Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice

Aongart Mahittikorn; Wickert, Hannes; Yaowalark Sukthana

Publication:
Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice

Issued Date

2010

Resource Type

Article

Language

eng

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Mahidol University

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PubMed

Bibliographic Citation

Experimental Parasitology. Vol.124, No. 2 (2010), 225-231

Suggested Citation

Aongart Mahittikorn, Wickert, Hannes, Yaowalark Sukthana Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice. Experimental Parasitology. Vol.124, No. 2 (2010), 225-231. Retrieved from: https://repository.li.mahidol.ac.th/handle/20.500.14594/10493

Title

Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice

Author(s)

Aongart Mahittikorn
Wickert, Hannes
Yaowalark Sukthana

Other Contributor(s)

Mahidol University. International College.

Abstract

Toxoplasmic encephalitis (TE) is caused by reactivation of dormant bradyzoites into rapidly dividing tachyzoites of the apicomplexan parasite Toxoplasma gondii in immune-compromised hosts. Diagnosis of this life-threatening disease is complicated, since it is difficult to distinguish between these two stages. It is,therefore, mainly based on a test positive for T. gondii antibodies, and specific clinical symptoms. We developed a duplex RT-PCR to detect the expression of bradyzoite (BAG1) and tachyzoite (SAG1) specific genes simultaneously during tachyzoite/bradyzoite stage conversion. The conversion reaction was observed in many organs of experimental mice, indicated by tachyzoites in the cerebrum, cerebellum, heart and lung, beginning in week 1 after the suppression period, and continuing until the end. Bradyzoites were also detected in nearly all organs throughout the study, suggesting that during the reactivation period, bradyzoites not only escape from cysts and reinvade neighboring cells as tachyzoites, but are also driven into developing new bradyzoites. The results of our study show that duplex RT-PCR is an easy, rapid, sensitive, and reproducible method, which is particularly valuable when numerous samples must be analyzed. This technique may usefully serve as an alternate tool for diagnosing TE in severely immunocompromised patients.

Keyword(s)

Duplex RT-PCR
Mice
Stage conversion
Toxoplasma gondii

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Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice

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Publication: Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice

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Publication:
Toxoplasma gondii: simple duplex RT-PCR assay for detecting SAG1 and BAG1 genes during stage conversion in immunosuppressed mice