ATG-anchored AFLP (ATG-AFLP) analysis in cotton

被引:9
作者
Lu, Yingzhi [1 ]
Curtiss, Jessica [1 ]
Miranda, Danielle [1 ]
Hughs, Ed [2 ]
Zhang, Jinfa [1 ]
机构
[1] New Mexico State Univ, Dept Plant & Environm Sci, Las Cruces, NM 88003 USA
[2] USDA ARS, SW Cotton Ginning Res Lab, Mesilla Pk, NM 88003 USA
关键词
Gossypium hirsutum; G; barbadense; AFLP; ATG-AFLP;
D O I
10.1007/s00299-008-0568-z
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
Amplified fragment length polymorphism (AFLP) marker system has had broad applications in biology. However, the anonymous AFLP markers are mainly amplified from non-coding regions, limiting their usefulness as a functional marker system. To take advantages of the traditional AFLP techniques, we propose substitution of a restriction enzyme that recognizes a restriction site containing ATG, called ATG-anchored AFLP (ATG-AFLP) analysis. In this study, we chose NsiI (recognizing ATGCAT) to replace EcoRI in combination with MseI to completely digest genomic DNA. One specific adaptor, one pre-selective primer and six selective amplification primers for the NsiI site were designed for ligation and PCR. Six NsiI and eight MseI primers generated a total of 1,780 ATG-AFLP fragments, of which 750 (42%) were polymorphic among four genotypes from two cultivated cotton species (Upland cotton, Gossypium hirsutum and Pima cotton, G. barbadense). The number of ATG-AFLP markers was sufficient to separate the four genotypes into two groups, consistent with their evolutionary and breeding history. Our results also showed that ATG-AFLP generated less number of total and polymorphic fragments per primer combination (2-3 vs. 4-5) than conventional AFLP within Upland cotton. Using a recombination inbred line (RIL) population, 62 polymorphic ATG-AFLP markers were mapped to 19 linkage groups with known chromosome anchored simple sequence repeat (SSR) markers. Of the nine ATG-AFLP fragments randomly chosen, three were found to be highly homologous to cotton cDNA sequences. An in-silico analysis of cotton and Arabidopsis cDNA confirmed that the ATG-anchored enzyme combination NsiI/MseI did generate more fragments than the EcoRI/MseI combination.
引用
收藏
页码:1645 / 1653
页数:9
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