牛支原体等温扩增冻干试剂盒研究

doi:10.3864/j.issn.0578-1752.2016.16.018

Abstract

Abstract: 【Objective】Mycoplasma bovis (M. bovis) is a pathogen related to a variety of syndromes of infected cattle, and it spreads widely in the world. For the survey of the epidemiology of M. bovis in China, simple and sensitive kits are needed.【Method】A recombinant plasmid with the uvrC gene of M. bovis was constructed and transfected into TOP10 competent cell, by which a strain of recombinant Escherichia coli was selected. The recombinant plasmid rP-uvrC was extracted, purified and diluted to the concentration of 10⁴copies/μL, which was used as the positive control. Betaine solution and color developing solution (mixture of SYBR Green I and HNB) were prepared to solve the freeze-dried amplification reagent and visualize the result of the amplification reaction, respectively, according to the published reports. Three kinds of freeze-drying protective agent which did not inhibit the amplification reaction were selected from 8 agents generally used to produce vaccine, then they were combined by different ratios to form 27 combinations, and the best combination was selected according to the physical characters. The isothermal amplification reagent made with the best freeze-drying protective agents were transported to the lyophilizer to detect the eutectic point, and the best heating-up time of the first drying, the first and the second drying times were determined. The best lyophilizing curve was selected to lyophilized the isothermal amplification reagent by testing of the physical characters, vacuum and residual water content. The lyophilized isothermal amplification kit consists of one tube of lyophilized isothermal amplification agent, betaine solution, positive control and color developing solution. The sensitivity of the kit was determined with a series of rP-uvrC solutions (10⁰-10⁵ copies), and the specificity was determined with 10⁴ CCU·mL^-1 solutions of M.bovis strains PG-45, HB-1, SD-2, 10⁸ CCU·mL^-1solutions of M. bovirhinis and M. agalactiae, and 10⁸CFU·mL^-1 Pasteurella multocida and Tuberculosis mycobacteria, respectively. The steady of the kit was also evaluated under different temperatures.【Result】Among the 8 freeze-drying protective agents, only trehalose, mannitol and bovine serum albumin did not interfere the isothermal amplification reaction, and the best freeze-drying protective agents composition is 5% trehalose +1.25% mannitol +1.25% bovine serum albumin. The eutectic point was -16℃, and the best heating-up time of the first drying was 3h, the first and the second drying times are 6h and 4h, respectively. The detection limit of the freeze-dried kit is 10 copies, 10⁴ CCU·mL^-1 solutions of M.bovis strains PG45, HB-1 and SD-2 showed positive results, 10⁸ CCU·mL^-1 solutions of M. bovirhinis and M. agalactiae, 10⁸CFU·mL^-1 Pasteurella multocida and Tuberculosis mycobacteria showed negative results. The sensitivity of the kit didn't change even it was stored for 6 months under 20℃ or 10 d under 37℃. So, the shelf life of the freeze-dried kit could be about 24 months.【Conclusion】The above results suggest that the freeze-dried kit has higher sensitivity, specificity and stability, could be used as a point-of-care (POC) test product since it is convenient for storage and very easy for the veterinarians to use in the farms.

Key words: Mycoplasma bovis, loop-mediated isothermal amplification, freeze-drying, kit, RT-PCR

WU Tong, LIU Xu, LI Jia-he, YAN Xin-bo, ZHANG Ning, WU Wen-xue. Development of a Freeze-Dried Kit for Isothermal Amplification Assay of Mycoplasma bovis[J].Scientia Agricultura Sinica, 2016, 49(16): 3251-3260.

0
/ / Recommend

Add to citation manager EndNote|Reference Manager|ProCite|BibTeX|RefWorks

URL: https://www.chinaagrisci.com/EN/10.3864/j.issn.0578-1752.2016.16.018

https://www.chinaagrisci.com/EN/Y2016/V49/I16/3251

References

[1] NICHOLAS R A, AYLING R D. Mycoplasma bovis: disease, diagnosis, and control. Research in Veterinary Science, 2003, 74(2): 105-112.

[2] MAUNSELL F P, WOOLUMS AR, FRANCOZ D, ROSENBUSCH R F, STEP D L, WILSON D J, JANZEN E D. Mycoplasma bovis infections in cattle. Journal of Veterinary Internal Medicine, 2001, 25:772-783.

[3] ADAMU J Y, WAWEGAMA N K, BROWNING, G F, MARKHAM, P F. Membrane proteins of Mycoplasma bovis and their role in pathogenesis. Research in Veterinary Science, 2013, 95:321-325.

[4] 胡长敏, 石磊, 龚瑞, 白智迪, 郭爱珍. 牛支原体病研究进展. 动物医学进展, 2009, 30(8): 73-77.

HU C M, SHI L, GONG R, BAI Z D, GUO A Z. Progress on Bovine Mycoplasmosis.Progress in Veterinary Medicine, 2009, 30(8):73-77. (in Chinese)

[5] HAINES D M, MARTIN K M, CLARK E G, JIM G K, JANZEN E D. The immunohistochemical detection of Mycoplasma bovis and bovine viral diarrhea virus in tissues of feedlot cattle with chronic, unresponsive respiratory disease and/or arthritis. The Canadian Veterinary Journal, 2001, 42: 857-860.

[6] SHAHRIAR F M, CLARK E G, JANZEN E, WEST K, WOBESER G. Coinfection with bovine viral diarrhea virus and Mycoplasma bovis in feedlot cattle with chronic pneumonia. The Canadian Veterinary Journal, 2002, 43: 863-868.

[7] GAGEA M I, BATEMAN K G, VAN DREUMEL T, MCEWEN B J, CARMAN S, ARCHAMBAULT M, SHANAHAN, R A, CASWELL J L. Diseases and pathogens associated with mortality in Ontario beef feedlots. Journal of Veterinary Diagnostic Investigation, 2006, 18: 18-28.

[8] NICHOLAS R A. Bovine mycoplasmosis: silent and deadly. The Veterinary Record, 2011, 168: 459-462.

[9] BALL H J, FINLAY D, REILLY G A. Sandwich ELISA detection of Mycoplasma bovis in pneumonic calf lungs and nasal swabs. The Veterinary Record, 1994, 135(22):531-532.

[10] BLACKBURN P, BROOKS C, BALL H J. Filtration of homogenised tissue samples to improve the diagnostic detection of Mycoplasma bovis by sandwich ELISA. The Veterinary Record, 2008, 163(17):514- 515.

[11] HELLER M, BERTHOLD E, PFÜTZNER H, LEIRER R, SACHSE K. Antigen capture ELISA using a monoclonal antibody for the detection of Mycoplasma bovis in milk. Veterinary of Microbiology, 1993, 37(1-2):127-133.

[12] BELL C J, BLACKBURN P, PATTERSON I A, ELLISON S, BALL H J. Real-time PCR demonstrates a higher prevalence of Mycoplasma bovis in Northern Ireland compared with sandwich ELISA. The Veterinary Record, 2012, 171(16):402.

[13] HERMEYER K, JACOBSEN B, SPERGSER J, ROSENGARTEN R, HEWICKER-TRAUTWEIN M. Detection of Mycoplasma bovis by in-situ hybridization and expression of inducible nitric oxide synthase, nitrotyrosine and manganese superoxide dismutase in the lungs of experimentally-infected calves. Journal of Comparative Pathology, 2011, 145(2-3):240-250.

[14] ADEGBOYE D S, RASBERRY U, HALBUR P G, ANDREWS J J, ROSENBUSCH R F. Monoclonal antibody-based immunohistochemical technique for the detection of Mycoplasma bovis in formalin-fixed, paraffin-embedded calf lung tissues. Journal of Veterinary Diagnostic Investigation, 1995, 7(2):261-265.

[15] HIGUCHI H, IWANO H, KAWAI K, OHTA T, OBAYASHI T, HIROSE K, ITO N, YOKOTA H, TAMURA Y, NAGAHATA H. A simplified PCR assay for fast and easy mycoplasma mastitis screening in dairy cattle. Journal of Veterinary Science, 2011, 12(2):191-193.

[16] CREMONESI P, VIMERCATI C, PISONI G, PEREZ G, RIBERA AM, CASTIGLIONI B, LUZZANA M, RUFFO G, MORONI P. Development of DNA extraction and PCR amplification protocols for detection of Mycoplasma bovis directly from milk samples, Veterinary Research Communications, 2007, 31(Suppl 1):225-227.

[17] ROSSETTI B C, FREY J, PILO P. Direct detection of Mycoplasma bovis in milk and tissue samples by real-time PCR. Molecular and Cellular Probes, 2010, 24(5):321-323.

[18] SACHSE K, SALAM HS, DILLER R, SCHUBERT E, HOFFMANN B, HOTZEL H. Use of a novel real-time PCR technique to monitor and quantitate Mycoplasma bovis infection in cattle herds with mastitis and respiratory disease, The Veterinary Journal, 2010, 186(3):299-303.

[19] BEN SHABAT M, MIKULA I, GERCHMAN I, LYSNYANSKY I. Development and evaluation of a novel single-nucleotide- polymorphism real-time PCR assay for rapid detection of fluoroquinolone-resistant Mycoplasma bovis. Journal of Clinical Microbiology, 2010, 48(8): 2909-2915.

[20] NOTOMI T, OKAYAMA H, MASUBUCHI H, YONEKAWA T, WATANABE K, AMINO N, HASE T. Loop-mediated isothermal amplification of DNA. Nucleic Acids Research, 2000, 28:E63.

[21] 黄火清, 郁昂. 环介导等温扩增技术的研究进展. 生物技术, 2012, 22(3): 90-94.

Huang H Q, Yu A. Advances of loop-mediated isothermal amplification. Biotechnology, 2012, 22(3):90-94. (in Chinese)

[22] 侯轩, 付萍, 张海燕, 张跃伟, 吴文学. 牛支原体的环介导等温扩增快速检测技术研究. 农业生物技术学报, 2012, 20(2):218-224.

HOU X, FU P, ZHANG H Y, ZHANG Y W, WU W X. Development of Loop-mediated Isothermal Amplification for Rapid Detection of Mycoplasma bovis. Journal of Agricultural Biotechnology, 2012, 20(2):218-224. (in Chinese)

[23] SUBRAMANIAM S, BERGONIER D, POUMARAT F, CAPAUL S, SCHLATTER Y, NICOLET J, FREY J. Species identification of Mycoplasma bovis and Mycoplasma agalactiae based on the uvrC genes by PCR. Molecular and Cellular Probes, 1998, 12(3):161-169.

[24] LI J H, MINION F C, PETERSEN A C, JIANG F, YANG S, GUO P P, LI J X, WU W X. Loop-mediated isothermal amplification for rapid and convenient detection of Mycoplasma hyopneumoniae, World Journal of Microbiology Bioanalytic Chemistry, 2013, 29:607-616.

[25] MARUYAMA F, KENZAKA T, YAMAGUCHI N, TANI K, NASU M. Detection of bacteria carrying the stx2 gene by in situ loop- mediated isothermal amplification. Applied and Environmental Microbiology, 2003, 69 (8):5023-5028.

[26] FUKUTA S, OHISHI K, YOSHIDA K, MIZUKAMI Y, ISHIDA A, KANBE M. Development of immunocapture reverse transcription loop-mediated isothermal amplification for the detection of tomato spotted wilt virus from chrysanthemum. Journal of Virology Methods, 2004, 121(1):49-55.

[27] KUBOKI N, INOUE N, SAKURAI T, DI CELLO F, GRAB DJ, SUZUKI H, SUGIMOTO C, IGARASHI I. Loop-Mediated Isothermal Amplification for Detection of African Trypanosomes. Journal of clinical microbiology, 2003, 41(12):5517-5524.

[28] Zhang Y W, Fu P, Li J H, Jiang F, Li J X, Wu W X. Development of loop-mediated isothermal amplification method for visualization detection of the highly virulent strains of porcine reproductive and respiratory syndrome virus (PRRSV) in China, African Journal of Biotechnology, 2011, 10(61): 13278-13283.

[29] 蒋菲, 黄书林, 徐威, 张跃伟, 刘金华, 吴文学. H9亚型禽流感病毒环介导等温扩增检测方法的建立与荧光显色剂的应用. 农业生物技术学报, 2010, 19(1):191-196.

JIANG F, HUANG S L, XU W, ZHANG Y W, LIU J H, WU W X. Detection of H9 avian influenza virus by Loop-mediated Isothermal Amplification and Application of Fluorescent Reagent. Journal of Agricultural Biotechnology, 2010, 19(1):191-196. (in Chinese)

[30] 李佳禾, 李一婧, 付萍, 张跃伟, 黄书林, 郭盼盼, 蒋菲, 吴文学. 胸膜肺炎放线杆菌的环介导等温扩增检测方法的研究. 农业生物技术学报, 2009, 17(6):948-953.

LI J H, LI Y J, FU P, ZHANG Y W, HUANG S L, GUO P P, JIANG F, WU W X.Detection ofActinobacillus pleuropneumoniae by Newly Developed Loop-mediated Isothermal Amplification Method, 2009, 17(6):948-953. (in Chinese)

[31] KLATSER P, KUIJPER S, VAN INGEN C W, KOLK A H. Stabilized, freeze-dried PCR mix for detection of mycobacteria. Journal of Clinical Microbiology, 1998, 36(6):1798-1800.

[32] 李美霞, 张庆利, 刘利平, 黄倢, 谢国驷. 海藻糖对冷冻干燥的LAMP反应体系的保护效果. 渔业科学进展, 2012, 33(5):95-101.

LI M X, ZHANG Q L, LIU L P, HUANG J, XIE G S. The protective effects of trehalose on freeze-drying and LAMP reagents storage. Progress in Fishery Sciences, 2012, 33(5):95-101. (in Chinese)

[33] Production Information of Bst DNA Polymerase, Large Fragment, http://www.neb.sg/products/m0275-bst-dna-polymerase-large-fragment

Related Articles 15

[1]	WANG YiDan,YANG FaLong,CHEN DiShi,XIANG Hua,REN YuPeng. One-Step Multiple TaqMan Real-time RT-PCR for Simultaneous Detection of Swine Diarrhea Viruses [J]. Scientia Agricultura Sinica, 2023, 56(1): 179-192.
[2]	WANG SiTong,CHEN Yan,LUO YuJia,YANG YuanYuan,JIANG ZhiYang,JIANG XinYi,ZHONG Fan,CHEN Hao,XU HongXing,WU Yan,DUAN HongXia,TANG Bin. Effect of Three Novel Compounds on Trehalose and Chitin Metabolism and Development of Spodoptera frugiperda [J]. Scientia Agricultura Sinica, 2022, 55(8): 1568-1578.
[3]	XIE LiXue,ZHANG XiaoYan,ZHANG LiJie,ZHENG Shan,LI Tao. Complete Genome Sequence Characteristics and TC-RT-PCR Detection of East Asian Passiflora Virus Infecting Passiflora edulis [J]. Scientia Agricultura Sinica, 2022, 55(22): 4408-4418.
[4]	KANG JunMei,ZHANG QiaoYan,JIANG Xu,WANG Zhen,ZHANG TieJun,LONG RuiCai,CUI HuiTing,YANG QingChuan. Cloning MsSQE1 from Alfalfa and Functional Analysis in Saponin Synthesis [J]. Scientia Agricultura Sinica, 2020, 53(2): 247-260.
[5]	XU JianJian,WANG YanJiao,DUAN Yu,MA ZhiMin,BIN Yu,ZHOU ChangYong,SONG Zhen. Construction of Genome-Length cDNA of Citrus Vein Enation Virus and Identification of Its Infectivity [J]. Scientia Agricultura Sinica, 2020, 53(18): 3707-3715.
[6]	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.
[7]	LIU YiRan,ZHANG Hong,JIN JiSu,ZHOU ZhongShi,GUO JianYing. Identification and Expression Analysis of the Halloween Gene Family in Agasicles hygrophila [J]. Scientia Agricultura Sinica, 2020, 53(10): 2009-2019.
[8]	DING YanJuan,LIU YongKang,LUO YuJia,DENG YingMei,XU HongXing,TANG Bin,XU CaiDi. Potential Functions of Nilaparvata lugens GSK-3 in Regulating Glycogen and Trehalose Metabolism [J]. Scientia Agricultura Sinica, 2019, 52(7): 1237-1246.
[9]	TANG Bin,SHEN QiDa,ZENG BoPing,XIAO ZhongJiu,QIU LingYu,PAN BiYing,LI Kun,ZHANG DaoWei. Characteristics, Developmental Expression and RNAi Effect Analysis of a Novel Trehalose-6-Phosphate Synthase Gene in Nilaparvata lugens [J]. Scientia Agricultura Sinica, 2019, 52(3): 466-477.
[10]	JunBo PENG,XingHong LI,Wei ZHANG,Ying ZHOU,JinBao HUANG,JiYe YAN. Pathogenicity and Gene Expression Pattern of the Exocrine Protein LtGH61A of Grape Canker Fungus [J]. Scientia Agricultura Sinica, 2019, 52(24): 4518-4526.
[11]	WAN DongLi,HOU XiangYang,DING Yong,REN WeiBo,WANG Kai,LI XiLiang,WAN YongQing. Response and the Expression of Pi-Responsive Genes in Leymus chinensis Under Inorganic Phosphate Treatment [J]. Scientia Agricultura Sinica, 2019, 52(23): 4215-4227.
[12]	YUAN JunHu,DING YiJuan,YANG WenJing,YAN BaoQin,CHAI YaRu,MEI JiaQin,QIAN Wei. Identification of Genes Encoding Secretory Proteins Related to the Pathogenicity of Sclerotinia sclerotiorum Using TRV-HIGS [J]. Scientia Agricultura Sinica, 2019, 52(23): 4274-4284.
[13]	LIU FanQi,WAN GuiJun,ZENG LuYing,LI ChunXu,PAN WeiDong,CHEN FaJun. Selection of Stable Internal Reference Genes for Transcript Expression Analyses in Laodelphax striatellus Under Near-Zero Magnetic Field [J]. Scientia Agricultura Sinica, 2019, 52(19): 3346-3356.
[14]	ZHANG DaoWei,YU YaYa,PAN BiYing,KANG Kui,ZENG BoPing,CHEN Jing,TANG Bin. Regulation Function of Trehalose-6-phosphate Synthase Genes on Chitin Synthesis in Sogatella furcifera [J]. Scientia Agricultura Sinica, 2019, 52(19): 3357-3366.
[15]	TANG YaFei,PEI Fan,LI ZhengGang,SHE XiaoMan,YU Lin,LAN GuoBing,DENG MingGuang,HE ZiFu. Identification of Viruses Infecting Peppers in Guangdong by Small RNA Deep Sequencing [J]. Scientia Agricultura Sinica, 2019, 52(13): 2256-2267.

Metrics

Viewed

Full text

Abstract

Cited

Shared

Discussed

Comments

Recommended 0

No Suggested Reading articles found!

Development of a Freeze-Dried Kit for Isothermal Amplification Assay of Mycoplasma bovis

RichHTML

PDF

Abstract

Cite this article

share this article

References

Related Articles 15

Metrics

Comments

Recommended 0