能源橡胶草GGPPS基因启动子的克隆及瞬时表达研究

doi:10.11686/cyxb2016034

草业学报 ›› 2016, Vol. 25 ›› Issue (12): 180-187.DOI: 10.11686/cyxb2016034

能源橡胶草GGPPS基因启动子的克隆及瞬时表达研究

李永梅, 冯玉杰, 曹新文, 赵李靖, 祝建波, 闫洁^*

石河子大学生命科学学院,新疆石河子 832000

收稿日期:2016-01-21 修回日期:2016-04-28 出版日期:2016-12-20 发布日期:2016-12-20
通讯作者: jiey@shzu.edu.cn
作者简介:李永梅(1988-),女,山西吕梁人,在读硕士。E-mail: liyongmeishzu@163.com
基金资助:
国家自然科学基金(No.31360060)资助

Cloning and transient expression of the GGPPS gene promoter from the energy plant Taraxacum kok-saghyz

LI Yong-Mei, FENG Yu-Jie, CAO Xin-Wen, ZHAO Li-Jing, ZHU Jian-Bo, YAN Jie^*

College of Life Science, Shihezi University, Shihezi 832000, China

Received:2016-01-21 Revised:2016-04-28 Online:2016-12-20 Published:2016-12-20

摘要/Abstract

摘要： 以多年生宿根型草本植物橡胶草为材料,根据已获得的橡胶草牻牛儿基牻牛儿基焦磷酸合酶(geranylgeranyl pyrophosphate synthase,GGPPS)基因序列设计引物,采用TAIL-PCR扩增到GGPPS基因5'上游大小为1131 bp的序列。采用PlantCare和PLACE软件分析,表明该序列不仅具有启动子的基本元件,同时还有与多个器官特异表达元件以及与胁迫相关的顺式作用元件,命名为pTkGGPPS(GenBank:KT901796)。将该序列代替pCAMBIA1304质粒上的CaMV 35S启动子序列,以GFP基因作为报告基因,构建pCAMBIA1304-pTkGGPPS-GFP植物表达载体,利用农杆菌介导法转化洋葱表皮细胞,结果表明,该启动子能够驱动GFP基因表达,具有一定的活性。TkGGPPS基因启动子克隆及瞬时表达为橡胶草中橡胶合成及组织特异性研究奠定了基础。

Abstract: Based on the known sequence of GGPPS, which encodes geranylgeranyl pyrophosphate synthase, the GGPPS promoter sequence was amplified from the root of the perennial herb Taraxacum kok-saghyz by thermal asymmetric interlaced PCR (TAIL-PCR) using nested specific primers. Analyses of the full-length 1131-bp fragment by PlantCare and PLACE software showed that the promoter sequence contained basic cis-acting elements, multiple organ-specific expression elements, and a number of stress-related cis-acting elements. The promoter sequence was designated as pTkGGPPS (GenBank: KT901796). The plant expression vector pCAMBIA1304-pTkGGPPS-GFP was constructed using this sequence to replace the CaMV 35S promoter sequence in the plasmid of pCAMBIA1304 with GFP as the reporter gene. The construct was transformed into onion epidermal cells using Agrobacterium tumefaciens, and the promoter successfully drove expression of the GFP gene. The cloning and transient expression of the GGPPS gene promoter from T. kok-saghyz provides a reference for further studies on the mechanisms and tissue-specificity of rubber synthesis.

李永梅, 冯玉杰, 曹新文, 赵李靖, 祝建波, 闫洁. 能源橡胶草GGPPS基因启动子的克隆及瞬时表达研究[J]. 草业学报, 2016, 25(12): 180-187.

LI Yong-Mei, FENG Yu-Jie, CAO Xin-Wen, ZHAO Li-Jing, ZHU Jian-Bo, YAN Jie. Cloning and transient expression of the GGPPS gene promoter from the energy plant Taraxacum kok-saghyz[J]. Acta Prataculturae Sinica, 2016, 25(12): 180-187.

参考文献

[1] Zeng L H,Wang H Y, Xie C C. Clone and identification of granule-bound starch synthase gene promoter in Maize. Plant Physiology Journal, 2015, 51(9): 1433-1439.
[2] Archer B L, Audley B G. New aspects of rubber biosynthesis. Botanical Journal of the Linnean Society, 1987, 94: 181-196.
[3] Cornish K, Siler D J. Effect of different allylic diphosphates on the initiation of new rubber molecules and on cis-1,4-polyisoprene biosynthesis in guayule ( Parthenium argentatum Gray). Journal of Plant Physiology, 1995, 147(3-4): 301-305.
[4] Liu B H, Wei X D. Tissue culture of Taraxacum kok-saghyz Rodin. Tropical Agricultural Engineering, 2009, 37(13): 5950-5951.
[5] Liu Y G, Chen Y L. High-efficiency thermal asymmetric interlaced PCR for amplification of unknown flanking sequences. Short Technical Reports, 2007, 43(5): 649-656.
[6] Liu Y G, Huang N. Efficient amplification of insert end sequences from bacterial artificial chromosome clones by thermal asymmetric interlaced PCR. Plant Molecular Biology Reporter, 1998, 16: 175-181.
[7] Miao J, Huo Y M, Yang Y Y, et al . Improvement of hiTAIL-PCR and its application in onion. Shandong Agricultural Sciences, 2009, 10: 1-4.
[8] Liu Y G, Whittier R F. Thermal asymmetric interlaced PCR: automatable amplification and sequencing of insert end fragments from PI and YAC clones for chromosome walking. Genomics, 1995, 25: 674-681.
[9] Zeng J, Huang F Z, Li B C, et al . An optimized method of Agrobacterium tumefaciens -mediated GFP subcelluar localization. Genomics and Applied Biology, 2014, 33(1): 159-162.
[10] Zhao W T, Wei J H, Meng D, et al . Subcellular localization of a sesquiterpene synthase from Aquilaria sinensis utilizing three transient expression system. Chinese Traditional and Herbology Drugs, 2013, 44(23): 3379-3385.
[11] Liu X F, Liang W H. Studies on subcellular localization GFP in onion epidermal cells mediated by Agrobacterium . Journal of Henan Normal University (Natural Science), 2009, 37(1): 123-125, 150.
[12] Liu H Y, Feng D R, Liu B, et al . Studies on subcellular localization MpASR in onion epidermal cells mediated by Agrobacterium . Journal of Tropical and Subtropical Botany, 2009, 17(3): 218-222.
[13] Liang C Z, Zhang R, Sun G Q, et al . Cloning of sress-related transcription factor gene from Cotton by optimized TAIL-PCR. Cotton Science, 2010, 22(3): 195-201.
[14] Qiu Y G, Tian J H, Ge R C, et al . A modified TAIL-PCR and its application in isolating gene promoter of Wheat. Chinese Journal of Biotechnology, 2008, 24(4): 695-699.
[15] Li Y M, Feng Y J, Li J, et al . Cloning and expression analysis of the TkGGPPS gene from Taraxacum kok-saghyz . Plant Physiology Journal, 2016, 52(3): 303-311.
[16] Hefner J, Ketchum R E B, Croteau R. Cloning and functional expression of a cDNA encoding geranylgeranyl diphosphate synthase from Taxus canadensis and assessment of the role of this prenyltransferase in cells induced for taxol production. Arch Biochem Biophys, 1998, 360(1): 62-74.
[17] Hua W P, Song S H, Zhi Y, et al . Cloning and expression analysis of SmGGPPS 3 gene from Salvia miltiorrhiza . Plant Science Journal, 2014, 32(1): 50-57.
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[7] 缪军, 霍雨猛, 杨妍妍, 等. 高效TAIL-PCR的改良及在洋葱中的应用. 山东农业科学, 2009, 10: 1-4.
[9] 曾洁, 黄凤智, 李本昌. 等. 一种根癌农杆菌介导的GFP亚细胞定位方法的优化. 基因组学与应用生物学, 2014, 33(1): 159-162.
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能源橡胶草GGPPS基因启动子的克隆及瞬时表达研究

Cloning and transient expression of the GGPPS gene promoter from the energy plant Taraxacum kok-saghyz

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