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应用农杆菌Ti质粒系统将外源基因转入籼稻细胞研究   总被引:17,自引:0,他引:17  
本文证明经复合酚类化合物预处理的菌株与籼稻培养细胞在普通培养液。特别是在复合诱导培养液(培养过番茄下胚轴切段、胡萝卜细胞及农杆菌的培养滤液)中共培养时,均可发现有较多的细菌附着于水稻细胞表面,并且菌体周围有纤维丝的形成。在复合处理组中,位于pGV3850::1103neo嵌合质粒T-DNA上的NPT Ⅱ基因及NOS基因在籼稻培养细胞中获得了转移与表达。Southern blot分析证明了外源基因整合到受体细胞的基因组中。  相似文献   
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After the cultured cells from Hyoscyamus muticus + Nicotiana tabacum somatic hybridswere cocultivated with different virulent strains of Agrobacterium tumefaciens harboringoctopine- type Ti plasmid or nopaline- type Ti plasmid using the transformation procedurein vitro developed in the present investigation, the TiT- DNA genes were introducedinto the host cells. The onc genes and ocs or nos genes located on TiT- DNA were expres-sed in transformed colonies derived from the cocultivated cells. Although the platingefficiencies of recipient cells were reduced by the agrobacterial treatment, the frequenciesof phytohormone autotrophy ranged from 33.9 to 76 .8% in the cells infected with viru-lent strains in hormone- free conditions, and the frequencies of opine synthase activityamounted to 9.7- 47 .5%. Teratomatous shoots were regenerated from the transformed col-onies. During the course of culture the shoots were no longer to lengthen when theygrew up to 1 -3 cm in length, and they could not be rooted. Follo  相似文献   
3.
携带章鱼碱型Ti质粒和胭脂碱型Ti质粒的根癌农杆菌不同菌株分别与天仙子+烟草体细胞杂种培养细胞经共培养离体转化程序后,Ti T-DNA基因在受体细胞中获得了转移与表达。虽然细菌处理对受体细胞的植板率具有一定的影响,但其激素自主型频率为33.9—76.8%,表现冠瘿碱合成酶活性的频率为9.7—47.5%。从转化细胞克隆再生的苗不易长大、难于生根,且其基部产生大量的次生瘤组织。在这种再生苗的叶组织及次生瘤组织中仍可检测到相应冠瘿碱合成酶的活性。  相似文献   
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Either bacterial attachment or cellulose fibrillar elaboration was hardly observedduring the cocultivation of the cultured suspension cells of Oryza sativa Indica with thestrain C58C1 Rif~r of Agrobacterium tumefaciens that was not specially pretreated. Onthe other hand, quite a lot of Agrobacterium cells were found to adhere to the surface ofcultured rice cells and a number of cellulose fibrils were produced around the specifiedbacteria when phenolics-pretreated bacteria were cocultivated with rice suspension cellsin common culture media, especially in complex culture solutions. The complex culturesolution was the bacterium-free filtrate of hormone-containing MS medium which hadbeen utilized to incubate carrot cells and the newly wounded hypocotyl segments fromtomato and Agrobacterium cells. Detecting experiments demonstrated that both NPT Ⅱ andNOS genes, located on the T-DNA segment of chimaeric plasmid pGV3850 :: 1103neo, weretransferred and expressed in the cultured cells of O. sativa Indica in the  相似文献   
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