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ACTA HORTICULTURAE SINICA ›› 2018, Vol. 45 ›› Issue (1): 159-167.doi: 10.16420/j.issn.0513-353x.2017-0166

• Research Notes • Previous Articles     Next Articles

Development of SSR Molecular Markers Based on Transcriptome Sequencing of Tagetes erecta

ZHANG Huali1,CONG Richen1,WANG Maoliang1,Dong Aixiang1,XIN Haibo1,*,YI Mingfang2,and GUO Hua3,*   

  1. 1Beijing Institute of Landscape Architecture,Beijing Key Laboratory of Greening Plants Breeding,Beijing 100102,China;2Department of Ornamental Horticulture and Landscape Architecture,China Agricultural University,Beijing 100193,China;3Biyang Forest Diseases and Insect Pests Quarantine Station in Henan Province,Biyang,Henan 463721,China
  • Online:2018-01-25 Published:2018-01-25

Abstract: A total of 48 953 Unigenes were obtained by transcriptome sequencing of flower buds of Tagetes erecata. MISA found 20 666 SSRs located in 13 849 unigenes with the frequency of 28.29% and a mean distance of 2.51 kb per one. Trinucleotide and tetranucleotide were major types with the percentages of 50.16% and 20.94%,respectively. ATG/ATG and AAAC/GTTT were most frequent motifs in trinucleotide and tetranucleotide repeats,accounting for 13.82% and 3.66%,respectively. Based on different dominant motifs types,36 primers were chosen randomly and verified with 20 different inbred lines of Tagetes erecta. The results showed that 30 primers were effective with a valid rate of 80.56%,and 13 primers showed polymorphism with He and PIC mean values of 0.275 and 0.608,respectively. These data indicated that the Unigenes generated from transcriptome sequencing can be used as an effective source to develop SSR markers,and the large quantities of SSR markers will provide reliable resources for analysis on genetic polymorphism and constructing genetic map in Tagetes erecta.

Key words: Tagetes erecta L., SSR, transcriptome