Sreevatsan S, Bookout J B, Ringpis F, Perumaalla V S, Ficht T A, Adams L G, Hagius S D, Elzer P H, Bricker B J, Kumar G K, Rajasekhar M, Isloor S, Barathur R R
ClinCyte, LLC, San Diego, California 92121, USA.
J Clin Microbiol. 2000 Jul;38(7):2602-10. doi: 10.1128/JCM.38.7.2602-2610.2000.
A multiplex amplification and detection platform for the diagnosis of Mycobacterium bovis and Brucella abortus infection simultaneously in bovine milk and nasal secretions was developed. This system (designated the bovine pathogen detection assay [BPDA]-PCR) consists of duplex amplification of species-specific targets (a region of the BCSP31K gene of B. abortus and a repeat-sequence region in the hsp65 gene of M. bovis, respectively). This is followed by a solid-phase probe capture hybridization of amplicons for detection. On the basis of spiking experiments with normal milk, the analytical sensitivity of the assay was 800 CFU equivalents/ml of milk for B. abortus and as low as 4 CFU equivalents per ml of milk for M. bovis. BPDA-PCR was validated with 45 liver samples from lemmings experimentally infected with B. abortus. The assay sensitivity, based on culture status as a "gold standard," was 93.9%. In this experiment, BPDA-PCR also identified five culture-negative liver samples as positive (41.7%). Field studies for the evaluation of BPDA-PCR were performed with samples from dairy animals from geographically distinct regions (India, Mexico, and Argentina). A high prevalence of shedding of B. abortus (samples from India) and M. bovis (samples from Mexico) was identified by BPDA-PCR. In samples from India, B. abortus shedding was identified in 86% of milk ring test-positive animals (n = 15) and 80% of milk ring test-negative cows (n = 5). In samples from Mexico, M. bovis was identified by PCR in 32.6% of pools (n = 46) of milk that each contained milk from 10 animals and in 56.2% of nasal swabs (n = 121) from cattle from tuberculin test-positive herds. In contrast, the Argentine cattle (n = 70) had a modest prevalence of M. bovis shedding in nasal swabs (2.9%) and milk (1.4%) and of B. abortus in milk (11.4%). On the basis of these analyses, we identify BPDA-PCR as an optimal tool for both screening of herds and testing of individual animals in a disease eradication program. A combination of the duplex assay, screening of milk samples in pools, and the proposed algorithm provides a highly sensitive, cost-effective, and economically viable alternative to serological testing.
开发了一种用于同时诊断牛乳和鼻分泌物中牛分枝杆菌和流产布鲁氏菌感染的多重扩增和检测平台。该系统(称为牛病原体检测分析[BPDA]-PCR)包括对物种特异性靶标进行双重扩增(分别为流产布鲁氏菌的BCSP31K基因区域和牛分枝杆菌hsp65基因中的重复序列区域)。随后进行扩增子的固相探针捕获杂交以进行检测。基于用正常牛奶进行的加标实验,该分析方法对流产布鲁氏菌的分析灵敏度为每毫升牛奶800 CFU当量,对牛分枝杆菌低至每毫升牛奶4 CFU当量。BPDA-PCR用45份来自实验感染流产布鲁氏菌的旅鼠肝脏样本进行了验证。以培养状态作为“金标准”,该检测方法的灵敏度为93.9%。在该实验中,BPDA-PCR还将5份培养阴性的肝脏样本鉴定为阳性(41.7%)。使用来自地理上不同地区(印度、墨西哥和阿根廷)的奶牛样本进行了评估BPDA-PCR的现场研究。通过BPDA-PCR鉴定出流产布鲁氏菌(来自印度的样本)和牛分枝杆菌(来自墨西哥的样本)的高流行率。在来自印度的样本中,在86%的乳环试验阳性动物(n = 15)和80%的乳环试验阴性奶牛(n = 5)中检测到流产布鲁氏菌 shedding。在来自墨西哥的样本中,通过PCR在32.6%的每组包含10头动物牛奶的牛奶池(n = 46)和56.2%的来自结核菌素试验阳性牛群的牛鼻拭子(n = 121)中检测到牛分枝杆菌。相比之下,阿根廷的牛(n = 70)鼻拭子(2.9%)和牛奶(1.4%)中牛分枝杆菌 shedding以及牛奶中流产布鲁氏菌的流行率较低(11.4%)。基于这些分析,我们确定BPDA-PCR是疾病根除计划中畜群筛查和个体动物检测的最佳工具。双重检测、牛奶样本混合筛查和所提出的算法相结合,为血清学检测提供了一种高度灵敏、具有成本效益且经济可行的替代方法。
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