首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Molecular cloning of Ehrlichia risticii and development of a gene probe for the diagnosis of Potomac horse fever.
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Molecular cloning of Ehrlichia risticii and development of a gene probe for the diagnosis of Potomac horse fever.

机译:埃希氏毛虫的分子克隆和用于诊断波托马克马热的基因探针的开发。

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摘要

A gene bank of Ehrlichia risticii was constructed in plasmid vector pUC13. Five clones representing discrete regions of the E. risticii genome were tested for their ability to hybridize specifically to E. risticii DNA. None of the clones cross-hybridized with Ehrlichia equi DNA, whereas four of these clones cross-hybridized with Ehrlichia canis and Ehrlichia sennetsu DNAs. However, one clone carrying a 1-kilobase HindIII fragment of E. risticii DNA failed to cross-react with the genomes of E. sennetsu, E. canis, and E. equi in dot blot hybridization assays. The sensitivity of this probe for the detection of E. risticii DNA was approximately 0.5 pg. By using this probe, the E. risticii DNA was detected in the peripheral blood mononuclear cells of 30 experimentally infected horses by 7 days postinfection (p.i.); the detection of E. risticii DNA peaked between 14 and 17 days p.i., a period immediately after the peak of the second rise in body temperature, during leukopenia and at the onset of diarrhea. E. risticii DNA was not detectable by 25 to 30 days p.i. E. risticii DNA was not detected in noninfected control horses.
机译:在质粒载体pUC13中构建了埃里希氏菌的基因库。测试了代表埃里希埃里希氏菌基因组离散区域的五个克隆与埃里希埃里希氏菌DNA特异性杂交的能力。没有一个克隆与马兜铃虫DNA交叉杂交,而这些克隆中有四个与犬埃里希氏菌和Sennetsu Sennetsu DNAs交叉杂交。然而,在斑点印迹杂交测定中,携带E.risticii DNA的1-千碱基HindIII片段的一个克隆未能与E. sennetsu,E。canis和E. equi的基因组交叉反应。该探针对大肠杆菌的DNA的检测灵敏度约为0.5 pg。通过使用该探针,在感染后7天(p.i.),在30只实验感染的马的外周血单核细胞中检测到了埃希氏大肠杆菌DNA。在白细胞减少症期间和腹泻开始时,在体温第二次升高的峰值之后不久的一个时间段内,埃里希埃里希氏体DNA的检测就达到峰值,时间为14至17天。 p.i.到25到30天时,无法检测到E. risticii DNA。在未感染的对照马中未检测到大肠杆菌。

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