We determined the location of the processing plant for each sampl

We determined the location of the processing plant for each sample from the code on the packaging that indicates the processing plant.

Most milk samples were either fresh or frozen at −20°C before DNA extraction. Unpasteurized Selleckchem Crenigacestat samples were autoclaved at 104°C for 20 minutes before being processed. IACUC oversight for all samples (including sampling individual cows) was not required. DNA was extracted in triplicate for each sample using a selleckchem proteinase K and chelex protocol (see Additional file 1). For each sample, a no template control (NTC) was also included in the DNA extraction protocol to detect any cross-contamination. The quality of the DNA extractions were assessed by running a generalized 16S rRNA assay [45] on each extraction to ensure that PCR quality DNA was obtained. Any samples that failed 16S rRNA quality controls were re-extracted. Detection and genotyping of C. burnetii DNA C. burnetii DNA was detected in samples using an assay designed to detect the multicopy IS1111 element [26]. For each DNA extract, this assay was run in triplicate with each of the three DNA extraction replicates and the extraction NTC. If the extraction NTC amplified, the sample was put through the extraction protocol again. If any of the nine extract replicates amplified, the sample was considered to be positive for C. burnetii DNA. Samples that were positive for C. burnetii DNA

were genotyped with TaqMan assays derived from signatures presented by Hornstra et al. [20]. Primer and probe designs as well as reaction conditions PRN1371 are included in Additional file 1. For each PCR, an additional NTC was included to help detect cross contamination during template addition. Selleckchem Neratinib Cross contamination was a concern as the genotype results from most samples were identical. It is important to note also that before genotyping these samples, we had not had any samples of ST20 in our laboratory. To further ensure the integrity

of positive PCR results and that shared genotypes across samples were not due to contamination from a positive control, we designed synthetic positive controls for each assay containing C. burnetii signatures as well as a non-bacterial sequence targeted by a probe with a different dye color (Additional file 1). Acknowledgements We would like to thank our many friends, families and colleagues who sent us milk while traveling around the country. This work was supported by a grant from the Department of Homeland Security (HSHQDC-10-C-00139) to PK. AVK was supported by the Science Education Program Grant No. 52006323 from the Howard Hughes Medical Institute to Washington and Jefferson College. The findings and conclusions in this report are those of the authors and do not necessarily represent the views of the Centers for Disease Control and Prevention or the Department of Health and Human Services.

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