Empirical verification of heterogeneous DNA fragments generated from wheat genome-specific SSR primers

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dc.creator Chen, Qijiao
dc.creator Zhang, Lianquan
dc.creator Yuan, Zhongwei
dc.creator Yan, Zehong
dc.creator Zheng, Youliang
dc.creator Sun, Genlou
dc.creator Liu, Dengcai
dc.date.accessioned 2013-07-30T18:18:17Z
dc.date.available 2013-07-30T18:18:17Z
dc.date.issued 2008
dc.identifier.issn 0008-4220
dc.identifier.uri http://library2.smu.ca/xmlui/handle/01/25039
dc.description Publisher's version/PDF
dc.description.abstract Due to the high polymorphisms between synthetic hexaploid wheat (SHW) and common wheat, SHW has been widely used in genetic studies. The transferability of simple sequence repeats (SSR) among common wheat and its donor species, Triticum turgidum and Aegilops tauschii, and their SHW suggested the possibility that some SSRs, specific for a single locus in common wheat, might appear in two or more loci in SHWs. This is an important genetic issue when using synthetic hexaploid wheat population and SSR for mapping. However, it is largely ignored and never empirically well verified. The present study addressed this issue by using the well-studied SSR marker Xgwm261 as an example. The Xgwm261 produced a 192 bp fragment specific to chromosome 2D in common wheat Chinese Spring, but generated a 176 bp fragment in the D genome of Ae. tauschii AS60. Chromosomal location and DNA sequence data revealed that the 176 bp fragment also donated by 2B chromosome of durum wheat Langdon. These results indicated that although a single 176 bp fragment was appeared in synthetic hexaploid wheat Syn-SAU-5 between Langdon and AS60, the fragment contained two different loci, one from chromosome 2D of AS60 and the other from 2B of Langdon which were confirmed by the segregating analysis of SSR Xgwm261 in 185 plants from a F2 population between Syn-SAU-5 and Chinese Spring. If Xgwm261 in Syn-SAU-5 was considered as a single locus in genetic analysis, distorted segregation or incorrect conclusions would be yielded. A proposed strategy to avoid this problem is to include SHW’s parental T. turgidum and Ae. tauschii in SSR analysis as control for polymorphism detection. en_CA
dc.description.provenance Submitted by Trish Grelot (trish.grelot@smu.ca) on 2013-07-30T18:18:17Z No. of bitstreams: 1 sun_genlou_et_al_article_2008.pdf: 279060 bytes, checksum: de3fd76d0814b1e133f28491dc02ac63 (MD5) en
dc.description.provenance Made available in DSpace on 2013-07-30T18:18:17Z (GMT). No. of bitstreams: 1 sun_genlou_et_al_article_2008.pdf: 279060 bytes, checksum: de3fd76d0814b1e133f28491dc02ac63 (MD5) Previous issue date: 2008 en
dc.language.iso en en_CA
dc.publisher Agricultural Institute of Canada en_CA
dc.subject.lcsh Wheat -- Genetics
dc.title Empirical verification of heterogeneous DNA fragments generated from wheat genome-specific SSR primers en_CA
dc.type Text en_CA
dcterms.bibliographicCitation Canadian Journal of Plant Science 88(6), 1065-1071. (2008)
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