Design of an internal amplification control for a duplex PCR used in the detection of Shiga toxin producing Escherichia coli in pediatric feces

A. G. SALINAS; C. LUCERO ESTRADA; C. S. CHIALVA; J. M. ZARATE; M. JURI AYUB; M. E. ESCUDERO

Molecular and Celluar Probes

El Sevier

Año: 2015 vol. 29 p. 351 - 357

0890-8508

A conventional PCR targeted directly to the detection of Shiga toxin-producing Escherichia coli (STEC) in diarrheal stools of symptomatic patients may require the introduction of internal controls to detect false negative results. In the present study, we designed a competitive internal amplification control (IAC) to be included in a well-known PCR protocol used to amplify the stx1 and stx2 genes from STEC isolates. The IAC was introduced in the PCR reaction and amplified when E. coli O157:H7 cultures and contaminated pediatric feces were assayed. When STEC concentration was 10^3 CFU ml-1 in pure culture and 10^4 CFU g-1 in contaminated stools, the IAC at concentration of 0.143 pg ul-1 in the PCR reaction mixture was co-amplified with the stx2 sequence, producing bands of 279 and 349 bp, respectively. These STEC values were considered the detection limits of the duplex PCR. The specific detection of STEC by duplex PCR including IAC might be achieved directly on pediatric feces when the pathogen load reaches concentrations of at least 10^4 CFU g-1.