Brussel Audrey, Brack Kerstin, Muth Erika, Zirwes Rudolf, Cheval Justine, Hebert Charles, Charpin Jean-Marie, Marinaci Alice, Flan Benoit, Ruppach Horst, Beurdeley Pascale, Eloit Marc
LFB, Courtaboeuf, France.
Charles River Laboratories Germany GmbH, Erkrath, Germany.
Biologicals. 2019 May;59:29-36. doi: 10.1016/j.biologicals.2019.03.008. Epub 2019 Apr 13.
The utilization of the current combination of in vitro, in vivo and PCR assays for the identification of adventitious viruses in production cells has a limited range of detection. While Next Generation Sequencing (NGS) has a broader breadth of detection, it is unable to differentiate sequences from replicating viruses versus background inert sequences. In order to improve NGS specificity, we have designed a new NGS approach which targets subsets of viral RNAs only synthesized during cell infection. In order to evaluate the performance of this approach for detecting low levels of adventitious viruses, we selected two difficult virus/cell systems. This included B95-8 cells persistently infected by Human herpesvirus 4 (HHV-4) and serially diluted into HHV-4 negative Ramos cells and Madin-Darby bovine kidney cells with an early infection produced via a low dose of Bovine viral diarrhea virus. We demonstrated that the sensitivity of our RNA NGS approach was equivalent to targeted PCR with an increased specificity for the detection of viral infection. We were also able to identify a previously undetected Murine Leukemia Virus contaminant in Ramos cells. Based on these results, we conclude that this new RNA NGS approach is suitable for conducting viral safety evaluations of cells.
目前用于鉴定生产细胞中潜在病毒的体外、体内和聚合酶链反应(PCR)检测方法组合的检测范围有限。虽然下一代测序(NGS)具有更广泛的检测范围,但它无法区分来自复制病毒的序列与背景惰性序列。为了提高NGS的特异性,我们设计了一种新的NGS方法,该方法仅针对细胞感染期间合成的病毒RNA子集。为了评估该方法检测低水平潜在病毒的性能,我们选择了两个具有挑战性的病毒/细胞系统。这包括被人类疱疹病毒4型(HHV-4)持续感染的B95-8细胞,并将其连续稀释到HHV-4阴性的拉莫斯细胞和经低剂量牛病毒性腹泻病毒早期感染的马-达二氏牛肾细胞中。我们证明,我们的RNA NGS方法的灵敏度与靶向PCR相当,且在检测病毒感染方面具有更高的特异性。我们还能够在拉莫斯细胞中鉴定出一种先前未检测到的鼠白血病病毒污染物。基于这些结果,我们得出结论,这种新的RNA NGS方法适用于进行细胞的病毒安全性评估。
