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Enhancement of the Molecular and Serological Assessment of Hepatitis E Virus in Milk Samples

机译:牛奶样品中丙型肝炎病毒分子和血清学评估的增强

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Hepatitis E virus (HEV) infection is endemic in developing and developed countries. HEV was reported to be excreted in the milk of ruminants, raising the possibility of transmission of HEV infection through the ingestion of contaminated milk. Therefore, the detection of HEV markers in milk samples becomes pivotal. However, milk includes inhibitory components that affect HEV detection assays. Previously it was reported that dilution of milk matrix improves the performance of HEV molecular assay, however, the dilution of milk samples is not the best strategy especially when the contaminated milk sample has a low HEV load. Therefore, the objective of this study is to compare the effect of extraction procedures on the efficiency of HEV RNA detection in undiluted milk samples. In addition, we assessed the effect of the removal of milk components such as fats and casein on the performance of the molecular and serological assays of HEV. Phosphate buffered saline (PBS) and different milk matrices (such as whole milk, skim milk, and milk serum) were inoculated with different HEV inoculums and subjected to two different extraction procedures. Method A includes manual extraction using spin column-based extraction, while method B includes silica-based automated extraction. Method A was more sensitive than method B in the whole milk and skim milk matrices with a LoD 95% of 300 IU/mL, and virus recovery yield of 47%. While the sensitivity and performance of method B were significantly improved using the milk serum matrix, with LoD 95% of 96 IU/mL. Interestingly, retesting HEV positive milk samples using the high sensitivity assay based on method B extraction and milk serum matrix increased the HEV RNA detection rate to 2-fold. Additionally, the performance of HEV serological assays such as anti-HEV IgG and HEV Ag in the milk samples was improved after the removal of the fat globules from the milk matrix. In conclusion, HEV RNA assay is affected by the components of milk and the extraction procedure. Removal of inhibitory substances, such as fat and casein from the milk sample increased the performance of HEV molecular and serological assays which will be suitable for the low load HEV milk with no further dilutions.
机译:乙型肝炎病毒(HEV)感染是发展中国家和发达国家的地方性。据报道,HEV被排泄在反刍动物牛奶中,通过摄入污染的牛奶来提高HEV感染的可能性。因此,牛奶样品中HEV标记的检测变为枢转。然而,牛奶包括影响HEV检测测定的抑制成分。此前据报道,乳基质的稀释性提高了HEV分子测定的性能,然而,乳液样品的稀释不是最好的策略,特别是当污染的乳汁具有低的HEV载荷时。因此,本研究的目的是比较提取程序对未稀释的牛奶样品中HEV RNA检测效率的影响。此外,我们评估了除去脂肪和酪蛋白等脂肪和酪蛋白的乳化成分的效果。用不同的HEV含量接种磷酸盐缓冲盐水(PBS)和不同的乳基质(例如全牛奶,脱脂牛奶和乳血清)并进行两种不同的提取程序。方法A包括使用基于旋转柱的提取的手动提取,而方法B包括基于二氧化硅的自动提取。方法A比全牛奶中的方法B更敏感,脱脂乳基质的含量为300μm/ ml的含量为95%,病毒回收率为47%。虽然使用乳血清基质的方法B的敏感性和性能显着改善,但LOD 95%的96 IU / mL。有趣的是,使用基于方法B萃取和乳血清基质的高灵敏度测定的重试HEV阳性乳样品增加了HEV的RNA检测率至2倍。另外,在从牛奶基质中除去脂肪球后,改善了HEV血清学测定的性能,例如抗HEV IgG和HEV Ag。总之,HEV RNA测定受牛奶组分和提取程序的影响。除去乳汁样品的抑制物质,例如脂肪和酪蛋白,增加了HEV分子和血清学测定的性能,这适用于低载荷HEV牛奶,没有进一步稀释。

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