Your search keyword '"Immunochromatographic test"' showing total 699 results

1. Rapid immunochromatographic test: An evolving tool for diagnosis of scrub typhus

Author

Sabyasachi Saha, Sanjit Kumar Patra, Mrinmoy Pathak, Jayanta Bikash Dey, Tapashi Ghosh, and Sohanjan Chakraborty

Subjects

rapid immunochromatographic test, diagnosis, scrub typhus, evolving tool, Medicine

Abstract

Background: Scrub typhus is prevalent in many districts of South Bengal throughout the year where an average temperature of 20–35°C, which contributes to the spread of Leptotrombidium deliense. However, its diagnosis remains complicated by the lack of readily available and validated assays, the non-specificity of clinical symptoms on admission, and even non-availability of the pathognomonic eschar in most of the cases. Aims and Objectives: This study was carried out to evaluate the rapid immunochromatographic test (RICT) for early detection of scrub typhus for using it as an early diagnostic tool at the field level. Materials and Methods: This cross-sectional study in which 181 serum samples from clinically suspected cases (after excluding dengue, malaria, Japanese encephalitis, and typhoid fever) collected over 13 months were processed for the detection of immunoglobulin M (IgM) antibodies for scrub typhus by enzyme-linked immunosorbent assay (ELISA) and rapid test. Results: Considering IgM ELISA for scrub typhus as the gold standard, the sensitivity, specificity, positive predictive value, and negative predictive value for RICT were found to be 100%, 86.87%, 50%, and 100%, respectively. Conclusion: RICT is a simple, rapid, and reliable assay for diagnosis of scrub typhus, capable of providing accurate results quickly and is highly suitable for field deployment in remote areas with limited medical support.

Published

2023

2. Analytical performance evaluation of a rapid immunochromatographic test for the diagnosis of bovine brucellosis based on a recombinant BP26 protein

Author

P.G. Souza, P.A. Lima, P.M. Soares Filho, R.N. Etges, R.R. Nicolino, A.G. Viana, T.A. Paixão, R.T. Fujiwara, and R.L. Santos

Subjects

Brucella abortus, BP26, serology, diagnosis, Animal culture, SF1-1100

Abstract

ABSTRACT Brucellosis is an important bacterial disease of global distribution with zoonotic potencial. Serological tests used in Brazil for diagnosis of bovine brucellosis, including the Rose Bengal test (RBT), 2-mercaptoethanol (2-ME), fluorescent polarization (FPA), and complement fixation (FC), are based on the smooth lipopolysaccharide antigen (S-LPS) of Brucella abortus. The aim of this study was to evaluate a recombinant BP26 protein used as antigen in a rapid lateral flow immunochromatographic assay (rBP26-LFIA) for serological diagnosis of bovine brucellosis. Analytical performance of rBP26-LFIA was evaluated in positive and negative bovine serum samples previously characterized by RBT and 2-ME. Estimates of analytical sensitivity and specificity were 73.91% and 97.14%, respectively. Bovine sera reactive to Neospora, Trypanosoma vivax or Leptospira were used to assess specificity because these diseases are commonly associated with abortion in cattle. In addition to a possible cross-reaction induced by commercial vaccines against Leptospira in serological tests for bovine brucellosis using S-LPS as an antigen. In conclusion, rBP26-LFIA, with its current standardization, had good analytical performance. However, a future evaluation of diagnostic performance by rBP26-LFIA with samples from regions with known prevalence is necessary for its recommendation for use in the Brazilian program for the control and eradication of bovine brucellosis.

Published

2024

3. Diagnostic performance of CL Detect rapid-immunochromatographic test for cutaneous leishmaniasis: a systematic review and meta-analysis

Author

Gebremeskele, Behailu Taye, Adane, Gashaw, Adem, Mohammed, and Tajebe, Fitsumbrhan

Published

2023

4. Diagnostic performance of CL Detect rapid-immunochromatographic test for cutaneous leishmaniasis: a systematic review and meta-analysis

Author

Behailu Taye Gebremeskele, Gashaw Adane, Mohammed Adem, and Fitsumbrhan Tajebe

Subjects

Cutaneous leishmaniasis, CL Detect rapid test, Diagnosis, Systematic review, Meta-analysis, Medicine

Abstract

Abstract Background Sensitive, robust, and fast point-of-care tests are needed for cutaneous leishmaniasis (CL) diagnosis. The recently developed CL Detect rapid test (InBios) for detecting Leishmania peroxidoxin antigen has been evaluated in several studies. However, diagnostic performances were controversial. Therefore, this systematic review and meta-analysis aimed to determine the pooled sensitivity and specificity of CL Detect for CL diagnosis. Methods PubMed, Scopus, EMBASE, ScienceDirect, and Google Scholar were sources of articles. We included studies reporting the diagnostic accuracy of CL Detect and CL-suspected patients in the English language. The methodological qualities of the included studies were appraised using the quality assessment of diagnostic accuracy studies-2 (QUADAS‐2). Meta-analysis was conducted using Stata 14.2 and R software. Results A total of 9 articles were included. The study sample size ranged from 11 to 274. The sensitivities of the individual studies ranged from 23 to 100%, and the specificities ranged from 78 to 100%. Pooled sensitivity and specificity were 68% (95% CI, 41–86%) and 94% (95% CI, 87–97%), respectively. AUC displayed 0.899. Pooled sensitivity was lower (47%, 95% CI, 34–61%) when PCR was used as a reference than microscopy (83%, 95% CI, 39–97%). Pooled sensitivity was lower (48%, 95% CI, 30–67%) for all lesion durations compared to ≤ 4 months (89%, 95% CI, 43–99%). Conclusions CL Detect has poor sensitivity and does not meet the minimal sensitivity of 95% of target product profiles designed for CL point-of-care tests. Currently, the CL Detect test looks unsuitable for CL diagnosis, despite its high specificity. Findings are limited by the low number of studies available. Further large-scale studies are recommended. Systematic review registration PROSPERO CRD42022323497.

Published

2023

5. Rapid immunochromatographic test: An evolving tool for diagnosis of scrub typhus.

Author

Saha, Sabyasachi, Patra, Sanjit Kumr, Pathak, Mrinmoy, Dey, Jayanta Bikash, Ghosh, Tapashi, and Chakraborty, Sohanjan

Subjects

*TSUTSUGAMUSHI disease, *JAPANESE B encephalitis, *IMMUNOGLOBULIN M, *ENZYME-linked immunosorbent assay, *TYPHOID fever, *DIAGNOSIS

Abstract

Background: Scrub typhus is prevalent in many districts of South Bengal throughout the year where an average temperature of 20-35°C, which contributes to the spread of Leptotrombidium deliense. However, its diagnosis remains complicated by the lack of readily available and validated assays, the non-specificity of clinical symptoms on admission, and even non-availability of the pathognomonic eschar in most of the cases. Aims and Objectives: This study was carried out to evaluate the rapid immunochromatographic test (RICT) for early detection of scrub typhus for using it as an early diagnostic tool at the field level. Materials and Methods: This cross-sectional study in which 181 serum samples from clinically suspected cases (after excluding dengue, malaria, Japanese encephalitis, and typhoid fever) collected over 13 months were processed for the detection of immunoglobulin M (IgM) antibodies for scrub typhus by enzyme-linked immunosorbent assay (ELISA) and rapid test. Results: Considering IgM ELISA for scrub typhus as the gold standard, the sensitivity, specificity, positive predictive value, and negative predictive value for RICT were found to be 100%, 86.87%, 50%, and 100%, respectively. Conclusion: RICT is a simple, rapid, and reliable assay for diagnosis of scrub typhus, capable of providing accurate results quickly and is highly suitable for field deployment in remote areas with limited medical support. [ABSTRACT FROM AUTHOR]

Published

2023

6. RAPID ETIOLOGICAL DIAGNOSIS OF NEONATAL CALF DIARRHEA WITH IMMUNOCHROMATOGRAPHIC TEST KITS IN ESME DISTRICT OF USAK.

Author

SEZER, SALIH and AKGUL, GULŞAH

Subjects

*DIARRHEA, *CALVES, *ESCHERICHIA coli, *DATA distribution, *CLOSTRIDIUM perfringens, *ROTAVIRUSES, *DIAGNOSIS

Abstract

This study was carried out for rapid etiological diagnosis of neonatal calf diarrhea by using immunochromatographic test kits in the Eşme district of Uşak. The animal material of the study consisted of 100 1-28 days old neonatal calves of different breeds and genders in the Eşme district of Uşak. Stool samples were taken from calves with diarrhea as a result of clinical examination. When stool samples were examined by a rapid diagnostic test, none of the disease factors sought in the study were found in 10 (10%) of 100 calves, while one or more disease factors were detected in 90 (90%) of calves. Rotavirus was detected in 27 (27%) calves, Escherichia coli 14 (14%) calves, Coronavirus in 8 (8%) calves, Clostridium perfringens in 19 (19%) calves, Cryptosporidium spp. in 17 (17%) calves, Rotavirus + Coronavirus in 2 (2%) calves, Rotavirus + Clostridium perfringens in 1 (1%) calf, Rotavirus + Cryptosporidium spp. in 1 (1%) calf, and Escherichia coli - Clostridium perfringens in 1 (1%) calf. As a result, data on the presence and distribution of enterogenous pathogens that cause diarrhea in neonatal calves in the Eşme district of Uşak were presented, and it was concluded that it would shed light on future studies on diarrheal calves in the Eşme. [ABSTRACT FROM AUTHOR]

Published

2022

7. Traditional Widal Agglutination Test Versus Rapid Immunochromatographic Test in the Diagnosis of Enteric Fever: A Prospective Study From South India

Author

Reewen George D Silva, Roopa Shahapur, Anand V Nimbal, Venkataramana Kandi, Praveen R Shahapur, and Tarun Kumar Suvvari

Subjects

Serotype, medicine.medical_specialty, medicine.diagnostic_test, business.industry, diagnosis, immunochromatographic test, General Engineering, Widal test, Antibody titer, Gastroenterology, Infectious Disease, Gold standard (test), Salmonella typhi, medicine.disease, Typhoid fever, salmonella typhi, Direct agglutination test, Internal medicine, medicine, Blood culture, widal test, Public Health, business, typhoid

Abstract

Introduction Early diagnosis and treatment are crucial to reducing the morbidity of patients with enteric fever/typhoid fever. Among the available diagnostic tests, the blood culture is considered a gold standard. However, in most of the developing and resource-limited settings, the diagnosis is made utilizing the traditional Widal test and rapid immunochromatographic test (ICT). This study was aimed to compare the diagnostic value and efficacy of ICT and traditional Widal test in the diagnosis of typhoid fever. Methods A prospective study was conducted, and 40 patients were included in the study. The Widal test and Salmonella enterica serovar Typhi IgM/IgG immunochromatographic test were performed for all the patients. The Widal is a tube agglutination test, and the rapid ICT utilizes the principle of enzyme-linked immunosorbent assay (ELISA). All the samples were also tested for the presence of antibodies (IgG and IgM) against the S. enterica serovar Typhi and the titers against 'O' and 'H' antigens of S. enterica serovar Typhi. An antibody titer of 1:80 or more against the 'O' and 'H' antigen was considered positive. Results In the ICT, 24 samples (60%) tested positive for the IgM antibodies, and only 15 samples tested positive and for IgG antibodies. In the Widal test, 27 samples (67.6%) returned positive for antibodies against the S. enterica serovar Typhi 'O' antigen. The sensitivity (90% vs 72.73%), specificity (81.25% vs 64%), and accuracy (82.12% vs 64.87%) for the Widal test were found to be more when compared to the ICT. Conclusion The results indicate that the traditional Widal agglutination test is superior to the rapid ICT in the diagnosis of enteric fever. However, both these tests cannot be considered as gold standards for the diagnosis owing to their low positive predictive values.

Published

2021

8. Accuracy and reliability of an NS1 rapid immunochromatographic test for DENV-1 diagnosis at point of care and in the laboratory

Author

Verónica Elizabeth Mata, Sonia Regina Lambert Passos, Yara Hahr Marques Hökerberg, Guilherme Miguéis Berardinelli, Maria Angelica Borges dos Santos, Levy Vilas Boas Fukuoka, Anna Carolina Fontoura Seixas Rangel Maciel, Cintia Damasceno dos Santos Rodrigues, Aline da Silva Santos, and Raquel de Vasconcellos Carvalhaes de Oliveira

Subjects

Dengue, Sensitivity and specificity, Diagnosis, Point-of-care systems, NS1, Reproducibility of results, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Rapid immunochromatographic tests (ICT) for dengue non-structural protein 1 (NS1) have shown good performance for diagnosing acute-phase dengue in serum in laboratory settings, but rarely have been assessed in whole blood and at point of care (POC). This study compare the accuracy and inter- and intra-observer reliability of the NS1 Bioeasy™ ICT in whole blood at POC versus serum in the laboratory, during a DENV-1 epidemic. Methods Cross-sectional study involving 144 adults spontaneously demanding care in an emergency department within 4 days of onset of acute febrile illness. Accuracy of NS1 Bioeasy™ ICT was compared in whole blood and serum, both at 15 and 30 min, blinded to the reference RT-PCR or NS1 ELISA. Non-dengue patients were also tested for Zika virus with RT-PCR. Reliability of whole blood and serum readings by the same or different observers was measured by simple kappa (95% CI). Results At 15 min, sensitivity (Sn) of NS1 Bioeasy™ ICT in whole blood/POC was 76.7% (95% CI: 68.0–84.1) and specificity (Sp) was 87.0% (95% CI: 66.4–97.2). Sn in serum/laboratory was 82% (95% CI: 74.1–88.6) and Sp 100% (95% CI: 85.8–100). Positive likelihood ratio was 5.9 (95% CI: 2.0–17.0) for whole blood/POC and 19.8 (95% CI: 2.9–135.1) for serum/laboratory. Reliability of matched readings of whole blood/POC and serum/laboratory by the same observer (k = 0.83, 95% CI: 0.74–0.93) or different observers (k = 0.81, 95% CI: 0.72–0.92) was almost perfect, with higher discordant levels in the absence of dengue. Results did not differ statistically at 5%. Conclusions NS1 Bioeasy™ ICT in DENV-1 epidemics is a potentially confirmatory test. Invalid results at 15 min should be reread at 30 min. To optimize impact of implementing ICT in the management of false-negatives it should be incorporated into an algorithm according to setting and available specimen. Trial registration UTN U1111-1145-9451 .

Published

2017

9. Development of a prototype immunochromatographic test for rapid diagnosis of respiratory adenovirus infection

Author

Paulini, Inarei, Siqueira-Silva, Joselma, Thomaz, Luciana, Rocha, Leticia, Harsi, Charlotte, Bellei, Nancy, and Granato, Celso

Published

2017

10. Diagnostic Efficacy of Rapid Immunochromatographic Test in Diagnosis of Dengue Infection.

Author

Kaur, Charanjeev and Sharma, Sarbjeet

Subjects

*ARBOVIRUS diseases, *DENGUE, *DENGUE viruses, *MEDICAL sciences, *VIRUS diseases, *DIAGNOSIS

Abstract

Dengue is a mosquito-borne arboviral disease of grave public health concern worldwide. Early diagnosis and treatment is required to reduce morbidity & mortality from complications caused by secondary dengue infection. According to WHO, the three main diagnostic modalities for the diagnosis of dengue infection are cultivation and identification of viruses, molecular methods, and serology. Whereas virus cultivation is labour intensive and available only in reference laboratories, molecular methods require expensive infrastructure & expertise. Serology on the other hand not only less tedious but is also able to differentiate between primary and secondary dengue. This study was undertaken to evaluate the diagnostic efficacy of rapid immunochromatographic assay in the diagnosis of dengue infection as compared to ELISA. The study was conducted in the serology section of the Microbiology laboratory, Sri Guru Ram Das Institute of Medical Sciences, Amritsar. Blood samples from 429 patients with clinical suspicion of dengue virus infection were received in the lab from August 2020 to December 2020. All samples were subjected to rapid ICT and ELISA to detect NS1 Ag and IgM antibodies. The majority number of cases were observed in the age group of 31 to 40 years while the gender-wise ratio was 1.43:1 showing male preponderance. Out of 429 samples tested, 156 were reactive for either NS1 antigen or IgM antibodies by the ELISA method. Results of rapid ICT for NS1Ag and results of NS1Ag by ELISA were analyzed and compared. A sensitivity of 81.25% was noted and specificity of 100%. IgM detection by rapid ICT in comparison to IgM ELISA shows a sensitivity of 82.14% and specificity of 100%. Rapid ICT kits performed at par with the ELISA. Rapid immunochromatographic assays are important diagnostic tools in the identification of dengue and early treatment of dengue patients is possible, reducing mortality significantly. [ABSTRACT FROM AUTHOR]

Published

2022

11. Evaluation of a new brand of immunochromatographic test for visceral leishmaniasis in Brazil made available from 2018

Author

Mariana Lourenço Freire, Tália Santana Machado de Assis, Daniel Moreira de Avelar, Ana Rabello, and Gláucia Cota

Subjects

Visceral leishmaniasis, Diagnosis, Rapid test, Antigen rK39, Arctic medicine. Tropical medicine, RC955-962, Infectious and parasitic diseases, RC109-216

Abstract

ABSTRACT Immunochromatographic tests based on the recombinant antigen K39 represent a major advance in diagnosing visceral leishmaniasis (VL) in recent years. Some performance variations are expected and have occurred in the use of several commercial rapid tests, especially in different geographical settings. This is the first evaluation in the Americas of the test recently provided by the public health system in Brazil for the diagnostic of VL, the OnSite™ Leishmania IgG/IgM Combo. In this first clinical test evaluation, 113 VL-positive patient samples and 73 negative controls were tested and a sensitivity of 91.2% and specificity of 94.5% were observed. These results indicate the need for further analysis and comparisons with the performance of other available commercial tests in order to define the impact of this new test on the quality of VL diagnosis in Brazil.

Published

2018

12. Pilot evaluation of a rapid immunochromatographic test for the diagnosis of gestational syphilis

Author

Mauro Cunha Ramos, Luiz Eduardo Bernardi, Marcia Susana Nunes da Silva, and Maria Lucia Rosa Rossetti

Subjects

syphilis, diagnosis, pregnancy, congenital syphilis, Medicine

Abstract

Introduction: Gestational syphilis is a global public health problem and one of the most common causes of adverse effects during pregnancy due to absence or inadequacy of treatment. Establishing a diagnosis of syphilis during prenatal care prevents the transmission of Treponema pallidum to the child. Objective: The objective of this study was to evaluate the performance of OL Syphilis (OrangeLife, Brazil), a rapid immunochromatographic test for gestational syphilis diagnosis. Methods: A total of 185 pregnant women in prenatal care were evaluated by OL Syphilis. The results were compared by traditional methods: Venereal Disease Research Laboratory and Rapid Plasma Reagin (VDRL and RPR) for screening and fluorescent treponemal antibody absorption test (FTA-Abs) for confirmation. Results: The prevalence of syphilis in this population was 6.49% (95%CI 3.40 to 11.06%). Rapid Test (RT) sensitivity was 91.67% (95%CI 61.52 to 99.79%) and specificity was 100% (95%CI 97.89 to 100%). Positive predictive value was 100% (95%CI 71.51 to 100%) and Negative predictive value was 99.43% (95%CI 96.84 to 100%). The agreement measured by Kappa coefficient was 0.954 (95%CI 0.863 to 1.000). Conclusion: The OL Syphilis test could be used for screening pregnant women, thus providing rapid diagnosis, increasing the probability of diagnosis and timely treatment, and preventing the devastating consequences of congenital syphilis.

Published

2017

13. AVALIAÇÃO DO DESEMPENHO DE UM TESTE RÁPIDO IMUNOCROMATOGRÁFICO NO DIAGNÓSTICO DE HANSENÍASE EM UMA REGIÃO ENDÊMICA NO NORTE DO BRASIL.

Author

Vieira Góis, Rosineide, Fideles Travaim, Sâmela, Calegari Prata, Gabrielle Melo, Nayara Degen, Andressa, Andrade Pereira, Giselle Cristina, Michel Wolf, Jonas, and Nunes Silva, Márcia Susana

Subjects

*HANSEN'S disease, *DIAGNOSIS, *PUBLIC health, *SKIN examination

Abstract

Introduction: Leprosy is of great importance for public health because of its epidemiology and disabling power. Efficiency in the diagnosis of this disease is limited. The objective of this study was to evaluate the performance of a rapid immunochromatographic test for multibacillary (MB) and paucibacillary (BP) leprosy, in positive and negative samples by skin smear examination in patients with leprosy, and to compare the rapid test analytically with World Health Organization (WHO) criteria. Methods: The study was conducted in the municipality of Ji-Paraná/RO, Brazil, between 2015 and 2016. In total, 140 individuals were evaluated. For a comparative analysis of the methods, sensitivity and specificity were calculated using SPSS® software. The Kappa (k) index was used to evaluate agreement between the methods. A p-value < 0.05 was considered significant. Results: Regarding agreement between the rapid test and WHO classification, k index was 0.94 (p < 0.01). When skin smear of individuals with BP leprosy was compared to the rapid test, agreement was non-significant (k = 0.01; p = 0.59). For agreement between skin smear of individuals with MB leprosy and the rapid test, a k index of 0.64 (p < 0.01) was detected. In addition, for PB leprosy sensitivity was 94% and specificity was 98%, while for MB leprosy sensitivity was 95% and specificity was 98%. Conclusion: The rapid test is a useful tool, fast and effective in aiding the diagnosis of leprosy. [ABSTRACT FROM AUTHOR]

Published

2018

14. An immunochromatographic test for serological diagnosis of scrub typhus.

Author

Yan, Shuhao, Lu, Qingyu, Tao, Qingyuan, Lu, Yawei, Gao, Bao, Wang, Sibo, Cai, Xusheng, Ai, Lele, Xiong, Xiaohui, Cao, Min, and Tan, Weilong

Subjects

*TSUTSUGAMUSHI disease, *SERODIAGNOSIS, *RECOMBINANT proteins, *ESCHERICHIA coli, *MEMBRANE proteins, *DIAGNOSIS

Abstract

A fluorescent immunochromatographic test (FM-ICT) was developed for rapid detection of anti- Orientia tsutsugamushi antibodies in serum samples. The FM-ICT was constructed based on the dual-antigen sandwich method. Truncated 56 kDa outer membrane protein of O. tsutsugamushi strain SJ, was expressed in E. coli and mixed with those of Ptan and Gillam strains. A thin line of the protein mixture was precisely sprayed across a nitrocellulose membrane making this the "Test" line. Polyclonal antibodies (pAbs) to O.tsutsugamushi were sprayed in another line across the membrane making this the "Control" line. Fluorescent microspheres conjugated 56 kDa proteins reacting with sample serum will be captured on the "Test" line if the sample contains antibodies to O.tsutsugamushi. Several experimental parameters were optimized. After optimizing the reaction procedure, the results are visible, within 6 min, with the naked eye under ultraviolet light. The limit of detection (LOD) was determined to be 7.63 ng/mL with prepared polyclonal antibodies. No cross-reaction was observed with sera samples from other febrile diseases. In clinical evaluations, the strips showed 94.92% sensitivity (106/112) and 93.75% specificity (56/60). The FM-ICT we developed will provide a new tool for on-site diagnosis of scrub typhus. • Recombinant proteins of three epidemic strains were mixed as diagnostic antigen. • Fuorescent microsphere were used in immunochromatographic strip for lower LOD. • Results can be read by naked eyes with the help of a portable UV lamp. • Suitable for on-site diagnosis in lab, families, even in the wild or remote areas. [ABSTRACT FROM AUTHOR]

Published

2024

15. Evaluation of urine sample for diagnosis of visceral leishmaniasis using rK-39 immunochromatographic test in Northwest Ethiopia.

Author

Eyayu, Tahir, Yasin, Melashu, Workineh, Lemma, Tiruneh, Tegenaw, Andualem, Henok, Sema, Meslo, Damtie, Shewaneh, Abebaw, Aynework, Getie, Birhanu, Andargie, Desalegn, Achaw, Barnabas, and Taklual, Wubet

Subjects

*VISCERAL leishmaniasis, *LEISHMANIASIS, *URINE, *CONTINGENCY tables, *BLOOD sampling, *DIAGNOSIS

Abstract

Background: Visceral leishmaniasis is the most severe form of leishmaniasis which ranks second in mortality and fourth in morbidity. Parasitological diagnostic techniques with splenic aspirate remain the gold standard. However, sample collection is risky, painful, and difficult. Alternatively, serological techniques provide good diagnostic accuracy using serum sample that is difficult for applying on small children and in the field. So, finding alternative non-invasive and self-collected samples like urine is very important. Thus, the study aimed to evaluate the diagnostic performance of the rK-39 strip test using urine for diagnosis of visceral leishmaniasis. Methods: A multicenter institutional-based cross-sectional study was conducted from November 2019 to March 2021 at Northwest Ethiopia. Sociodemographic information was collected using a structured questionnaire. Blood sample and midstream urine sample were collected for rK-39 test. Data were entered into Epi-data version 4.2 and analyzed using SPSS version 24.0. Diagnostic performance parameters of urine-based rK-39 rapid test, i.e. sensitivity, specificity, positive and negative predictive values, positive and negative likelihood ratios (LR+/−), and diagnostic accuracy were determined on contingency table by using serum-based rK-39 test result as a reference. An agreement between urine and serum-based rK-39 test was statistically determined by kappa value. Result: In total, 300 subjects, age ranged between 7 and 60 years, were included in the study. The overall sensitivity, specificity, positive predictive value, negative predictive value and diagnostic accuracy of urine-based rK-39 test were found to be 98.0% (95% CI: 93.0% - 99.8%), 95.5% (95% CI: 91.6% - 97.9%), 91.6% (95% CI: 85.2%– 95.4%), 98.9 (95% CI: 96.0%– 99.7%), and 96.33% (95% CI: 93.53–98.16%), respectively. Additionally, there was a strong agreement between the results obtained on rK-39 ICT using urine and serum samples (kappa = 0.92; P < 0.001). Conclusion: Urine-based rK-39 ICT had an excellent high sensitivity, specificity and strong agreement with serum-based rK-39 ICT results. This indicates that urine sample would be a promising noninvasive and easy to collect sample for diagnosis of VL in field and rural settings. [ABSTRACT FROM AUTHOR]

Published

2022

16. Identification of novel biomarkers for anti-Toxoplasma gondii IgM detection and the potential application in rapid diagnostic fluorescent tests

Author

Minh-Ngoc Nguyen, Seon-Ju Yeo, and Hyun Park

Subjects

Toxoplasma gondii, diagnosis, IgM detection, point-of-care test, fluorescence immunochromatographic test, 2DE immunoblotting, Microbiology, QR1-502

Abstract

Toxoplasmosis, while often asymptomatic and prevalent as a foodborne disease, poses a considerable mortality risk for immunocompromised individuals during pregnancy. Point-of-care serological tests that detect specific IgG and IgM in patient sera are critical for disease management under limited resources. Despite many efforts to replace the T. gondii total lysate antigens (TLAs) by recombinant antigens (rAgs) in commercial kits, while IgG detection provides significant specificity and sensitivity, IgM detection remains comparatively low in sensitivity. In this study, we attempted to identify novel antigens targeting IgM in early infection, thereby establishing an IgM on-site detection kit. Using two-dimensional gel electrophoresis (2DE) and mouse serum immunoblotting, three novel antigens, including EF1γ, PGKI, and GAP50, were indicated to target T. gondii IgM. However, rAg EF1γ was undetectable by IgM of mice sera in Western blotting verification experiments, and ELISA coated with PGKI did not eliminate cross-reactivity, in contrast to GAP50. Subsequently, the lateral flow reaction employing a strip coated with 0.3 mg/mL purified rAg GAP50 and exhibited remarkable sensitivity compared with the conventional ELISA based on tachyzoite TLA, which successfully identified IgM in mouse sera infected with tachyzoites, ranging from 103 to 104 at 5 dpi and 104 at 7 dpi, respectively. Furthermore, by using standard T. gondii-infected human sera from WHO, the limit of detection (LOD) for the rapid fluorescence immunochromatographic test (FICT) using GAP50 was observed at 0.65 IU (international unit). These findings underline the particular immunoreactivity of GAP50, suggesting its potential as a specific biomarker for increasing the sensitivity of the FICT in IgM detection.

Published

2024

17. Comparison of Immunochromatographic Test and Conventional Polymerase Chain Reaction as Diagnostic Methods for Canine Parvovirus Infection

Author

Chigozie S Ukwueze, Chika I Nwosuh, Boniface M Anene, and Romanus C Ezeokonkwo

Subjects

diagnosis, canine parvovirus type 2, dogs, immunochromatographic test, polymerase chain reaction, Agriculture

Abstract

Canine parvovirus type 2 infection is one of the aetiological agents of contagious gastroenteritis in dogs associated with high morbidity and mortality. Early diagnosis and treatment is very crucial for the survival of infected dog. This study was conducted to compare two diagnostic methods of canine parvovirus. Namely; Immunochromatographic (IC) test and Conventional Polymerase Chain Reaction (PCR). Eighty two (82) faecal specimens were collected per rectum from diarrhoeic dogs presented to various Veterinary Clinics and Hospitals in South Eastern Nigeria between the months of June 2017 March 2018. Three states, namely Abia, Anambra and Enugu were randomly selected and purposive/convenience sampling method was used to select two clinics/hospitals in each state. The faecal samples were both subjected to Immunochromatographic (IC) test and Conventional Polymerase Chain Reaction (PCR) simultaneously. IC test revealed that 83% positivity (68/82), while PCR showed 96% positivity (79/82). The sensitivity of IC test over PCR was 86%, with specificity of 100%, while the positive predictive value 100%, negative predictive value 21%, positive likely hood ratio 0.86 and negative likely hood ratio 0.14. McNemar test showed a significant difference between the two diagnostic methods. PCR was found to be more sensitive than IC test, though IC test is comparable with PCR and can be used in routine daily clinical practice. [J Bangladesh Agril Univ 2021; 19(4.000): 514-520]

Published

2021

18. Preparation of colloidal gold immunochromatographic test strips for the diagnosis of Toxoplasma gondii.

Author

Shen, Yuanxi, Wang, Zhaozhe, Li, Jiajing, Xu, Rui, Ji, Rongyi, Lin, Jiaojiao, and Zhu, Chuangang

Subjects

*COLLOIDAL gold, *TOXOPLASMA gondii, *TOXOPLASMOSIS, *SYMPTOMS, *WESTERN immunoblotting, *DIAGNOSIS

Abstract

As a severely harmful zoonotic disease, toxoplasmosis has complex clinical symptoms with atypical lesions, thus making it difficult for diagnosis in a timely manner. Therefore, developing an appropriate technique to diagnose and prevent toxoplasmosis has become a subject of many studies. In this study, a colloidal gold immunochromatographic test strips for the diagnosis of Toxoplasma gondii was established on the basis of the optimization of antigenic epitopes of GRA1 and GRA7 genes. Western blot and ELISA results showed that expressed rGRA exhibited specifically reaction with Toxoplasma gondii-positive mouse serum. This strip could be used to diagnose the toxoplasmosis of mouse. Moreover, compared with ELISA and PCR, GICA strip exhibited similar sensitivity in the diagnosis of Toxoplasma gondii in pigs. Here, we preliminarily established a diagnostic method for rapidly detecting toxoplasmosis, which may provide technical support for large-scale screening of Toxoplasma gondii. [ABSTRACT FROM AUTHOR]

Published

2020

19. Evaluation of a new brand of immunochromatographic test for visceral leishmaniasis in Brazil made available from 2018

Author

Ana Rabello, Tália Santana Machado de Assis, Gláucia Fernandes Cota, Mariana Lourenço Freire, and Daniel Moreira de Avelar

Subjects

Adult, Male, 0301 basic medicine, medicine.medical_specialty, lcsh:Arctic medicine. Tropical medicine, Adolescent, Leishmania IgG, Recombinant antigen, Test evaluation, lcsh:RC955-962, 030106 microbiology, 030231 tropical medicine, Immunochromatographic test, Protozoan Proteins, Antibodies, Protozoan, Antigens, Protozoan, Brief Communication, Sensitivity and Specificity, Chromatography, Affinity, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, parasitic diseases, Diagnosis, medicine, Humans, Child, Aged, Visceral leishmaniasis, Rapid test, Diagnostic Tests, Routine, business.industry, Infant, Newborn, Infant, Middle Aged, medicine.disease, Immunoglobulin M, Child, Preschool, Immunoglobulin G, Leishmaniasis, Visceral, Female, business, Antigen rK39

Abstract

Immunochromatographic tests based on the recombinant antigen K39 represent a major advance in diagnosing visceral leishmaniasis (VL) in recent years. Some performance variations are expected and have occurred in the use of several commercial rapid tests, especially in different geographical settings. This is the first evaluation in the Americas of the test recently provided by the public health system in Brazil for the diagnostic of VL, the OnSite™ Leishmania IgG/IgM Combo. In this first clinical test evaluation, 113 VL-positive patient samples and 73 negative controls were tested and a sensitivity of 91.2% and specificity of 94.5% were observed. These results indicate the need for further analysis and comparisons with the performance of other available commercial tests in order to define the impact of this new test on the quality of VL diagnosis in Brazil.

Published

2018

20. Development of an immunochromatographic test based on monoclonal antibodies against surface antigen 3 (TgSAG3) for rapid detection of Toxoplasma gondii.

Author

Luo, Jiaqing, Sun, Hongchao, Zhao, Xianfeng, Wang, Suhua, Zhuo, Xunhui, Yang, Yi, Chen, Xueqiu, Yao, Chaoqun, and Du, Aifang

Subjects

*MONOCLONAL antibodies, *TOXOPLASMA gondii, *ENZYME-linked immunosorbent assay, *TOXOPLASMOSIS diagnosis, *DIAGNOSIS, PARASITE physiology

Abstract

The immunochromatographic test (ICT) is a convenient and low-cost method that can rapidly obtain results (10 min) under normal conditions. In this study, we established an ICT assay with two monoclonal antibodies: TgSAG3-3A7 and TgSAG3-4D5 based on the conserved protein of TgSAG3 that can be expressed in all the infective stages of T. gondii. 20 nm gold particles were prepared and conjugated with TgSAG3-3A7 MAb at the concentration of 12.5 μg/mL. TgSAG3-4D5 MAb were used as the capture antibody because of its higher affinity tested by ELISA. The detection limit of the ICT assay was 100 ng with visual detection under optimal conditions of analysis. Positive porcine serum of Cryptosporidium suis , Mycoplasma suis , Streptococcus suis , Salmonella choleraesuis , Cysticercus cellulosae , Isospora suis , and Trichinella spiralis were used to evaluate the specificity of this ICT and no cross-reactivity was observed. 310 porcine serum samples obtained from pig farms in Zhejiang Province, China were detected by this ICT and ELISA kit, 23 positive samples were found by the developed strip with the rate of 7.42% comparing with 22 positive samples detected by the commercially ELISA kit which the positive rate was 7.1%, the relative sensitivity and specificity of this ICT are 100% and 99.65%. Therefore, the ICT established in this study is proved effective, simple, specific and sensitive of T. gondii detection. [ABSTRACT FROM AUTHOR]

Published

2018

21. Evaluation of a rapid immunochromatographic test kit to the gold standard fluorescent antibody test for diagnosis of rabies in animals in Bhutan.

Author

Tenzin, Tenzin, Lhamo, Kelzang, Rai, Purna B., Tshering, Dawa, Jamtsho, Pema, Namgyal, Jamyang, Wangdi, Thrinang, Letho, Sangay, Rai, Tuku, Jamtsho, Sonam, Dorji, Chendu, Rinchen, Sangay, Lungten, Lungten, Wangmo, Karma, Wangchuk, Pema, Gempo, Tshewang, Jigme, Kezang, Phuntshok, Karma, Tenzinla, Tenzinla, and Gurung, Ratna B.

Subjects

*RABIES, *FELIDAE, *GOAT diseases, *ANIMAL species, *IMMUNOGLOBULINS, *DIAGNOSIS

Abstract

Background: Rabies kills approximately 59,000 people each year worldwide. Rapid and accurate diagnosis of rabies is important for instituting rapid containment measures and for advising the exposed people for postexposure treatment. The application of a rapid diagnostic tests in the field can greatly enhance disease surveillance and diagnostic activities, especially in resource poor settings. In this study, a total of 179 brain tissue samples collected from different rabies suspect animal species (113 dogs, 50 cattle, 10 cats, 3 goats, 2 horses, and 1 bear) were selected and tested using both rapid immunochromatographic kit and the reference standard fluorescent antibody test (FAT). We evaluated the sensitivity, specificity, positive predictive value (PPV) and negative predictive value (NPV) of a rapid antigen detection test kit produced by BioNote, Inc. (Hwaseong-si, Korea) relative to a FAT for its fit-for-purpose for confirmation of clinical cases of rabies for early response and enhancing rabies surveillance. Results: Among 179 samples examined in this study, there was a concordance in results by the rapid test and FAT in 115 positive samples and 54 negative samples. Test results were discordant in 10 samples which were positive by FAT, but negative (false negative) by rapid kit. The rapid test kit showed a sensitivity of 92% (95% CI: 85.9–95.6) and specificity of 100% (95% CI: 93.4–100) using FAT as the reference standard. The positive and negative predictive values were found to be 100% (95% CI:96.7–100) and 84.4% (95% CI: 73.6–91.3), respectively. Overall, there was 94.4% (95% CI: 90–96.9) test agreement between rapid test and FAT (Kappa value = 0.874) with a positive percent agreement and negative percent agreement of 92 and 100%, respectively. Conclusions: Our finding demonstrated that the rapid test kit (BioNote) can be used for rabies surveillance and confirming clinical case of rabies in animals for making rapid decisions particularly controlling rabies outbreaks in resource poor settings. [ABSTRACT FROM AUTHOR]

Published

2020

22. Rapid diagnosis of cryptococcosis using an antigen detection immunochromatographic test.

Author

Rivet-Dañon, Diane, Guitard, Juliette, Grenouillet, Frédéric, Gay, Frédérick, Ait-Ammar, Nawel, Angoulvant, Adela, Marinach, Carine, and Hennequin, Christophe

Abstract

Summary Objectives Current methods for cryptococcal antigen detection have some limitations. This study aimed at evaluating a lateral flow assay (LFA) for the diagnosis of cryptococcosis in a French University medical center. Methods A retrospective study was performed on samples collected from patients with a definitive diagnosis of cryptococcosis (group I 66 samples; 28 patients) or with non- Cryptococcus invasive fungal infection (group II 18 samples; 17 patients). In addition, 274 samples from 205 consecutive patients, either suspected of cryptococcal infection or routinely screened during their follow-up, were prospectively tested (group III). Cryptococcal antigen was assayed using LFA and an EIA. A latex-based test was used for confirmation. Results Sensitivity calculated on group I and specificity on group II, were respectively at 100% and 90.0%. Two false positives were related to Trichosporon fungemia. Per-sample analysis on group III revealed sensitivity, specificity, positive and negative predictive values all at 100% for CSF, and at 100%, 98.9%, 75% and 100%, respectively for serum samples. LFA enabled the diagnosis of two cases of asymptomatic cryptococcosis. Conclusion The excellent diagnostic value and practicality (visual reading results in 15 min) of LFA make it fully appropriate for the diagnosis of cryptococcosis in this particular setting. [ABSTRACT FROM AUTHOR]

Published

2015

23. Multiplexed Immunochromatographic Test-System for Rapid Diagnosis of Acute Heart Failure.

Author

Gorshkova, R. M., Slobodova, D. A., Novoselov, N. P., and Gladyshev, P. P.

Subjects

*SEMICONDUCTOR nanocrystals, *HEART failure, *QUANTUM dots, *DIAGNOSIS

Abstract

A new approach to a multiplexed immunochromatographic system for rapid diagnosis of acute heart failure that included the use of colloidal quantum dots as labels was developed. The analysis was based on separation of analytes into bands and the use of biomarkers with various properties in the mixture being analyzed. The ability to use quantum dots synthesized in two different solutions for qualitative and quantitative analysis was demonstrated. The developed approach optimized the analytical capabilities of rapid diagnosis and increased its effectiveness and availability. [ABSTRACT FROM AUTHOR]

Published

2020

24. Accuracy and reliability of an NS1 rapid immunochromatographic test for DENV-1 diagnosis at point of care and in the laboratory

Author

Yara Hahr Marques Hökerberg, Anna Carolina Fontoura Seixas Rangel Maciel, Levy Vilas Boas Fukuoka, Guilherme Miguéis Berardinelli, Raquel de Vasconcellos Carvalhaes de Oliveira, Sonia Regina Lambert Passos, Verónica Elizabeth Mata, Cintia Damasceno dos Santos Rodrigues, Aline Caroline da Silva Santos, and Maria Angelica Borges dos Santos

Subjects

0301 basic medicine, Reproducibility of results, medicine.medical_specialty, business.industry, 030106 microbiology, NS1, Febrile illness, Emergency department, medicine.disease, Likelihood ratios in diagnostic testing, Dengue fever, lcsh:Infectious and parasitic diseases, Dengue, 03 medical and health sciences, Infectious Diseases, Sensitivity and specificity, Internal medicine, Diagnosis, Medicine, Point-of-care systems, lcsh:RC109-216, business, Kappa, Whole blood

Abstract

Background Rapid immunochromatographic tests (ICT) for dengue non-structural protein 1 (NS1) have shown good performance for diagnosing acute-phase dengue in serum in laboratory settings, but rarely have been assessed in whole blood and at point of care (POC). This study compare the accuracy and inter- and intra-observer reliability of the NS1 Bioeasy™ ICT in whole blood at POC versus serum in the laboratory, during a DENV-1 epidemic. Methods Cross-sectional study involving 144 adults spontaneously demanding care in an emergency department within 4 days of onset of acute febrile illness. Accuracy of NS1 Bioeasy™ ICT was compared in whole blood and serum, both at 15 and 30 min, blinded to the reference RT-PCR or NS1 ELISA. Non-dengue patients were also tested for Zika virus with RT-PCR. Reliability of whole blood and serum readings by the same or different observers was measured by simple kappa (95% CI). Results At 15 min, sensitivity (Sn) of NS1 Bioeasy™ ICT in whole blood/POC was 76.7% (95% CI: 68.0–84.1) and specificity (Sp) was 87.0% (95% CI: 66.4–97.2). Sn in serum/laboratory was 82% (95% CI: 74.1–88.6) and Sp 100% (95% CI: 85.8–100). Positive likelihood ratio was 5.9 (95% CI: 2.0–17.0) for whole blood/POC and 19.8 (95% CI: 2.9–135.1) for serum/laboratory. Reliability of matched readings of whole blood/POC and serum/laboratory by the same observer (k = 0.83, 95% CI: 0.74–0.93) or different observers (k = 0.81, 95% CI: 0.72–0.92) was almost perfect, with higher discordant levels in the absence of dengue. Results did not differ statistically at 5%. Conclusions NS1 Bioeasy™ ICT in DENV-1 epidemics is a potentially confirmatory test. Invalid results at 15 min should be reread at 30 min. To optimize impact of implementing ICT in the management of false-negatives it should be incorporated into an algorithm according to setting and available specimen. Trial registration UTN U1111-1145-9451 .

Published

2017

25. Development and characterization of an immunochromatographic test for the rapid diagnosis of Talaromyces (Penicillium) marneffei.

Author

Pruksaphon, Kritsada, Intaramat, Akarin, Ratanabanangkoon, Kavi, Nosanchuk, Joshua D., Vanittanakom, Nongnuch, and Youngchim, Sirida

Subjects

*DIAGNOSIS, *MYCOSES, *TALAROMYCES, *DIMORPHISM (Biology), *HIV, *COMPLICATIONS from organ transplantation, *FUNGI

Abstract

Talaromyces (Penicillium) marneffei is a thermally dimorphic fungus that can cause opportunistic systemic mycoses in patients infected with the human immunodeficiency virus (HIV). It has also been reported among patients with other causes of immunodeficiency, such as systemic lupus erythematosus, cancer, organ transplanted patients receiving immunosuppressive drug and adult onset immunodeficiency syndromes. Recent studies indicate that the clinical manifestations, laboratory findings and treatment strategies of talaromycosis (penicilliosis) marneffei are different between patients with and without HIV infection. Therefore early and accurate diagnosis of talaromycosis marneffei is crucial to the proper management and treatment. Since current diagnostic methods are currently inadequate, the aim of this study was to develop an immunochromatographic test (ICT) for the detection of T. marneffei yeast antigens in urine samples. The highly T. marneffei-specific monoclonal antibody 4D1 (MAb 4D1) conjugated with gold colloid at pH 6.5 was used as signal generator. The nitrocellulose membrane was lined with T. marneffei cytoplasmic yeast antigen (TM CYA) to serve as the test line, and rabbit anti-mouse IgG was the control line. Subjecting the assembled test strip to urine samples containing T. marneffei antigen produced a visible result within 20 minutes. The sensitivity limit of the assay was 3.125μg/ml of TM CYA. The ICT was used to test urine samples from 66 patients with blood culture confirmed talaromycosis marneffei, 42 patients with other fungal or bacterial infections, and 70 normal healthy individuals from endemic area of T. marneffei. The test exhibited sensitivity, specificity and accuracy of 87.87%, 100% and 95.5%, respectively. This rapid, user-friendly test holds great promise for the serodiagnosis of T. marneffei infection. [ABSTRACT FROM AUTHOR]

Published

2018

26. Validation of rK39 immunochromatographic test and direct agglutination test for the diagnosis of Mediterranean visceral leishmaniasis in Spain.

Author

Bangert, Mathieu, Flores-Chávez, María D., Llanes-Acevedo, Ivonne P., Arcones, Carolina, Chicharro, Carmen, García, Emilia, Ortega, Sheila, Nieto, Javier, and Cruz, Israel

Subjects

*VISCERAL leishmaniasis, *ANTIGEN analysis, *AGGLUTINATION tests, *MIXED infections, *SENSITIVITY analysis, *DIAGNOSIS

Abstract

Background: Visceral leishmaniasis (VL), the most severe form of leishmaniasis, is endemic in Europe with Mediterranean countries reporting endemic status alongside a worrying northward spread. Serological diagnosis, including immunochromatographic test based on the recombinant antigen rK39 (rK39-ICT) and a direct agglutination test (DAT) based on the whole parasite antigen, have been validated in regions with high VL burden, such as eastern Africa and the Indian subcontinent. To date, no studies using a large set of patients have performed an assessment of both methods within Europe. Methodology/Principal findings: We selected a range of clinical serum samples from patients with confirmed VL (including HIV co-infection), Chagas disease, malaria, other parasitic infections and negative samples (n = 743; years 2009–2015) to test the performance of rK39-ICT rapid test (Kalazar Detect Rapid Test; InBios International, Inc., USA) and DAT (ITM-DAT/VLG; Institute of Tropical Medicine Antwerp, Belgium). An in-house immunofluorescence antibody test (IFAT), was included for comparison. Estimated sensitivities for rK39-ICT and DAT in HIV-negative VL patients were 83.1% [75.1–91.2] and 84.2% [76.3–92.1], respectively. Sensitivity was reduced to 67.3% [52.7–82.0] for rK39 and increased to 91.3% [82.1–100.0] for DAT in HIV/VL co-infected patients. The in-house IFAT was more sensitive in HIV-negative VL patients, 84.2% [76.3–92.1] than in HIV/VL patients, 79.4% [73.3–96.2]. DAT gave 32 false positives in sera from HIV-negative VL suspects, compared to 0 and 2 for rK39 and IFAT, respectively, but correctly detected more HIV/VL patients (42/46) than rK39 (31/46) and IFAT (39/46). Conclusions/Significance: Though rK39-ICT and DAT exhibited acceptable sensitivity and specificity a combination with other tests is required for highly sensitive diagnosis of VL cases in Spain. Important variation in the performance of the tests were seen in patients co-infected with HIV or with other parasitic infections. This study can help inform the choice of serological test to be used when screening or diagnosing VL in a European Mediterranean setting. [ABSTRACT FROM AUTHOR]

Published

2018

27. Evaluation of a rapid immunochromatographic test for the detection of low burden Dirofilaria immitis (heartworm) in dogs and cats.

Author

Genchi, Marco, Mangia, Carlo, Ferrari, Nicola, and Loukeri, Sofia

Subjects

*DIROFILARIA immitis, *CANINE heartworm disease, *TRANSMISSION of parasitic diseases, *FELINE heartworm disease, *VETERINARY vaccines, *DIAGNOSIS

Abstract

The performance of a rapid immunochromatographic test for the detection of Dirofilaria immitis antigens (Speed Diro™; BVT-Virbac, France) was assessed in 49 experimentally infected dogs and in 244 naturally infected animals; 142 dogs and 102 cats. In experimentally infected dogs, Speed Diro™ showed a sensitivity of 90.9% in dogs infected with one adult female worm and 100% in dogs infected with more than one female worm. Specificity was 100%. For naturally infected dogs, the Knott test and PetChek HTWM PF served as reference methods for microfilaremia and antigenemia, respectively. All microfilaemic dogs (55/142) were positive with Speed Diro™. Importantly, none of the 21 dogs infected with D. repens were positive. The results of Speed Diro™ for the detection of antigenemia were compared with two in-house tests, SNAP HTWM and Witness Dirofilaria, and all three tests were 100% specific and sensitive in comparison to PetChek HTWM PF. For the evaluation of feline samples, 102 cats were examined by echocardiography. Sera from 87 heartworm-infected cats were tested by Speed Diro™ and SNAP HTWM. The results of Speed Diro™ were equivalent to SNAP HTWM, with a sensitivity of 98.9% and a specificity of 100%. [ABSTRACT FROM AUTHOR]

Published

2018

28. Highly sensitive sandwich immunoassay and immunochromatographic test for the detection of Clostridial epsilon toxin in complex matrices.

Author

Féraudet-Tarisse, Cécile, Mazuet, Christelle, Pauillac, Serge, Krüger, Maren, Lacroux, Caroline, Popoff, Michel R., Dorner, Brigitte G., Andréoletti, Olivier, Plaisance, Marc, Volland, Hervé, and Simon, Stéphanie

Subjects

*CLOSTRIDIAL enteritis, *IMMUNOASSAY, *BACTERIAL toxins, *CELL-mediated cytotoxicity, *WATER pollution, *DIAGNOSIS

Abstract

Epsilon toxin is one of the four major toxins of Clostridium perfringens. It is the third most potent clostridial toxin after botulinum and tetanus toxins and is thus considered as a potential biological weapon classified as category B by the Centers for Disease Control and Prevention (CDC). In the case of a bioterrorist attack, there will be a need for a rapid, sensitive and specific detection method to monitor food and water contamination by this toxin, and for a simple human diagnostic test. We have produced and characterized five monoclonal antibodies against common epitopes of epsilon toxin and prototoxin. Three of them neutralize the cytotoxic effects of epsilon toxin in vitro. With these antibodies, we have developed highly sensitive tests, overnight and 4-h sandwich enzyme immunoassays and an immunochromatographic test performed in 20 min, reaching detection limits of at least 5 pg/mL (0.15 pM), 30 pg/mL (0.9 pM) and 100 pg/mL (3.5 pM) in buffer, respectively. These tests were also evaluated for detection of epsilon toxin in different matrices: milk and tap water for biological threat detection, serum, stool and intestinal content for human or veterinary diagnostic purposes. Detection limits in these complex matrices were at least 5-fold better than those described in the literature (around 1 to 5 ng/mL), reaching 10 to 300 pg/mL using the enzyme immunoassay and 100 to 2000 pg/mL using the immunochromatographic test. [ABSTRACT FROM AUTHOR]

Published

2017

29. Diagnostic Performance of a Rapid Immunochromatographic Test Kit for Detecting Canine Parvovirus Infection.

Author

Shima, Felix K., Gberindyer, Fidelis A., Tion, Matthew T., Fagbohun, Olusegun A., Omobowale, Temidayo O., and Nottidge, Helen O.

Published

2021

30. Preparation and evaluation of a lateral flow immunochromatographic nanogold diagnostic kit for brucellosis in sheep

Author

Zainab Mohammed Aboelqassem, Hazem Mohammed Ibrahim, Rafik Hamed Sayed, Hassan Mohamed Sobhy, and Sahar Hussein Abdalla Hekal

Subjects

brucellosis, diagnosis, enzyme-linked immunosorbent assay, lateral flow assay, lateral flow immunochromatographic test, rose bengal plate test, Animal culture, SF1-1100, Veterinary medicine, SF600-1100

Abstract

Background and Aim: Brucellosis is a zoonotic disease with a worldwide distribution. It has a serious impact on the health of humans and animals, along with a negative impact on the economy. This study aimed to prepare and evaluate the diagnostic performance of a lateral flow immunochromatographic test (LFIT) nanogold diagnostic kit for detecting brucellosis in sheep. Materials and Methods: A rapidly developed LFIT, in which lipopolysaccharide conjugates with nanogold molecules, was placed on the conjugate pad. One hundred ovine serum samples were tested to detect Brucella antibodies (Ab) using the prepared lateral flow immunochromatography assay (LFA) kit and Rose Bengal test. The evaluation of specificity, sensitivity, and accuracy for LFIT and Rose Bengal plate test was conducted using the P04310-10 IDEXX brucellosis ovine/ caprine Ab enzyme-linked immunosorbent assay (ELISA) test (gold standard). Results: The lower amount of Brucella Ab in the ovine serum samples was detected and was 1.58 S/P ratio ELISA titer/100 μL using LFIT and with Rose Bengal to detect 1.86 S/P ratio ELISA. The results showed that the developed LFIT had high specificity with no cross-reactivity with other tested bacteria. The calculated sensitivity, specificity, and accuracy of LFIT and Rose Bengal test using the P04310-10 IDEXX brucellosis ovine/caprine Ab ELISA test (gold standard) were 74% and 89%, 81% and 59%, and 76.9% and 66%, respectively. Conclusion: The present results showed interesting results implying that the LFIA strip test could be used as a substantial diagnostic tool for field screening ovine Brucella as an essential step in the control of brucellosis. However, further studies for the validation of the present findings are necessary.

Published

2022

31. Comparison between an immunochromatographic test with an amplified ELISA for detecting e antigen and anti-e antigen antibodies in chronic Hepatitis B

Author

Damián Mainet-González, Daniel O Palenzuela-Gardon, and Julio C Aguilar-Rubido

Subjects

chronic hepatitis b, diagnosis, antibodies, e antigen, enzyme-immunoassay, immunochromatographic test, Biotechnology, TP248.13-248.65

Abstract

The disappearance of the e antigen and the appearance of anti-e antigen antibodies are two biomarkers that indicate favorable prognosis in Hepatitis B. In this study the Advanced QualityTM immunochromatographic test for detecting those biomarkers was compared to the Vidas® semi-quantitative ELISA test. Our hypothesis was that it is possible to use these biomarkers measured in a rapid and simple Advanced QualityTM immunochromatographic test for evaluating the therapeutic response in clinical trials with chronic hepatitis B patients. The two methods were done following the manufacturer’s instructions. The sera were taken from 69 patients with chronic hepatitis B of the clinical trial of the CIGB 440 therapeutic candidate. The immunochromatographic test and ELISA for detecting e antigen and anti-e antigen antibodies presented from substantial to almost perfect agreement in the evaluation of the sera of chronic Hepatitis B patients in a clinical trial. The immunochromatographic test for detecting e antigen had a low positive average agreement and a high negative average agreement compared to the ELISA. Nevertheless, the immunochromatographic test for detecting anti-e antigen antibodies had a high negative and positive average agreement in comparison to the ELISA. The immunochromagraphic test for the e antigen had a lower positive average agreement compared to the ELISA and some patients infected with Hepatitis B virus could not be detected by the former assay. The immunochromatographic test for anti-e antigen antibodies showed a similar performance to that of ELISA and could therefore be used in clinical trials for chronic Hepatitis B in health institutions without the need of a highly qualified lab technician.

32. Time window for positive cerebrospinal fluid broad-range bacterial PCR and Streptococcus pneumoniae immunochromatographic test in acute bacterial meningitis.

Author

Brink, Magnus, Welinder-Olsson, Christina, and Hagberg, Lars

Subjects

*STREPTOCOCCAL disease diagnosis, *ACADEMIC medical centers, *ANTIBIOTICS, *BACTERIAL antigens, *CEREBROSPINAL fluid, *CULTURES (Biology), *IMMUNOASSAY, *MICROBIOLOGY, *POLYMERASE chain reaction, *PROBABILITY theory, *RESEARCH funding, *LUMBAR puncture, *STREPTOCOCCUS, *DATA analysis software, *DESCRIPTIVE statistics, *BACTERIAL meningitis, *KRUSKAL-Wallis Test, *ONE-way analysis of variance, *DIAGNOSIS

Abstract

Background:Reliable microbiological tests are essential for the diagnosis of acute bacterial meningitis (ABM). In this study we investigated the time period after the start of antibiotic therapy during which culture, polymerase chain reaction (PCR) and the immunochromatographic test (ICT) are able to detect bacteria in cerebrospinal fluid (CSF).Methods:The study was performed on CSF samples from adults with ABM admitted to the Department of Infectious Diseases, Sahlgrenska University Hospital, Gothenburg, Sweden, from January 2007 to April 2014. In addition to the initial lumbar puncture (LP), the participants underwent one or two more LPs during 10 days following the start of antibiotics. The analyses performed on the CSF samples were culture, PCR and ICT.Results:The study comprised 70 CSF samples from 25 patients with ABM. A bacterium could be identified by CSF culture in 44%, by blood culture in 58% and by PCR in 100% of the patients. There were no positive CSF cultures in samples taken later than the day of starting antibiotics. PCR was positive in 89% on days 1–3, 70% on days 4–6 and 33% on days 7–10. For cases of pneumococcal meningitis, the ICT was positive in 88% on days 1–3, 90% on days 4–6 and 75% on days 7–10.Conclusions:This study shows that PCR is highly sensitive for bacterial detection in CSF samples taken up to 1 week into antibiotic therapy. The ICT is highly sensitive for the detection of pneumococci in CSF samples taken during the first week of antibiotic treatment. [ABSTRACT FROM AUTHOR]

Published

2015

33. Evaluation of the NOW Malaria Immunochromatographic Test for Quantitative Diagnosis of Falciparum and Vivax Malaria Parasite Density.

Author

Yuko Katakai, Komaki-Yasuda, Kanako, Tangpukdee, Noppadon, Wilairatana, Polrat, Krudsood, Srivicha, and Shigeyuki Kano

Subjects

*MALARIA, *PLASMODIUM, *DIAGNOSIS, *CLINICAL medicine, *INFECTION

Abstract

The NOW® Malaria Test, an immunochromatographic test (ICT), was evaluated to determine its ability test to quantitatively detect malaria parasites using 100 blood samples from Thailand, including 50 Plasmodium falciparum (Pf) infections and 50 P. vivax (Pv) infections. Intensities of the thickness of the visible bands of the positive ICT were compared with the parasite densities. In cases of Pf infection, the intensities of both HRP-2 bands (T1 bands: Pf specific bands) and aldolase bands (T2 bands: pan-Plasmodium bands) correlated with the parasite densities. The intensities of T2 bands in Pf positive samples showed better correlation with the parasitedensities than the T1 bands. In the cases of Pv infection, the intensities of T2 bands were also well correlated with parasite density. These results suggest that the ICT is useful not only for rapid detection of malaria parasites but also for estimating parasite density. [ABSTRACT FROM AUTHOR]

Published

2011

34. Clinical Performance of a New Soluble CD14-Subtype Immunochromatographic Test for Whole Blood Compared with Chemiluminescent Enzyme Immunoassay: Use of Quantitative Soluble CD14-Subtype Immunochromatographic Tests for the Diagnosis of Sepsis.

Author

Sato, Masayuki, Takahashi, Gaku, Shibata, Shigehiro, Onodera, Makoto, Suzuki, Yasushi, Inoue, Yoshihiro, and Endo, Shigeatsu

Subjects

*CD14 antigen, *BLOOD testing, *COMPARATIVE studies, *CHEMILUMINESCENCE, *ENZYME-linked immunosorbent assay, *SEPSIS, *DIAGNOSIS

Abstract

We previously reported that a soluble CD14-subtype (sCD14-ST) immunochromatographic test (ICT) for plasma is more convenient than chemiluminescent enzyme immunoassay (CLEIA), but plasma separation makes bedside measurements difficult. We developed a new sCD14-ST ICT for whole blood and investigated whether quantitative determinations of sCD14-ST by ICT were useful for diagnosing sepsis and severe sepsis/septic shock. We studied 20 patients who fulfilled two or more systemic inflammatory response syndrome (SIRS) criteria and 32 patients who had been diagnosed with sepsis or severe sepsis/septic shock. Whole blood was collected on day 0 (on admission) and day 7, and the sCD14-ST concentration was quantitatively measured by CLEIA and ICT for whole blood. The patients’ Acute Physiology and Chronic Health Evaluation (APACHE) II, Sequential Organ Failure Assessment (SOFA), and Mortality in Emergency Department Sepsis (MEDS) scores were also calculated. The cut-off values obtained by the quantitative measurements made by ICT were 464.5 pg/mL for sepsis and 762.7 pg/mL for severe sepsis/septic shock (P < 0.0001). A Bland–Altman plot showed that no fixed bias or proportional bias was detected between CLEIA and quantitative ICT for whole blood. sCD14-ST concentrations were significantly correlated with APACHE II, SOFA, and MEDS scores (P < 0.0001). These results suggest that the new sCD14-ST ICT for whole blood may be a useful tool for the convenient, rapid bedside diagnosis and treatment of sepsis. [ABSTRACT FROM AUTHOR]

Published

2015

35. Evaluation of an Immunochromatographic Test to the Diagnosis of Canine Brucellosis Caused by Brucella canis.

Author

Keid, LB, Diniz, JA, Oliveira, TMFS, Ferreira, HL, and Soares, RM

Subjects

*BRUCELLOSIS in animals, *CHROMATOGRAPHIC analysis, *IMMUNODIFFUSION, *POLYMERASE chain reaction, *MERCAPTOETHANOL, *MEDICAL screening, *DIAGNOSIS

Abstract

Contents This study evaluated the performance of an immunochromatographic test ( ICT) for the diagnosis of canine brucellosis caused by Brucella canis, comparing its results with that of the rapid slide agglutination test with and without the use of 2-mercaptoethanol and the agar gel immunodiffusion test ( AGID). The microbiological culture, PCR and clinical examination were used as reference. According to the results obtained in clinical examination, blood culture, culture of semen and vaginal swab and PCR in blood, semen and vaginal swab, a total of 102 dogs were divided into three groups: B. canis-infected dogs (Group 1), B. canis-non-infected dogs (Group 2) and dogs with suspected brucellosis (Group 3). The diagnostic sensitivity of RSAT, 2 ME- RSAT, AGID and ICT in Group 1 was, respectively, 75%, 37.5%, 27.8% and 89.58%. The diagnostic specificity of RSAT, 2 ME- RSAT, AGID and ICT in Group 2 was, respectively, 91%, 100%, 100%, and 100%. In dogs with suspected brucellosis, 9.67% were RSAT positive, none was positive by 2 ME- RSAT, 3.22% were AGID positive and 6.45% were ICT positive. The main drawback concerning canine brucellosis diagnosis is the lack of a highly sensitive serological assay to be used as a screening test to the rapid identification of infected animals. The ICT showed a high diagnostic specificity and a diagnostic sensitivity value greater than that observed in the RSAT, 2 ME- RSAT and AGID. However, 10.41% of infected dogs had negative results by ICT. These dogs were positive by microbiological culture and/or PCR, indicating active infection and consequently a higher potential of spreading Brucella. Although rapid and simple to perform, the ICT lacked sensitivity to be used as a screening test. [ABSTRACT FROM AUTHOR]

Published

2015

36. Surra Sero K-SeT, a new immunochromatographic test for serodiagnosis of Trypanosoma evansi infection in domestic animals.

Author

Birhanu, Hadush, Rogé, Stijn, Simon, Thomas, Baelmans, Rudy, Gebrehiwot, Tadesse, Goddeeris, Bruno Maria, and Büscher, Philippe

Subjects

*SERODIAGNOSIS, *TRYPANOSOMA, *TRYPANOSOMIASIS, *DOMESTIC animal diseases, *IMMUNOGLOBULINS, *CHROMATOGRAPHIC analysis, *DIAGNOSIS

Abstract

Trypanosoma evansi , the causative agent of surra, infects different domestic and wild animals and has a wide geographical distribution. It is mechanically transmitted mainly by haematophagous flies . Parasitological techniques are commonly used for the diagnosis of surra but have limited sensitivity. Therefore, serodiagnosis based on the detection of T. evansi specific antibodies is recommended by the World Organisation for Animal Health (OIE). Recently, we developed a new antibody detection test for the serodiagnosis of T. evansi infection, the Surra Sero K -SeT. Surra Sero K -SeT is an immunochromatographic test (ICT) that makes use of recombinant variant surface glycoprotein rVSG RoTat 1.2, produced in the yeast Pichia pastoris . In this study, we compared the diagnostic accuracy of the Surra Sero K -SeT and the Card Agglutination Test for T. evansi Trypanosomososis (CATT/ T. evansi ) with immune trypanolysis (TL) as reference test on a total of 806 sera from camels, water buffaloes, horses, bovines, sheep, dogs and alpacas. Test agreement was highest between Surra Sero K -SeT and TL ( κ = 0.91, 95% CI 0.841–0.979) and somewhat lower between CATT/ T. evansi and TL ( κ = 0.85, 95% CI 0.785–0.922) and Surra Sero K -SeT and CATT/ T. evansi ( κ = 0.81, 95% CI 0.742–0.878). The Surra Sero K -SeT displayed a somewhat lower overall specificity than CATT/ T. evansi (94.8% versus 98.3%, χ 2 = 13.37, p < 0.001) but a considerably higher sensitivity (98.1% versus 84.4%, χ 2 = 33.39, p < 0.001). We conclude that the Surra Sero K -SeT may become an alternative for the CATT/ T. evansi for sensitive detection of antibodies against T. evansi in domestic animals. [ABSTRACT FROM AUTHOR]

Published

2015

37. Development of an Immunochromatographic Test for Diagnosis of Visceral Leishmaniasis Based on Detection of a Circulating Antigen.

Author

Gao, Chun-hua, Yang, Yue-tao, Shi, Feng, Wang, Jun-yun, Steverding, Dietmar, and Wang, Xia

Subjects

*VISCERAL leishmaniasis, *SERODIAGNOSIS, *ANTIGENS, *LEISHMANIA donovani, *AGGLUTINATION tests, *DIAGNOSIS, *PUBLIC health, *TRICHOMONIASIS

Abstract

Background: Visceral leishmaniasis (VL) is a life-threatening disease caused by protozoan parasites of the Leishmania donovani complex. Early case detection followed by adequate treatment is essential to the control of VL. However, the available diagnostic tests are either invasive and require considerable expertise (parasitological demonstration of the parasite in tissue smears) or unable to distinguish between past and active infection (serological methods). Therefore, we aimed to develop a lateral flow assay in the form of an immunochromatographic test (ICT) device based on the detection of a circulating Leishmania antigen using monoclonal antibodies (mAbs). Methodology/Principal Findings: mAbs were produced by fusion of murine myeloma cells with splenocytes isolated from a mouse immunized with L. donovani soluble crude antigen. Out of 12 cloned hybridoma cell lines, two secreted mAbs recognizing the same leishmanial protein. These mAbs were used to produce an ICT as a sandwich assay for the detection of circulating antigen in serum and blood samples. The ICT was evaluated with 213 serum samples from VL patients living in VL endemic areas in China, and with 156 serum samples from patients with other diseases as well as 78 serum samples from healthy donors. Sensitivity, specificity and diagnostic efficiency of the new ICT was 95.8%, 98.7% and 97.3%, respectively. Compared with a commercially available antibody detecting ICT, our antigen-based ICT performed slightly better. Conclusion/Significance: The newly developed ICT is an easy to use and more accurate diagnostic tool which fulfils the performance and operational characteristics required for VL case detection under field and laboratory conditions. As our ICT detects a circulating antigen, it will also be useful in monitoring treatment success and diagnosing VL in immunocompromised patients. Author Summary: Visceral leishmaniasis is a neglected disease caused by different species of protozoan parasites of the genus Leishmania. The disease is endemic in 61 countries, and in many of them it poses a serious public health issue. As visceral leishmaniasis is fatal if left untreated, early diagnosis is essential for treatment and control of the disease. Current available diagnostic tests are either difficult to carry out under field conditions or insufficiently accurate. In this study we developed a new diagnostic test which detects a circulation parasite-derived antigen in serum or blood samples of patients with visceral leishmaniasis. We found that our test performed better than most other tests based on the detection of parasite-specific antibodies. In addition, as our test is a device for the detection of an acute infection, it will be useful to validate treatment and in the diagnosis of the disease in patients with deficient antibody production (as in AIDS patients). [ABSTRACT FROM AUTHOR]

Published

2015

38. Development of an immunochromatographic point-of-care test for detection of IgG antibody in serodiagnosis of human trichinellosis

Author

Tongjit Thanchomnang, Lakkhana Sadaow, Oranuch Sanpool, Pewpan M. Intapan, Rutchanee Rodpai, Patcharaporn Boonroumkaew, Penchom Janwan, Somjintana Tourtip, and Wanchai Maleewong

Subjects

Trichinellosis, Trichinella, Diagnosis, Immunochromatographic test, Screening test, Rapid test, Infectious and parasitic diseases, RC109-216

Abstract

Objective: Trichinellosis is a globally distributed food-borne parasitic disease. Initially, diagnosis is usually made based on clinical signs, symptoms, and history of eating raw or undercooked meat. In the present study, an immunochromatographic test (ICT) kit was developed to diagnose trichinellosis by detecting IgG antibodies in sera of infected humans.Methods: Somatic extract from Trichinella spiralis larvae was used as the antigen for the ICT kit development. Diagnostic efficacy was evaluated using human serum samples from proven trichinellosis patients, healthy persons, and those with other parasitic infections.Results: The diagnostic sensitivity, specificity, positive and negative predictive values and accuracy of the ICT kit were 100.0% (95%; CI 88.8 to 100.0%), 92.5% (95% CI; 86.9 to 96.2%), 73.8% (95% CI; 58.0 to 86.1%), 100.0% (95% CI; 97.3 to 100.0%) and 93.8% (95% CI; 89.2 to 96.9%), respectively.Conclusions: This ICT diagnostic kit can be used as a testing tool for human trichinellosis. This test should permit rapid detection of infection to enable prompt anthelminthic treatment. It can also be used for retrospective diagnoses and field surveys based at laboratories where sophisticated equipment is lacking.

Published

2021

39. Rapid diagnosis of cryptococcosis using an antigen detection immunochromatographic test

Author

Diane Rivet-Dañon, Juliette Guitard, Frédéric Grenouillet, Frédérick Gay, Nawel Ait-Ammar, Adela Angoulvant, Carine Marinach, Christophe Hennequin, Immunité et Infection, Université Pierre et Marie Curie - Paris 6 (UPMC)-IFR113-Institut National de la Santé et de la Recherche Médicale (INSERM), Parasitologie-Mycologie CHU Besançon, Centre Hospitalier Régional Universitaire [Besançon] (CHRU Besançon), Laboratoire Chrono-environnement - UFC (UMR 6249) (LCE), Université Bourgogne Franche-Comté [COMUE] (UBFC)-Centre National de la Recherche Scientifique (CNRS)-Université de Franche-Comté (UFC), Ecologie fonctionnelle et biogéochimie des sols et des agro-écosystèmes (UMR Eco&Sols), Institut National de la Recherche Agronomique (INRA)-Institut de Recherche pour le Développement (IRD)-Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-Centre international d'études supérieures en sciences agronomiques (Montpellier SupAgro)-Institut national d’études supérieures agronomiques de Montpellier (Montpellier SupAgro), Anofel Cryptosporidium National Network, CHU Saint-Antoine [APHP], Mucoviscidose: physiopathologie et phénogénomique [CRSA], Centre de Recherche Saint-Antoine (CRSA), Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU), CHU Saint-Antoine [AP-HP], Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Sorbonne Université (SU), Laboratoire Chrono-environnement (UMR 6249) (LCE), Centre National de la Recherche Scientifique (CNRS)-Université de Franche-Comté (UFC), Université Bourgogne Franche-Comté [COMUE] (UBFC)-Université Bourgogne Franche-Comté [COMUE] (UBFC), Cellule Pasteur UPMC, Institut Pasteur [Paris] (IP)-Sorbonne Université (SU), Dynamic Microbiology - EA 7380 (DYNAMIC), École nationale vétérinaire - Alfort (ENVA)-Agence nationale de sécurité sanitaire de l'alimentation, de l'environnement et du travail (ANSES)-Université Paris-Est (UPE)-Université Paris-Est Créteil Val-de-Marne - Paris 12 (UPEC UP12), Hôpital Bicêtre, Université Paris-Sud - Paris 11 (UP11)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Hôpital Bicêtre, Université Paris-Sud - Paris 11 (UP11), Centre d'Immunologie et de Maladies Infectieuses (CIMI), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU), Service de parasitologie et mycologie [CHRU de Besançon], Centre Hospitalier Régional Universitaire de Besançon (CHRU Besançon), Laboratoire Chrono-environnement - CNRS - UBFC (UMR 6249) (LCE), Université de Franche-Comté (UFC), Université Bourgogne Franche-Comté [COMUE] (UBFC)-Université Bourgogne Franche-Comté [COMUE] (UBFC)-Centre National de la Recherche Scientifique (CNRS), Institut national d’études supérieures agronomiques de Montpellier (Montpellier SupAgro), Institut national d'enseignement supérieur pour l'agriculture, l'alimentation et l'environnement (Institut Agro)-Institut national d'enseignement supérieur pour l'agriculture, l'alimentation et l'environnement (Institut Agro)-Centre international d'études supérieures en sciences agronomiques (Montpellier SupAgro)-Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-Institut de Recherche pour le Développement (IRD)-Institut National de la Recherche Agronomique (INRA), Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-Institut de Recherche pour le Développement (IRD)-Institut National de la Recherche Agronomique (INRA)-Centre international d'études supérieures en sciences agronomiques (Montpellier SupAgro)-Institut national d’études supérieures agronomiques de Montpellier (Montpellier SupAgro), Université Pierre et Marie Curie - Paris 6 ( UPMC ) -IFR113-Institut National de la Santé et de la Recherche Médicale ( INSERM ), Centre Hospitalier Régional Universitaire [Besançon] ( CHRU Besançon ), Laboratoire Chrono-environnement ( LCE ), Université Bourgogne Franche-Comté ( UBFC ) -Centre National de la Recherche Scientifique ( CNRS ) -Université de Franche-Comté ( UFC ), Ecologie fonctionnelle et biogéochimie des sols et des agro-écosystèmes ( Eco&Sols ), and Centre international d'études supérieures en sciences agronomiques ( Montpellier SupAgro ) -Institut National de la Recherche Agronomique ( INRA ) -Institut de Recherche pour le Développement ( IRD ) -Centre de Coopération Internationale en Recherche Agronomique pour le Développement ( CIRAD ) -Institut national d’études supérieures agronomiques de Montpellier ( Montpellier SupAgro )

Subjects

Microbiology (medical), Male, medicine.medical_specialty, Pathology, Antigens, Fungal, [SDV]Life Sciences [q-bio], Cryptococcus, Lateral flow assay, Asymptomatic, Gastroenterology, Sensitivity and Specificity, Rapid diagnosis test, Chromatography, Affinity, Serotype, Antigen, Internal medicine, Positive predicative value, Trichosporon, Diagnosis, medicine, Humans, [ SDV.MP.MYC ] Life Sciences [q-bio]/Microbiology and Parasitology/Mycology, Fungemia, [SDV.MP.MYC]Life Sciences [q-bio]/Microbiology and Parasitology/Mycology, Aged, Retrospective Studies, Academic Medical Centers, biology, business.industry, Retrospective cohort study, Cryptococcus gattii, Cryptococcosis, Middle Aged, biology.organism_classification, medicine.disease, 3. Good health, Infectious Diseases, Asymptomatic Diseases, Cryptococcus neoformans, Female, France, medicine.symptom, business, Bronchoalveolar Lavage Fluid

Abstract

Summary Objectives Current methods for cryptococcal antigen detection have some limitations. This study aimed at evaluating a lateral flow assay (LFA) for the diagnosis of cryptococcosis in a French University medical center. Methods A retrospective study was performed on samples collected from patients with a definitive diagnosis of cryptococcosis (group I 66 samples; 28 patients) or with non- Cryptococcus invasive fungal infection (group II 18 samples; 17 patients). In addition, 274 samples from 205 consecutive patients, either suspected of cryptococcal infection or routinely screened during their follow-up, were prospectively tested (group III). Cryptococcal antigen was assayed using LFA and an EIA. A latex-based test was used for confirmation. Results Sensitivity calculated on group I and specificity on group II, were respectively at 100% and 90.0%. Two false positives were related to Trichosporon fungemia. Per-sample analysis on group III revealed sensitivity, specificity, positive and negative predictive values all at 100% for CSF, and at 100%, 98.9%, 75% and 100%, respectively for serum samples. LFA enabled the diagnosis of two cases of asymptomatic cryptococcosis. Conclusion The excellent diagnostic value and practicality (visual reading results in 15 min) of LFA make it fully appropriate for the diagnosis of cryptococcosis in this particular setting.

Published

2015

40. Development of a immunochromatographic test with avidin-biotin for the detection of antibodies against antigen e of hepatitis B in human plasma.

Author

Mainet-González, Damián, Palenzuela-Gardon, Daniel O., and Díaz-Argudín, Tamara

Subjects

*ANTIGENS, *HEPATITIS B treatment, *IMMUNOGLOBULINS, *AVIDIN, *BLOOD plasma, *MONOCLONAL antibodies

Abstract

The disappearance of antigen e of hepatitis B in the presence of the plasmatic antibodies against antigen e may indicate a satisfactory therapeutic response in patients with chronic hepatitis B. The immunochromatographic test carried out in the diagnosis of diseases use different antibody combinations and may employ the avidin or streptavidinbiotin technology to develop a rapid immunochromatographic test for the detection of antibodies anti-antigen e in the plasma. They were detected in the laboratory by means of two fast immunochromatographic tests when using in one of them the avidin-biotin technology. These tests are carried out with a one-step competitive inhibition format and amplified or not with avidin-biotin. Monoclonal antibodies against antigen e obtained by cellular hybridization were used. Forty-six plasmatic samples classified as possitive and negative to the anti-antigen antibodies were evaluated with a reference immunochromatographic test Advanced Quality™. The possible expiry time of the biological reagents forming part of these tests were studied with accelerated thermal-stability experiments. The possible interference in the plasma of some of the biochemical compounds used in these trials was analyzed. Four murine monoclonal antibodies anti-antigen e were obtained and only one of them was used in these immunochromatographic tests with an anti-antigene polyclonal antibody conjugated with gold. Both tests and their stable biological reagents discriminated the positive and negative samples to the antibodies anti-antigen e, as well as the commercial test. There was no interference in the biochemical compounds studied in these tests. Both immunochromatographic tests made in the laboratory are useful to detect antibodies anti-antigen e in the plasma. The avidin-biotin increased the analytical sensitivity of this type of fast immunochromatographic test without altering its performance features. [ABSTRACT FROM AUTHOR]

Published

2007

41. A rapid immunochromatographic test to detect the lily mottle virus.

Author

Zhang, Yubao, Wang, Yajun, Yang, Wanrong, Xie, Zhongkui, Wang, Ruoyu, Kutcher, Hadley Randal, and Guo, Zhihong

Subjects

*CHROMATOGRAPHIC analysis, *POTYVIRUSES, *IMMUNOGLOBULIN G, *COLLOIDAL gold, *POLYMERASE chain reaction, *DIAGNOSIS, *THERAPEUTICS, *VIRUS diseases of plants

Abstract

We developed a rapid immunochromatographic strip (ICS) test for lily mottle virus (LMoV). The test is based on a double-antibody sandwich format and employs two distinct anti-LMoV polyclonal antibodies (IgG 3 and IgG 4 ). The first antibody, IgG 3 was conjugated with colloidal gold, and the second antibody, IgG 4 was used as the capture antibody at the test line. The performance of the ICS test was evaluated and the results obtained were compared with a quadruplex RT-PCR assay. When serial dilutions of purified LMoV were tested, the LMoV detection limit of the ICS test was 8.0 × 10 −9 mg/mL, which was in complete agreement with the results of quadruplex RT-PCR. Compared with quadruplex RT-PCR, the specificity and sensitivity of ICS were 98.7 and 100%, respectively. There was therefore significant agreement between the results obtained from the two tests ( κ = 0.982). The ICS test therefore appears to be broadly applicable, and will be especially useful in the field, as well as in areas without laboratory facilities, to support efforts to detect and control LMoV. [ABSTRACT FROM AUTHOR]

Published

2015

42. Bedside immunochromatographic test for enterovirus 71 infection in children.

Author

Huang, Kuan-Ying Arthur, Yang, Shuan, Tsao, Kuo-Chien, Chen, Chih-Jung, Hsieh, Yu-Chia, Chiu, Cheng-Hsun, Hsieh, Juo-Yu, Yang, Jyh-Yuan, and Huang, Yhu-Chering

Subjects

*CHROMATOGRAPHIC analysis, *ENTEROVIRUS diseases, *VIRAL diseases in children, *PUBLIC health, *PREVENTIVE medicine, *VIRUS diseases, *IMMUNOLOGY, *DIAGNOSIS

Abstract

Abstract: Background: Enterovirus 71 (EV71) causes frequent outbreaks worldwide, particularly in the Asia-Pacific area. Its quick spread is a critical challenge for public health and timely preventive measures and clinical management therefore rely on early detection. There is a need for a rapid, easy-to-use, and reliable method for detecting EV71 infections. Objective: The study aimed to evaluate a bedside immunochromatography (ICT) kit for diagnosing acute EV71 infection in children. Study design: Pediatric patients with herpangina or hand–foot–mouth disease were randomly and prospectively enrolled from hospitals across Taiwan. Throat or rectal swabs were collected for viral culture and reverse-transcriptase polymerase chain reaction (RTPCR). For the ICT kit, whole blood was obtained by ear piercing, finger-sticking, or venipuncture. The results of ICT, virus isolation and RTPCR in clinical samples were compared. Results: Of the 156 patients enrolled, 91 (58%), 64 (41%) and 72 (46%) had positive results of the ICT kit, viral culture and RTPCR, respectively. Laboratory-confirmed infection with either positive EV71 culture or RTPCR was used as the diagnostic standard. The sensitivity and specificity of the ICT kit was 84% and 77%, respectively. The viral culture and RTPCR had relatively lower sensitivity but higher specificity. The patient's age did not affect the performance of the ICT, viral culture and RTPCR. However, a low sensitivity of ICT kit was noted before the second day of disease onset. Conclusions: The ICT kit may serve as a simple, quick and reliable method for the bedside diagnosis of acute EV71 infection in children. [Copyright &y& Elsevier]

Published

2013

43. Assessment of a rapid immunochromatographic test for the diagnosis of norovirus gastroenteritis.

Author

Pombubpa, K. and Kittigul, L.

Subjects

*NOROVIRUS diseases, *NOROVIRUSES, *ABDOMINAL pain, *GASTROENTERITIS, *DIARRHEA, *DIAGNOSIS

Abstract

Noroviruses are the leading cause of acute gastroenteritis in people of all ages. Since the viruses are highly infectious, rapid and early diagnosis is important to prevent and control the disease. The present study aimed to evaluate the commercial immunochromatographic test RIDA® QUICK Norovirus for the detection of norovirus in stool samples from patients with acute gastroenteritis in Thailand. As compared with reference RT-PCR results, the RIDA® QUICK Norovirus assay provided a sensitivity of 48.2 and 83.3% with a specificity of 87.5%. False positive results were observed in 12.5% of norovirus-negative stool samples. Based on commercial quantitative real-time RT-PCR, the RIDA® QUICK Norovirus assay revealed a highly significant association, p-value <0.001, and good agreement (kappa = 0.6). The assay could detect norovirus in stool samples ranging from 3.22 × 10 to 3.26 × 10 copies/ml. False negative results occurred in the stool samples containing 5.9 × 10 copies/ml of norovirus GI or 1.85 × 10 - 4.28 × 10 copies/ml of GII. The immunochromatographic RIDA® QUICK Norovirus assay may be useful for rapid screening of norovirus infections in patients with acute gastroenteritis in both developed and developing countries where the RT-PCR method has not been established for routine diagnosis. [ABSTRACT FROM AUTHOR]

Published

2012

44. Development of a colloidal gold-based immunochromatographic test strip for the rapid, on-site detection of Pseudomonas aeruginosa in clinical samples.

Author

Wang, Yan, Dou, Hengli, Chen, Kuixiang, Zhang, Hua, and Hu, Chengjin

Subjects

*ANALYSIS of variance, *ANIMAL experimentation, *CHROMATOGRAPHIC analysis, *DIAGNOSTIC reagents & test kits, *ENZYME-linked immunosorbent assay, *IMMUNOASSAY, *MICE, *MONOCLONAL antibodies, *POLYMERASE chain reaction, *PSEUDOMONAS diseases, *RABBITS, *RESEARCH funding, *TIME, *WESTERN immunoblotting, *DIAGNOSIS

Abstract

Background: Current procedures for the detection of Pseudomonas aeruginosa require sophisticated equipment, skilled technicians, and a great deal of time. Immunochromatography assays (ICA) are simple and rapid diagnostic procedures that can be performed and interpreted on the spot or at the bedside without a machine. Methods: We developed a rapid, 1-step immunochromatographic test strip that is well suited to the on-site detection of P. aeruginosa with high sensitivity and specificity. In brief, a monoclonal antibody targeting the outer membrane protein F (OprF) of P. aeruginosa, 3C3B5, was conjugated to colloidal gold and used as a detection antibody. An OprF polyclonal antibody was developed as the capture antibody. Eighty-three clinical samples were examined for P. aeruginosa by rapid 1-step ICA and compared with Multiplex-polymerase chain reation (M-PCR). Results: The detection limit of this method is 5 ×× 105 CFU/ml for P. aeruginosa and 10 ng/ml for the OprF protein. The immunochromatographic strip test demonstrated a slightly lower sensitivity (84.8%), but a similar specificity (100%), to multi-PCR, which is an accurate method for the detection of P. aeruginosa in the laboratory. We observed no cross-reactivity with non-P. aeruginosa bacterial microbes. The detection of P. aeruginosa by the ICA strip can be completed within 5--10 min and is at least 10-fold faster than M-PCR. Conclusions: The ICA test strip developed in this study has proved to be a rapid, simple, effective and economical method for the detection of P. aeruginosa infection in clinical samples. To our knowledge, this is the first report of an ICA method being used to detect P. aeruginosa. [ABSTRACT FROM AUTHOR]

Published

2011

45. An evaluation of the RIDASCREEN and IDEIA enzyme immunoassays and the RIDAQUICK immunochromatographic test for the detection of norovirus in faecal specimens

Author

Kirby, Andrew, Gurgel, Ricardo Q., Dove, Winifred, Vieira, Sarah Cristina F., Cunliffe, Nigel A., and Cuevas, Luis E.

Subjects

*ENZYME-linked immunosorbent assay, *CHROMATOGRAPHIC analysis, *NOROVIRUSES, *GASTROENTERITIS, *REVERSE transcriptase polymerase chain reaction, *NOSOCOMIAL infections, *EPIDEMIOLOGY, *FECES, *DIAGNOSIS

Abstract

Abstract: Background: The detection of norovirus by ELISA and immunochromatographic methods may facilitate epidemiological studies into the global disease burden associated with norovirus gastroenteritis and provide a quick method of testing for norovirus infection. Objectives: To evaluate the new RIDASCREEN norovirus ELISA (3rd generation) and RIDAQUICK norovirus immunochromatographic test on a collection of samples from Brazilian children with acute gastroenteritis, and compare them against the established 2nd generation IDEIA norovirus assay. Study design: Reverse transcriptase PCR, the study reference standard, was used to test 726 specimens for the presence of norovirus. All 96 norovirus positive samples and a systematic selection of negative samples were tested by RIDASCREEN, RIDAQUICK and IDEIA norovirus tests. Results: The sensitivity of RIDASCREEN for the detection of norovirus was 63% (95% CI: 53–72%) and RIDAQUICK 69% (95% CI: 58–78%); both were >98% specific. The IDEIA had a sensitivity of 45% (95% CI: 35–55%), significantly lower than RIDASCREEN and RIDAQUICK (p ≤0.01). The sensitivity of RIDASCREEN and RIDAQUICK in detecting GII.4 noroviruses, the principal norovirus strain identified in community and nosocomial infection globally, was 78% and 88% respectively. Conclusion: The norovirus RIDASCREEN test may be useful in epidemiological studies of norovirus infection and the norovirus RIDAQUICK test offers an accurate and rapid method of detecting norovirus infection. [ABSTRACT FROM AUTHOR]

Published

2010

46. An Immunochromatographic Test for the Diagnosis of Ricin Inhalational Poisoning.

Author

Guglielmo-Viret, Valérie, Splettstoesser, Wolf, and Thullier, Philippe

Subjects

*RICIN, *BIOLOGICAL weapons, *IMMUNOGLOBULINS, *TOXINS, *CHROMATOGRAPHIC analysis, *DIAGNOSIS

Abstract

Introduction. Aerosolized ricin is a feared bioweapon for which no diagnostic protocol is currently available. Methods. We obtained antibodies to develop an immunochromatographic test (ICT) that would be part of such a protocol. Results. Our ICT, that can be read with the naked eye, has a sensitivity of 1 ng ricin/mL buffer, without enhancement, making it the most sensitive rapid test available for this toxin as far as we know. Its dynamic range extends to 10 μg/mL, with a plateau from 10 to at least 250 μg/mL (no "hook effect"), and it has limited cross-reactivity with other lectins. Discussion. Calculated from experimental and animal data, sampling with nasal swabs and testing with the devised ICT should give more than a thousand times the sensitivity required to diagnose ricin inhalational poisoning. Such a margin is particularly valuable in the absence of clinical data. Conclusion. This cost-effective and easy to use diagnostic tool could assist in the diagnosis of inhalational exposure from ricin aerosols. [ABSTRACT FROM AUTHOR]

Published

2007

47. Development of immunochromatographic device as a point-of-care tool for serodiagnosis of human strongyloidiasis cases

Author

Sadaow, Lakkhana, Sanpool, Oranuch, Rodpai, Rutchanee, Boonroumkaew, Patcharaporn, Maleewong, Wanchai, and Intapan, Pewpan M.

Published

2020

48. Rapid Immunochromatographic Test for the Identification and Discrimination of Mycobacterium tuberculosis Complex Isolates from Non-tuberculous Mycobacteria.

Author

SHENOY, VISHNU PRASAD and MUKHOPADHYAY, CHIRANJAY

Subjects

*MYCOBACTERIUM tuberculosis, *TUBERCULOSIS diagnosis, *CHROMATOGRAPHIC analysis, *TUBERCULIN test, *DRUGS, *MYCOBACTERIAL disease treatment, *MYCOBACTERIA, *DIAGNOSIS

Abstract

Background: A new rapid Immunochromatographic test (ICT) kit (SDBioline TB Ag MPT64RAPID®) developed by Standard Diagnostics, South Korea was evaluated for rapid differentiation of M. tuberculosis from non tuberculous mycobacteria (NTM). It detects MPT 64 antigen in M. tuberculosis isolates using mouse monoclonal MPT 64 antibody. The kit was assessed for routine identification of the Acid Fast Bacilli(AFB) isolated in our laboratory. Materials and Methods: Two hundred eight culture isolates of Mycobacteria were tested using ICT test kit for detection of MPT 64 antigen from liquid and solid culture. H37Rv strain was employed as the positive reference control. Any negative result was referred for confirmation by Gen Probe Accu Probe assay for MTB Complex (Gen-Probe, San Diego, Calif.). Speciation of NTM was performed using genotypic Mycobacterium CM assay (Hain's life sciences, Germany). Results: Of the 208 culture positive isolates tested, 182 (87.5%) were found positive for Mycobacterium tuberculosis Complex and remaining 26 (12.5%) were considered as NTM. These results were further confirmed by Gen Probe Accu probe assay that served as the reference method for detection of MTBC. H37Rv reference strain was taken as a control for ICT test and molecular tests. The reference strain showed the presence of MPT64 antigen band in the ICT test. Similar bands were formed in all MTBC (182) isolates tested, proving 100 per cent sensitivity and no bands were detected in 48 (100%) NTM isolates tested, proving 100 per cent specificity of the ICT kit. Conclusion: Tuberculosis is a global pandemic. Rapid identification of Mycobacteria as MTB complex or non-tuberculous Mycobacteria from culture is important for treatment of infected cases and drug susceptibility testing of the culture isolate. MPT 64 TB antgen detection using SD Bioline Immunochromatographic test is a simple and cost effective method for differentiation of Mycobacterial cultures as MTB complex from non- tuberculous Mycobacteria. [ABSTRACT FROM AUTHOR]

Published

2014

49. Pressure/colorimetric dual-readout immunochromatographic test strip for point-of-care testing of aflatoxin B1.

Author

Jiang, Shan, Zhang, Lvxia, Li, Jizhou, Ouyang, Hui, and Fu, Zhifeng

Subjects

*POINT-of-care testing, *AFLATOXINS, *PLATINUM nanoparticles, *DIAGNOSIS, *HYDROGEN peroxide, *FOOD quality, *FAULT diagnosis

Abstract

Immunochromatographic test strip (ITS) for point-of-care testing (POCT) has attracted prominent attention due to the advantages including rapid response, low cost and good portability. Here, we developed a sensitive ITS for detecting aflatoxin B 1 (AFB 1) by using dendritic platinum nanoparticles (DPNs) as novel pressure/colorimetric dual-readout probes. DPNs-labeled antibody of AFB 1 were used as the signal tracer of the immunochromatographic process. After 10-min competitive immunoreaction, black color appeared on the test line of ITS due to the accumulation of DPNs, which was observed visually as a colorimetric readout for qualitation purpose. Furthermore, DPNs with peroxidase-like activity caused decomposition of hydrogen peroxide aqueous solution to produce pressure change signal in vials, which was detected by a hand-held pressure meter for quantitation purpose. With the pressure readout mode, the detection range was 0.05–10 ng mL−1, and the detection limit was 0.03 ng mL−1 (S/N = 3) for AFB 1. The proposed ITS was successfully utilized for detecting AFB 1 in herbal medicine samples, and the acceptable recoveries of 93.77–114.09% indicated the reliability for real sample detection. It provides a new avenue for POCT with great application potential in various area including drug and food quality control, pollutants monitoring as well as medical diagnosis. Dendritic platinum nanoparticles were adopted as colorimetric/pressure probes to develope a dual-readout immunochromatographic test strip for detecting aflatoxin B 1. [Display omitted] • Dendritic platinum nanoparticles were utilized as dual-readout signal probes for immunochromatographic test strip. • A hand-held pressure meter was used as a portable detector for realizing sensitive and precise quantitation. • It provides a point-of-care testing device suitable for resource-limited countries or institutes. [ABSTRACT FROM AUTHOR]

Published

2021

50. Comparison between an immunochromatographic test with an amplified ELISA for detecting e antigen and anti-e antigen antibodies in chronic Hepatitis B.

Author

Mainet-González, Damián, Palenzuela-Gardon, Daniel O., and Rubido, Julio C. Aguilar

Subjects

*HEPATITIS associated antigen, *ENZYME-linked immunosorbent assay, *ANTIGENS, *BIOMARKERS, *HEPATITIS B, *HEPATITIS B virus, *SERUM, *PATIENTS

Abstract

The disappearance of the e antigen and the appearance of anti-e antigen antibodies are two biomarkers that indicate favorable prognosis in Hepatitis B. In this study the Advanced Quality™ immunochromatographic test for detecting those biomarkers was compared to the Vidas® semi-quantitative ELISA test. Our hypothesis was that it is possible to use these biomarkers measured in a rapid and simple Advanced Quality™ immunochromatographic test for evaluating the therapeutic response in clinical trials with chronic hepatitis B patients. The two methods were done following the manufacturer's instructions. The sera were taken from 69 patients with chronic hepatitis B of the clinical trial of the CIGB 440 therapeutic candidate. The immunochromatographic test and ELISA for detecting e antigen and anti-e antigen antibodies presented from substantial to almost perfect agreement in the evaluation of the sera of chronic Hepatitis B patients in a clinical trial. The immunochromatographic test for detecting e antigen had a low positive average agreement and a high negative average agreement compared to the ELISA. Nevertheless, the immunochromatographic test for detecting anti-e antigen antibodies had a high negative and positive average agreement in comparison to the ELISA. The immunochromagraphic test for the e antigen had a lower positive average agreement compared to the ELISA and some patients infected with Hepatitis B virus could not be detected by the former assay. The immunochromatographic test for anti-e antigen antibodies showed a similar performance to that of ELISA and could therefore be used in clinical trials for chronic Hepatitis B in health institutions without the need of a highly qualified lab technician. [ABSTRACT FROM AUTHOR]

Published

2009