BackgroundLeptospirosis has long been a major public health concern in the southwestern Indian Ocean. However, in Madagascar, only a few, old studies have provided indirect serological evidence of the disease in humans or animals.Methodology/Principal FindingsWe conducted a large animal study focusing on small-mammal populations. Five field trapping surveys were carried out at five sites, from April 2008 to August 2009. Captures consisted of Rattus norvegicus (35.8%), R. rattus (35.1%), Mus musculus (20.5%) and Suncus murinus (8.6%). We used microbiological culture, serodiagnosis tests (MAT) and real-time PCR to assess Leptospira infection. Leptospira carriage was detected by PCR in 91 (33.9%) of the 268 small mammals, by MAT in 17 of the 151 (11.3%) animals for which serum samples were available and by culture in 9 of the 268 animals (3.3%). Rates of infection based on positive PCR results were significantly higher in Moramanga (54%), Toliara (48%) and Mahajanga (47.4%) than in Antsiranana (8.5%) and Toamasina (14%) (p = 0.001). The prevalence of Leptospira carriage was significantly higher in R. norvegicus (48.9%), S. murinus (43.5%) and R. rattus (30.8%) than in M. musculus (9.1%) (p<0.001). The MAT detected antibodies against the serogroups Canicola and Icterohaemorrhagiae. Isolates were characterized by serology, secY sequence-based phylogeny, partial sequencing of rrs, multi-locus VNTR analysis and pulsed field gel electrophoresis. The 10 isolates obtained from nine rats were all identified as species L. interrogans serogroup Canicola serovar Kuwait and all had identical partial rrs and secY sequences.Conclusions/SignificanceWe present here the first direct evidence of widespread leptospiral carriage in small mammals in Madagascar. Our results strongly suggest a high level of environmental contamination, consistent with probable transmission of the infection to humans. This first isolation of pathogenic Leptospira strains in this country may significantly improve the detection of specific antibodies in human cases.
The equine disease strangles, which is characterized by the formation of abscesses in the lymph nodes of the head and neck, is one of the most frequently diagnosed infectious diseases of horses around the world. The causal agent,
Streptococcus equi
subspecies
equi
, establishes a persistent infection in approximately 10 % of animals that recover from the acute disease. Such ‘carrier’ animals appear healthy and are rarely identified during routine veterinary examinations pre-purchase or transit, but can transmit
S. equi
to naïve animals initiating new episodes of disease. Here, we report the analysis and visualization of phylogenomic and epidemiological data for 670 isolates of
S. equi
recovered from 19 different countries using a new core-genome multilocus sequence typing (cgMLST) web bioresource. Genetic relationships among all 670 S.
equi
isolates were determined at high resolution, revealing national and international transmission events that drive this endemic disease in horse populations throughout the world. Our data argue for the recognition of the international importance of strangles by the Office International des Épizooties to highlight the health, welfare and economic cost of this disease. The Pathogenwatch cgMLST web bioresource described herein is available for tailored genomic analysis of populations of
S. equi
and its close relative
S. equi
subspecies
zooepidemicus
that are recovered from horses and other animals, including humans, throughout the world. This article contains data hosted by Microreact.
20The major role of EHV-1 in equine abortion is widely reported in the literature but the 21 contribution of EHV-2, EHV-3, EHV-4 or EHV-5 remains less well documented. The 22 objective of this study is to evaluate the contribution of these five different EHVs to equine 23 abortion in a variety of biological tissues using a consensus polymerase chain reaction (PCR). 24The test was validated for specificity and sensitivity in horses before screening specimens 25 from 407 foetuses, stillbirths and premature foals collected over a 2½-year interval. Positive 26 results obtained with this assay were compared to other EHV type-specific PCR or by 27 sequencing. EHV-1 was identified as the major cause of abortion in French mares (59/407 28 cases). However, there was evidence to suggest some variation in the potential of EHV-1 29 strains to induce abortion. Indeed, DNA samples from EHV-2 (in three cases) and EHV-5 (in 30 one case) inferred a role of these viruses in abortion. The presence of viral DNA from EHV-3 31 or EHV-4 strains was not detected in the specimens studied. The data obtained suggest that 32 the consensus herpesvirus PCR is an efficient screening tool. In association with a specific 33 PCR, the test provides a rapid identification of the type of herpesvirus involved in abortion 34 and is useful for routine diagnostic tests as it allows the identification of herpesviruses other 35 than the EHV-1 strain. 36 37
Abstract. Studies were carried out to determine the cause of death in a prematurely born Thoroughbred foal that died 24 hours after birth. Necropsy revealed gross lesions suggestive of septicemia. A commercial Leptospira polymerase chain reaction (PCR) assay designed to specifically amplify the hemolysis-associated protein 1 (hap1) gene present only in pathogenic Leptospira strains detected the presence of Leptospira DNA in various tissues of the foal. Histologic examination of lung, liver, kidney, and myocardium revealed numerous spirochetes in Warthin-Starry-stained tissue sections. Results of PCR analysis and histologic examination suggested a leptospiral infection in the newborn foal. At the moment of death, the infection coexisted with a streptococcal-associated aspiration bronchopneumonia and postpartum septicemia. These findings indicate that the PCR assay based on the amplification of the hap1 gene represents a useful tool for specific detection of pathogenic leptospira in field samples taken from horses.
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