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一种特定的顺式发夹状核酶促进基于烟草花叶病毒的DNA载体在烟草原生质体中的感染。

A specific cis-hairpin ribozyme facilitates infection of a TMV-based DNA vector in tobacco protoplasts.

作者信息

Wu Ligang, Fan Jihua, Jiang Lubin, Wang Hui, Song Rentao, Zhang Qingqi, Zhu Huihui, Li Ning, Liu Zhixue, Xu Zhengkai

机构信息

Institute of Plant Physiology and Ecology, Shanghai Institutes for Biological Sciences, The Chinese Academy of Sciences, 300 Fenglin Road, Shanghai 200032, China.

出版信息

J Virol Methods. 2003 Aug;111(2):101-9. doi: 10.1016/s0166-0934(03)00153-8.

Abstract

The effect of a specific cis-hairpin ribozyme on TMV-based vectors in the infection of tobacco protoplasts was studied. Vectors contained full-length TMV genome cDNA linked to a T7 promoter or a CaMV 35S promoter at the 5'-end and an NOS gene polyadenylation signal at the 3'-end. The coat protein (CP) gene was replaced with the green fluorescent protein (GFPuv) gene allowing quantification of protoplast infection. In plasmids pTMVGFPRIB (T7-driven) and pSTMVGFPRIB (CaMV 35S-driven), the cDNA fragment of the cis-hairpin ribozyme (designed to specifically cleave the transcripts immediately downstream of the 3'-terminus of TMV RNA) was inserted between the 3'-terminus of TMV genome and NOS sequence. The in vitro transcript TMVGFPRIB was three- to fivefold more infectious than the control TMVGFPNOS. Northern blot analysis indicated that the 3'-terminal non-viral sequence had been cleaved from the in vitro transcripts by the cis-hairpin ribozyme soon after in vitro transcription. pSTMVGFPRIB and pSTMVGFPNOS plasmid DNAs were, as expected, less infectious than their in vitro transcript counterparts. However, pSTMVGFPRIB was somewhat more infectious than pSTMVGFPNOS. Northern blot analysis indicated that pSTMVGFPRIB synthesized more genomic and sub-genomic RNAs in the protoplasts. The significant increase in infectivity and viral RNA synthesis is due to the specific activity of the cis-hairpin ribozyme in vivo. Therefore, the cis-hairpin ribozyme described here may improve TMV-based vectors in the expression of foreign protein in plants.

摘要

研究了一种特定的顺式发夹状核酶对基于烟草花叶病毒(TMV)的载体感染烟草原生质体的影响。载体包含在5'端与T7启动子或花椰菜花叶病毒(CaMV)35S启动子相连的全长TMV基因组cDNA,以及在3'端的NOS基因聚腺苷酸化信号。外壳蛋白(CP)基因被绿色荧光蛋白(GFPuv)基因取代,从而能够对原生质体感染进行定量分析。在质粒pTMVGFPRIB(T7驱动)和pSTMVGFPRIB(CaMV 35S驱动)中,顺式发夹状核酶的cDNA片段(设计用于特异性切割TMV RNA 3'末端下游的转录本)插入到TMV基因组的3'末端和NOS序列之间。体外转录本TMVGFPRIB的感染性比对照TMVGFPNOS高3至5倍。Northern印迹分析表明,体外转录后不久,顺式发夹状核酶就从体外转录本中切割掉了3'末端的非病毒序列。正如预期的那样,pSTMVGFPRIB和pSTMVGFPNOS质粒DNA的感染性低于它们的体外转录本对应物。然而,pSTMVGFPRIB的感染性略高于pSTMVGFPNOS。Northern印迹分析表明,pSTMVGFPRIB在原生质体中合成了更多的基因组RNA和亚基因组RNA。感染性和病毒RNA合成的显著增加归因于顺式发夹状核酶在体内的特异性活性。因此,本文所述的顺式发夹状核酶可能会改进基于TMV的载体在植物中表达外源蛋白的能力。

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