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Comparison of molecular markers for determining the viability and infectivity of Cryptosporidium oocysts and validation of molecular methods against animal infectivity assay

机译:用于确定隐孢子虫卵囊活力和感染性的分子标记的比较,以及针对动物传染性测定的分子方法的验证

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Background: Globally, disinfectants are widely used to intervene in the dissemination of Cryptosporidium oocysts. However, extensive investigations of oocyst inactivation by various disinfectants are not feasible due to the limitations imposed by animal infectivity methods. Molecular techniques provide an alternative strategy; however, non-metabolic genes have been used as markers for determining viability/infectivity. Methods: In this study we used amyloglucosidase (AG) - a metabolic protein - as a marker to determine viability/infectivity of Cryptosporidium. Oocysts were exposed to 6% hydrogen peroxide for 2min. Samples were analyzed by cell culture polymerase chain reaction (CC-PCR) using PCR primers specific for heat shock protein 70 (hsp70) and AG. Both target genes were amplified with the same level of intensity. Results: Based on the results it can be concluded that AG is a valid target for the study of environmental survival and for the evaluation of the efficacy of microbicides against Cryptosporidium using molecular and cellular assays. Comparison of the CC-PCR assay and mouse infectivity assay showed a fairly good correlation under these test conditions. Conclusion: Results indicate that the CC-PCR assay presents a valid and cost-effective alternative to the mouse infectivity assay.
机译:背景:在全球范围内,消毒剂被广泛用于干预隐孢子虫卵囊的传播。然而,由于动物感染方法的局限性,对各种消毒剂对卵囊灭活的广泛研究是不可行的。分子技术提供了另一种策略。然而,非代谢基因已被用作确定生存力/传染性的标记。方法:在这项研究中,我们使用了一种代谢蛋白淀粉淀粉葡萄糖苷酶(AG)作为确定隐孢子虫的生存力/感染力的标志物。卵囊暴露于6%的过氧化氢2分钟。使用对热休克蛋白70(hsp70)和AG特异的PCR引物,通过细胞培养聚合酶链反应(CC-PCR)分析样品。两种靶基因均以相同强度扩增。结果:根据结果可以得出结论,AG是用于环境生存研究以及使用分子和细胞分析评估杀菌剂对隐孢子虫功效的有效靶标。在这些测试条件下,CC-PCR分析与小鼠感染性分析的比较显示出相当好的相关性。结论:结果表明,CC-PCR测定法是替代小鼠感染测定法的一种有效且具有成本效益的选择。

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