Ismaila Muritala scite author profile

Ismaila Muritala

2Publications

9Citation Statements Received

107Citation Statements Given

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Affiliations

Federal University of Agriculture

Publications

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Detecting the existence of gene flow between Spanish and North African goats through a coalescent approach

Martínez

Manunza

Delgado

et al. 2016

Sci Rep

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Human-driven migrations are one of the main processes shaping the genetic diversity and population structure of domestic species. However, their magnitude and direction have been rarely analysed in a statistical framework. We aimed to estimate the impact of migration on the population structure of Spanish and African goats. To achieve this goal, we analysed a dataset of 1,472 individuals typed with 23 microsatellites. Population structure of African and Spanish goats was moderate (mean FST = 0.07), with the exception of the Canarian and South African breeds that displayed a significant differentiation when compared to goats from North Africa and Nigeria. Measurement of gene flow with Migrate-n and IMa coalescent genealogy samplers supported the existence of a bidirectional gene flow between African and Spanish goats. Moreover, IMa estimates of the effective number of migrants were remarkably lower than those calculated with Migrate-n and classical approaches. Such discrepancies suggest that recent divergence, rather than extensive gene flow, is the main cause of the weak population structure observed in caprine breeds.

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Comparative study of molecular and non-molecular tools for peste des petits ruminants virus detection in West African Dwarf goats

Muritala

Bemji

Ozoje

et al. 2023

Preprint

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Peste des petits ruminants (PPR) causes severe economic losses to many countries of the world where the disease is endemic. It has been targeted for global eradication by 2030 following the successful eradication of rinderpest in 2011. The proposed eradication program would benefit from efficient and relatively reliable diagnostic tools for early PPR virus (PPRV) detection. A total of 33 eight to 12 months old West African Dwarf (WAD) goats were used. Nineteen goats infected by comingling with two PPR virus positive animals formed the infected group (PPRV-infected goats) while 14 non-infected goats formed the control group (CTG). The suitability of a molecular method (Hydroxyl naphthol blue (HNB) staining of reverse transcription loop mediated isothermal amplification (RT-LAMP)) and a non-molecular tool (haemagluttination assay (HA)) were compared for their sensitivity to detect the PPRV in PPRV-infected goats and non-infected CTG. PPR disease severity in WAD goats at different days post infection (dpi) was evaluated by clinical scoring and haemagluttination titre (HAT). HNB staining RT-LAMP reaction and HA showed sensitivities of 100% and 73.68%, respectively, for PPRV detection. Expression of PPR clinical signs began from 3 dpi, attained peak at 5 dpi, thereafter showed irregular patterns till 24 dpi. Evaluation of HAT in PPRV-infected goats at 12 dpi ranged from 2 to 64 haemagluttination units (HAU), while CTG goats had 0 HAU. In conclusion, HNB staining RT-LAMP assay demonstrated reasonable potential for accurate diagnoses of PPRV and as an important diagnostic tool in areas with poor electricity supply and less sophisticated laboratory equipment.

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