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国家自然科学基金(30170457)

作品数:3 被引量:17H指数:3
相关作者:李明王幼群刘国琴姜世玲更多>>
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基因转录后沉默信号可以在拟南芥嫁接体内快速双向传递被引量:9
2006年
RNA干扰(RNAi)是引起生物体基因转录后沉默的新技术之一,已成功用于基因功能研究.利用拟南芥动蛋白异型体KatB和KatC两个基因上共有的一段同源编码序列(168bp)构建了能导致目标基因KatB和KatC双基因转录后沉默的DEX(dexamethazone)诱导性RNAi载体.RT-PCR和Northernblot结果显示,转基因拟南芥纯合体植株(简称RNAi型植株)经DEX诱导后,KatB和KatC的mRNA逐渐减少,表明这两个基因发生了转录后沉默作用.用改进后的简易方法将RNAi型与野生型拟南芥植株进行高效率嫁接,对砧木和接穗中目标基因mRNA变化进行了半定量RT-PCR检测.结果表明,无论用RNAi型植株作为砧木或接穗,DEX诱导产生的基因沉默信号均能导致相应野生型接穗或砧木中KatB和KatCmRNA的减少,说明基因转录后沉默信号可以通过嫁接面在拟南芥体内双向传递;与已报道的基因沉默信号在烟草嫁接体内传递速度相比,拟南芥基因沉默信号的传递更为迅速.
李明姜世玲王幼群刘国琴
关键词:拟南芥RNAI嫁接
Soluble expression and characterization of a GFP-fused pea actin isoform (PEAc1)被引量:3
2004年
A pea actin isoform PEAc1 with green fluorescent protein (GFP) fusion to its C-terminus and His-tag to its N- terminus, was expressed in prokaryotic cells in soluble form, and highly purified with Ni-Chelating SepharoseTM Fast Flow column. The purified fusion protein (PEAc1-GFP) efficiently inhibited DNase I activities before polymerization, and activated the myosin Mg-ATPase activities after polymerization. The PEAc1-GFP also polymerized into green fluorescent filamentous structures with a critical concentration of 0.75 μM. These filamentous structures were labeled by TRITC-phalloidin, a specific agent for staining actin microfilaments, and identified as having 9 nm diameters by negative staining. These results indicated that PEAc1 preserved the essential characteristics of actin even with His-tag and GFP fusion, suggesting a promising potential to use GFP fusion protein in obtainning soluble plant actin isoform to analyze its physical and biochemical properties in vitro. The PEAc1-GFP was also expressed in tobacco BY2 cells, which offers a new pathway for further studying its distribution and function in vivo.
Ai Xiao LIUShao Bin ZHANGXiao Jing XUDong Tao RENGuo Qin LIU
关键词:POLYMERIZATION
AtKP1, a kinesin-like protein, mainly localizes to mitochondria in Arabidopsis thaliana被引量:5
2005年
Kinesins and kinesin-like proteins (KLPs) constitute a large family of microtubule-based motors that play important roles in many fundamental cellular and developmental processes. To date, a number of kinesins or KLPs have been identified in plants including Arabidopsis thaliana. Here, a polyclonal antibody against AtKP1 (kinesin-like protein 1 in A.thaliana) was raised by injection the expressed AtKP1 specific C-terminal polypeptides in rabbits, and immunoblot analysis was conducted with the affinity-purified anti-AtKP1 antibody. The results indicated that this antibody recognized the AtKP1 fusion proteins expressed in E. coli and proteins of ~125 kDa in the soluble fractions of Arabidopsis extracts. The molecular weight was consistent with the calculated molecular weight based on deduced amino acids sequence of AtKP1. To acquire the subcellular localization of the protein, AtKP1 in Arabidopsis root cells was observed by indirect immunofluorescence microscopy. AtKP1 was localized to particle-like organelles in interphase or dividing cells, but not to mitotic microtubule arrays. Relatively more AtKP1 was found in isolated mitochondria fraction on immunoblot of the subcellular fractions. The AtKP1 protein could not be released following a 0.6 M KI washing,indicating that AtKP1 is tightly bind to mitochondria and might function associated with this kind of organelles.
Cheng Zhi NI Hai Qing WANG Tao XU Zhe QU Guo Qin LIU
关键词:线粒体基因表达细胞功能
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