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Characterization of Arabidopsis thaliana Pinoresinol Reductase a New Type of Enzyme Involved in Lignan Biosynthesis

机译:拟南芥拟南芥松脂醇还原酶的表征 木质素中涉及的一种新型酶 生物合成

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摘要

A lignan, lariciresinol, was isolated from Arabidopsis thaliana, the most widely used model plant in plant bioscience sectors, for the first time. In the A. thaliana genome database, there are two genes (At1g32100 and At4g13660) that are annotated as pinoresinol/lariciresinol reductase (PLR). The recombinant AtPLRs showed strict substrate preference toward pinoresinol but only weak or no activity toward lariciresinol, which is in sharp contrast to conventional PLRs of other plants that can reduce both pinoresinol and lariciresinol efficiently to lariciresinol and secoisolariciresinol, respectively. Therefore, we renamed AtPLRs as A. thaliana pinoresinol reductases (AtPrRs). The recombinant AtPrR2 encoded by At4g13660 reduced only (–)-pinoresinol to (–)-lariciresinol and not (+)-pinoresinol in the presence of NADPH. This enantiomeric selectivity accords with that of other PLRs of other plants so far reported, which can reduce one of the enantiomers selectively, whatever the preferential enantiomer. In sharp contrast, AtPrR1 encoded by At1g32100 reduced both (+)- and (–)-pinoresinols to (+)- and (–)-lariciresinols efficiently with comparative kcat/Km values. Analysis of lignans and spatiotemporal expression of AtPrR1 and AtPrR2 in their functionally deficient A. thaliana mutants and wild type indicated that both genes are involved in lariciresinol biosynthesis. In addition, the analysis of the enantiomeric compositions of lariciresinol isolated from the mutants and wild type showed that PrRs together with a dirigent protein(s) are involved in the enantiomeric control in lignan biosynthesis. Furthermore, it was demonstrated conclusively for the first time that differential expression of PrR isoforms that have distinct selectivities of substrate enantiomers can determine enantiomeric compositions of the product, lariciresinol.
机译:首次从植物生物科学领域中使用最广泛的模型植物拟南芥中分离出木脂素lariciresinol。在拟南芥基因组数据库中,有两个基因(At1g32100和At4g13660)被注释为松脂醇/ lariciresinol还原酶(PLR)。重组AtPLRs对松脂醇具有严格的底物偏爱性,但对lariciresinol的活性却很弱或没有活性,这与其他植物的常规PLR形成鲜明对比,后者可以分别将松脂醇和lariciresinol分别有效地还原为lariciresinol和secoisolariciresinol。因此,我们将AtPLRs重命名为拟南芥松脂醇还原酶(AtPrRs)。在NADPH存在下,由At4g13660编码的重组AtPrR2仅将(–)-松脂醇还原为(–)-lariciresinol,而不还原(+)-松脂醇。该对映异构体选择性与迄今报道的其他植物的其他PLR一致,其可以选择性地还原一种对映异构体,而不管优先的对映异构体如何。与之形成鲜明对比的是,由At1g32100编码的AtPrR1可以将(+)-和(-)-松油菜皮酚有效地降低为(+)-和(-)-油菜豆素醇,并且具有相对的kcat / Km值。 木质素和AtPrR1和At的时空表达分析 AtPrR2在其功能缺陷的拟南芥突变体中 野生型表明这两个基因均参与了lariciresinol 生物合成。此外,分析了 从突变体和野生型中分离出的lariciresinol表明,PrRs 与一种或多种蛋白质一起参与对映体控制 在木脂素生物合成中。此外,对于 首次发现具有不同特征的PrR亚型的差异表达 底物对映体的选择性可以确定对映体组成 产品lariciresinol。

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