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首页> 外文期刊>Applied and Environmental Microbiology >Peptide aMptD-Mediated Capture PCR for Detection of Mycobacterium avium subsp. paratuberculosis in Bulk Milk Samples
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Peptide aMptD-Mediated Capture PCR for Detection of Mycobacterium avium subsp. paratuberculosis in Bulk Milk Samples

机译:肽Amptd介导的捕获PCR检测分枝杆菌亚空间。散装牛奶样品的副植物

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A peptide-mediated capture PCR for the detection of Mycobacterium avium subsp. paratuberculosis in bulk milk samples was developed and characterized. Capture of the organism was performed using peptide aMptD, which had been shown to bind to the M. avium subsp. paratuberculosis MptD protein (J. Stratmann, B. Strommenger, R. Goethe, K. Dohmann, G. F. Gerlach, K. Stevenson, L. L. Li, Q. Zhang, V. Kapur, and T. J. Bull, Infect. Immun. 72:1265-1274, 2004). Consistent expression of the MptD receptor protein and binding of the aMptD ligand were demonstrated by capturing different Mycobacterium avium subsp. paratuberculosis type I and type II strains and subsequent PCR analysis using ISMav2-based primers. The analytical sensitivity of the method was determined to be 5 × 102 CFU ml?1 for artificially contaminated milk. The specificity of aMptD binding was confirmed by culture and competitive capture assays, showing selective enrichment of M. avium subsp. paratuberculosis (at a concentration of 5 × 102 CFU ml?1) from samples containing 100- and 1,000-fold excesses of other mycobacterial species, including M. avium subsp. avium and M. avium subsp. hominissuis. The aMptD-mediated capture of M. avium subsp. paratuberculosis using paramagnetic beads, followed by culture, demonstrated the ability of this approach to capture viable target cells present in artificially contaminated milk. Surface plasmon resonance experiments revealed that the aMptD peptide is a high-affinity ligand with a calculated association rate constant of 9.28 × 103 and an association constant of 1.33 × 109. The potential use of the method on untreated raw milk in the field was investigated by testing 423 bulk milk samples obtained from different dairy farms in Germany, 23 of which tested positive. Taken together, the results imply that the peptide-mediated capture PCR might present a suitable test for paratuberculosis screening of dairy herds, as it has an analytical sensitivity sufficient for detection of M. avium subsp. paratuberculosis in bulk milk samples under field conditions, relies on a defined and validated ligand-receptor interaction, and is adaptable to routine diagnostic laboratory automation.
机译:肽介导的捕获PCR,用于检测分枝杆菌亚空分枝杆菌。散装牛奶样品中的分析性并表现出来。使用肽AMPTD进行有机体的捕获,该肽AMPTD已被证明与M. Avium Subsp结合。 Paratuberculosis MPTD蛋白(J. Stratmann,B. Stratmenger,R.Goethe,K. Dohmann,GF Gerlach,K. Stevenson,LL Li,Q. Zhang,V. Kapur和TJ Bull,Infect。Immun。72:1265- 1274,2004)。通过捕获不同的分枝杆菌载BP来证明MPTD受体蛋白的一致表达和AMPTD配体的结合。 Paratuberculosis I和II型菌株和随后使用基于ISMAV2的引物的PCR分析。该方法的分析敏感性被测定为5×102 CFU mlα1,用于人工受污染的牛奶。通过培养和竞争性捕获测定证实了AMPTD结合的特异性,显示出钙胚子的选择性富集。从含有100-和1,000倍的其他分枝杆菌物种的样品(包括M. Avium Subsp,以含有100-倍和1,000倍的5×102 CFU mlα1)的副刺激(以5×102cfu mlα1)。 Avium和M. Avium subsp。 hominissuis。 Amptd介导的M. Avium Subsp捕获。对植物沟珠的分析性,随后进行培养,证明了这种方法捕获在人为受污染的牛奶中存在的活靶细胞的能力。表面等离子体共振实验表明,AMPTD肽是高亲和力配体,具有9.28×103的计算缔置速率常数和1.33×109的关联常数。研究了该方法对该领域未处理的原料牛奶的潜在使用测试从德国的不同乳制品农场获得的423个散装牛奶样品,其中23个测试阳性。在一起,结果意味着肽介导的捕获PCR可能为乳制品牛群的分析敏感性呈现适当的抗菌筛查测试,因为它具有足以检测M. Avium Subsp的分析敏感性。在散装牛奶样品下的甲状腺抑制在现场条件下,依赖于定义和验证的配体 - 受体相互作用,并适应常规诊断实验室自动化。

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