ST, DW, MD, BDB and AN participated in the molecular 3-Methyladenine order studies. KL helped in the collection of isolates from poultry farms in France and participated in the design of the study. DW collected isolates from poultry farms in China. FB participated in draft of the manuscript.
All the authors read and approved the final manuscript.”
“Background A group of diverse pathogens has the potential to cause high morbidity and mortality in humans -especially if carried by aerosols- even though they do not pose a major threat to public health under normal circumstances. The most menacing bacterial pathogens of this group are Bacillus anthracis, Francisella tularensis and Yersinia pestis, and these organisms are listed as category A biothreat agents (classification of the CDC, USA, http://www.bt.cdc.gov/agent/agentlist-category.asp) because of the potential danger of their deliberate release. Selleck SB-715992 Exposure to aerosolized B. anthracis spores and F. tularensis can lead to inhalational
anthrax and tularemia. Y. pestis may cause pneumonic plague, which, unlike the other two diseases, may also spread from person to person. To reduce the public health impact Selleck Entinostat of such highly pathogenic micro-organisms, rapid and accurate diagnostic tools for their detection are needed. Timely recognition of disease agents will enable appropriate treatment of exposed individuals which will be critical to their survival, and the spread of disease can be reduced by taking appropriate public health measures. Classical identification involves culturing suspect pathogens, but although culturing can be very sensitive, these methods are time consuming, PAK6 not very specific, involve extensive biosafety measures and some organisms simply resist cultivation. Real-time qPCR methods for the detection of pathogens can be equally or more sensitive, and can also provide higher speed and specificity. Also, molecular methods require only preparatory handling of samples under biosafety conditions and can be easily scaled-up, which is important for speeding
up investigations and control of disease progression in outbreak situations. Despite these manifold advantages, detection of DNA does not yield information about the presence of viable organisms. Multiplexing qPCR detection offers several advantages, including reduction of sample volume and handling time (reducing the analysis time, cost and opportunities for lab contamination). Also, false-negative results can be reduced through co-amplification of internal controls in each sample, and using multiple redundant genetic markers for each organism reduces the chance that strain variants are missed. Amplification of multiple signature sequences per organism will also reduce false-positive results in complex samples.