Preparation of Polyclonal Antibody Containing CPN60-β for Controlling Rice Stripe Virus Disease
-
摘要:
目的 制备针对水稻叶绿体蛋白Chaperonin-60-beta(CPN60-β)多克隆抗体,为进一步研究CPN60-β蛋白在由NSvc4蛋白所介导的水稻条纹病毒(Rice stripe virus, RSV)的运动和致病过程中的调控功能及作用机制提供技术支持和材料准备。 方法 通过RT-PCR从水稻幼嫩叶片基因组扩增CPN60-β基因的功能片段,与原核表达质粒pET-28a(+)构建重组质粒pET-CPN60-β,然后将重组质粒转化大肠杆菌BL21细胞进行诱导表达;将表达纯化的CPN60-β融合蛋白免疫雄性新西兰大白兔获得高效价高浓度的多克隆抗体。 结果 RT-PCR扩增获得的水稻叶绿体CPN60-β基因片段约为657 bp,构建的重组质粒pET-CPN60-β转化大肠杆菌BL21后在诱导剂IPTG浓度0.5 mmol·L−1、摇床温度37 ℃、转速220 r·min−1振荡培养3.5 h条件下成功表达CPN60-β融合蛋白。ELISA和SDS-PAGE检测表明,以纯化CPN60-β融合蛋白免疫雄性新西兰大白兔获得的多克隆抗体效价为1∶1 000 000,抗体质量浓度约300 μg·mL−1。 结论 明确CPN60-β基因原核表达条件;制备获得的水稻叶绿体CPN60-β蛋白的多克隆抗体质量浓度和效价较高,可用于后续研究CPN60-β蛋白在RSV病毒运动和致病过程中发挥的功能。 Abstract:Objective To elucidate the regulatory function and mechanism of the pathogenic processes mediated by the rice stripe virus (RSV)-encoding NSvc4 protein in rice, the high titer concentrated polyclonal antibody containing the chloroplast-related chaperonin-60-beta (CPN60-β) protein against the RSV disease was prepared. Method The CPN60-β fragment was amplified by RT-PCR from rice genome. The recombinant plasmid pET-CPN60-β was constructed with prokaryotic expression plasmid pET-28a (+) and further expressed in Escherichia coli BL21 cells. The CPN60-β fusion protein was purified and immunized into New Zealand rabbits to obtain polyclonal antibody. Titer and concentration of the polyclonal antibody against CPN60-β protein were detected by ELISA and SDS-PAGE for confirmation. Result The approximately 657bp chloroplast-related CPN60-β fragment was successfully amplified by RT-PCR. The reconstructed plasmid pET-CPN60-β positively expressed the CPN60-β fusion protein in E. coli BL21 cells under IPTG concentration of 0.5mmol·L−1 at 37 ℃ with a rotate speed of 220 r·min−1 and an induction time of 5 h. The purified polyclonal antibody had a high titer of 1:106 and a concentration of 300 μg·mL−1 as detected separately by ELISA and SDS-PAGE. Conclusion The conditions of CPN60-β prokaryotic expression were confirmed and the polyclonal antibody against chloroplast-related CPN60-β protein with high titer and concentration successfully prepared for further studies. -
Key words:
- rice /
- chloroplast /
- CPN60-β /
- polyclonal antibody /
- titer
-
图 1 重组质粒pET-CPN60-β构建
注:A–CPN60-β基因RT-PCR产物琼脂糖凝胶电泳:M, DNA Marker;1, 阴性对照(水);2, 水稻叶片样品。B– 重组质粒pET-CPN60-β PCR产物琼脂糖凝胶电泳:M, DNA Marker;1, 阴性对照(水);2, 单克隆菌落。
Figure 1. Construction of recombinant plasmid pET-CPN60-β
Note: A–Agarose gel electrophoresis of CPN60-β RT-PCR products: M-DNA marker, 1-negative control (water), 2-rice leaf samples. B– Agarose gel electrophoresis of recombinant plasmid pET-CPN60-β PCR products: M-DNA marker, 1-negative control (water), 2-monoclonal colonies.
图 2 CPN60-β基因的表达与鉴定
注:A– SDS-PAGE检测CPN60-β基因的表达:M, 蛋白Marker;1, 不加IPTG的阴性对照;2, 加0.5 mmol·L−1 IPTG样品。B–Western blot鉴定CPN60-β基因的表达:M, 蛋白Marker;1, 加0.5 mmol·L−1 IPTG样品;2, 不加IPTG的阴性对照。
Figure 2. Expression and confirmation of CPN60-β gene
Note: A– Expression of CPN60-β detected by SDS-PAGE: M-protein marker, 1-negative control without IPTG, 2-0.5mM IPTG samples. B– Expression of CPN60-β protein confirmed by western blot: M-protein marker, 1-0.5 mmol·L−1 IPTG samples, 2-negative control without IPTG.
图 3 抗CPN60-β抗体的效价测定
注:A, 免疫过程中抗体效价测定。B, 免疫完成后抗体效价测定:1, 兔子编号1;2, 兔子编号2。
Figure 3. Titer of antibodies against CPN60-β
Note: A–Titer detection of antibodies before immunity. B–Titer detection of antibodies after immunity: 1-rabbit No. 1, 2-rabbit No. 2.
-
[1] 陈晓英, 方荣祥. 中国植物病毒研究40年 [J]. 微生物学通报, 2014, 41(3):437−444.CHEN X Y, FANG R X. The study of plant viruses in China during the last 40 years [J]. Microbiology China, 2014, 41(3): 437−444.(in Chinese) [2] TORIYAMA S, TAKAHASHI M, SANO Y, et al. Nucleotide sequence of RNA 1, the largest genomic segment of rice stripe virus, the prototype of the tenuiviruses [J]. The Journal of General Virology, 1994, 75(12): 3569−3579. [3] DU Z G, XIAO D L, WU J G, et al. p2 of Rice stripe virus (RSV) interacts with OsSGS3 and is a silencing suppressor [J]. Molecular Plant Pathology, 2011, 12(8): 808−814. doi: 10.1111/j.1364-3703.2011.00716.x [4] HIBINO H. Biology and epidemiology of rice viruses [J]. Annual Review of Phytopathology, 1996, 34(1): 249−274. doi: 10.1146/annurev.phyto.34.1.249 [5] XIONG R Y, WU J X, ZHOU Y J, et al. Characterization and subcellular localization of an RNA silencing suppressor encoded by Rice stripe Tenuivirus [J]. Virology, 2009, 387(1): 29−40. doi: 10.1016/j.virol.2009.01.045 [6] TORIIYAMA S. Chemical composition of coat protein of rice stripe virus and rice stripe disease specific protein [J]. Annuals of The Phytopathological Society of Japan, 1983, 49: 432. [7] XIONG R Y, WU J X, ZHOU Y J, et al. Identification of a movement protein of the Tenuivirus rice stripe virus [J]. Journal of Virology, 2008, 82(24): 12304−12311. doi: 10.1128/JVI.01696-08 [8] LIU L, SAUNDERS K, THOMAS C L, et al. Bean yellow dwarf virus RepA, but not rep, binds to maize retinoblastoma protein, and the virus tolerates mutations in the consensus binding motif [J]. Virology, 1999, 256(2): 270−279. doi: 10.1006/viro.1999.9616 [9] 唐超, 陈远超, 朱春晖, 等. 小西葫芦黄花叶病毒研究进展 [J]. 江苏农业科学, 2016, 44(9):18−20.TANG C, CHEN Y C, ZHU C H, et al. Progress in zucchini yellow mosaic virus [J]. Jiangsu Agricultural Sciences, 2016, 44(9): 18−20.(in Chinese) [10] SOELLICK T R, UHRIG J F, BUCHER G L, et al. The movement protein NSm of tomato spotted wilt Tospovirus (TSWV): RNA binding, interaction with the TSWV N protein, and identification of interacting plant proteins [J]. PNAS, 2000, 97(5): 2373−2378. doi: 10.1073/pnas.030548397 [11] LI Y, WU M Y, SONG H H, et al. Identification of a tobacco protein interacting with tomato mosaic virus coat protein and facilitating long-distance movement of virus [J]. Archives of Virology, 2005, 150(10): 1993−2008. doi: 10.1007/s00705-005-0554-5 [12] DESVOYES B, FAURE-RABASSE S, CHEN M H, et al. A novel plant homeodomain protein interacts in a functionally relevant manner with a virus movement protein [J]. Plant Physiology, 2002, 129(4): 1521−1532. doi: 10.1104/pp.004754 [13] XU Y, ZHOU X P. Role of rice stripe virus NSvc4 in cell-to-cell movement and symptom development in Nicotiana benthamiana [J]. Frontiers in Plant Science, 2012, 3: 269. [14] ZHANG C, PEI X W, WANG Z X, et al. The Rice stripe virus pc4 functions in movement and foliar necrosis expression in Nicotiana benthamiana [J]. Virology, 2012, 425(2): 113−121. doi: 10.1016/j.virol.2012.01.007 [15] 贾慧娜, 罗海玲. 多克隆抗体制备方法的研究进展 [J]. 中国草食动物科学, 2012, 32(S1):66−69.JIA H N, LUO H L. Progress in preparation of polyclonal antibodies [J]. China Herbivore Science, 2012, 32(S1): 66−69.(in Chinese) [16] TILLER K E, TESSIER P M. Advances in antibody design [J]. Annual Review of Biomedical Engineering, 2015, 17: 191−216. doi: 10.1146/annurev-bioeng-071114-040733 -
下载:
点击查看大图
计量
- 文章访问数: 1032
- HTML全文浏览量: 190
- PDF下载量: 17
- 被引次数: 0
