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Establishing elements of a synthetic biology platform for Vaccinia virus production: BioBrick™ design serum-free virus production and microcarrier-based cultivation of CV-1 cells

机译：建立用于牛痘病毒生产的合成生物学平台的要素：BioBrick™设计无血清病毒生产和基于微载体的CV-1细胞培养

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Vaccinia virus (VACV) is an established vector for vaccination and is beginning to prove effective as an oncolytic agent. Industrial production of VACV stands to benefit in future from advances made by synthetic biology in genome engineering and standardisation. The CV-1 cell line can be used for VACV propagation and has been used extensively with the CRISPR/Cas9 system for making precise edits of the VACV genome. Here we take first steps toward establishing a scalable synthetic biology platform for VACV production with CV-1 cells featuring standardised biological tools and serum free cell cultivation. We propose a new BioBrick™ plasmid backbone format for inserting transgenes into VACV. We then test the performance of CV-1 cells in propagation of a conventional recombinant Lister strain VACV, VACVL-15 RFP, in a serum-free process. CV-1 cells grown in 5% foetal bovine serum (FBS) Dulbecco’s Modified Eagle Medium (DMEM) were adapted to growth in OptiPRO and VP-SFM brands of serum-free media. Specific growth rates of 0.047 h⁻¹ and 0.044 h⁻¹ were observed for cells adapted to OptiPRO and VP-SFM respectively, compared to 0.035 h⁻¹ in 5% FBS DMEM. Cells adapted to OptiPRO and to 5% FBS DMEM achieved recovery ratios of over 96%, an indication of their robustness to cryopreservation. Cells adapted to VP-SFM showed a recovery ratio of 82%. Virus productivity in static culture, measured as plaque forming units (PFU) per propagator cell, was 75 PFU/cell for cells in 5% FBS DMEM. VP-SFM and OptiPRO adaptation increased VACV production to 150 PFU/cell and 350 PFU/cell respectively. Boosted PFU/cell from OptiPRO-adapted cells persisted when 5% FBS DMEM or OptiPRO medium was observed during the infection step and when titre was measured using cells adapted to 5% FBS DMEM or OptiPRO medium. Finally, OptiPRO-adapted CV-1 cells were successfully cultivated using Cytodex-1 microcarriers to inform future scale up studies.

机译：牛痘病毒（VACV）是已建立的疫苗接种载体，并已开始证明它是有效的溶瘤剂。 VACV的工业生产将受益于合成生物学在基因组工程和标准化方面的进步。 CV-1细胞系可用于VACV繁殖，已与CRISPR / Cas9系统广泛用于对VACV基因组进行精确编辑。在这里，我们朝着建立可扩展的合成生物学平台迈出第一步，该平台可利用具有标准化生物学工具和无血清细胞培养功能的CV-1细胞生产VACV。我们提出了一种新的BioBrick™质粒主链形式，用于将转基因插入VACV。然后，我们在无血清的过程中测试了常规重组李斯特菌VACV，VACVL-15 RFP繁殖中CV-1细胞的性能。在5％胎牛血清（FBS）Dulbecco的改良Eagle培养基（DMEM）中生长的CV-1细胞适合在无血清培养基的OptiPRO和VP-SFM品牌中生长。与Opti35和VP-SFM相适应的细胞分别观察到0.047 h ^{-1 和0.044 h ^{-1 的比生长速率，而0.035 h ^{-1 ^{-1 < / sup>在5％FBS DMEM中。适应OptiPRO和5％FBS DMEM的细胞实现了超过96％的回收率，这表明它们对冷冻保存的坚固性。适应VP-SFM的细胞的回收率为82％。静态培养中的病毒生产率（以每个繁殖细胞的噬斑形成单位（PFU）衡量）对于5％FBS DMEM中的细胞为75 PFU /细胞。 VP-SFM和OptiPRO的适应性将VACV产量分别提高到150 PFU /单元和350 PFU /单元。当在感染步骤中观察到5％FBS DMEM或OptiPRO培养基时，以及使用适应5％FBS DMEM或OptiPRO培养基的细胞测定滴度时，来自OptiPRO适应细胞的升压PFU /细胞持续存在。最后，使用Cytodex-1微载体成功培养了适应OptiPRO的CV-1细胞，为将来的大规模研究提供了信息。}}}}

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期刊名称 Heliyon
作者
Shuchang Liu; Ludmila Ruban; Yaohe Wang; Yuhong Zhou; Darren N. Nesbeth;
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年(卷),期 2017(3),2
年度 2017
页码 e00238
总页数 20
原文格式 PDF
正文语种
中图分类
关键词
Biological sciences Biochemistry Bioengineering Cell biology Microbiology History;

机译：生物科学;生物化学;生物工程;细胞生物学;微生物学历史;

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7. Establishing elements of a synthetic biology platform for Vaccinia virus production: BioBrick™ design, serum-free virus production and microcarrier-based cultivation of CV-1 cells [O] . Shuchang Liu, Ludmila Ruban, Yaohe Wang, 2017

机译：建立痘苗病毒生产合成生物学平台的要素：BioBrick™设计，无血清病毒生产和基于微载体的CV-1细胞培养

Establishing elements of a synthetic biology platform for Vaccinia virus production: BioBrick™ design serum-free virus production and microcarrier-based cultivation of CV-1 cells

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