金黄色葡萄球菌双组分系统反应调节蛋白AgrA的原核表达、纯化及活性鉴定

doi:10.13523/j.cb.20150505

中国生物工程杂志

2015, Vol. 35

Issue (5): 32-40 DOI: 10.13523/j.cb.20150505

研究报告

金黄色葡萄球菌双组分系统反应调节蛋白AgrA的原核表达、纯化及活性鉴定

张旭宁¹, 权春善^2,3, 廖颖玲^2,3, 柳科欢^2,3, 熊文^2,3, 范圣第^2,3

1. 大连工业大学生物工程学院大连 116034;
2. 大连民族学院生物技术与资源利用国家民委-教育部重点实验室大连 116600;
3. 大连民族学院生命科学学院大连 116600

Expression,Purification and Identification of AgrA, a Response Regulator Protein of Two-component Signal Transduction System in Staphylococcus aureus

ZHANG Xu-ning¹, QUAN Chun-shan^2,3, LIAO Ying-ling^2,3, LIU Ke-huan^2,3, XIONG Wen^2,3, FAN Sheng-di^2,3

1. School of Biological Engineering, Dalian Polytechnic University, Dalian 116034, China;
2. Key Laboratory of Biotechnology and Resource Utilization, State Ethnic Affairs Commission and Ministry of Education, Dalian Nationalities University, Dalian 116600, China;
3. Department of Life Science, Dalian Nationalities University, Dalian 116600, China

全文: PDF(1026 KB) HTML

摘要：

AgrA作为金黄色葡萄球菌双组分信号转导系统(two-component signal transduction system, TCST)的反应调节因子,能调控细菌毒力因子的表达,在金黄色葡萄球菌致病过程中起着重要的作用。采用无限制克隆法构建AgrA表达载体,在AgrA蛋白的C端融合绿色荧光蛋白(GFP)标签,通过实时监测GFP的荧光强度来快速检测重组蛋白的表达水平。首先利用单因素实验,筛选出宿主菌株BL21-(DE3)-PlysS;其次,结合Box-Behnken试验设计,筛选出最优蛋白质表达条件:诱导时间为22h、转速为222r/min、诱导剂浓度为0.5mmol/L,AgrA产量达到5.56mg/L。最后,基于AgrA蛋白LytTR区域的非放射性凝胶阻滞实验(non-radioactive electrophoretic mobility shift assay, EMSA)验证了AgrA的生物活性。提出了反应调节蛋白AgrA在大肠杆菌高效可溶性表达的策略,为双组分信号转导系统的体外研究奠定基础,也为其他反应调节蛋白的可溶性表达与分离纯化提供了一个可行借鉴。

关键词： 金黄色葡萄球菌; AgrA; GFP; 响应面分析; EMSA

Abstract:

As a response regulator in the two-component signal transduction system (TCST) of Staphylococcus aureus, AgrA, which transmits signals to downstream promoter and then regulates genes expression and transcription, plays an important role in the pathogenesis of S. aureus. A expression vector using Restriction-free (RF) cloning was constructed. In order to monitor the protein expression level in real time, a C-terminal green fluorescent protein (GFP) was fused to AgrA to serve as a reporter. Firstly, BL21-(DE3)-PlysS was screened as the best host cell by single-factor experiment. Secondly, combined with the Box-Behnken designed response surface method test, the cultured conditions which include culture time、RPM and IPTG concentration were optimized. The optimum conditions selected are as follows: induction time is 22h, speed is 222r/min, IPTG is 0.5mmol/L. Then, the expressed AgrA were purified using immobilized metal affinity chromatography (IMAC) and size exclusion chromatography (SEC) with the yield of AgrA is 5.56mg/L. Finally, the activity of AgrA was assessed by using non-radioactive electrophoretic mobility shift assay (EMSA) based on AgrA protein LytTR region. In short, A strategy through which response regulator protein AgrA could be expressed in E. coli efficiently and solublely. It not only establishes the foundation for the two-component signal transduction system in vitro studies, but also provides a viable reference for other response regulator proteins which need soluble expression, separation and purification.

Key words: Staphylococcus aureus AgrA GFP Response surface method EMSA

收稿日期: 2015-01-22 出版日期: 2015-05-25

ZTFLH:

Q78

通讯作者: 权春善 E-mail: mikyeken@dlnu.edu.cn

	服务
	把本文推荐给朋友
	加入引用管理器
	E-mail Alert
	RSS
	作者相关文章

引用本文:

张旭宁, 权春善, 廖颖玲, 柳科欢, 熊文, 范圣第. 金黄色葡萄球菌双组分系统反应调节蛋白AgrA的原核表达、纯化及活性鉴定[J]. 中国生物工程杂志, 2015, 35(5): 32-40.

ZHANG Xu-ning, QUAN Chun-shan, LIAO Ying-ling, LIU Ke-huan, XIONG Wen, FAN Sheng-di. Expression,Purification and Identification of AgrA, a Response Regulator Protein of Two-component Signal Transduction System in Staphylococcus aureus. China Biotechnology, 2015, 35(5): 32-40.

链接本文:

https://manu60.magtech.com.cn/biotech/CN/10.13523/j.cb.20150505 或 https://manu60.magtech.com.cn/biotech/CN/Y2015/V35/I5/32

[1] Larsen A, Stegger M, Goering R,et al. Emergence and dissemination of the methicillin resistant Staphylococcus aureus USA300 clone in Denmark. Euro Surveill, 2007,12(2): 22-24.

[2] Chambers H F, Deleo F R Waves of resistance: Staphylococcus aureus in the antibiotic era. Nat Rev Microbiol,2009,7(9): 629-641.

[3] Miller M B, Bassler B L. Quorum sensing in bacteria. Annu Rev Microbiol, 2001,55:165-199.

[4] Cheung A L, Nishina K A, Trotonda M P, et al. The SarA protein family of Staphylococcus aureus. Biochem Cell Biol, 2008,40(3):355-361.

[5] Waters C M, Bassler B L. Quorum sensing: cell-to-cell communication in bacteria. Annu Rev Cell Dev Biol, 2005,21:319-346.

[6] Geisinger E R P, Adhikari R, Jin H F,et al. Inhibition of rot translation by RNAIII, a key feature of agr function. Mol Microbiol, 2006,61(4):1038-1048.

[7] Chakrabarti S K, Misra T K, SarA represses agr operon expression in a purified in vitro Staphylococcus aureus transcription system.J Bacteriol, 2000,182(20):5893-5897.

[8] Novick R P. Autoinduction and signal transduction in the regulationof staphylo- coccal virulence. Mol Microbiol, 2003,48(6):1429-1449.

[9] Leonard PG, Bezar I F, Sidote D J, et al. Identification of a hydrophobic cleft in the LytTR domain of AgrA as a locus for small molecule interactions that inhibit DNA binding. Biochemistry, 2012,51(50):10035-10043.

[10] 朱红裕, 李强. 外源蛋白在大肠杆菌中的可溶性表达策略.过程工程学报, 2006,6(1):151-155. Zhu H Y, Li Q. Strategies for expression of soluble heterologous proteins in Escherichia coli. The Chinese Journal of Process Engineering, 2006,6(1):151-155.

[11] 胡建广,尹艳. GFP与微管结合蛋白和肌动蛋白结合区融合蛋白载体构建与表达.中国生物工程杂志, 2004,24(1):53-56. Hu J G, YIN Y, Construction of two vectors for expressing the fusion genes of GFP with microtubules associated protein 4 and actin filaments talinand their expression. China Biotecnology, 2004,24(1):53-56.

[12] Drew D, Slotboom D J, Friso G A. GFP-based pipeline for membrane protein overexpression screening and purification. Protein Sci, 2005,14(8):2011-2017.

[13] Drew D, Lerch M, Kunji E. Optimization of membrane protein overexpression and purification using GFP fusions. Nat Methods, 2006, 3(4):303-313.

[14] Stephen R B, Christian C N. RF-Cloning org: an online tool for the design of restriction-free cloning projects. Nucleic Acids Research,2012,40(w1):209-213.

[15] Fusinita V E, Jan L. RF cloning: a restriction-free method for inserting target genes into plasmids. J Biochem Biophys,2006,67(1):67-74.

[16] Wang L N, Quan C S, Xiong W, et al. GFP-based overexpression screening and characterization of AgrC, a receptor protein of quorum sensing in Staphyloc- occus aureus. Int J Mol Sci, 2013,14(9):18470-18487.

[17] Dindo R, Diego O A, Antoinette M, et al. Coordinated regulation by AgrA, SarA, and SarR to control expression in agr Staphylococcus aureus. J Bact- eriol, 2011,193(21):6020-6031.

[18] Fowler S A, Stacy D M, Blackwell H E. Design and synthesis of macrocyclic peptomers as mimics of a quorum sensing signal from Staphylococcus aureus. Org Lett, 2008,10(12):2329-2332.

[19] Mansson M, Nielsen A, Kjaerulff L, et al. Inhibition of virulence gene expression in Staphylococcus aureus by novel depsipeptides from a marine photobacterium. Mar Drugs, 2011,9(12):2537-2552.

[20] Jensen R O, Winzer K, Clarke S R, et al. Differential recognition of Staphylo- coccus aureus quorum-sensing signals depends on both extracellular loops 1 and 2 of the transmembrane sensor AgrC. J Mol Biol, 2008,381(2):300-309.

[21] 陈来同,茄炳根. 在大肠杆菌表达体系中以包涵体形式存在的真核生物蛋白质的分离复性和二硫键的形成. 中国生化药物杂志, 1997,18(1):46-49. Chen L T, Qie B G. Isolation, renaturation, and formation of disulfide bonds of eukaryotic proteins expressed in E. coli as inclusion bondies. Chinese Journal of Biochemical Phar- maceutics,1997,18(1):46-49.

[22] 朱希强,袁勤生.EC-SOD在大肠杆菌中的可溶性表达. 食品与药品, 2005, 7(4A): 31-33. Zhu X Q, Yuan Q S. The resolution expression of EC- SOD in supernatant by E. coli. Food and Drug, 2005,7(4A):31-33.

[23] Koenig R L, Ray J L, Maleki S J. Staphylococcus aureus AgrA binding to the RNAIII-agrrReg- ulatory region. J Bacteriol, 2004,186(22):7549-7555.

[24] María F D P, Marta P. Enterococcus faecalis virulence regulator FsrA binding to target promoters. J Bacteriol, 2011,193(7):1527-1532.

[1]	马占兵,党洁,杨继辉,霍正浩,徐广贤. 基于慢病毒系统的双荧光标记多功能自噬流监测系统建立与应用 ^*[J]. 中国生物工程杂志, 2019, 39(5): 88-95.
[2]	何亚南,孙钰椋,任雅坤,梁盛英,杨芬,刘彦礼,林俊堂. 金黄色葡萄球菌类肠毒素K与GFP融合蛋白工程菌的构建及其表达蛋白生物学活性分析 ^*[J]. 中国生物工程杂志, 2018, 38(12): 14-20.
[3]	王曦, 陈熙明, 浦铜良. 溶葡球菌酶高效表达与应用[J]. 中国生物工程杂志, 2017, 37(9): 118-125.
[4]	徐安健, 李艳萌, 李斯文, 乌姗娜, 张蓓, 黄坚. 人组氨酸磷酸酶蛋白PHPT1的细胞定位及其对细胞层状伪足形成的影响[J]. 中国生物工程杂志, 2017, 37(6): 17-21.
[5]	倪璇, 高金欣, 余传金, 刘铜, 李雅乾, 陈捷. *玉米弯孢叶斑病菌clt-1基因生物信息学分析和启动子的功能鉴定*[J]. 中国生物工程杂志, 2017, 37(3): 37-42.
[6]	王路路, 权春善, 许永斌, 陈金利, 吴懿, 王冠天, 董悦生. 金黄色葡萄球菌arl双组分信号转导系统受体蛋白ArlS_CA的表达、纯化及活性研究[J]. 中国生物工程杂志, 2017, 37(11): 52-58.
[7]	叶雨辰, 赵俊龙, 王琳, 段娟丽, 高春辰, 秦鸿雁, 窦科峰. EGFP-Luc-Hepa1-6细胞系的构建及其在小鼠肝癌模型中的应用[J]. 中国生物工程杂志, 2015, 35(5): 1-7.
[8]	陆路, 熊文, 张钰琨, 王丽娜, 权春善, 范圣第. RF克隆结合巢式PCR构建金黄色葡萄球菌组氨酸蛋白激酶AgrC表达载体[J]. 中国生物工程杂志, 2014, 34(10): 55-60.
[9]	达飞, 侯征, 孟静茹, 贾敏, 罗晓星. 反义锁核酸阻断耐甲氧西林金黄色葡萄球菌agr群体感应系统[J]. 中国生物工程杂志, 2013, 33(5): 1-6.
[10]	吴迎春, 马琴琴, 丁先锋, 张凯, 刘立丽, 郭江峰. 响应面法优化产XRN1蛋白发酵培养基[J]. 中国生物工程杂志, 2013, 33(4): 121-128.
[11]	陈杰, 魏鸿刚, 罗远婵, 张道敬, 李淑兰, 田黎, 李元广. 海洋芽胞杆菌B-9987产新型抗菌环脂肽Marinhysin A的培养基优化[J]. 中国生物工程杂志, 2013, 33(1): 84-89.
[12]	陈洁梅, 徐聪聪, 常磊, 刘永萍, 缪冰旋. 响应面分析法优化豆粕固态发酵工艺生产大豆抗氧化肽的研究[J]. 中国生物工程杂志, 2012, 32(12): 59-65.
[13]	艾佐佐, 颜日明, 袁锦云, 张志斌, 朱笃. 响应面法优化木薯淀粉发酵生产单细胞油脂工艺[J]. 中国生物工程杂志, 2012, 32(07): 66-72.
[14]	闫兴, 师明磊, 陈娜, 王洋, 张彦, 王政, 李晓晨, 赵志虎. HCV NS3/4A蛋白酶胞内荧光检测方法的建立[J]. 中国生物工程杂志, 2012, 32(07): 84-88.
[15]	刘春光, 权春善, 王剑锋, 于桂梅, 范圣第. 重组蛋白AgrC的表达纯化及人工超分子体系的构建[J]. 中国生物工程杂志, 2012, 32(04): 1-6.

Viewed

Full text

Abstract

Cited

Shared

Discussed