转基因植物生物反应器中存在的问题及解决途径

利用转基因植物作为生物反应器,可以大量生产重组药物蛋白质和工业化酶,但是表达量低、下游处理复杂、糖基化结构改变是植物反应器中经常遇到的困难,这些困难限制了转基因植物的商业化发展。针对这些问题,人们分别采用不同的生物技术策略加以解决。     

谷氨酰胺合成酶基因GS1和GS2的高效表达增强转基因水稻对氮素缺乏的耐性

构建了同时含有胞质谷氨酰胺合成酶(GS1)cDNA和叶绿体谷氨酰胺合成酶(GS2)cDNA的植物表达载体p2GS,通过农杆菌介导法用它们转化了水稻品种"中花10号"的成熟胚愈伤组织,经潮霉素(Hyg)筛选培养及分化再生,获得了抗Hyg的转基因水稻植株.PCR和基因组Southern杂交分析结果证明,GS1和GS2基因均已经整合到转基因水稻的基因组内.Northern杂交实验结果证实,GS1和GS2基因在转基因水稻的转录水平上得到了有效表达.在以0.7 mmol/L的(NH4)2SO4取代了其中氮成分的MS培养基上测试植株生长量,结果表明转基因植株鲜重增长量显著高于对照,证明高效表达GS增强了转基因水稻对土壤氮素缺乏的耐性.     

两种阳离子纳米基因载体及植物基因介导效果的研究

以阳离子聚乙烯亚胺(polyethylenimine, PEI)和壳聚糖(chitosan, CS)作为两种植物基因载体,分别制备了载基因PEI纳米粒(PEI/DNA)和壳聚糖-DNA纳米粒(CS/DNA),并对其形态、粒度分布、包封率、DNA结合的稳定性及纳米颗粒对DNA的保护等方面进行表征.并以GFP基因为报告基因进行植物细胞转染,比较两者转化效率.结果表明PEI/DNA纳米粒稳定性,对DNA的保护以及转染效率等方面均优于壳聚糖-DNA纳米粒.     

Antiporter Gene from Hordum brevisubulatum （Trin.） Link and Its Overexpression in Transgenic Tobaccos

A vacuolar Na^ /H^ antiporter cDNA gene was successfully isolated fromHordeum brevisubulatum (Trin.) Link using the rapid amplification ofcDNA ends (RACE) method. The gene was named HbNHXI and was found to consist of 1 916 bp encoding a predicted polypeptide of 540 amino acids with a conserved amiloride-binding domain. Phylogenetic tree analysis of the Na^ /H^ antiporters showed that the HbNHXI gene shares 55.3%-74.8% similarity with the vacuolar-type Na^ /H^ antiporters. Transgenic tobaccos that contain the HbNHXI gene, integrated by forward insertion into the tobacco genome, were obtained via Agrobacterium tumerfaciens and characterized for the determination of the concentration of Na^ and K^ ions, as well as proline, in the presence of 300 mmol/L NaCl. The T1 transgenic plants showed more tolerance to salt and drought than did wild-type plants. Our data suggest that overexpression of the HbNHXI gene could improve the tolerance of transgenic tobaccos to salt and drought through the function of the vacuolar Na^ /H^ antiporter.     

aroA-In融合基因载体的构建、表达及对烟草的转化

PCR扩增突变的5’-烯醇丙酮酸莽草酸-3-磷酸合成酶(5’-enolpyruvylshikimate-3-phosphate synthetase,EPSPS)cDNA全长序列,插入pLitmus28得到pLEPSPS,进而通过反向PCR在EPSPS235／236aa之间将其打断为无功能的片段。选用人工构建的具有顺式和反式剪接功能的mini型蛋白内含子Ssp DnaB和Rma DnaB,插入被打断的aroA(抗除草剂基因),构建了质粒pLEBC、pLEBT、pLERC和pLERT。将4种重组质粒中的aroA-In(蛋白内含子Intein插入aroA)融合基因插入pET-32得到表达载体pETLEBC、pETLEBT、pETLERC和pETLERT,lPTG诱导后,SDS-PAGE分析显示其能在DE。中有效表达并发生相应的蛋白剪接。将aroA-cis Ssp DnaB和aroA-cis Rma DnaB融合基因分别插入pLYM中进一步构建成植物表达载体,农杆菌叶盘法转化烟草。基因组PCR分析表明融合基因整合入植物核基因组;RT-PCR分析显示其可在高等植物细胞中成功表达。结果说明蛋白内含子基因可以转化高等真核细胞,蛋白剪接技术可应用于高等植物细胞,从而为防止植物转基因扩散提供了一条新的途径。     

胡萝卜HRGP启动子调控GUS基因的某些特点

HRG(hydroxyproline rich glycoproteins)是高等植物细胞壁中一类富含羟脯氨酸的糖蛋白,是植物细胞壁中主要的结构蛋白。早期研究认为其在细胞壁的形成过程中起作用并称之为伸展蛋白(extensin)。在双子叶植物中,HRGP基因以多基因家族形式存在,具有特定的表达模式。许多条件及处理都能引起HRGP表达量的增加,如伤害、真菌感染、病毒感染、乙烯、细胞培养、红光等,同时也受到发育水平的调节。在单子叶植物中,玉米HRGP的表达是在发育水平上受伤害调节的。HRGP基因还具有组织专一性表达的特点。在大豆种子中,HRGP主要存在于种皮的外两层、表皮栅栏组织和滴漏细胞中,属于起支持作用的厚壁组织。在胡萝卜根韧皮部薄壁细胞中HRGP含量最丰富,而在健康的番茄根中     

转基因烟草生产霍乱毒素B亚单位的纯化

提取转基因烟草叶片总蛋白,用经溴化氰活化的Ｓｅｐｈａｒｏｓｅ ４Ｂ偶联有抗ＣＴ ＩｇＧ色谱柱,得到了表达产物ＣＴＢ蛋白质。经ＰＡＧＥ、Ｗｅｓｔｅｒｎ ｂｌｏｔ、琼脂糖免疫扩散和免疫电泳等方法鉴定表明该蛋白与天然ＣＴＢ相同。     

表达尾穗苋凝集素基因的转基因烟草对桃蚜(Myzus persicae)繁殖的影响(英文)

To investigate the possible function of the agglutinin from Amaranthus caudatus L. (ACA) in plant defending against insect pests, ACA cDNA was cloned by RT-PCR and the 5‘ and 3‘ sequences were confirmed by rapid amplification of cDNA ends (RACE). The phloem-specific expression vector of ACA gene, pBCACAc, was constructed based on the plant binary vector pBC438 and transfered into tobacco plants via Agrobacterium-mediated transformation method. Results from PCR and Southern blotting analysis showed that AOA gene was integrated into the genomes of transformed plants and the transgene integration varied from one to four estimated copies per genome. Western blotting analysis indicated that ACA gene was transcribed and translated in the transgenic plants. The bioassay of Myzus persicae Sulzer on detached leaves demonstrated that the 78% transgenic tobacco plants displayed an average aphid-resistant rate of more than 75%. Some apterous progeny of M. persicae were found dead on the resistant plants. These results indicate that ACA gene should be an effective aphid-resistant gene and could be valuable for application in crop breeding for aphid resistance.     

Abiotic Stress Tolerance： From Gene Discovery in Model Organisms to Crop Improvement

Productive and sustainable agriculture necessitates growing plants in sub-optimal environments with less input of precious resources such as fresh water. For a better understanding and rapid improvement of abiotic stress tolerance, it is important to link physiological and biochemical work to molecular studies in genetically tractable model organisms. With the use of several technologies for the discovery of stress tolerance genes and their appropriate alleles, transgenic approaches to improving stress tolerance in crops remarkably parallels breeding principles with a greatly expanded germplasm base and will succeed eventually.