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首页> 外文期刊>Journal of Veterinary Diagnostic Investigation >Pooling of porcine fecal samples for quantification of Lawsonia intracellularis by real-time polymerase chain reaction
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Pooling of porcine fecal samples for quantification of Lawsonia intracellularis by real-time polymerase chain reaction

机译:收集猪粪便样品,通过实时聚合酶链反应定量测定胞内劳森菌

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Procedures in which biological specimens are mixed and tested as 1 sample (pooling) have been applied for various biological specimens and laboratory examinations. The objective of the current study was to investigate agreement between laboratory testing of fecal pools and theoretical values obtained by averaging test results from individual fecal samples in relation to a quantitative polymerase chain reaction (qPCR) test for Lawsonia intracellularis. Ten diarrheic and 10 normal fecal samples were submitted from each of 43 Danish swine herds (n = 860 fecal samples). Pools (n = 43), each containing 20 individual fecal samples from the same herd, were prepared in the laboratory by pooling 10% fecal phosphate buffered saline solutions. All pools and individual fecal samples were subjected to qPCR testing for L. intracellularis. The theoretical number of L. intracellularis in the pools was calculated as the mean number of bacteria from the 20 individual fecal samples contributing to each pool. Agreement between the laboratory testing of pools and theoretical calculations based on individual sample results was evaluated. Pooling resulted in fewer L. intracellularis-positive herds (41.9%) compared with testing 20 fecal samples (53.5%). Agreement between the laboratory and the theoretical pools for dichotomized test results was 100% (95% confidence interval: 91.8-100%). For the quantitative test results, Lin concordance correlation coefficient was 0.997. The mean difference between the laboratory testing and the theoretical values was not different from zero (mean difference = 0.039 log(10) bacteria/g feces; P = 0.26).
机译:将生物样本混合并作为1个样本进行测试(合并)的程序已用于各种生物样本和实验室检查。当前研究的目的是调查粪便池的实验室测试与通过将单个粪便样品的测试结果与细胞内劳森菌定量聚合酶链反应(qPCR)测试相关的平均值得出的理论值之间的一致性。从43个丹麦猪群中分别提交了10个腹泻样品和10个正常粪便样品(n = 860个粪便样品)。在实验室中,通过合并10%的粪便磷酸盐缓冲盐溶液,制备了每个样本池(n = 43),每个样本池包含来自同一群的20个粪便样品。对所有的池和单个粪便样品进行细胞内劳森氏菌的qPCR测试。计算池中胞内劳森氏菌的理论数,作为贡献于每个池的20个单独粪便样品中细菌的平均数。评估池的实验室测试与基于单个样本结果的理论计算之间的一致性。与测试20个粪便样品(53.5%)相比,合并导致更少的细胞内劳森氏菌阳性牛群(41.9%)。实验室和二分法化验结果的理论库之间的一致性为100%(95%置信区间:91.8-100%)。对于定量测试结果,Lin一致性相关系数为0.997。实验室测试与理论值之间的平均差异不为零(平均值差异= 0.039 log(10)细菌/ g粪便; P = 0.26)。

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