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吕亮杰,宿振起,孙丽静,王莉梅,李 辉.利用VIGS技术初步验证WSR1基因功能的研究[J].麦类作物学报,2019,(3):268
利用VIGS技术初步验证WSR1基因功能的研究
Preliminary Validation of WSR1 Gene Function by VIGS Technology
  
DOI:10.7606/j.issn.1009-1041.2019.03.03
中文关键词:  小麦  淀粉合成  转录因子  病毒诱导的基因沉默
英文关键词:Wheat(Triticum aestivum L.)  Starch synthesis  Transcription factor  Virus-induced gene silencing
基金项目:国家转基因生物新品种培育重大专项(2016ZX08002005-002);河北省农林科学院财政专项(F17R0013;2018060303);河北省农林科学院粮油作物研究所开放课题资助项目(LYS2016004)
作者单位
吕亮杰,宿振起,孙丽静,王莉梅,李 辉 (河北省农林科学院粮油作物研究所/河北省作物遗传育种实验室河北石家庄 050035) 
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中文摘要:
      为进一步了解小麦淀粉合成酶转录因子对淀粉合成的影响,以水稻RSR1基因为探针,首先利用同源克隆技术和RACE技术获得了小麦WSR1基因的全长cDNA;生物信息学分析表明,该基因含有AP2保守结构域。随后,以大麦条纹花叶病毒(BSMV)为载体,八氢番茄红素脱氢酶(PDS)基因为指示基因,利用VIGS技术和qRT-PCR技术对WSR1基因的功能进行研究。结果表明,在接种5 d 后,WSR1基因的相对表达量下降到 50%, 25 d后下降到12%;WSR1基因沉默后的冀麦325籽粒内支链淀粉、总淀粉和抗性淀粉含量均较对照显著增加;直链淀粉含量、千粒重较对照极显著增加。以上结果表明WSR1基因负向调控小麦的淀粉合成。
英文摘要:
      To further understand the effect of wheat starch synthase transcription factors on starch synthesis,the riceRSR1 gene was used as the probe to obtain the homologous RSR1 fragment from wheat genome. The full-length cDNA of the wheat WSR1 gene was cloned using RACE technology. The bioinformatics analysis showed that the gene contains an AP2 conserved domain,namely WSR1. The barley stripe mosaic virus(BSMV) was used as the vector,and the phytoene desaturase(PDS) gene was used as the indicator gene. The function of WSR1 gene was studied by virus induced gene silencing(VIGS) and qRT-PCR. The result showed that after five days of inoculation,the relative expression level of WSR1 gene was reduced to 50%,and remained at a relatively low level(about 12%) after 25 days of inoculation. The contents of amylopectin,total starch and resistant starch were much higher in the WSR1-silenced Jimai 325 than that in the control of Jimai 325 without BSMV:WSR1 transformation. The proportion of amylose was increased from 14.47% to 15.60% and the 1 000-grain weight was increased from 43.1 g to 45.8 g. It was demonstrated that the WSR1 gene negatively regulates starch synthesis in wheat.
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