Simple Low-Cost Production of DNA MS2 Virus-Like Particles As Molecular Diagnostic Controls.

IF 2 Q3 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Michael A Crone, Paul S Freemont
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Abstract

Suitable controls are integral for the validation and continued quality assurance of diagnostic workflows. Plasmids, DNA, or in vitro transcribed RNA are often used to validate novel diagnostic workflows, however, they are poorly representative of clinical samples. RNA phage virus-like particles (VLPs) packaged with exogenous RNA have been used in clinical diagnostics as workflow controls, serving as surrogates for infectious viral particles. Comparable controls for DNA viruses are more challenging to produce, with analogous DNA phages being infectious and packaging of DNA within RNA phages requiring complex purification procedures and expensive chemical linkers. We present a simple and inexpensive method to produce Emesvirus zinderi (MS2) VLPs, packaged with DNA, that makes use of affinity chromatography for purification and enzymatic production of exogenous DNA suitable for packaging. The produced VLPs were packaged with hepatitis B virus DNA and were then quantified using droplet digital PCR and calibrated against the WHO international standard using a commercial assay in an accredited clinical laboratory.

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Abstract Image

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简单低成本生产DNA MS2病毒样颗粒作为分子诊断控制。
适当的控制对于诊断工作流程的验证和持续质量保证是不可或缺的。质粒、DNA或体外转录RNA通常用于验证新的诊断工作流程,然而,它们对临床样品的代表性很差。外源性RNA包装的RNA噬菌体病毒样颗粒(VLPs)已被用于临床诊断,作为工作流程控制,作为感染性病毒颗粒的替代品。DNA病毒的可比对照更具挑战性,因为类似的DNA噬菌体具有传染性,而在RNA噬菌体中包装DNA需要复杂的纯化程序和昂贵的化学连接物。我们提出了一种简单、廉价的方法来生产用DNA包装的Emesvirus zinderi (MS2) VLPs,该方法利用亲和层析纯化和酶促生产适合包装的外源DNA。生产的VLPs用乙型肝炎病毒DNA包装,然后使用液滴数字PCR进行定量,并在经认可的临床实验室使用商业测定法根据世卫组织国际标准进行校准。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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