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Identifying a Cinnamoyl Coenzyme A Reductase (CCR) Activity with 4-Coumaric Acid: Coenzyme A Ligase (4CL) Reaction Products in Populus tomentosa

机译:识别4-香豆酸的肉桂酰基辅酶A还原酶(CCR)活性:毛白杨中的辅酶A连接酶(4CL)反应产物

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摘要

A cinnamoyl coenzyme A reductase (CCR, EC 1.2.1.44), one of the key enzyme involved in lignin biosynthesis, was cloned from Populus tomentosa (Chinese white poplar). At the same time, a 4CL1 gene was cloned from P. tomentosa, too. The two genes were subcloned in pQE31 vector and expressed in Escherichia coli M15. Both of them were purified by Ni-NTA. Purified CCR protein was digested by trypsin and analyzed by HPLC-MS; the peptide segments had 27% similarity with the sequence of the CCR protein. 4CL was thought to be a neighbor enzyme of CCR in lignin biosynthesis. In this paper, a 4CL1 from P. tomentosa was cloned, and its enzyme reaction products were extracted for the substrates of CCR. Three 4CL1 enzyme reaction products were monitored by HPLC-MS and then the CCR enzyme reaction was detected by GC-MS. In the CCR reaction, the three corresponding aldehyde (p-coumaraldehyde, caffealdehyde, and coniferaldehyde) were detected and identified by Frontier3 software. The results showed that the CCR that we cloned from P. tomentosa had affinities with 4CL1 enzyme reaction products and a ptCCR that was cloned from aspen (Li et al., Plant Cell Physiol 46(7):1073–1082, 2005) only had affinity with feruloyl-CoA. The different results maybe depend on the different study method. The method of exacting 4CL enzyme products as the substrates of CCR in the paper was reliable and can be used in lignin biosynthesis network to detect the enzymes in the neighborhood that depended on the polarity of the substrates and products. This CCR gene had eight homology sequence CCR gene when a BLAST was conducted in Populus trichocarpa genome database. The CCR homology genes in Populus suggested that some CCRs may take part in the lignin biosynthesis, too. The gene family would be the hot spot in the future study.
机译:从毛白杨(Populus tomentosa)(中国白杨)中克隆了一种肉桂酰辅酶A还原酶(CCR,EC 1.2.1.44),这是一种参与木质素生物合成的关键酶。同时,也从毛白球菌中克隆了4CL1基因。将这两个基因亚克隆到pQE31载体中,并在大肠杆菌M15中表达。它们都通过Ni-NTA纯化。用胰蛋白酶消化纯化的CCR蛋白,并用HPLC-MS分析。该肽段与CCR蛋白的序列具有27%的相似性。 4CL被认为是木质素生物合成中CCR的邻近酶。本文克隆了毛白杨的4CL1,并提取了其酶反应产物作为CCR的底物。通过HPLC-MS监测3种4CL1酶反应产物,然后通过GC-MS检测CCR酶反应。在CCR反应中,通过Frontier3软件检测并鉴定了三个相应的醛(对香豆醛,咖啡醛和松柏醛)。结果表明,我们从毛白球菌克隆的CCR与4CL1酶反应产物和从白杨克隆的ptCCR具有亲和力(Li等人,Plant Cell Physiol 46(7):1073-1082,2005)与阿魏酰辅酶A的亲和力。不同的结果可能取决于不同的研究方法。本文中将4CL酶产物作为CCR底物的方法是可靠的,可用于木质素生物合成网络中,根据底物和产物的极性检测附近的酶。当在毛果杨基因组数据库中进行BLAST时,该CCR基因具有八个同源序列CCR基因。胡杨中的CCR同源基因表明,一些CCR也可能参与木质素的生物合成。基因家族将成为未来研究的热点。

著录项

  • 来源
    《Journal of Plant Biology》 |2009年第5期|482-491|共10页
  • 作者单位

    College of Life Sciences and Biotechnology Beijing Forestry University No 35 Qinghua Donglu Haidian District P.O.Box 162 Beijing 100083 People’s Republic of China;

    College of Life Sciences and Biotechnology Beijing Forestry University No 35 Qinghua Donglu Haidian District P.O.Box 162 Beijing 100083 People’s Republic of China;

    College of Life Sciences and Biotechnology Beijing Forestry University No 35 Qinghua Donglu Haidian District P.O.Box 162 Beijing 100083 People’s Republic of China;

    College of Life Sciences and Biotechnology Beijing Forestry University No 35 Qinghua Donglu Haidian District P.O.Box 162 Beijing 100083 People’s Republic of China;

    College of Life Sciences and Biotechnology Beijing Forestry University No 35 Qinghua Donglu Haidian District P.O.Box 162 Beijing 100083 People’s Republic of China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    Lignin; CCR; 4CL; HPLC-MS; GC-MS;

    机译:木质素;CCR;4CL;HPLC-MS;GC-MS;

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