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Acta Agron Sin ›› 2010, Vol. 36 ›› Issue (10): 1691-1697.doi: 10.3724/SP.J.1006.2010.01691

• CROP GENETICS & BREEDING·GERMPLASM RESOURCES·MOLECULAR GENETICS • Previous Articles     Next Articles

Establishment of Agrobacterium tumefaciens -mediated Anther Calli Transformation System in Hevea brasiliensis

HUANG Tian-Dai,LI Zhe,SUN Ai-Hua,ZHOU Quan-Nan,HUA Yu-Wei,HUANG Hua-Sun*   

  1. Rubber Research Institute of Chinese Academy of Tropical Agricultural Sciences / National Rubber Tree Breeding Centre / Key Laboratory of Rubber Biology / Ministry of Agriculture / State Key Laboratory Breeding Base of Cultivation & Physiology of Tropical Crops, Danzhou 571737, China
  • Received:2010-02-05 Revised:2010-04-20 Online:2010-10-12 Published:2010-07-05
  • Contact: HUANG Hua-Sun,E-mail:xjshhs@163.com

Abstract: Developping a new Hevea variety by crossing breeding will take 20-30 years, but genetic transformation provides an effective alternative for shortening breeding cycle. Until now, two kinds of recipient materials, anther compact embryogenic calli (ACEC) and maintained friable embryogenic calli (MFEC), have been used successfully for Hevea genetic transformation. However, few transformed plants are produced from ACEC-derived embyos, and plants regenerated from MFEC are abnormal, showing that they have poorer performance in growth, yield and disease resistance than the budded control. In order to establish Agrobacterium tumefaciens-mediated Hevea factors influencing transformation frequency, including strains of Agrobacteriumembryos regeneration. GUS transient expression frequency was significantly affected by Agrobacterium strains and co-culture temperature/time, which was 5.07 blue spots/callus for EHA105, higher than that for GV3101 and LBA4404. The highest GUS transient expression frequency was 8.43 and 19.10 blue spots/callus under 22℃ co-cultured temperature and 6 days co-cultured time respectively. Twenty-two thousand ACEC were transformed by the strain EHA105 with pCAMBIA2301, and then transferred to the medium without AS and incubated at 22℃ for 6 days in the dark. Subsequently, 11 transformants were identified by GUS staining, PCR amplification of target genes, sequencing of PCR products and Southern hybridization. Among them, three planted directly in the field died; three as scions were budded onto seedlings, producing five budded transgenic plants; five were multiplicated at embryo phase by secondary embryogenesis, producing 676 transgenic plantlets, among which 248 survived in the field. The results showed that the present transformation system and the plant propagation by transgenic embryos secondary embryogenesis are efficient for the production of transgenic rubber plants., co-culture temperature/time and acetosyringone (AS), and the methods for anther calli transformation system, we surveyed the

Key words: Hevea brasiliensis, Agrobacterium tumefaciens, Anther calli, Genetic transformation, Secondary embryogenesis

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