Resolution of multiclonal infections of Trypanosoma cruzi from naturally infected triatomine bugs and from experimentally infected mice by direct plating on a sensitive solid medium |
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Authors: | Yeo Matthew Lewis Michael D Carrasco Hernan J Acosta Nidia Llewellyn Martin da Silva Valente Sebastião Aldo de Costa Valente Vera de Arias Antonieta Rojas Miles Michael A |
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Affiliation: | Department of Infectious and Tropical Diseases, London School of Hygiene and Tropical Medicine, Keppel Street, London, WC1E 7HT, UK. Matthew.yeo@lshtm.ac.uk |
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Abstract: | The isolation of biological clones of Trypanosoma cruzi by microscopically dispensing individual organisms or by serial dilution is laborious and time consuming. The inability to resolve mixed T. cruzi infections, from vectors and hosts, and to isolate clones of slow growing genotypes by efficient plating on solid media, has hindered characterisation studies and downstream applications. We have devised and validated a sensitive, solid medium plating technique for rapid in vitro isolation of clones representative of all the recognised T. cruzi lineages (TCI, TCIIa-e), including the slow growing strain CANIII (TC IIa) and Trypanosoma rangeli, with high plating efficiencies. Furthermore, the method is effective for the isolation of clones directly from silvatic triatomine bugs and from experimentally infected mice harbouring mixed infections, allowing resolution of multiclonal infections from varied sources. |
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Keywords: | Cloning Culture Lineage Multiclonal Trypanosoma cruzi Trypanosoma rangeli |
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