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Changes in the levels of Cryspovirus during in vitro development of Cryptosporidium parvum

机译:小隐隐孢子虫体外发育过程中隐球菌水平的变化

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The purpose of this study was to develop and utilize semi-quantitative RT-PCR and PCR assays for measuring the level of Cryspovirus, the viral symbiont of Cryptosporidium parvum, during in vitro development of the protozoan. Cultures of human carcinoma cells (HCT-8) were inoculated with excysting C. parvum sporozoites, followed by harvest of cells and culture medium at 2-, 24-, 48-, and 72-h post-infection. Changes in viral RNA levels were detected by RT-PCR using primers specific for RNA encoding the 40-kDa capsid protein (CP) or RNA-dependent RNA polymerase (RdRp). Parasite or host DNA was quantified by PCR specific for C. parvum or human glyceraldehyde-3-phosphate dehydrogenase (HuGAPDH). An internal standard (competitor) was incorporated into all assays as a control for PCR inhibition. Intracellular levels of C. parvum DNA increased between 2- and 48-h post-infection, and then decreased at 72 h. Culture medium overlying these C. parvum-infected cells displayed a similar increase in CP and RdRp signal, reaching peak levels at 48 h. However, the CP and RdRp levels in cellular RNA displayed only a modest increase between 2 and 48 h, and exhibited no change (CP) or decreased (RdRp) at 72 h. These data suggest that during the first 48 h of C. parvum in vitro development, Cryspovirus is released into the media overlying cells but remains at fairly constant levels within infected cells.
机译:这项研究的目的是开发和利用半定量RT-PCR和PCR分析方法来测量原生动物体外发育过程中小隐隐孢子虫的病毒共生体隐孢子虫病毒的水平。将人癌细胞(HCT-8)的培养物接种囊状小球藻子孢子,然后在感染后2、24、48和72小时收获细胞和培养基。病毒RNA水平的变化通过RT-PCR使用编码40 kDa衣壳蛋白(CP)或RNA依赖性RNA聚合酶(RdRp)的RNA特异性引物检测。寄生虫或宿主DNA通过特异于衣原体梭状芽胞杆菌或人甘油醛-3-磷酸脱氢酶(HuGAPDH)的PCR定量。将内标(竞争者)掺入所有测定中,作为PCR抑制的对照。感染后2小时至48小时之间,小球藻DNA的细胞内水平升高,然后在72小时时降低。覆盖这些细小衣原体感染细胞的培养基显示出CP和RdRp信号类似的增加,在48小时达到峰值。然而,细胞RNA中的CP和RdRp水平在2至48小时之间仅显示出适度的增加,而在72小时时则无变化(CP)或下降(RdRp)。这些数据表明,在小球藻体外培养的最初48小时内,结晶病毒被释放到覆盖细胞的培养基中,但在感染细胞中仍保持相当恒定的水平。

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