Scientia Agricultura Sinica ›› 2016, Vol. 49 ›› Issue (20): 3927-3933.doi: 10.3864/j.issn.0578-1752.2016.20.007

• PLANT PROTECTION • Previous Articles     Next Articles

Construction and Transformation of RNAi Vector for Citrus tristeza virus Gene p23

LI Fang, DENG Zi-niu, ZHAO Ya, LI Da-zhi, DAI Su-ming   

  1. Horticulture and Landscape College, Hunan Agricultural University/National Center for Citrus Improvement (Changsha), Changsha 410128
  • Received:2016-04-15 Online:2016-10-16 Published:2016-10-16

RichHTML

3

PDF

350

Abstract: 【Objective】 The objective of this study is to construct RNAi vector containing p23 gene of Citrus tristeza virus (CTV), and obtain transgenic orange plants with virus resistance. 【Method】 Based on the pathogen-derived resistance and the CTV genome sequences published by NCBI, two specific conserved fragments of p23 with different lengths were cloned. Two segments and vector pBI 121 were double-digested and connected for RNAi construction. Subsequently, to initially estimate the antiviral feasibility, the Mexican lime (CTV indicator plant) leaves were injected with Agrobacterium contained the RNAi vector for transient expression, and observed using GUS histochemical staining method. The leaves were inoculated with CTV T36 isolate, and detected by enzyme-linked immunosorbent assay (ELISA). The RNA of leaves was also extracted and reverse transcript to cDNA. Quantitative real-time PCR (q-PCR) was performed to observe the CTV p20 gene expression which could reflect the virus in hosts. The RNAi vector was also transferred into the epicotyl stem of ‘DA HONG’ sweet orange seedlings via Agrobacterium-mediated transformation. Resistant buds were engrafted onto Carrizo Citrange in vitro seedlings. DNA extracted from the ‘DA HONG’ sweet orange leaves was used as the PCR template to identify the transgenic plants. Plants containing the target gene were re-engrafted onto sour orange seedlings and stored in the greenhouse. The expression of the p23 within the transgenic plants was evaluated by q-PCR. The skin buds of CTV T36 isolate hosts were collected and inoculated onto the transgenic sweet orange. The leaves from the sprouted branch tips were collected and analyzed the pathogen resistance capability with the same method that the transient expression leaves detected. Plants without detectable virus infection after the first inoculation were also inspected and analyzed by the same manner in the second round. 【Result】 Long (513 bp) and short (291 bp) fragments of the p23 were cloned. These p23 fragments are then cloned into the pBI121 vector, named p23-RNAi. This p23-RNAi vector was then delivered in the Mexican lime leaves using the Agrobacterium-mediated transient expression assay. The leaves were identified based on the presence of blue stains after GUS staining, indicating that the Agrobacterium contained vector p23-RNAi may induce transient expression in Mexican lime leaves. On the 15th and 30th day after the CTV inoculation, the ELISA detection results for the transgenic Mexican lime leaves in p23-RNAi plants were all negative, whereas the q-PCR detection results showed that the accumulation level of p20 expression was significantly lower than that of the control plants. It indicated that the transient expression of p23-RNAi may, in a defined period, inhibit the CTV infection. Introduction of p23-RNAi via Agrobacterium-mediated genetic transformation led to the production of resistant buds for the ‘DA HONG’ sweet orange, and PCR amplification confirmed a total of seven transgenic plants. The expression of the p23 in all seven transgenic plants was further confirmed by q-PCR amplification, and the gene expression level exhibited a certain degree of difference, with expression level in plant E being the highest, followed by C, F, H, A, B, and G. After inoculation with CTV, the level of expression of p20 varied among these seven transgenic plants, with plant A having the highest level of p20 expression, followed by G, F, E, B, H and C. The transgenic plants showed higher pathogen resistance, albeit to different degrees, when compared to the control plants. However, the virus resistance degrees in the transgenic plants were not closely related to the expression levels of the exogenous gene. For example, plant E, which had the highest expression level of the exogenous gene, did not exhibit powerful CTV resistance. By contrast, the transgenic plant C displayed complete resistance after the two rounds of virus inoculation. 【Conclusion】The p23-RNAi construct that generated confers plant disease resistance to CTV. Transient expression assay can be applied for the high efficiency identification of resistance and screening for high efficiency RNAi vectors.

Key words: Citrus tristeza virus (CTV), p23, RNAi, ‘DA HONG&rsquo, sweet orange, transient expression, genetic transformation

[1]    周彦, 周常勇, 李中安, 王雪峰, 刘科宏. 利用弱毒株交叉保护技术防治甜橙茎陷点型衰退病. 中国农业科学, 2008, 41(12): 4085-4091.
Zhou Y, Zhou C Y, Li Z A, Wang X F, Liu K H. Mild strains cross protection against stem-pitting tristeza of sweet orange. Scientia Agricultura Sinica, 2008, 41(12): 4085-4091. (in Chinese)
[2]    Kreuze J F, Klein I S, Lázaro M U, Chuquiyuri W C, Morgan G L, Mejía P G C, Ghislain M, Valkonen J P. RNA silencing-mediated resistance to a crinivirus (Closteroviridae) in cultivated sweetpotato (Ipomoea batatas L.) and development of sweet potato virus disease following co-infection with a potyvirus. Molecular Plant Pathology, 2008, 9(5): 589-598.
[3]    Soler N, Plomer M, Fagoaga C, Moreno P, Navarro L, Flores R, Peña L. Transformation of Mexican lime with an intron-hairpin construct expressing untranslatable versions of the genes coding for the three silencing suppressors of Citrus tristeza virus confers complete resistance to the virus. Plant Biotechnology Journal, 2012, 10: 597-608.
[4]    Cheng C Z, Yang J W, Yan H B, Bei X J, Zhang Y Y, Lu Z M, Zhong G Y. Expressing p20 hairpin RNA of Citrus tristeza virus confers Citrus aurantium with tolerance/resistance against stem pitting and seedling yellow CTV strains. Journal of Integrative Agriculture, 2015, 14(9): 1767-1777.
[5]    Voinnet O, Lederer C, Baulcombe D C. A viral movement protein prevents spread of the gene silencing signal in Nicotiana benthamiana. Cell, 2000, 103: 157-167.
[6]    Lu R, Folimonov A, Shintaku M, Li W X, Falk B W, Dawson W O, DING S W. Three distinct suppressors of RNA silencing encoded by a 20-kb viral RNA genome. Proceedings of the National Academy of Sciences of the United States of America, 2004, 101(44): 15742-15747.
[7]    Costa Â, Marques N, Nolasco G. Citrus tristeza virus p23 may suppress systemic silencing but is not related to the kind of viral syndrome. Physiological & Molecular Plant Pathology, 2014, 87: 69-75.
[8]    Ghorbel R, López C, Fagoaga C, Moreno P, Navarro L, Flores R, Peña L. Transgenic citrus plants expressing the Citrus tristeza virus p23 protein exhibit viral like symptoms. Molecular Plant Pathology, 2001, 2(1): 27-36.
[9]    Fagoaga C, López C, Moreno P, Navarro L, Flores R, Peña L. Viral-like symptoms induced by the ectopic expression of the p23 gene of Citrus tristeza virus are citrus-specific and do not correlate with the pathogenicity of the virus strain. Molecular Plant-Microbe Interactions, 2005, 18(5): 435-445.
[10]   Jones H D, Doherty A, Sparks C A. Transient transformation of plants. Methods in Molecular Biology, Plant Genomics, 2009, 513: 131-152.
[11]   王关林, 方宏筠. 植物基因工程. 2版. 北京: 科学出版社, 2002: 831-834.
WANG G L, FANG H Y. Plant Genetic Engineering. 2nd ed. Beijing: Science Press, 2002: 831-834. (in Chinese)
[12]   敖小平, 胡新喜, 郭琛, 焦徕, 邓子牛, 熊兴耀. 用rol B基因转化大红甜橙的初步研究. 湖南农业大学学报 (自然科学版), 2005, 31(6): 623-626.
Ao X P, Hu X X, Guo C, Jiao L, Deng Z N, Xiong X Y. Genetic transformation of ‘Dahong’ sweet orange with rol B gene. Journal of Hunan Agricultural University (Natural Sciences), 2005, 31(6): 623-626. (in Chinese)
[13]   Blue R L, Roistacher C N, Cartia G, Calavan E C. Leaf-disc grafting-a rapid indexing method for detection of some citrus viruses//Proceedings of the seventh IOCV conference. University of California, Riverside, 1976: 207-212.
[14]   刘红光, 王中康, 曹月青, 夏玉先, 殷幼平. 应用常规RT-PCR和荧光定量RT-PCR 检测柑桔衰退病毒. 植物病理学报, 2008, 38(1): 24-30.
Liu H G, Wang Z K, Cao Y E, Xia Y X, Yin Y P. Detection of Citrus tristeza virus using conventional and fluorescence quantitative RT-PCR assays. Acta phytopathologica sinica, 2008, 38(1): 24-30. (in Chinese)
[15]   MenzeL W, Jelkmann W, Maiss E. Detection of four apple viruses by multiplex RT-PCR analysis assays with coamplification of plant mRNA as internal control. Journal of Virological Methods, 2002, 99: 81-92.
[16]   Yadav J S, Ogwok E, Wagaba H, L. Patil B, Bagewadi B, Alicai T, Gaitan-solis E, Taylor N J, Fauquet C M. RNAi-mediated resistance to Cassava brown streak uganda virus in transgenic cassava. Molecular Plant Pathology, 2011, 12(7): 677-687.
[17]   Patil B L, Ogwol E, Wagaba H, Mohammed I U, Yadav, J S, Bagewadi B, Taylor N J, Kreuze J F, Maruthi M N, Alicai T, Fauquet C M. RNAi-mediated resistance to diverse isolates belonging to two virus species involved in cassava brown streak disease. Molecular Plant Pathology, 2011, 12(1): 31-41.
[18]   Fagoaga C, LÓpez C, Mendoza A H D, Moreno P, Navarro L, Flores R, Peña L. Post-transcriptional gene silencing of the p23 silencing suppressor of Citrus tristeza virus confers resistance to the virus in transgenic Mexican lime. Plant Molecular Biology, 2006, 60: 153-165.
[19]   Kapila J, Rycke R D, Montagu M V, Angenon G. An Agrobacterium-mediated transient gene expression system for intact leaves. Plant Science, 1997, 122(1): 101-108.
[20]   Almeida W A B, Mourão Filho F A A, Pino L E, Boscariol R L, Rodriguez A P M, Mendes B M J. Genetic transformation and plant recovery from mature tissues of Citrus sinensis L. Osbeck. Plant Science, 2003, 164: 203-211.

[21]   LÓpez C, Cervera M, Fagoaga C, Moreno P, Navarro L, Flores R, Peña L. Accumulation of transgene-derived siRNAs is not sufficient for RNAi-mediated protection against Citrus tristeza virus in transgenic Mexican lime.Molecular plant pathology, 2010, 11(1): 33-41.
[22]   Bhaskar P B, Venkateshwaran M, Wu L, Ané J M, Jiang J M. Agrobacterium-mediated transient gene expression and silencing: a rapid tool for functional gene assay in potato. Plos One,2009, 4(6): e5812.
[23]   Llave C, Kasschau K D, Carrington J C. Virus-encoded suppressor of posttranscriptional gene silencing targets a maintenance step in the silencing pathway. Proceedings of the National Academy of Sciences of the United States of America, 2000, 97(24): 13401-13406.
[24]   Xu K D, Huang X H, Wu M M, Wang Y, Chang Y X, Liu K, Zhang Ju, Zhang Y, Zhang F L, Yi L M, Li T T, Wang R Y, Tan G X, Li C W. A rapid, highly efficient and economical method of Agrobacterium-mediated in planta transient transformation in living onion epidermis. PLoS One, 2014, 9(1): e83556.
[25]   Send?n L N, Filippone M P, Orce I G, Rigano L, Enrique R, Peña L, Vojnov A A, Marano M R, Castagnaro A P. Transient expression of pepper Bs2 gene in Citrus limon as an approach to evaluate its utility for management of citrus canker disease. Plant Pathology, 2012, 61: 648-657.
[26]   Wydro M, Kozubek E, Lehmann P. Optimization of transient Agrobacterium-mediated gene expression system in leaves of Nicotiana benthamiana. Acta Biochimica Polonica, 2006, 53(2): 289-298.
[27]   Kim M J, Baek K, Park C M. Optimization of conditions for transient Agrobacterium-mediated gene expression assays in Arabidopsis. Plant Cell Reports, 2009, 28: 1159-1167.
[28]   Pang S Z, Jan F J, Carney K, Stout J, Tricoli D M, Quemada H D, Gonsalves D. Post-transcriptional transgene silencing and consequent tospovirus resistance in transgenic lettuce are affected by transgene dosage and plant development. The Plant Journal, 1996, 9(6): 899-909.
[29]   Kalantidis K, Psaradakis S, Tabler M, Tsagris M. The occurrence of CMV-specific short RNAs in transgenic tobacco expressing virus-derived double-stranded RNA is indicative of resistance to the virus. Molecular plant-microbe interactions, 2002, 15(8): 826-833.
[1] GUAN RuoBing,LI HaiChao,MIAO XueXia. Commercialization Status and Existing Problems of RNA Biopesticides [J]. Scientia Agricultura Sinica, 2022, 55(15): 2949-2960.
[2] YIN Fei,LI ZhenYu,SAMINA Shabbir,LIN QingSheng. Expression and Function Analysis of Cytochrome P450 Genes in Plutella xylostella with Different Chlorantraniliprole Resistance [J]. Scientia Agricultura Sinica, 2022, 55(13): 2562-2571.
[3] WU Wei,XU HuiLi,WANG ZhengLiang,YU XiaoPing. Cloning and Function Analysis of a Serine Protease Inhibitor Gene Nlserpin2 in Nilaparvata lugens [J]. Scientia Agricultura Sinica, 2022, 55(12): 2338-2346.
[4] CHEN ErHu,MENG HongJie,CHEN Yan,TANG PeiAn. Cuticle Protein Genes TcCP14.6 and TcLCPA3A are Involved in Phosphine Resistance of Tribolium castaneum [J]. Scientia Agricultura Sinica, 2022, 55(11): 2150-2160.
[5] Xiang XU,Yi XIE,LiYun SONG,LiLi SHEN,Ying LI,Yong WANG,MingHong LIU,DongYang LIU,XiaoYan WANG,CunXiao ZHAO,FengLong WANG,JinGuang YANG. Screening and Large-Scale Preparation of dsRNA for Highly Targeted Degradation of Tobacco Mosaic Virus (TMV) Nucleic Acids [J]. Scientia Agricultura Sinica, 2021, 54(6): 1143-1153.
[6] GE XinZhu,SHI YuXing,WANG ShaSha,LIU ZhiHui,CAI WenJie,ZHOU Min,WANG ShiGui,TANG Bin. Sequence Analysis of Harmonia axyridis Pyruvate Kinase Gene and Its Regulation of Trehalose Metabolism [J]. Scientia Agricultura Sinica, 2021, 54(23): 5021-5031.
[7] TAN YongAn,JIANG YiPing,ZHAO Jing,XIAO LiuBin. Expression Profile of G Protein-Coupled Receptor Kinase 2 Gene (AlGRK2) and Its Function in the Development of Apolygus lucorum [J]. Scientia Agricultura Sinica, 2021, 54(22): 4813-4825.
[8] LI Qing,YU HaiPeng,ZHANG ZiHao,SUN ZhengWen,ZHANG Yan,ZHANG DongMei,WANG XingFen,MA ZhiYing,YAN YuanYuan. Optimization of Cotton Mesophyll Protoplast Transient Expression System [J]. Scientia Agricultura Sinica, 2021, 54(21): 4514-4524.
[9] FU ChaoRan, LI YaZi, WU Han, ZHAO Dan, GUO Wei, GUO XiaoChang. Cloning, Expression and Functional Analysis of SeDuox from Spodoptera exigua [J]. Scientia Agricultura Sinica, 2021, 54(18): 3881-3891.
[10] LI YanLin,SHAHID Iqbal,SHI Ting,SONG Juan,NI ZhaoJun,GAO ZhiHong. Isolation of PmARF17 and Its Regulation Pattern of Endogenous Hormones During Flower Development in Prunus mume [J]. Scientia Agricultura Sinica, 2021, 54(13): 2843-2857.
[11] YU WeiDong,PAN BiYing,QIU LingYu,HUANG Zhen,ZHOU Tai,YE Lin,TANG Bin,WANG ShiGui. The Structure Characteristics and Biological Functions on Regulating Trehalose Metabolism of Two NlTret1s in Nilaparvata lugens [J]. Scientia Agricultura Sinica, 2020, 53(23): 4802-4812.
[12] ZHANG DaoWei,KANG Kui,YU YaYa,KUANG FuPing,PAN BiYing,CHEN Jing,TANG Bin. Characteristics and Immune Response of Prophenoloxidase Genes in Sogatella furcifera [J]. Scientia Agricultura Sinica, 2020, 53(15): 3108-3119.
[13] LIU XiaoJian,GUO Jun,ZHANG XueYao,MA EnBo,ZHANG JianZhen. Molecular Characteristics and Function Analysis of Nuclear Receptor Gene LmE75 in Locusta migratoria [J]. Scientia Agricultura Sinica, 2020, 53(11): 2219-2231.
[14] YAO LiXiao,FAN HaiFang,ZHANG QingWen,HE YongRui,XU LanZhen,LEI TianGang,PENG AiHong,LI Qiang,ZOU XiuPing,CHEN ShanChun. Function of Citrus Bacterial Canker Resistance-Related Transcription Factor CitMYB20 [J]. Scientia Agricultura Sinica, 2020, 53(10): 1997-2008.
[15] MA Wen,LIU Jiao,ZHANG XueYao,SHEN GuoHua,QIN XueMei,ZHANG JianQin. Enzymatic Characteristics and Metabolic Analysis to Malathion and p,p’-DDT of LmGSTS2 from Locusta migratoria [J]. Scientia Agricultura Sinica, 2019, 52(8): 1389-1399.
Viewed
Full text


Abstract

Cited
  Shared   
  Discussed   
No Suggested Reading articles found!
京ICP备09089781号-30
Copyright 2018 © Editorial office of Scientia Agricultura Sinica
Tel: 86-010-82106279    E-mail: zgnykx@mail.caas.net.cn
Supported by Beijing Magtech Co.Ltd