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文昌鱼GFP基因的鉴定及表达分析
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作者 徐炜 李伟业 王义权 《Zoological Research》 CAS CSCD 北大核心 2012年第3期304-313,共10页
近年在隶属头索动物亚门的文昌鱼体内发现有内源性绿色荧光蛋白存在,并发现文昌鱼荧光蛋白的发光现象在不同发育时期以及个体间有较大的差异。为了进一步揭示GFP基因在文昌鱼中的进化模式,探索其可能执行的功能,该文首先对白氏文昌鱼(Br... 近年在隶属头索动物亚门的文昌鱼体内发现有内源性绿色荧光蛋白存在,并发现文昌鱼荧光蛋白的发光现象在不同发育时期以及个体间有较大的差异。为了进一步揭示GFP基因在文昌鱼中的进化模式,探索其可能执行的功能,该文首先对白氏文昌鱼(Branchiostoma belcheri)GFP基因作了全面鉴定,并对其不同发育阶段胚胎及成体不同区域中的荧光信号进行了实时观察记录,进而对GFP基因在绿色荧光表达强烈的两个特定时期做了绝对定量检测。研究结果表明,文昌鱼基因组中至少有12个内源性GFP基因,在个体发育的不同时期,内源性荧光出现的位置有所变化,而且在变态后的个体之间出现荧光的情况差异较大,荧光蛋白基因的表达由多个GFP同源基因共同参与,这些基因在不同的发育时期表达量有较大的差异,提示不同的GFP基因在特定发育阶段可能行使各自的功能。 展开更多
关键词 文昌鱼 gfp 基因克隆 表达
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Identification of neutral genome integration sites with high expression and high integration efficiency in Fusarium venenatum TB01
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作者 Sheng Tong Kexin An +4 位作者 Wuxi Chen Mengdan Chai Yuanxia Sun Qinhong Wang Demao Li 《Synthetic and Systems Biotechnology》 SCIE CSCD 2023年第1期141-147,共7页
CRISPR/Cas9-mediated homology-directed recombination is an efficient method to express target genes.Based on the above method,providing ideal neutral integration sites can ensure the reliable,stable,and high expressio... CRISPR/Cas9-mediated homology-directed recombination is an efficient method to express target genes.Based on the above method,providing ideal neutral integration sites can ensure the reliable,stable,and high expression of target genes.In this study,we obtained a fluorescent transformant with neutral integration and high expression of the GFP expression cassette from the constructed GFP expression library and named strain FS.The integration site mapped at 4886 bp upstream of the gene FVRRES_00686 was identified in strain FS based on a Y-shaped adaptor-dependent extension,and the sequence containing 600 bp upstream and downstream of this site was selected as the candidate region for designing sgRNAs(Sites)for CRISPR/Cas9-mediated homology-directed recombination.PCR analysis showed that the integration efficiency of CRISPR/Cas9-mediated integration of target genes in designed sites reached 100%.Further expression stability and applicability analysis revealed that the integration of the target gene into the above designed sites can be stably inherited and expressed and has no negative effect on the growth of F.venenatum TB01.These results indicate the above designed neutral sites have the potential to accelerate the development of F.venenatum TB01 through overexpression of target genes in metabolic engineering. 展开更多
关键词 gfp expression library Neutral integration site Y-shaped adaptor-dependent extension CRISPR/Cas9 Fusarium venenatum
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