Evaluation of a real-time PCR assay based on the repetitive B1 gene for the detection of Toxoplasma gondii in human peripheral blood

Kompalic-Cristo, Alicia; Frotta, Cassia; Suárez-Mútis, Martha Cecília; Fernandes, Octávio; Britto, Constança

doi:10.1007/s00436-007-0524-9

Cited by 87 publications

(51 citation statements)

References 32 publications

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“…Furthermore, in our laboratory, peripheral blood of patients suspected of acute toxoplasmosis was also analyzed ( (Guy & Joynson, 1995). In a study involving patients with acute toxoplasmosis in southeastern Brazil, the rate of parasite DNA-positive peripheral blood samples was 48.6% (17/35) (Kompalic-Cristo et al, 2007). Interestingly, both of these studies used B1 as the target gene, which is considered to be of lower sensitivity than the AF146527 marker that we used; however, the total number of analyzed samples was smaller and the patient selection criteria may have differed.…”

Section: Clinical Significance In Various Biological Samplesmentioning

confidence: 94%

Molecular Detection and Genotyping of Toxoplasma gondii from Clinical Samples

Ivović¹,

Vujanić²,

Živković³

et al. 2012

Toxoplasmosis - Recent Advances

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Section: Clinical Significance In Various Biological Samplesmentioning

confidence: 94%

Molecular Detection and Genotyping of Toxoplasma gondii from Clinical Samples

Ivović¹,

Vujanić²,

Živković³

et al. 2012

Toxoplasmosis - Recent Advances

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“…The inclusion in PCR assays of genes that constitute cells such as β-actin, β-globin, albumin and G3PD has been useful to evaluate the quality of samples in qPCR and PCR experiments (20,34,47,48). Due to the recognized need for evaluating the integrity of DNA, controls are usually used in separate reactions, generating more costs and consuming more time to establish the diagnosis (49).…”

Section: Discussionmentioning

confidence: 99%

Application of the mammalian glyceraldehyde-3-phosphate dehydrogenase gene for sample quality control in multiplex PCR for diagnosis of leishmaniasis

Gonçalves¹,

Régis-da-Silva²,

Brito³

et al. 2012

J. Venom. Anim. Toxins incl. Trop. Dis

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Leishmaniasis is a neglected disease endemic in five continents. It is a severe disease that may lead to death, and its early detection is important to avoid severe damage to affected individuals. Molecular methods to detect Leishmania are considered alternatives to overcome the limitations presented by conventional methods. The aim of this study was to develop multiplex PCR systems able to detect small amounts of target DNA of Leishmania infantum and Leishmania braziliensis, and the gene coding for glyceraldehyde-3-phosphate dehydrogenase (G3PD) in mammals, enabling quality evaluation of the sample simultaneously with detection of the specific target. The systems created for G3PD recognition were combined with detection systems for L. infantum and L. braziliensis to compose multiplex PCR systems for visceral (mVL) and cutaneous (mACL) leishmaniasis diagnosis. The multiplex PCR systems developed were assessed in blood samples from five different species of mammal reservoirs involved in the disease cycle in Brazil, and 96 and 52 human samples from patients with suspected visceral leishmaniasis (VL) and cutaneous leishmaniasis (ACL), respectively. Three G3PD detection systems were created (G3PD1, G3PD2 and G3PD3) with different product sizes, G3PD2 was chosen for the formation of multiplex PCR systems. The two multiplex PCR systems (mVL and mACL) were reproducible in all species evaluated. Results of test samples (sensitivity, specificity and efficiency) suggest its use in routine diagnosis, research activities in medicine and veterinary medicine. Additionally, the systems designed to detect the G3PD gene are capable of combining with other targets used for molecular diagnosis of infectious diseases. Concerning leishmaniasis, the multiplex PCR systems can be used in epidemiological studies for the detection of new and classic reservoirs, which may contribute to the reliability of results and development of actions to control the disease.

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“…This study determines the mouse infectivity status primarily by animal health followed by a novel confirmation by a duplex qPCR assay instead of serology or immunohistochemistry. The B1 qPCR assay used to detect T. gondii in infected tissues was adopted from an assay developed by Kompalic-Cristo et al (39). This approach is very reliable and less labor-intensive than serology and immunohistochemistry and resulted in a dual detection of both mouse tissue and the presence or absence of T. gondii.…”

Section: Discussionmentioning

confidence: 99%

Determining UV Inactivation of Toxoplasma gondii Oocysts by Using Cell Culture and a Mouse Bioassay

Ware

Augustine²,

Erisman³

et al. 2010

Appl Environ Microbiol

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The effect of UV exposure on Toxoplasma gondii oocysts has not been completely defined for use in water disinfection. This study evaluated UV-irradiated oocysts by three assays: a SCID mouse bioassay, an in vitro T. gondii oocyst plaque (TOP) assay, and a quantitative reverse transcriptase real-time PCR (RT-qPCR) assay. The results from the animal bioassay show that 1-and 3-log 10 inactivation is achieved with 4 mJ/cm 2 UV and 10 mJ/cm 2 low-pressure UV, respectively. TOP assay results, but not RT-qPCR results, correlate well with bioassay results. In conclusion, a 3-log 10 inactivation of T. gondii oocysts is achieved by 10-mJ/cm 2 low-pressure UV, and the in vitro TOP assay is a promising alternative to the mouse bioassay.

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Evaluation of a real-time PCR assay based on the repetitive B1 gene for the detection of Toxoplasma gondii in human peripheral blood

Cited by 87 publications

References 32 publications

Molecular Detection and Genotyping of Toxoplasma gondii from Clinical Samples

Molecular Detection and Genotyping of Toxoplasma gondii from Clinical Samples

Application of the mammalian glyceraldehyde-3-phosphate dehydrogenase gene for sample quality control in multiplex PCR for diagnosis of leishmaniasis

Determining UV Inactivation of Toxoplasma gondii Oocysts by Using Cell Culture and a Mouse Bioassay

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