Teste rápido de aglutinação utilizando partículas de látex para a detecção de anticorpos anti-cisticercos em amostras de líquido cefalorraquidiano (LCR)

Simple and rapid latex-based diagnostic tests have been used for detecting specific antigens or antibodies in several diseases. In this article, we present the preliminary results obtained with a latex agglutination test (LAT) for diagnosing neurocysticercosis by detection of antibodies in CSF. A total of 43 CSF samples were assayed by the LAT: 19 CSF samples from patients with neurocysticercosis and 24 CSF samples from patients with other neurologic disorders (neurosyphilis, n = 8; neurotoxoplasmosis, n = 3; viral meningitis, n = 4, chronic headache, n = 9). The LAT exhibited 89.5% sensitivity and 75% specificity. The use of LAT seems to be an additional approach for the screening of neurocysticercosis with advantage of simplicity and rapidity. Further studies could be performed using purified antigens and serum samples.Testes diagnósticos simples e rápidos baseados na aglutinação de partículas de látex têm sido utilizados para a pequisa de antígenos ou anticorpos específicos em muitas doenças. No presente trabalho, é descrito um teste de aglutinação em lâmina para a pesquisa de anticorpos contra cisticercos de Taenia solium, utilizando partículas de látex revestidas com um extrato bruto do parasita. Anticorpos anti-cisticercos foram pesquisados em 19 amostras de LCR de pacientes com neurocisticercose e em 24 amostras de LCR de pacientes com outros problemas neurológicos (neurosífilis, n = 8; neurotoxoplasmose, n = 3; meningite viral, n = 4; cefaléia crônica, n = 9). O teste de aglutinação apresentou sensibilidade e especificidade de 89,5% e 75%, respectivamente. O teste de aglutinação para cisticercose idealizado é simples, rápido e barato. Essas características tornam o teste um meio promissor de expansão e simplificação do imunodiagnósico da neurocisticercose. Estudos futuros poderiam testar a sensibilização das partículas de látex com antígenos de cisticercos purificados e a pesquisa de anticorpos em amostras de soros

Teste rápido de aglutinação utilizando partículas de látex para a detecção de anticorpos anti-cisticercos em amostras de líquido cefalorraquidiano (LCR)

Simple and rapid latex-based diagnostic tests have been used for detecting specific antigens or antibodies in several diseases. In this article, we present the preliminary results obtained with a latex agglutination test (LAT) for diagnosing neurocysticercosis by detection of antibodies in CSF. A total of 43 CSF samples were assayed by the LAT: 19 CSF samples from patients with neurocysticercosis and 24 CSF samples from patients with other neurologic disorders (neurosyphilis, n = 8; neurotoxoplasmosis, n = 3; viral meningitis, n = 4, chronic headache, n = 9). The LAT exhibited 89.5% sensitivity and 75% specificity. The use of LAT seems to be an additional approach for the screening of neurocysticercosis with advantage of simplicity and rapidity. Further studies could be performed using purified antigens and serum samples.Testes diagnósticos simples e rápidos baseados na aglutinação de partículas de látex têm sido utilizados para a pequisa de antígenos ou anticorpos específicos em muitas doenças. No presente trabalho, é descrito um teste de aglutinação em lâmina para a pesquisa de anticorpos contra cisticercos de Taenia solium, utilizando partículas de látex revestidas com um extrato bruto do parasita. Anticorpos anti-cisticercos foram pesquisados em 19 amostras de LCR de pacientes com neurocisticercose e em 24 amostras de LCR de pacientes com outros problemas neurológicos (neurosífilis, n = 8; neurotoxoplasmose, n = 3; meningite viral, n = 4; cefaléia crônica, n = 9). O teste de aglutinação apresentou sensibilidade e especificidade de 89,5% e 75%, respectivamente. O teste de aglutinação para cisticercose idealizado é simples, rápido e barato. Essas características tornam o teste um meio promissor de expansão e simplificação do imunodiagnósico da neurocisticercose. Estudos futuros poderiam testar a sensibilização das partículas de látex com antígenos de cisticercos purificados e a pesquisa de anticorpos em amostras de soros.575

How much leaf area do insects eat? A data set of insect herbivory sampled globally with a standardized protocol

Herbivory is ubiquitous. Despite being a potential driver of plant distribution and performance, herbivory remains largely undocumented. Some early attempts have been made to review, globally, how much leaf area is removed through insect feeding. Kozlov et al., in one of the most comprehensive reviews regarding global patterns of herbivory, have compiled published studies regarding foliar removal and sampled data on global herbivory levels using a standardized protocol. However, in the review by Kozlov et al., only 15 sampling sites, comprising 33 plant species, were evaluated in tropical areas around the globe. In Brazil, which ranks first in terms of plant biodiversity, with a total of 46,097 species, almost half (43%) being endemic, a single data point was sampled, covering only two plant species. In an attempt to increase knowledge regarding herbivory in tropical plant species and to provide the raw data needed to test general hypotheses related to plant–herbivore interactions across large spatial scales, we proposed a joint, collaborative network to evaluate tropical herbivory. This network allowed us to update and expand the data on insect herbivory in tropical and temperate plant species. Our data set, collected with a standardized protocol, covers 45 sampling sites from nine countries and includes leaf herbivory measurements of 57,239 leaves from 209 species of vascular plants belonging to 65 families from tropical and temperate regions. They expand previous data sets by including a total of 32 sampling sites from tropical areas around the globe, comprising 152 species, 146 of them being sampled in Brazil. For temperate areas, it includes 13 sampling sites, comprising 59 species

Intrathecal Synthesis Of Specific Immunoglobulin G Antibodies In Neurocysticercosis: Evaluation Of Antibody Concentrations By Enzyme-linked Immunosorbent Assay Using A Whole Cysticercal Extract And Cyst Vesicular Fluid As Antigens.

The demonstration of intrathecal antibody production has proven useful for showing the involvement of the central nervous system (CNS) in several diseases. In the present study, the intrathecal synthesis of cysticercus-specific immunoglobulin G (IgG) antibodies was investigated in 30 patients with neurocysticercosis based on calculation of the specific IgG antibody index (AI(IgG)). An AI(IgG) > or =1.5 was considered to be indicative of intrathecal antibody production. Antibody concentrations in serum and cerebrospinal fluid samples were evaluated using an enzyme-linked immunosorbent assay with 2 antigen preparations from Taenia solium cysticerci, namely, a whole cysticercal extract (TsoW) and the vesicular fluid of the parasite (TsoVF). Intrathecal, cysticercus-specific IgG antibody synthesis was observed in 21 (70%) and 23 (76.6%) patients using the TsoW and TsoVF antigens, respectively. The detection of the intrathecal synthesis of specific antibodies may be a potentially useful tool in establishing the involvement of CNS in cysticercosis.5445-

A Rapid Latex Agglutination Test For The Detection Of Anti-cysticercus Antibodies In Cerebrospinal Fluid (csf).

Simple and rapid latex-based diagnostic tests have been used for detecting specific antigens or antibodies in several diseases. In this article, we present the preliminary results obtained with a latex agglutination test (LAT) for diagnosing neurocysticercosis by detection of antibodies in CSF. A total of 43 CSF samples were assayed by the LAT: 19 CSF samples from patients with neurocysticercosis and 24 CSF samples from patients with other neurologic disorders (neurosyphilis, n = 8; neurotoxoplasmosis, n = 3; viral meningitis, n = 4, chronic headache, n = 9). The LAT exhibited 89.5% sensitivity and 75% specificity. The use of LAT seems to be an additional approach for the screening of neurocysticercosis with advantage of simplicity and rapidity. Further studies could be performed using purified antigens and serum samples.4457-