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一种用于检测生物体液中致病性钩端螺旋体的免疫磁珠分离-聚合酶链反应方法。

An immunomagnetic separation-PCR method for detection of pathogenic Leptospira in biological fluids.

作者信息

Fernandes Cláudia Pinho Hartleben, Seixas Fabiana Kömmling, Coutinho Mariana Loner, Vasconcellos Flávia Aleixo, Moreira Angela Nunes, Conceição Fabricio Rochedo, Dellagostin Odir Antônio, Aleixo José Antonio Guimarães

机构信息

Centro de Biotecnologia, Universidade Federal de Pelotas, Pelotas, Brazil.

出版信息

Hybridoma (Larchmt). 2008 Oct;27(5):381-6. doi: 10.1089/hyb.2008.0029.

Abstract

Abstract Leptospirosis is a zoonotic disease that occurs worldwide and is caused by pathogenic bacteria of the genus Leptospira. Clinical manifestations of leptospirosis are similar to other febrile illnesses and this fact frequently retards the beginning of antibiotic therapy. Thus, early and accurate diagnosis is a prerequisite for proper treatment of leptospirosis. Antigen and DNA-based detection tests offer potential advantage over tests based on antibody detection for early diagnosis of leptospirosis since antibodies only reach detectable levels several days after the onset of the infection. This work describes a method for detection of pathogenic Leptospira that associates an immunoseparation step with a PCR assay and uses an internal amplification control (IAC) to ensure accuracy of the test. The immunoseparation was performed with protein A-magnetic beads in house coated with an MAb specific for LipL32, the major outer membrane protein of pathogenic Leptospira; PCR was performed using lipL32 specific primers. The IMS-PCR method enhanced detection of Leptospira in experimentally contaminated human sera and urine when compared to PCR performed alone. IMS-PCR was able to detect 10(2) Leptospira cells per mL of human sera and urine, corresponding to 25 genomic copies per PCR reaction.

摘要

摘要 钩端螺旋体病是一种在全球范围内发生的人畜共患病,由钩端螺旋体属的致病细菌引起。钩端螺旋体病的临床表现与其他发热性疾病相似,这一事实常常延迟抗生素治疗的开始。因此,早期准确诊断是正确治疗钩端螺旋体病的先决条件。基于抗原和DNA的检测试验在钩端螺旋体病的早期诊断方面比基于抗体检测的试验具有潜在优势,因为抗体在感染发生几天后才达到可检测水平。这项工作描述了一种检测致病性钩端螺旋体的方法,该方法将免疫分离步骤与PCR检测相结合,并使用内部扩增对照(IAC)来确保检测的准确性。免疫分离使用内部包被有针对致病性钩端螺旋体主要外膜蛋白LipL32的单克隆抗体的蛋白A磁珠进行;PCR使用lipL32特异性引物进行。与单独进行的PCR相比,IMS-PCR方法增强了在实验污染的人血清和尿液中钩端螺旋体的检测。IMS-PCR能够检测每毫升人血清和尿液中10(2)个钩端螺旋体细胞,相当于每个PCR反应25个基因组拷贝。

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