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重组新城疫病毒的拯救:当前的克隆策略和RNA聚合酶供应系统

Rescue of recombinant Newcastle disease virus: current cloning strategies and RNA polymerase provision systems.

作者信息

Molouki Aidin, Peeters Ben

机构信息

Department of Avian Disease Research and Diagnostic, Razi Vaccine and Serum Research Institute, Karaj, Iran.

Reproductive Biotechnology Research Center, Avicenna Research Institute, ACECR, Tehran, Iran.

出版信息

Arch Virol. 2017 Jan;162(1):1-12. doi: 10.1007/s00705-016-3065-7. Epub 2016 Oct 1.

Abstract

Since the first rescue of a recombinant Newcastle disease virus (rNDV) in the late 1990s, many more rNDVs have been rescued by researchers around the world. Regardless of methodology, the main principle behind rescue of the virus has remained the same, i.e., the formation of a functional replication complex by simultaneously providing the full-length viral RNA and the viral NP, P and L proteins. However, different strategies have been reported for the insertion of the full-length genome into a suitable transcription vector, which remains the most challenging step of the rescue. Moreover, several systems have been published for provision of the DNA-dependent RNA polymerase, which is needed for transcription of viral RNA (vRNA) from the transfected plasmid DNA. The aim of this article is to consolidate all of the current cDNA assembly strategies and transcription systems used in rescue of rNDV in order to attain a better understanding of the advantages and disadvantages of each approach.

摘要

自20世纪90年代末首次拯救重组新城疫病毒(rNDV)以来,世界各地的研究人员已经拯救了更多的rNDV。无论采用何种方法,拯救该病毒背后的主要原理都是相同的,即通过同时提供全长病毒RNA以及病毒核蛋白(NP)、磷蛋白(P)和大蛋白(L)来形成功能性复制复合体。然而,关于将全长基因组插入合适转录载体的方法已有不同报道,这仍然是拯救过程中最具挑战性的步骤。此外,已经发表了几种用于提供依赖DNA的RNA聚合酶的系统,这种酶是从转染的质粒DNA转录病毒RNA(vRNA)所必需的。本文的目的是整合目前在rNDV拯救中使用的所有cDNA组装策略和转录系统,以便更好地了解每种方法的优缺点。

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