR and the agreement between the rapid test and the ELISA APGL1 were fair. The agreement between the PCR of the samples stored in the alcohol and the PCR of the samples stored on the filter paper was perfect. We conclude that the clinical examination is still essential for the diagnosis of leprosy, especially in paucibacillary forms. We also concluded that the methods of storing the material collected by intradermal scraping (filter paper x alcohol) do not interfere in the final result of the PCR, therefore the storage in the filter paper can be done preferentially because it presents a lower cost for the extraction of DNA. Rapid serological test and the anti-PGL1 ELISA have low specificity, but may have other different applications than the diagnosis of leprosy.

Diagnóstico

ELISA antiPGL1

Hanseníase

PCR

Teste sorológico

anti-PGL1 ELISA

Diagnosis

Leprosy

PCR

Serological test

Estudo da sensibilização de cães com dermatite atópica na região central do Rio Grande do Sul / Sensitization study of the dogs with atopic dermatitis in central region of Rio Grande do Sul

Pereira, Desydere Trindade

12 February 2015

Canine atopic dermatitis (CAD) is a common dermatosis, defined as a genetic-based disease, which predisposes to cutaneous inflammation and pruritus, mediated by class IgE immunoglobulins directed against specific antigens in most cases. Clinical diagnosis may be later complemented by skin allergic and/or serological tests (ELISA). The aim of these tests is to identify possible allergens in order to enable the clinicians to select candidate antigens for allergen specific immunotherapy. This work aimed to identify the sensitization profile of 58 dogs with atopic dermatitis diagnosis. All animals were submitted to intradermic test (IDT) and screened for the presence of antibodies against different allergens using a serologic test. House dust mites are described as the most frequent allergens in all continents. However, the positivity to C. dactylon is not commonly described and may be characteristic for the region. With this work it was possible to identify the main allergens involved in the immunologic response of atopic dogs residing in Rio Grande do Sul, pointing to the importance to include C. dactylon in screening tests for allergy. / A dermatite atópica canina (DAC) é uma dermatose comum, definida como uma doença de cunho genético que predispõe à inflamação e ao prurido cutâneo, mediada por imunoglobulinas da classe IgE dirigidas contra antígenos específicos na maior parte dos casos. O diagnóstico da DAC é clínico e pode ser posteriormente complementado por testes alérgicos cutâneos e/ou sorológicos. O objetivo desses testes é identificar possíveis alérgenos e, com isso, possibilitar ao clínico a seleção de antígenos candidatos para a imunoterapia alérgeno-específica. No presente trabalho buscou-se identificar o perfil de sensibilização de 58 cães diagnosticados com dermatite atópica. Todos os animais foram submetidos ao teste intradérmico (TID) e à detecção de anticorpos específicos para diferentes alérgenos através de teste sorológico (ELISA). Os ácaros domiciliares são descritos como os alérgenos mais frequentes em todos os continentes. Entretanto, a positividade ao C. dactylon não é usualmente descrita e pode ser característica da região. Com esse trabalho foi possível identificar os principais alérgenos envolvidos na resposta imunológica de cães atópicos residentes no Rio Grande do Sul, ressaltando-se a importância da inclusão do extrato de C. dactylon em testes alérgicos.

Teste intradérmico

Teste sorológico

Ácaros da poeira domiciliar

Ácaros de produtos armazenados

Cynodon dactylon

Intradermal test

Serological test

House dust mites

Storage mites

Cynodon dactylon

A Quantitative ELISA to Detect Anti-SARS-CoV-2 Spike IgG Antibodies in Infected Patients and Vaccinated Individuals

Luo, Ji, Klett, Jennifer, Gabert, Jörg, Lipp, Thomas, Karbach, Julia, Jäger, Elke, Borte, Stephan, Hoffmann, Ralf, Milkovska-Stamenova, Sanja

14 March 2024

There is an ongoing need for high-precision serological assays for the quantitation of anti-SARS-CoV-2 antibodies. Here, a trimeric SARS-CoV-2 spike (S) protein was used to develop an ELISA to quantify specific IgG antibodies present in serum, plasma, and dried blood spots (DBS) collected from infected patients or vaccine recipients. The quantitative S-ELISA was calibrated with international anti-SARS-CoV-2 immunoglobulin standards to provide test results in binding antibody units per mL (BAU/mL). The assay showed excellent linearity, precision, and accuracy. A sensitivity of 100% was shown for samples collected from 54 patients with confirmed SARS-CoV-2 infection more than 14 days after symptom onset or disease confirmation by RT-PCR and 58 vaccine recipients more than 14 days after vaccination. The assay specificity was 98.3%. Furthermore, antibody responses were measured in follow-up samples from vaccine recipients and infected patients. Most mRNA vaccine recipients had a similar response, with antibody generation starting 2–3 weeks after the first vaccination and maintaining positive for at least six months after a second vaccination. For most infected patients, the antibody titers increased during the second week after PCR confirmation. This S-ELISA can be used to quantify the seroprevalence of SARS-CoV-2 in the population exposed to the virus or vaccinated.

info:eu-repo/classification/ddc/570

ddc:570

info:eu-repo/classification/ddc/610

ddc:610