期刊文献+

APEC强毒力岛核心基因irp2、fyuA敲除对其致病性影响的研究 被引量:10

The relationship between the core gene irp2、fyuA deletion of the high pathogenicity island and the pathogenicity of APEC
原文传递
导出
摘要 采用Red同源重组技术分别构建出APEC irp2单基因敲除株△AE17和irp2、fyuA双基因敲除株△△AE17。运用活菌计数法分别观察AE17、△AE17、△△AE17黏附鸡胚成纤维细胞DF-1的能力。并且应用Real-time PCR检测AE17、△AE17和△△AE17中的luxs,pfs,tsh,ibeA,stx2f,iss,ompA,fimC 8个毒力基因转录水平。结果成功构建出基因敲除株△AE17和△△AE17,它们黏附DF-1细胞的能力分别下降为AE17的66.04%和53.54%。同时,Real-time PCR结果显示,△AE17的luxs,iss,ompA和fimC等4个毒力基因的转录水平均极显著下降(P<0.01),△△AE17的luxs,pfs,tsh,iss,ompA和fimC等6个毒力基因的转录水平极显著的下降(P<0.01)。结果表明强毒力岛中核心基因的敲除能够减弱APEC黏附DF-1的能力,并且使其毒力基因的转录水平有所降低。irp2、fyuA双基因敲除较irp2单基因敲除对APEC的致病性影响更显著。 Abstract:The the Red homologous recombination method was used to construct the irp2 gene dele- tion strain △AE17 and the irp2, fyuA genes deletion strain △△AE17. Viable bacteria counting method was used to evaluate the effects of AE17, △AE17 and △△AE17 on the capability of APEC to adhere and invade DF-lcell. Their effects on the mRNA levels of the luxs,pfs,tsh,ibeA, stx2f,iss,ompA and fimC virulence genes were analyzed using real-time PCR. The results showed that succeed constructed APEC strains △AE17 and △△AE17 were. The adherences of △AE17 and △△AE17 were decreased by 66.04% and 53.54%. Real-time PCR showed that the transcrip- tion of luxs,iss,ompA, fimC genes of △AE17 was decreased and the transcription of luxs, pfs, tsh,iss,ompA,fimC genes of △△AE17 was decreased. The invasion to DF 1 cells of the bacteria were decreased and transcription of the virulence genes were decreased by the core gene deletion of high pathogenicity island in the APEC. The influence of irp2, fyuA genes deletion is more impor- tant to the pathogenicity in APEC when compared with the irp2 gene deletion.
出处 《中国兽医学报》 CAS CSCD 北大核心 2014年第4期564-570,共7页 Chinese Journal of Veterinary Science
基金 国家自然科学基金资助项目(30871851)
关键词 APEC 强毒力岛 irp2 fyuA 致病性 APEC high pathogenicity island irp2 fyuA pathogenicity
  • 相关文献

参考文献14

  • 1Schotulcr C, Schaeffer B, Bree A, et al. Diagnostic strategy for idcmifying avian pathogenic Escherichia col; based on four patterns of virulence genes[J]. Clin Microbi,2012,50(5) : 1673-1678. 被引量:1
  • 2Hem X G,Bai H,Lei L,et al. The luxS gene functions in lhc pathogenesis of avian pathogenic Esccherichia coli[J]. Microbial Pathogenesis, 2013,6 ( 55 ) : 21-27. 被引量:1
  • 3Carniel E, Guilvout I, Prentice M. Characterization of a large chromosomal ‘ high-pathogenicity island ' in hiotype IB Yersinia enterocolitica[J]. Bacteriology, 1996.178(23) :6743-6751. 被引量:1
  • 4Rakin A, Noclting C,Schubert S,et al. Common and spccific eharactcristics of the high-pathogenicity island of Yersimia emerocolitica[J]. Infect Immun, 1999,67 (10) :5265-5271. 被引量:1
  • 5Christoph A,Gregm S,Rakin A,et al, Expression a naiysis of the Yersbdahactin receptor gene fyuA and tile heine receptor hemR of Yersinia enterocolitica in witra. and in vivo using the reporter genes for green fluorescent prmein and lueiferase[J]. Infect Immun, 200! ,69(12) :7772. 被引量:1
  • 6Karch H, Sclmberl S. Zhang D, et al. A genomic is- land, lermcd high pathogenicity island, is present in cerlain non-O 157 Shiga toxin-producing Escherichia coli clonal lineages[J]. Infect immune, 1999,67(11) : 5994-6001. 被引量:1
  • 7Bach S, Almeida A, Carniel E. The Yersinia high- pathogenicity island is present in different members of the family Enteroba cteriaceae[J]. FEMS Microbiol LeE, 2000,183 (2) : 289-294. 被引量:1
  • 8Schubert S,Rakin A,Karch H, et al. Prevalence of the "high-pathogenicity island" of Yersinia species among Escherichia coli strains that are pathogenic to humans [J]. Infect immun,1998,66(2) :480-485. 被引量:1
  • 9陈文静,韩先干,何亮,胡青海,于圣青.鸭致病性大肠杆菌的分离鉴定及其生物学特性分析[J].中国动物传染病学报,2010,18(2):34-40. 被引量:41
  • 10Muyrers J P, Zhang Y, Stewart A F. Techniques. Recombinogenic engineering-new options for cloning and manipulating DNA[J]. Trends Biochem Sci,2001,26(5) :325-331. 被引量:1

二级参考文献6

  • 1胡青海,刘晓文,苗晋锋,赵东伟,张知良,丁铲.当前我国鸭病de流行动态与防制对策[J].中国禽业导刊,2001,18(23):18-18. 被引量:4
  • 2Zhao S,Muarer J J,Htlbert S,et al.Antimicrobialsusceptibility and molecular characterization of avianpathogenicEscherichia coliisolates. Veterinary Microbiology . 2005 被引量:1
  • 3Dozois CM,Fairbrother JM,Harel J,et al.Pap-and pil-related DNA sequences and other virulence determinants associated with Escherichia coli isolated from septicemic chickens and turkeys. Infection and Immunity . 1992 被引量:1
  • 4Christa Ewers,Traute JanBen,Sabine KieBling,et al.Molecular epidemiology of avian pathogenic Escherichia coli (APEC) isolated from colisepticemia in poultry. Veterinary Microbiology . 2004 被引量:1
  • 5Dho-Moulin M,Fairbrother J M.Avian pathogenic Escherichia coli(APEC). Veterinary Research . 1999 被引量:1
  • 6Cloud S S,Rosenberger J K,Fries P A,et al.In Vitro and Vivo Characterization of Avian Escherichta coil.I. Serotypes,Metabolic Activity and Antiiotic Sensitivity. Avian Diseases . 1985 被引量:1

共引文献40

同被引文献58

引证文献10

二级引证文献18

相关作者

内容加载中请稍等...

相关机构

内容加载中请稍等...

相关主题

内容加载中请稍等...

浏览历史

内容加载中请稍等...
;
使用帮助 返回顶部