Abstract
BackgroundStreptococcus equi subsp equi (S. equi) is the cause of “equine strangles” which is a highly infectious upper respiratory disease. Detection of S. equi is influenced by site of specimen collection, method of sampling, and type of diagnostic test that is performed. We hypothesized i) that a loop-mediated isothermal amplification (LAMP) assay that targets the S. equi-specific eqbE gene would be more sensitive than a realtime PCR assay that targets the S. equi-specific seeI gene and ii) that LAMP of specimens obtained by guttural pouch lavage (GPL) would be more sensitive than LAMP of nasopharyngeal specimens to identify S. equi carriers.MethodsA nasopharyngeal flocked swab, nasopharyngeal wash, and GPL specimen was collected from 44 convalescent horses and the eqbE LAMP assay was performed. The seeI realtime PCR assay and aerobic culture were also performed on the GPL specimen. Logistic regression was performed to compare sampling sites and test methods (P-values ≤0.05 were considered significant).ResultsOne of 41 nasopharyngeal flocked swabs, 6/38 nasopharyngeal wash and 24/44 GPL specimens were positive by eqbE LAMP. 18/44 GPL specimens were positive by seeI PCR and S. equi was isolated from 4/44 of these specimens. Detection of S. equi DNA was 51 times more likely from the GPL samples than nasopharyngeal samples (OR 51.0, P < 0.0001). When eqbE LAMP GPL samples were positive, it was eight times more likely that the guttural pouch had any abnormality on endoscopy (OR 8.2, P ≤ 0.005), almost 20 times more likely that mild empyema was found (OR 19.7, P ≤ 0.002), and eight times more likely that the SeeI PCR was positive for S. equi DNA (OR 8.1, P ≤ 0.006).ConclusionThis study demonstrates that guttural pouch lavage specimens should be used to detect S. equi and that the eqbE LAMP assay was comparable to the seeI PCR.
Highlights
Streptococcus equi subsp equi (S. equi) is the cause of “equine strangles” which is a highly infectious upper respiratory disease
One hundred and twenty-three samples were analyzed (Additional file 2: Table S2): 41 nasopharyngeal flocked swabs, 38 nasopharyngeal washes, and 44 guttural pouch lavages were obtained from 40 different horses on 44 separate occasions from all 6 different strangles outbreaks that occurred from November 2013 to November 2014 (Fig. 1)
This study provides strong evidence that the eqbE Loop-mediated isothermal amplification (LAMP) assay performed with guttural pouch specimens is more sensitive for the detection of S. equi than nasopharyngeal flocked swab or a nasopharyngeal wash taken from the same horse at the same time
Summary
Streptococcus equi subsp equi (S. equi) is the cause of “equine strangles” which is a highly infectious upper respiratory disease. Strangles, caused by Streptococcus equi subsp equi (S. equi), is a highly infectious upper respiratory disease that has a high morbidity rate and poses a high financial burden for the equine industry [1,2,3]. Bacterial culture and PCR of nasopharyngeal wash and guttural pouch lavage (GPL) specimens have been used to detect S. equi for diagnostic testing of clinical suspects and for the detection of carrier animals [2, 3, 5]. During the carrier state organisms may present at a very low number, may be shed intermittently or may be dead; yet their DNA will still be detectable by PCR. Practitioners must obtain multiple sequential samples from convalescing animals in order to ensure a 90% chance of true negatives before comingling with susceptible animals [5]
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