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一种完全由非模板、化学合成 DNA 片段衍生而来的杆状病毒表达载体。

A Baculovirus Expression Vector Derived Entirely from Non-Templated, Chemically Synthesized DNA Parts.

机构信息

Stylus Medicine, Inc., 200 Berkeley St., Boston, MA 02116, USA.

Voyager Therapeutics, 64 Sidney St., Cambridge, MA 02139, USA.

出版信息

Viruses. 2023 Sep 23;15(10):1981. doi: 10.3390/v15101981.

Abstract

Baculovirus expression system1s are a widely used tool in recombinant protein and biologics production. To enable the possibility of genome modifications unconstrained through low-throughput and bespoke classical genome manipulation techniques, we set out to construct a baculovirus vector (>130 kb dsDNA) built from modular, chemically synthesized DNA parts. We constructed a synthetic version of multiple nucleopolyhedrovirus (MNPV) through two steps of hierarchical Golden Gate assembly. Over 140 restriction endonuclease sites were removed to enable the discrimination of the synthetic genome from native baculovirus genomes. A head-to-head comparison of our modular, synthetic MNPV genome with native baculovirus vectors showed no significant difference in baculovirus growth kinetics or recombinant adeno-associated virus production-suggesting that neither baculovirus replication nor very-late gene expression were compromised by our design or assembly method. With unprecedented control over the MNPV genome at the single-nucleotide level, we hope to ambitiously explore novel MNPV vectors streamlined for biologics production and development.

摘要

杆状病毒表达系统 1 是重组蛋白和生物制剂生产中广泛使用的工具。为了能够进行不受低通量和定制化经典基因组操作技术限制的基因组修饰,我们着手构建一种由模块化、化学合成 DNA 片段组成的杆状病毒载体(>130kb dsDNA)。我们通过两步层次 Golden Gate 组装构建了一种多角体核型多角体病毒 (MNPV) 的合成版本。为了能够区分合成基因组和天然杆状病毒基因组,我们去除了超过 140 个限制酶切位点。我们的模块化、合成的 MNPV 基因组与天然杆状病毒载体的头对头比较表明,杆状病毒生长动力学或重组腺相关病毒生产没有明显差异——这表明我们的设计或组装方法既没有损害杆状病毒复制,也没有损害晚期基因表达。通过在单核苷酸水平上对 MNPV 基因组进行前所未有的控制,我们希望雄心勃勃地探索新型 MNPV 载体,使其简化生物制剂的生产和开发。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7949/10612064/3ad04b4ebd5d/viruses-15-01981-g001.jpg

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