灰葡萄孢<em>BcKMO</em>基因的原核表达分析

doi:10.7668/hbnxb.2017.01.011

摘要/Abstract

摘要： 为构建灰葡萄孢犬尿氨酸单加氧酶（BcKMO）基因的原核表达载体并进行高效表达，获得纯化的BcKMO蛋白。以灰葡萄孢野生型BC22为试材，通过反转录PCR扩增BcKMO基因，回收BcKMO基因片段克隆到pMD19-T载体中，测序正确后，酶切pMD19-T-BcKMO和带有GST标签蛋白的pGEX4T-1质粒，将目的片段进行连接，构建BcKMO基因的原核表达载体pGEX4T-1-BcKMO-GST。经酶切和测序鉴定正确后，将构建好的原核载体转化大肠杆菌BL21。经IPTG诱导，在大肠杆菌BL21菌株中成功表达了与GST标签蛋白融合的BcKMO蛋白，大小约71 kDa。SDS-PAGE分析表明，该蛋白在0.2 mmol/L IPTG诱导12 h时高效表达；Western Blot结果发现目的蛋白能与GST特异性抗体起特异性反应，表明BcKMO基因的体外诱导表达成功。

关键词: 灰葡萄孢, BcKMO, 原核表达, 纯化, PCR

Abstract: The aim of this study is prokaryotic expression analysis of BcKMO gene from Botrytis cinerea and obtain the purified BcKMO protein.The BcKMO gene was amplified by RT-PCR technology using the cDNA of the Botrytis cinerea wild type BC22,cloned into the pMD19-T vector and sequenced.The results of sequencing showed that the BcKMO gene sequence was right.The pMD19-T-BcKMO and pGEX4T-1 plasmids were digested using restriction enzyme.The BcKMO gene segments were collected and cloned into the pGEX4T-1 vector.The results of restriction enzyme digestion and sequencing showed that the vector pGEX4T-1-BcKMO-GST was successfully constructed.The vector pGEX4T-1-BcKMO-GST was transformed into E.coli BL21 strain.The results of IPTG inducement indicated that the pGEX4T-1- BcKMO -GST was successfully expressed in E.coli BL21 strain,with the molecular weight 71 kDa.The optimal conditions of the prokaryotic expression of BcKMO were determined as 0.2 mmol/L IPTG treatment 12 h.Western Blot results showed that the GST antibody could specifically bound to purified pGEX4T-1-BcKMO-GST fusion protein,suggesting that the expression of BcKMO gene was successfully in vitro.

Key words: Botrytis cinerea, BcKMO, Prokaryotic expressin, Purification, PCR

中图分类号:

S431.03
Q78

王敏, 刘媛媛, 周帆, 姜婷婷, 郑旭, 张靖, 时翠平, 邢继红, 董金皋. 灰葡萄孢BcKMO基因的原核表达分析[J]. 华北农学报, 2017, 32(1): 68-72. doi: 10.7668/hbnxb.2017.01.011.

WANG Min, LIU Yuanyuan, ZHOU Fan, JIANG Tingting, ZHENG Xu, ZHANG Jing, SHI Cuiping, XING Jihong, DONG Jingao. Prokaryotic Expression Analysis of BcKMO Gene from Botrytis cinerea[J]. ACTA AGRICULTURAE BOREALI-SINICA, 2017, 32(1): 68-72. doi: 10.7668/hbnxb.2017.01.011.

http://www.hbnxb.net/CN/Y2017/V32/I1/68

参考文献

[1] Levis C,Giraud T,Dutertre M,et al.Telomeric DNA of Botrytis cinerea:a useful tool for strain identification[J].FEMS Microbiology Letters,1997,157(2):267-272.
[2] Rui O,Hahn M.The Botrytis cinerea hexokinase,Hxk1,but not the glucokinase,Glk1,is required for normal growth and sugar metabolism,and for pathogenicity on fruits[J].Microbiology,2007,153(Pt 8):2791-2802.
[3] Schumacher J,De Larrinoa I F,Tudzynski B.Calcineurin-responsive Zinc finger transcription factor CRZ1 of Botrytis cinerea is required for growth,development,and full virulence on bean plants[J].Eukaryotic Cell,2008,7(4):584-601.
[4] Yin Y N,Kim Y K,Xiao C L.Molecular characterization of boscalid resistance in field isolates of Botrytis cinerea from apple[J].Phytopathology,2011,101(8):986-995.
[5] Chen S C,Liu A R,Wang F H,et al.Combined overexpression of chitinase and defens in genes in transgenic tomato enhances resistance to Botrytis cinerea[J].African Journal of Biotechnology,2009,8(20):5182-5188.
[6] Jeon E H,Chung E S,Lee H Y,et al.Ectopic expression of wild rice OgGRP gene encoding a glycine rich cell wall protein confers resistance to Botrytis cinerea pathogen on Arabidopsis[J].Plant Pathology Journal,2009,25(2):193-198.
[7] Alberati-Giani D,Cesura A M,Broger C,et al.Cloning and functional expression of human kynurenine 3-monooxygenase[J].FEBS Letters,1997,410(2/3):407-412.
[8] Dantzer R,O'connor J C,Lawson M A,et al.Inflammation-associated depression:from serotonin to kynurenine[J].Psychoneuroendocrinology,2011,36(3):426-436.
[9] Wilson K,Mole D J,Binnie M,et al.Bacterial expression of human kynurenine 3-monooxygenase:solubility,activity,purification[J].Protein Expression and Purification,2014,95:96-103.
[10] Zwilling D,Huang S Y,Sathyasaikumar K V,et al.Kynurenine 3-monooxygenase inhibition in blood ameliorates neurodegeneration[J].Cell,2011,145(6):863-874.
[11] Amaral M,Levy C,Heyes D J,et al.Structural basis of kynurenine 3-monooxygenase inhibition[J].Nature,2013,496(7445):382-385.
[12] Reignault P,Valette-Collet O,Boccara M.The importance of fungal pectinolytic enzymes in plant invasion,host adaptability and symptom type[J].European Journal of Plant Pathology,2008,120(1):1-11.
[13] Siegmund U,Heller J,Van Kan J A,et al.The NADPH oxidase complexes in Botrytis cinerea:evidence for a close association with the ER and the tetraspanin Pls1[J].PLoS One,2013,8(2):e55879.
[14] Gourgues M,Brunet-Simon A,Lebrun M H,et al.The tetraspanin BcPls1 is required for appressorium-mediated penetration of Botrytis cinerea into host plant leaves[J].Molecular Microbiology,2004,51(3):619-629.
[15] Choquer M,Becker H F,Vidal-Cros A.Identification of two group A chitinase genes in Botrytis cinerea which are differentially induced by exogenous chitin[J].Mycological Research,2007,111(Pt 5):615-625.
[16] Patel R M,Van Kan J A,Bailey A M,et al.RNA-mediated gene silencing of superoxide dismutase (bcsod1) in Botrytis cinerea[J].Phytopathology,2008,98(12):1334-1339.
[17] Wojtaszek P.Oxidative burst:an early plant response to pathogen infection[J].The Biochemical Journal,1997,322(3):681-692.
[18] 李培芬.灰葡萄孢 BcKMO 基因对病菌生长发育和致病力的影响[D].保定:河北农业大学,2014.
[19] 李培芬,赵福鑫,董丽萍,等.灰葡萄孢BcKMO在病菌生长、发育和致病过程中的功能[J].中国农业科学,2014,47(15):2971-2979.
[20] 李培芬,赵福鑫,董丽萍,等.灰葡萄孢犬尿氨酸单氧酶基因 BcKMO 调控病菌致病力的机制分析[J].中国农业科学,2014,47(16):3169-3175.
[21] 李波,倪志勇,李晓东,等.棉花 GhCOMT1 基因原核表达载体构建及蛋白纯化和Western鉴定[J].西北植物学报,2012,32(10):1971-1976.
[22] Wu C,Wang Y Y,Zou M,et al.Prokaryotic expression,purification,and production of polyclonal antibody against human polypeptide N-acetylgalactosaminyl transferase 14[J].Protein Expression and Purification,2007,56(1):1-7.
[23] Han X Q,Lin X M,Chen H J,et al.The prokaryotic expression and bioactivity of the recombinant red fire ant venom allergen soli 4[J].Agricutural Sciences in China,2009,8(2):182-187.
[24] 柴政斌,张更林,韩金祥.GST-pulldown技术在蛋白质相互作用中的应用[J].中国生物制品学杂志,2014,27(10):1354-1358.
[25] 蒋琛茜,瓮巧云,樊锦涛,等.拟南芥抗病相关基因 T1N6_22 的原核表达分析[J].华北农学报,2015,30(1):73-76.

选择文件类型/文献管理软件名称

选择包含的内容

灰葡萄孢BcKMO基因的原核表达分析

Prokaryotic Expression Analysis of BcKMO Gene from Botrytis cinerea

PDF

可视化

被引次数

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价

[1]	冯清香, 朱哈修, 杜洋, 徐艳茹, 王晨晨, 刘雪, 李大勇, 周军, 张彬. *菊苣ANS基因的克隆及表达分析*[J]. 华北农学报, 2025, 40(3): 51-59.
[2]	殷冬冬, 朱星星, 兰梦蝶, 彭梦玲, 尹磊, 戴银, 沈学怀, 王洁茹, 赵瑞宏, 潘孝成. 新型鹅星状病毒 AH-2021 株的分离鉴定及其VP27-VP34蛋白多克隆抗体的制备[J]. 华北农学报, 2025, 40(2): 210-217.
[3]	刘永宁, 单乙戈, 潘晨帆, 刘倩琳, 李翌琳, 段思彰, 安健, 张建军. *柔嫩艾美耳球虫AMA1的原核表达及其免疫保护效果评价*[J]. 华北农学报, 2025, 40(1): 232-238.
[4]	张玉倩, 吕志航, 刘春红, 廉春杨, 张雪莲. 禽戊型肝炎病毒CaHEV-GDSZ01株ORF2蛋白的生物信息学分析、原核表达及多克隆抗体制备[J]. 华北农学报, 2024, 39(6): 231-238.
[5]	龚珂珂, 张梦雅, 李志勇, 刘佳, 马继芳, 董志平, 贾小平, 白辉. 谷子抗锈病反应相关MAPKK家族成员的鉴定与分析[J]. 华北农学报, 2024, 39(5): 193-203.
[6]	邵文先, 王冬梅. TaMAPK5蛋白的抗体制备及其在小麦与叶锈菌互作过程中的表达特征[J]. 华北农学报, 2024, 39(5): 186-192.
[7]	张元臣, 苏圣盈, 张家祺, 薛爽, 王景顺. *东方黏虫溶菌酶基因MseLYS的克隆与表达分析*[J]. 华北农学报, 2024, 39(4): 206-214.
[8]	王晓玥, 陈双双, 齐香玉, 冯景, 陈慧杰, 孙明, 邓衍明. 绣球花铝转运蛋白HmALMT11的生物信息学及其表达特性分析[J]. 华北农学报, 2024, 39(4): 94-101.
[9]	郭昭阳, 殷宇航, 刘钰, 解一桐, 裴玉贺, 宋希云, 赵美爱. *玉米ZmPAP26b基因的克隆及其在干旱胁迫下表达模式分析*[J]. 华北农学报, 2024, 39(4): 10-19.
[10]	宋普文, 邓佳乐, 杜玉新, 陈家美, 敬月婷, 刘俊彤, 李澳, 胡海燕. 小麦mRNA剪接因子TaSR与TaHis的互作鉴定及其基因表达分析[J]. 华北农学报, 2024, 39(3): 166-172.
[11]	霍秀鹏, 宋照哲, 马红, 汪亮, 刘娣, 郝丽. UCP3对民猪前脂肪细胞产热相关基因表达的影响[J]. 华北农学报, 2024, 39(3): 208-214.
[12]	张玉倩, 李长乐, 吕志航, 姚鑫炎, 张雪莲. 禽戊型肝炎病毒CaHEV-GDSZ01株ORF3蛋白的原核表达及其多克隆抗体的制备[J]. 华北农学报, 2024, 39(3): 224-229.
[13]	胡馨月, 王津, 聂婉虹, 龚超, 许本波, 张学昆, 赵福永. 海甘蓝发育种子中FAE1的表达模式与芥酸积累[J]. 华北农学报, 2024, 39(3): 35-42.
[14]	王鑫淼, 赵孟良, 邵登魁, 尕桑, 任延靖. *球茎甘蓝MYB62转录因子的克隆与表达特征分析*[J]. 华北农学报, 2024, 39(2): 62-70.
[15]	吴茵茵, 温思怡, 韩卓然, 孙敬锋. *半滑舌鳎突触体相关蛋白29基因(SNAP29)克隆及其组织分布和时序表达分析*[J]. 华北农学报, 2024, 39(2): 231-238.

模态框（Modal）标题

选择文件类型/文献管理软件名称

选择包含的内容

灰葡萄孢BcKMO基因的原核表达分析

Prokaryotic Expression Analysis of BcKMO Gene from Botrytis cinerea

PDF

可视化

被引次数

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价