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Vol. 15. Issue 3.
Pages 204-210 (May - June 2011)
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Vol. 15. Issue 3.
Pages 204-210 (May - June 2011)
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Comparison of different primes for PCR-based diagnosis of cutaneous leishmaniasis
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Diego Molina de Oliveira1, Maria Valdrinez Campana Lonardoni2, Ueslei Teodoro2, Thais Gomes Verzignassi Silveira2,
Corresponding author
tgvsilveira@uem.br

Departamento de Análises Clínicas e Biomedicina, Universidade Estadual de Maringá, Av. Colombo 5790, Maringá, Paraná, Brazil 87020-900.
1 Postgraduate Student, Universidade Estadual de Maringá, PR, Brazil
2 Departament of Clinical Analysis, Universidade Estadual de Maringá, PR, Brazil
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Abstract
Objective

The objective of this study was to analyze different primers that are commonly used in epidemiological studies for the detection of Leishmania DNA by PCR, and to compare them to the conventional direct parasite search for American cutaneous leishmaniasis (ACL) diagnosis.

Material and methods

Five pairs of primers, four of them derived from Leishmania kDNA sequences (MP3H-MP1L; B1-B2; LBF1-LBR1; 13A-13B), and one derived from the SL RNA (mini-exon) gene repeat (LU5A-LB3C), reported previously, were used

Results and discussion

The MP3H-MP1L primers were the best at amplifying the DNA, detecting 2 fg of Leishmania spp. DNA. The 13A-13B primers presented the worst performance, detecting 512 x 103 fg of DNA.

Conclusion

The wide variation in the analytical sensitivity of the primers used in the PCR, and the significant differences from the conventional method of ACL diagnosis found in this study, emphasize the importance of standardizing the PCR technique, analyzing sensitivity, and selecting suitable oligonucleotide primers.

Keywords:
leishmaniasis
polymerase chain reaction
Leishmania
DNA primers
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