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应用聚合酶链反应和DNA测序技术检测一名血培养阴性感染性心内膜炎患者主动脉瓣中的五日热巴尔通体。

Use of the polymerase chain reaction and DNA sequencing for detection of Bartonella quintana in the aortic valve of a patient with culture-negative infective endocarditis.

作者信息

Jalava J, Kotilainen P, Nikkari S, Skurnik M, Vänttinen E, Lehtonen O P, Eerola E, Toivanen P

机构信息

Department of Medical Microbiology, Turku University, Turku University Central Hospital, Finland.

出版信息

Clin Infect Dis. 1995 Oct;21(4):891-6. doi: 10.1093/clinids/21.4.891.

Abstract

We used the polymerase chain reaction (PCR) and broad-range bacterial primers, combined with DNA sequencing, to identify Bartonella quintana as the etiologic agent in a case of culture-negative infective endocarditis; all blood cultures, as well as the bacterial cultures of the resected aortic valve and vegetations, remained negative. PCR was used to amplify bacterial 16S rDNA from a template prepared from the aortic valve vegetation. The amplified 16S rDNA produced a nucleotide sequence that was 99.79% identical to the B. quintana rDNA sequence. The patient had a highly elevated level of serum antibodies to Bartonella antigen (1:8,192).

摘要

我们使用聚合酶链反应(PCR)和广谱细菌引物,并结合DNA测序,以确定五日热巴尔通体是一例血培养阴性感染性心内膜炎的病原体;所有血培养以及切除的主动脉瓣和赘生物的细菌培养均为阴性。PCR用于从主动脉瓣赘生物制备的模板中扩增细菌16S rDNA。扩增的16S rDNA产生的核苷酸序列与五日热巴尔通体rDNA序列的相似度为99.79%。该患者血清中抗巴尔通体抗原的抗体水平极高(1:8,192)。

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