植物RNA病毒载体构建策略

作为对传统的植物转化载体的补充,植物ＲＮＡ病毒载体具有受体植物广泛,且转化需要的时间短,特别适宜于大量表达外源基因．虽然外源基因的稳定性存在一定的问题,但大量的事例说明,作为一种新型的外源基因在植物中表达的载体,它具有其独到的特点．本文就最新利用ＲＮＡ病毒转化植物的报道进行了综述     

植物病毒载体系统研究进展

植物病毒基因组小,易于进行遗传操作而且感染过程简单,因而利用植物病毒载体表达外源基因在生物技术领域具有潜在的应用优势。本文主要介绍了抗原展示系统和多肽表达系统,并分别列举一些植物病毒作为表达载体的研究进展情况以及应用前景。     

外源基因在转基因植物中的表达

外源基因在转基因植物中的表达王忠华夏英武舒庆尧（浙江农业大学核农所,杭州３１００２９）近十几年来,人们通过各种方法将外源基因导入植物体内产生许多转基因植物,包括水稻、小麦、棉花、烟草、大豆、番茄、马铃薯等重要粮食作物和经济作物。据不完全统计目前已获得...     

外源基因在叶绿体表达系统中高效表达研究进展

综述叶绿体表达系统的特点,转化方法,同质化研究及提高外源基因在叶绿体基因组中表达水平的研究状况。     

植物病毒表达载体研究进展

利用ＤＮＡ或ＲＮＡ植物病毒作载体表达外源蛋白是几年发展较快的一种新的遗传转化方式,它具有以下几个优点,表达量大,表达速度快,地进行基因操作和接种以及适用对象广泛。已发展的四种载体构建策略包括：基因取代,基因插入,融合抗原和基因互补。植物病毒表达载体可以用于基因的重组、病毒的移动和基因功能的检测等基础性研究,也可用于商业上表达多种药用蛋白或疫苗,植物病毒表达载体的稳定性主要取决于存在同源序列而引起的     

植物病毒表达载体研究进展

利用DNA或RNA植物病毒作载体表达外源蛋白是近几年发展较快的一种新的遗传转化方式,它具有以下几个优点:表达量大,表达速度快,易于进行基因操作和接种以及适用对象广泛。已发展的四种载体构建策略包括:基因取代,基因插入,融合抗原和基因互补。植物病毒表达载体可以用于基因的重组、病毒的移动和基因功能的检测等基础性研究,也可用于商业上表达多种药用蛋白或疫苗。植物病毒表达载体的稳定性主要取决于存在同源序列而引起的基因重组。本文还对病毒载体的生物安全性进行了讨论。     

转基因植物中外源基因及其表达产物转移的途径

随着转基因植物商品化应用的增多,全面了解转基因植物潜在的生态风险性尤为重要。国内外对“转基因植物中外源基因向野生亲缘物种漂移的可能性”、“昆虫对抗虫转基因植物的耐受性”以及“转基因植物对生物多样性的潜在影响”等问题已进行了广泛研究。对转基因植物中外源基因及其表达产物的几种可能转移途径作了概述。着重介绍了“经花粉散布或与野生亲缘物种杂交等途径引起的外源基因转移”以及“转基因植物对土壤生态系统的影响”等方面的研究情况。此外,还对“鉴定外源基因及其表达产物存在的方法”进行了简要探讨。     

水稻草矮病毒NS6基因在大肠杆菌中的表达及植物表达载体的构建

Large amount of disease-specific protein(SP) accumulated in the rice plant cells infected by rice grassy stunt virus(RGSV). It was deduced that the protein was encoded by NS6 gene on genomic vRNA6 and thus referred to as NS6 protein.But its function is unknown. In an effort to prove the above deduction and to elucidate the function of NS6 protein of RGSV, we constructed a bacterial expression plasmid pGTNS6 producing a fusion protein of glutathione S-transferase (GST) and NS6 protein, and a plant expression vector pCBTNSv6 containing NS6 gene. A recombinant plasmid pTNSv 6 containing the coding region of NS6 gene and the non-coding region at its 5' terminus, cloned by RT-PCR from purified RNAs of Shaxian isolate of RGSV, was used as the start point. Western blot analysis showed that the fusion protein reacted strongly with antisera raised against RGSV-SP, which served as evidence of the deduction.EHA105 of Agrobacterium tumefasciens containing pCBTNSv6 has been obtained and the transformation of rice is underway.     

利用病毒载体在烟草中瞬时表达融合HBsAg基因

利用马铃薯PVX病毒载体构建了外源人工融合乙肝表面抗原HBsAg基因的表达载体,在烟草中利用农杆菌介导进行瞬时表达,以快速鉴定外源基因瞬时表达的状况以及重组蛋白的免疫活性。利用PCR技术从含有人工融合HBsAg基因的表达载体中分别扩增出LP PreS1 PreS2 S、PreS1 PreS2 S、PreS2 S序列,将其分别与PVX病毒载体pgR106连接,构建成PVX-LP、PVX-S1和PVX-S2等3个转化载体,并将此载体导入农杆菌菌株GV3101中用于侵染烟草植株叶片。感染植株经RT-PCR、RNA Dot blotting和HBsAg蛋白的ELISA检测显示,3个人工融合的HBsAg基因均可在植物体内得到转录,翻译成具有活性的蛋白。结果表明,外源融合HB-sAg基因经过植物病毒载体瞬时表达系统可以在植物系统中正常转录和翻译。     

A plant virus vector for systemic expression of foreign genes in cereals

Inserts bearing the coding sequences of NPT II and beta-glucuronidase (GUS) were placed between the nuclear inclusion b (NIb) and coat protein (CP) domains of the wheat streak mosaic virus (WSMV) polyprotein ORF. The WSMV NIb-CP junction containing the nuclear inclusion a (NIa) protease cleavage site was duplicated, permitting excision of foreign protein domains from the viral polyprotein. Wheat, barley, oat and maize seedlings supported systemic infection of WSMV bearing NPT II. The NPT II insert was stable for at least 18-30 days post-inoculation and had little effect on WSMV CP accumulation. Histochemical assays indicated the presence of functional GUS protein in systemically infected wheat and barley plants inoculated with WSMV bearing GUS. The GUS constructs had greatly reduced virulence on both oat and maize. RT-PCR indicated that the GUS insert was subject to deletion, particularly when expressed as a GUS-NIb protein fusion. Both reporter genes were expressed in wheat roots at levels comparable to those observed in leaves. These results clearly demonstrate the utility of WSMV as a transient gene expression vector for grass species, including two important grain crops, wheat and maize. The results further indicate that both host species and the nature of inserted sequences affect the stability and expression of foreign genes delivered by engineered virus genomes.     

口蹄疫病毒VP1高效植物表达载体构建及鉴定

采用高保真PCR方法从pGEM-VP1-T质粒扩出VP1基因,定向克隆到含DHA的融合中间载体pUC18-DHA,得到pUC18-VP1-DHA,经测序证实核酸序列正确后,再亚克隆到转化范围广,转化效率高,且含有双增强子的高效植物双元表达载体pGreen0029-GFP上,获得含VP1融合DHA基因的植物双元表达载体pGreen0029-VP1-DHA,采用电击法将含VP1的植物表达载体转入根癌农杆菌G3101中,获得了含VP1基因的双元植物表达载体,为下一步的广范围转基因植物表达研究奠定了基础。     

香蕉花叶病毒外壳蛋白基因克隆及表达载体的构建

从海南大田感染香蕉花叶病的香蕉叶片 ,获得香蕉花叶病毒 ,提纯其 RNA,在 AMV反转录酶作用下合成 c DNA第一链 ,经 PCR扩增 ,获得一约 70 0 bp的 DNA片段 ,测序结果显示所克隆的 DNA片段包含一完整的香蕉花叶病毒株系 ( CMV-BHI)外壳蛋白基因 ,长度为 6 5 7bp,然后将此 DNA片段 ,分别克隆到p BI1 2 1和 p KHG4质粒 ,构成两个含 Ca MV35 s启动子 ( 5 '-端 )、NOS终止子 ( 3'-端 )和分别含 NPT 标记基因和 NPT 及 HPT标记基因的植物表达载体 ( p TBB和 p TBK)。然后用 p AHC1 8中的 UBI promoter换下p BI1 2 1的 Ca MV35 s promoter,构成 p BIAH;再用 CMV-BHI外壳蛋白基因换下 p BIAH中 GUS基因 ,构成一含单子叶植物启动子 UBI和 NPT 标记基因的植物表达载体 ( p TBBU)。从而为 CMV-BHI外壳蛋白基因在香蕉中表达打下了基础     

Cauliflower mosaic virus as a gene expression vector for plants

It is possible to replace the CaMV (cauliflower mosaic virus) ORF (open reading frame) II with foreign sequences without interfering with virus viability. Such recom-binants can induce the synthesis of substantial amounts of a foreign protein in infected plants and confer new properties to these plants. However, so far only three genes have been successfully cloned and expressed in this way. The expression mechanism of CaMV demands precise replacement of ORF II and probably certain structural features of the viral 35S RNA, which should not be disturbed by inserted sequences. Since these features are largely unknown, it cannot at present be pre-dicted whether an insert will be tolerated. It is more likely that larger inserts will disturb the viral gene expression mechanism than smaller ones.     

Geminivirus vectors for high-level expression of foreign proteins in plant cells

Bean yellow dwarf virus (BeYDV) is a monopartite geminivirus that can infect dicotyledonous plants. We have developed a high-level expression system that utilizes elements of the replication machinery of this single-stranded DNA virus. The replication initiator protein (Rep) mediates release and replication of a replicon from a DNA construct ("LSL vector") that contains an expression cassette for a gene of interest flanked by cis-acting elements of the virus. We used tobacco NT1 cells and biolistic delivery of plasmid DNA for evaluation of replication and expression of reporter genes contained within an LSL vector. By codelivery of a GUS reporter-LSL vector and a Rep-supplying vector, we obtained up to 40-fold increase in expression levels compared to delivery of the reporter-LSL vectors alone. High-copy replication of the LSL vector was correlated with enhanced expression of GUS. Rep expression using a whole BeYDV clone, a cauliflower mosaic virus 35S promoter driving either genomic rep or an intron-deleted rep gene, or 35S-rep contained in the LSL vector all achieved efficient replication and enhancement of GUS expression. We anticipate that this system can be adapted for use in transgenic plants or plant cell cultures with appropriately regulated expression of Rep, with the potential to greatly increase yield of recombinant proteins.     

Development of the binary vector pTACAtg1 for stable gene expression in plant: Reduction of gene silencing in transgenic plants carrying the target gene with long flanking sequences

Genetic modification in plants helps us to understand molecular mechanisms underlying on plant fitness and to improve profitable crops. However, in transgenic plants, the value of gene expression often varies among plant populations of distinct lines and among generations of identical individuals. This variation is caused by several reasons, such as differences in the chromosome position, repeated sequences, and copy number of the inserted transgene. Developing a state-of-art technology to avoid the variation of gene expression levels including gene silencing has been awaited. Here, we developed a novel binary plasmid (pTACAtg1) that is based on a transformation-competent artificial chromosome (TAC) vector, harboring long genomic DNA fragments on both sides of the cloning sites. As a case study, we cloned the cauliflower mosaic virus 35S promoter:β-glucuronidase (35S:GUS) gene cassettes into the pTACAtg1, and introduced it with long flanking sequences on the pTACAtg1 into the plants. In isolated transgenic plants, the copy number was reduced and the GUS expressions were detected more stably than those in the control plants carrying the insert without flanking regions. In our result, the reduced copy number of a transgene suppressed variation and silencing of its gene expression. The pTACAtg1 vector will be suitable for the production of stable transformants and for expression analyses of a transgene.     

抗旱基因HDCS1的植物表达载体构建

在克隆了二棱大麦第３组ＬＥＡｃＤＮＡ,抗旱基因ＨＤＣＳ１的基因上,将其连接于ｐＢ１１２１的ＣａＭＶ３５Ｓ启动子和ＮＯＳ终止子之间,,构建了ＨＤＣＳ１的植物表达载体ｐＢＨＣ,并进行了ＰＣＲ和酶切鉴定,为进行植物抗旱基因工程研究创造了条件。