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Showing 2 results for Heterozygosity

M. H. Banabazi, S. Esmaeilkhanian, S. R. Miraei Ashtiani, M. Moradi Shahrbabak,
Volume 10, Issue 4 (1-2007)
Abstract

Genetic variation within and between five Iranian sheep populations including Sanjabi (SAN), Kordi Kordistan (KKO), Kordi Khorasan (KKH), Mehraban (MEH) and Moghani (MOG) was assessed using six microsatellite markers (McMA2, McMA26, MAF64, OarAE64, OarCP26 and OarFCB304). The PCR reactions were successfully perfomed with all primers except OarAE64. All locus-population combinations were at Hardy-Weinberg equilibrium except McMA2 in MOG population (P<0.005). Polymorphism criteria showed that the five studied loci were polymorphic in all populations. The lowest DA genetic distance (0.234) was observed between KKH and KKO and the highest (0.388) between SAN and MOG populations. The dendrograms based on DA distances were drawn using unweighted pair-group method using an arithmetic average (UPGMA) and neighbor-joining (NJ) method. KKO, KKH and SAN were grouped together at one cluster and MEH and MOG at another by both methods. The average expected heterozygosity for each populations (as interpopulation variation) ranged from 0.744 to 0.847 for KKH and MEH, respectively. The estimated time of divergence for two Kordi populations (KKO and KKH) was 445 years that complies with historical evidences. The findings of this research confirmed that microsatellite variation could be a useful tool for screening of investigating biodiversity among domestic animals.
S. Esmail Khanian, A. Negati Javaremi, F. Afraz, P. Daneshyar, S. Ghanbari,
Volume 11, Issue 41 (10-2007)
Abstract

In order to identify polymorphic microsatellite markers and evaluae genetic variation within Baluchi sheep population, nineteen microsatellite loci were studied. Whole Blood samples were collected from 156 sheep at north eastern animal breeding station of Iran (Abbasabad-Mashhad). DNA was extracted by salting-out procedure with some modifications. Polymerase chain reactions were successfully done except for UNC5C locus. PCR products were electrophoresed on 8% denaturing polyacrylamide gels stained according to rapid silver staining procedure. The genotype and allelic frequencies were calculated by direct counting and used for estimating of different polymorphism and genetic variation criteria. This population wasn't at Hardy-Weinberg equilibrium except for OarAE101 locus (P<0.005). Heterozygosity (gene variation) ranged from 0.1 to 0.93. BULGE5E and BM1329 loci were monomorphic. In conclusion, this investigation showed high polymorphism at the studied loci, so they could be used in future studies.

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