fusion cell culture 中文意思是什麼
fusion cell culture
解釋
融合細胞培養-
This paper introduced the application of biotechnology in rice genetics and breeding, including tissue culture, cell mutants selection, protoplast fusion, apomixis, molecular mark assisted breeding and genic transformation
簡要綜述了生物技術在水稻遺傳育種中的應用,主要包括組織培養、細胞突變體的篩選、原生質體融合、無融合生殖以及分子標記輔助育種和轉基因技術等方面。 -
Different from mammals, the early embryos of fish can not be preserved for the long period at the very low temperature ( - 196 ). therefore, three methods were usually applied to cryogenic preservation of the fine and rare species of fish : 1 ) perserving fish spermatozoon in cryogenic condition. researchers have had systematically studied on this technique for many years, and this technique has been utilized in application and made a lot of effects ; 2 ) combining with the techniques of cell engineering ( nuclear transplantation and electric fusion etc. ), and through the process of culturing histiocyte of fish, cryopreservation and re - culture after thawing, carrying out somatic cell breeding of fish. the past studies showed that the nucleolus of somatic cells of fish have totipotency
多年來,國內外學者對各種魚類精液的冷凍保存進行了大量的系統研究,目前這項技術已達到實用水平,並日益發揮作用;二是對魚類培養的組織細胞冷凍保存,通過魚類細胞的培養、超低溫凍存、解凍后再培養過程,結合細胞工程技術(如核移植、電融合等)進行體細胞育種;大量的研究結果表明魚類體細胞核具有發育的全能性,隨著細胞培養技術、細胞工程技術日益發展成熟,完全具備實現魚類物種種質長期保存的理論基礎和技術條件。 -
This study we acquired the coding region of hcv ns5b gene by pcr of hcv full length genome and construct the recombinant plasmid pegep n3 - ns5b ; with the different concentration of g418 in the culture medium, we think the selection concentration of g418 for hepg2 cell is 800 g / ml ; the recombinant plasmid was transfected into hepg2 cell by lipofectamine2000 cells containing stable transformants were selected by the ability of resistance to g418 and isolated with the limited dilution. the stably transfected cell line expressing ns5b - egfp fusion protein was obtained by the detection under fluorescence microscope and rt - pcr
本研究首先從hcv基因組中擴增出nssb基因,構建了nssb基因與報告分子egfp (增強型綠色熒光蛋白)基因的融合基因真核表達質粒pegfpn30 ;通過含有不同g418濃度梯度的培養液培養hepgz細胞,確定了篩選用g4181作濃度為800pg ml ;利用脂質體法將該重組質粒轉染hepgz細胞,經過有限稀釋法和g4壓力選擇,應用熒光顯微鏡和rtpcr檢測,獲得可穩定表達nssbegfp融合蛋白的hepgz細胞克隆。
分享友人