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细胞凋亡相关新基因Apr-3转录剪接体的克隆、测序及亚细胞定位
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作者 张静 王文亮 +5 位作者 晏伟 郭双平 张志培 李擒龙 王丽 严晓昱 《临床与实验病理学杂志》 CAS CSCD 北大核心 2006年第3期344-347,共4页
目的克隆Apr-3基因的一个转录剪接体,并对其进行测序及亚细胞定位。方法培养HL-60细胞,提取HL-60细胞总RNA,应用RT-PCR获取Apr-3的转录剪接体的编码区cDNA序列,将该cDNA与质粒pcDNA3·1/myc-His(-)B连接,构建克隆载体,将其转化E.col... 目的克隆Apr-3基因的一个转录剪接体,并对其进行测序及亚细胞定位。方法培养HL-60细胞,提取HL-60细胞总RNA,应用RT-PCR获取Apr-3的转录剪接体的编码区cDNA序列,将该cDNA与质粒pcDNA3·1/myc-His(-)B连接,构建克隆载体,将其转化E.coli DH5α,进行测序,与GenBank中登录序列比对结果正确后将该cDNA与质粒pEGFP-C3连接,并将其转染COS-7细胞。结果对测序结果进行序列分析,与GenBank中登录的Apr-3编码区完全一致。pEGFP-Apr-3基因表达产物定位于COS-7细胞的细胞膜和细胞质。结论对Apr-3基因的一个转录剪接体进行克隆,构建了真核表达载体,首次发现Apr-3的该转录剪接体主要在真核细胞的细胞膜和细胞质表达,为后期对该基因的结构和功能的研究奠定基础。 展开更多
关键词 apr-3 细胞凋亡 转录剪接体 克隆 亚细胞定位
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细胞凋亡相关新基因Apr-3的一个转录剪接体的克隆、初步表达及纯化
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作者 张静 王文亮 +3 位作者 晏伟 张志培 李擒龙 王丽 《现代肿瘤医学》 CAS 2006年第7期781-783,共3页
目的克隆Apr-3基因的一个转录剪接体,进行原核表达,并进行初步纯化。方法培养HL-60细胞,提取HL-60细胞总RNA,应用RT-PCR获取Apr-3编码区cDNA序列的前366bp,将该cDNA与质粒pcDNA3.0连接,构建克隆载体,将其转化E.coliDH5α,进行测序,与Gen... 目的克隆Apr-3基因的一个转录剪接体,进行原核表达,并进行初步纯化。方法培养HL-60细胞,提取HL-60细胞总RNA,应用RT-PCR获取Apr-3编码区cDNA序列的前366bp,将该cDNA与质粒pcDNA3.0连接,构建克隆载体,将其转化E.coliDH5α,进行测序,与GenBank中登录序列比对,结果正确后将该cDNA与质粒pET28a连接,构建原核表达载体,转化大肠杆菌,诱导表达获得Apr-3蛋白。结果对测序结果进行序列分析,与GenBank中登录的Apr-3编码区完全一致。Apr-3融合蛋白主要以包涵体形式存在。结论成功构建了Apr-3的原核表达载体,获得了较纯的Apr-3融合蛋白。 展开更多
关键词 apr-3 细胞凋亡 转录剪接体 克隆 表达 融合蛋白
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H2O2-Activated Up-Regulation of Glutathione in Arabidopsis Involves Induction of Genes Encoding Enzymes Involved in Cysteine Synthesis in the Chloroplast 被引量:10
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作者 Guillaume Queval Dorothée Thominet Hélène Vanacker Myroslawa Miginiac-Maslow Bertrand Gakière Graham Noctor 《Molecular Plant》 SCIE CAS CSCD 2009年第2期344-356,共13页
Glutathione is a key player in cellular redox homeostasis and, therefore, in the response to H2O2, but the factors regulating oxidation-activated glutathione synthesis are still unclear. We investigated H2O2-induced g... Glutathione is a key player in cellular redox homeostasis and, therefore, in the response to H2O2, but the factors regulating oxidation-activated glutathione synthesis are still unclear. We investigated H2O2-induced glutathione synthesis in a conditional Arabidopsis catalase-deficient mutant (cat2). Plants were grown from seed at elevated CO2 for 5 weeks, then transferred to air in either short-day or long-day conditions. Compared to cat2 at elevated CO2 or wild-type plants in any condition, transfer of cat2 to air in both photoperiods caused measurable oxidation of the leaf glutathione pool within hours. Oxidation continued on subsequent days and was accompanied by accumulation of glutathione. This effect was stronger in cat2 transferred to air in short days, and was not linked to appreciable increases in the extractable activities of or transcripts encoding enzymes involved in the committed pathway of glutathione synthesis. In contrast, it was accompanied by increases in serine, O-acetylserine, and cysteine. These changes in metabolites were accompanied by induction of genes encoding adenosine phosphosulfate reductase (APR), particularly APR3, as well as a specific serine acetyltransferase gene (SAT2.1) encoding a chloroplastic SAT. Marked induction of these genes was only observed in cat2 transferred to air in short-day conditions, where cysteine and glutathione accumulation was most dramatic. Unlike other SAT genes, which showed negligible induction in cat2, the relative abundance of APR and SAT2.1 transcripts was closely correlated with marker transcripts for H2O2 signaling. Together, the data underline the importance of cysteine synthesis in oxidant-induced up-regulation of glutathione synthesis and suggest that the chloroplast makes an important contribution to cysteine production under these circumstances. 展开更多
关键词 Oxidative stress CATALASE PHOTOPERIOD 3 -glutamylcysteine synthetases (γ-ECS) adenosine phosphosulfate reductase (APR) serine acetyltransferase (SAT).
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