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Cloning and Analysis of Full-Length cDNA of PumNPR1 Gene from Pyrus ussuriensis Maxim 被引量:2
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作者 CHE Daidi FAN Jinping +3 位作者 WANG Jingang XU Ping YANG Tao LIU Shenkui 《Journal of Northeast Agricultural University(English Edition)》 CAS 2008年第2期12-17,共6页
The purpose of this study is to find a new gene resource for the researches of molecular breeding of Rosaceae plants disease-resistance. Pyrus ussuriensis Maxim is used as a starting material to clone the full-length ... The purpose of this study is to find a new gene resource for the researches of molecular breeding of Rosaceae plants disease-resistance. Pyrus ussuriensis Maxim is used as a starting material to clone the full-length cDNA of NPR1(nonexpressor of pathogenesis- related genes 1) which is a key regulator in SA (salicylic acid)-mediated systemic acquired resistance (SAR) by homologous cloning and RACE techniques. The length of the cDNA sequence was 1 767 bp, the ORF was 1 761 bp, it coded 586 amino acids, pi=5.58, the relative molecular weight was 65.009 ku, contained 19 kinds of amino acids, and had full BTB/POZ and ANK domains. Compared the homology of NPR1 gene in GenBank database, the homology with Pyrus pyrifolia, Arabidopsis thaliana, Nicotiana tabacum, Lycopersicon esculentum, Oryza sativa, Helianthus annuus were 98%, 62%, 68%, 65%, 57%, 63%. The homology offunctional area were 99%, 78%, 82%, 79%, 74%, 77%. This NPR1 gene was considered as homologic gene of Pyrus ussuriensis Maxim and named PumNPR1. 展开更多
关键词 Pyrus ussuriensis Maxim npr1 gene cloning RACE
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甘薯NPR1基因半定量RT-PCR检测方法的建立 被引量:8
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作者 陈观水 潘大仁 +3 位作者 周以飞 林生 高丽华 杨志伟 《福建农林大学学报(自然科学版)》 CSCD 北大核心 2007年第1期56-59,共4页
为进一步研究甘薯病原微生物的侵染对甘薯病程相关非表达子1基因(NPR1)表达的影响,以甘薯肌动蛋白(β-ac-tin)基因为内参照基因,提取甘薯叶片总RNA,反转录为cDNA,同批异管对该2个基因进行PCR扩增.通过对循环数的优化和对体系重复性、准... 为进一步研究甘薯病原微生物的侵染对甘薯病程相关非表达子1基因(NPR1)表达的影响,以甘薯肌动蛋白(β-ac-tin)基因为内参照基因,提取甘薯叶片总RNA,反转录为cDNA,同批异管对该2个基因进行PCR扩增.通过对循环数的优化和对体系重复性、准确性的分析,建立了一个稳定、方便的半定量RT-PCR体系. 展开更多
关键词 甘薯 病程相关非表达子1(npr1) 基因表达 半定量RT-PCR
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NPR1多肽抗体的制备和应用 被引量:6
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作者 陈卓 刘家驹 +6 位作者 毕亮 李向阳 胡德禹 于丹丹 王贞超 杨松 宋宝安 《生物技术通报》 CAS CSCD 北大核心 2012年第1期145-150,共6页
根据NCBI GenBank中报道的NPR1一级结构信息,采用Blastn、Blastx、ExPASy和Protean等软件进行序列同源性和抗原性指数分析,获得三段序列特异性较高的多肽,并从中优选一段序列特异性多肽,采用9-氟甲氧羰基固相合成法获得序列特异性最好... 根据NCBI GenBank中报道的NPR1一级结构信息,采用Blastn、Blastx、ExPASy和Protean等软件进行序列同源性和抗原性指数分析,获得三段序列特异性较高的多肽,并从中优选一段序列特异性多肽,采用9-氟甲氧羰基固相合成法获得序列特异性最好的多肽,采用HPLC和LC-MS测定合成多肽的浓度和分子量,试验表明目的多肽纯度达88%、目的多肽分子量为1.92234 kD。采用碳化二亚胺法将多肽与KLH进行偶联获得免疫原Pep-KLH,并将其免疫新西兰大白兔以获得抗血清和多克隆抗体,采用ELISA和Western blotting测定其效价和特异性,经ELISA检测表明抗血清和多克隆抗体可与Pep发生特异性免疫反应,经Western blotting试验表明抗血清和多克隆抗体可识别烟草叶片特异性条带,其相对分子量为65 kD,与预测分子量相符,表明利用该方法制备的NPR1多肽抗体具有较高特异性和灵敏度。 展开更多
关键词 非表达型病程相关蛋白 序列分析 多肽 合成 多克隆抗体
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RT-PCR克隆广谱抗病基因NPR1及其蛋白表达载体构建 被引量:2
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作者 刘永光 刘克锋 孙向阳 《安徽农业科学》 CAS 北大核心 2011年第21期12707-12709,共3页
[目的]克隆植物广谱抗病基因NPR1并构建其蛋白表达载体。[方法]提取拟南芥总RNA,设计相关引物,采用反转录PCR方法克隆NPR1基因;利用酶切连接方法,将该基因正向导入蛋白表达载体。[结果]经过相关检验,将NPR1正向插入pMXB10载体中,得到了p... [目的]克隆植物广谱抗病基因NPR1并构建其蛋白表达载体。[方法]提取拟南芥总RNA,设计相关引物,采用反转录PCR方法克隆NPR1基因;利用酶切连接方法,将该基因正向导入蛋白表达载体。[结果]经过相关检验,将NPR1正向插入pMXB10载体中,得到了pMXB10-NPR1蛋白表达载体。[结论]成功构建了包含NPR1的蛋白表达载体。 展开更多
关键词 npr1 广谱抗病 载体构建
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GmSKP1,a Novel S-phase Kinase-associated Protein 1 in Glycine max,Enhancing Resistance Against Phytophthora sojae Infection
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作者 Ning Bin Li Wei-wei +9 位作者 Liu Xin Ji Wei Wang Yu-hong Zhao Ming He Sheng-fu Zhang Chuan-zhong Rong Tian-yu Liu Dong-xue Xu Peng-fei Zhang Shu-zhen 《Journal of Northeast Agricultural University(English Edition)》 CAS 2023年第1期1-12,共12页
Phytophthora root and stem rot of soybean caused by Phytophthora sojae(P.sojae)is a devastating disease that affects soybean[Glycine max(L.)Merr.]all over the world.S-phase kinase-associated protein 1(SKP1)proteins ar... Phytophthora root and stem rot of soybean caused by Phytophthora sojae(P.sojae)is a devastating disease that affects soybean[Glycine max(L.)Merr.]all over the world.S-phase kinase-associated protein 1(SKP1)proteins are key members of the SKP1/Cullin/F-box protein(SCF)ubiquitin ligase complex and play diverse roles in plant biology.However,the role of SKP1 in soybean against the phytopathogenic oomycete P.sojae remains unclear.In this study,a novel member of the soybean SKP1 gene family,GmSKP1 which was significantly induced by P.sojae,was reported.The expression of GmSKP1 was simultaneously induced by methyl jasmonate(MeJA),salicylic acid(SA)and ethylene(ET),which might suggest an important role for GmSKP1 of plant in responses to hormone treatments.Functional analysis using GmSKP1 overexpression lines showed that GmSKP1 enhanced resistance to P.sojae in transgenic soybean plants.Further analyses showed that GmSKP1 interacted with a homeodomain-leucine zipper protein transcription factor(GmHDL56)and a WRKY transcription factor(GmWRKY31),which could positively regulate responses to P.sojae in soybean.Importantly,several pathogenesis-related(PR)genes were constitutively activated,including GmPR1a,GmPR2,GmPR3,GmPR4,GmPR5a and GmPR10,in GmSKP1-OE soybean plants.Taken together,these results suggested that GmSKP1 enhanced resistance to P.sojae in soybean,possibly by activating the defense-related PR genes. 展开更多
关键词 Phytophthora sojae SOYBEAN SKP1 OVEREXPRESSION pathogenesis-related gene
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