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Prevalence, Molecular Identification, and Phylogenetic Analysis of Strongylus equinus in Horses in Al-Muthanna Province, Iraq | ||
| Iranian Journal of Veterinary Medicine | ||
| مقاله 10، دوره 20، شماره 2، خرداد و تیر 2026، صفحه 311-320 اصل مقاله (1.63 M) | ||
| نوع مقاله: Original Articles | ||
| شناسه دیجیتال (DOI): 10.32598/ijvm.20.2.1005901 | ||
| نویسندگان | ||
| Hussein Jabar Jasim* 1؛ Naer Abdulbari Madlool Alkaabawi1؛ Zahraa Abd Alhammza Abbass2؛ Mohammed Mijbas Mohammed Alomari1 | ||
| 1Department of Microbiology and Parasitology, College of Veterinary Medicine, Al-Muthanna University, Al-Muthanna, Iraq. | ||
| 2Department of Parasitology, College of Medicine, University of Al-Muthanna, Al-Muthanna, Iraq. | ||
| چکیده | ||
| Background: Gastrointestinal parasites, particularly Strongylus spp., represent a critical challenge to equine health and productivity in developing nations. Objectives: This study aims to provide the first molecular and phylogenetic characterization of Strongylus equinus in horses in Iraq, using the internal transcribed spacer (ITS-1) region of rDNA as a marker for species-level identification. It has not been reported previously in the Middle East. Additionally, it establishes baseline data on age, sex, and season-linked risk factors influencing Strongylus spp. prevalence in Al-Muthanna Province, Iraq, a previously unstudied region, thereby addressing critical gaps in the epidemiology of equine parasites. Methods: The flotation technique was performed on 118 horse fecal samples, randomly collected from stables in Al-Muthanna Governorate, Southern Iraq, from January to the end of October 2023. Then, polymerase chain reaction (PCR) was performed using species-specific primers (StrongF/StrongR) for 50 samples. Three high-quality PCR products with strong band intensity from local S. equinus isolates were sent for sequencing. Results: The epidemiological analysis discovered that 50(42.3%) out of 118 horses were positive for Strongylus spp. infection via the flotation technique. Infection rates were significantly higher in horses under 4 years of age (57.1%); this difference was not statistically significant (P>0.05). Also, the highest prevalence rate was recorded during March (83.3%), and in females (56.2%) (P≤0.05). Moreover, PCR confirmed the presence of S. equinus in 22(44%) out of 50 morphologically positive samples. Partial ITS-1 sequence analysis of the local isolates (PQ900954.1, PQ900955.1, and PQ900956.1) revealed a high degree of similarity to strains from Australia (97%–100%) and to a Chinese isolate (94%). Conclusion: Strongylosis is an important veterinary disease in local horses, with a 42.3% prevalence and significant association with the month and sex. Phylogenetic analysis revealed significant genetic similarity between strains from Iraq and Australia, highlighting the importance of molecular diagnostics to improve parasite management, prevent the spread of zoonotic diseases, and enhance livestock health. | ||
| کلیدواژهها | ||
| Horses؛ Phylogenetic tree؛ Polymerase chain reaction (PCR)؛ Prevalence؛ Strongylos | ||
| اصل مقاله | ||
|
Introduction
Sample size (n=118) was calculated based on an expected prevalence of 50% from previous studies, a 95% confidence interval, and a precision ±9%. Five-gram fecal samples were obtained from each horse, either during rectal examination by a plastic glove or from fresh fecal deposits. Each sample was individually stored in a container, clearly labeled with age, sex, and date of collection, and transported to the laboratory in insulated containers with ice packs for direct examination using the flotation method. Then, samples that tested positive by microscopic examination were kept at 4 °C for later DNA extraction. Horses were divided into three age categories, namely under four years, four to seven years, and over seven years, based on owner-provided information and dental formulas, as per the methods outlined by Mezgebu et al. (2013).
The PCR amplification mixture for the detection of the ITS-1 region of rDNA included 25 µL of GoTaq® DNA polymerase 2X Master Mix (Promega, USِِA, and Cat. No. M7122) that contains (Taq polymerase, dNTPs, MgCl₂, and buffer), 5 µL DNA template (normalized to 150 ng), 1.5 μL of a 10 μM working stock of each primer (StrongF, StrongR), resulting in a final concentration of 0.3 µM for each primer, and completed the volume to 50 µL with nuclease-free water. The PCR amplification protocol consisted of an initial denaturation at 94 °C for 5 minutes, followed by 35 cycles of denaturation at 94 °C for 25 seconds, annealing at 56 °C (optimized based on primer Tm calculations and gradient PCR) for 25 seconds, and extension at 72 °C for 40 seconds. A final extension step at 72 °C for 5 minutes was performed. The specificity of the 220 bp product was confirmed by DNA sequencing. After amplification, 5 µL of each PCR product was subjected to electrophoresis on a 1.5% agarose gel and visualized under UV light using a transilluminator (Abdullah & Ali, 2021).
Epidemiologically, out of the 118 horses examined from January to the end of October 2023, 50 tested positive for Strongylus spp., with a prevalence rate of 42.3% based on the flotation technique. Concerning risk factors, infection rates were considerably higher in horses under 4 years of age (57.1%); however, this disparity was not statistically significant (P>0.05) (Table 2).
Also, the analysis demonstrated a statistically significant difference in infection rates based on sex, with female horses showing notably higher prevalence (56.2%) compared to male horses (32.8%) (P≤0.05) (Table 2). Moreover, the study identified significant seasonal variations in infection prevalence, with peak rates recorded in March (83.3%) and April (72.2%); these variations were statistically highly significant (P≤0.05) (Table 3).
Finally, the result of ITS-1 in local S. equinus based on phylogenetic analyses were recorded outstanding 100% and 97% identity matching between the current study isolates (PQ900954.1, PQ900955.1., and PQ900956.1) and an Australian strain isolated from horses (AJ228250.1, AJ228248.1), and 94% with Chinese isolate (KP693438.1) (Figure 4).
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