Fig. 1

Diagram illustrating experimental procedures of the present study. Two horses (Group 1) were exposed to rickettsial infection through infestation with Rickettsia rickettsii-infected Amblyomma sculptum ticks. Two other horses (Group 2) were infected through intraperitoneal inoculation of a homogenate of R. rickettsii-infected guinea pig organs. The four horses were clinically evaluated and infested with uninfected A. sculptum ticks (larvae, nymphs and adults) during 30 days. Recovered ticks were reared to the next developmental stage and/or tested by real-time PCR for detection of rickettsial DNA. Molted, unfed ticks were allowed to feed on tick-naïve rabbits, which were clinically evaluated for 21 days and tested by seroconversion through testing paired serum samples (days 0 and 21 post-infestation) against R. rickettsii antigens. Solely for horse 1, a sample of unfed nymphs and adults, resulting from molting of engorged larvae and nymphs, respectively, was subjected to real-time PCR, and the remaining unfed ticks were fed on the rabbits. For the other three horses, all unfed nymphs and adults were placed on rabbits