种子特异启动子的克隆及植物表达载体构建
충자특이계동자적극륭급식물표체재체구건
Cloning of Seed-specific Promoter and Construction of Plant Transformation Vector
  • 万方数据
    安徽农业科学 안휘농업과학
    JOURNAL OF ANHUI AGRICULTURAL SCIENCES
    2010年 1期 63-67 ,共5页

    张梦晗%谢伟红%曾洪斌%徐超%李宏业%杨维东%刘洁生

    장몽함%사위홍%증홍빈%서초%리굉업%양유동%류길생

    启动子%PCR%基因组步移%绿豆8S球蛋白%种子特异表达载体 啟動子%PCR%基因組步移%綠豆8S毬蛋白%種子特異錶達載體
    계동자%PCR%기인조보이%록두8S구단백%충자특이표체재체
    Promoter%PCR%Genome-walking%Vigna radiate 8S globulin%Seed-specific expression vector
    [目的]启动子是植物基因工程中一个重要工具,对构建植物生物反应器有着重要意义.8S球蛋白是绿豆中含量最丰富的种子贮藏蛋白,因此,其调控序列可能提供了一个很好来源的种子特异性启动子.[方法]通过基因组步移技术克隆了绿豆8S球蛋白a亚基基因8SGα的启动子区域,基因组步移使用的引物根据绿豆8SGα的cDNA序列设计.[结果]通过3轮PCR的扩增,得到了472 bp的上游序列片段,构建了植物双元表达载体pBI-8SGα-GUS.[结论]研究结果可用于转化植物,并于转基因植物中分析启动表达的时空特异性及表达强度,并为植物种子生物反应器提供重要元件.
    [목적]계동자시식물기인공정중일개중요공구,대구건식물생물반응기유착중요의의.8S구단백시록두중함량최봉부적충자저장단백,인차,기조공서렬가능제공료일개흔호래원적충자특이성계동자.[방법]통과기인조보이기술극륭료록두8S구단백a아기기인8SGα적계동자구역,기인조보이사용적인물근거록두8SGα적cDNA서렬설계.[결과]통과3륜PCR적확증,득도료472 bp적상유서렬편단,구건료식물쌍원표체재체pBI-8SGα-GUS.[결론]연구결과가용우전화식물,병우전기인식물중분석계동표체적시공특이성급표체강도,병위식물충자생물반응기제공중요원건.
    [Objective] Promoter is an important tool in plant genetic engineering, which is critical for developing an efficient plant bioreactor. 8S globulin is the most abundant seed storage protein in Vigna radiate, its regulator sequence may provide a good source of seed-specific promoter. [Method]Vigna radiate 8S globulin α subunit promoter sequence was amplified by the method of Genome-walking in accordance with the Vigna radiate 8S globulin α subunit cDNA sequence. [Result]The amplified sequence was cloned into pMD18-T vector, and then transformed into E. coli cells. Resultant plasmid was extracted and subjected to DNA sequencing. The cloned sequence was analyzed by various promoter prediction servers. The sequence was shown to contain a number of key components of seed-specific promoters; suggesting that we have successfully obtained the Vigna radiate 8SGα promoter. [Conclusion]Subsequently, 8SGα was subcloned into plant binary vector pBI121 by replacing CaMV35S promoter upstream of GUS reporter gene with 8SGα promoter, thus providing a basis for investigation of 8SGα promoter function in planta.
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