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基于马铃薯X病毒(PVX)在体外培养物中重组绿色荧光蛋白(GFP)的长期瞬时表达

Long-Term Potato Virus X (PVX)-Based Transient Expression of Recombinant GFP Protein in Culture In Vitro.

作者信息

Sindarovska Yana, Kuchuk Mykola

机构信息

Department of Genetic Engineering, Institute of Cell Biology and Genetic Engineering of NAS of Ukraine, 148 Akad. D.K. Zabolotnogo Str., 03143 Kyiv, Ukraine.

出版信息

Plants (Basel). 2021 Oct 15;10(10):2187. doi: 10.3390/plants10102187.

Abstract

Plant molecular farming has a great potential to produce valuable proteins. Transient expression technology provides high yields of recombinant proteins in greenhouse-grown plants, but every plant must be artificially agroinfiltrated, and open greenhouse systems are less controlled. Here, we propose to propagate agrobacteria-free plants with high-efficient long-term self-replicated transient gene expression in a well-controlled closed in vitro system. plant tissue culture in vitro, with transient expression of recombinant GFP, was obtained through shoot induction from leaf explants infected by a PVX-based vector. The transient expression occurs in new tissues and regenerants due to the natural systemic distribution of viral RNA carrying the target gene. Gene silencing was delayed in plants grown in vitro, and GFP was detected in plants for five to six months. Agrobacteria-free, GFP-expressing plants can be micropropagated in vitro (avoiding an agroinfiltration step), "rejuvenated" through regeneration (maintaining culture for years), or transferred in soil. The mean GFP in the regenerants was 18% of the total soluble proteins (TSP) (0.52 mg/g of fresh leaf weight (FW). The highest value reached 47% TSP (2 mg/g FW). This study proposes a new method for recombinant protein production combining the advantages of transient expression technology and closed cultural systems.

摘要

植物分子农业在生产有价值的蛋白质方面具有巨大潜力。瞬时表达技术可在温室种植的植物中高产重组蛋白,但每株植物都必须进行人工农杆菌浸润,且开放的温室系统较难控制。在此,我们提议在一个控制良好的封闭体外系统中繁殖无农杆菌的植物,使其具有高效的长期自我复制瞬时基因表达。通过基于PVX的载体感染叶片外植体诱导芽再生,获得了体外植物组织培养物,并伴有重组绿色荧光蛋白(GFP)的瞬时表达。由于携带靶基因的病毒RNA的自然系统分布,瞬时表达发生在新组织和再生植株中。体外培养的植物中基因沉默延迟,GFP在植物中可检测到五到六个月。无农杆菌、表达GFP的植物可在体外进行微繁殖(避免农杆菌浸润步骤),通过再生“复壮”(保持培养数年),或转移到土壤中。再生植株中GFP的平均含量为总可溶性蛋白(TSP)的18%(0.52毫克/克鲜叶重(FW)),最高值达到47%TSP(2毫克/克FW)。本研究提出了一种结合瞬时表达技术和封闭培养系统优势的重组蛋白生产新方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1001/8537016/0d30152e7f98/plants-10-02187-g001.jpg

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