Huang Tyng-Shyan, Anzellotti Dominique, Dedaldechamp Fabienne, Ibrahim Ragai K
Plant Biochemistry Laboratory and Centre for Structural and Functional Genomics, Concordia University, Montreal, Quebec, Canada H4B 1R6.
Plant Physiol. 2004 Apr;134(4):1366-76. doi: 10.1104/pp.103.036442.
Serratula tinctoria (Asteraceae) accumulates mainly 3,3'-dimethylquercetin and small amounts of 3-methylquercetin as an intermediate. The fact that 3-methylquercetin rarely accumulates in plants in significant amounts, and given its important role as an antiviral and antiinflammatory agent that accumulates in response to stress conditions, prompted us to purify and characterize the enzyme involved in its methylation. The flavonol 3-O-methyltransferase (3-OMT) was partially purified by ammonium sulfate precipitation and successive chromatography on Superose-12, Mono-Q, and adenosine-agarose affinity columns, resulting in a 194-fold increase of its specific activity. The enzyme protein exhibited an expressed specificity for the methylation of position 3 of the flavonol, quercetin, although it also utilized kaempferol, myricetin, and some monomethyl flavonols as substrates. It exhibited a pH optimum of 7.6, a pI of 6.0, and an apparent molecular mass of 31 kD. Its K(m) values for quercetin as the substrate and S-adenosyl-l-Met (AdoMet) as the cosubstrate were 12 and 45 microm, respectively. The 3-OMT had no requirement for Mg(2+), but was severely inhibited by p-chloromercuribenzoate, suggesting the requirement for SH groups for catalytic activity. Quercetin methylation was competitively inhibited by S-adenosyl-l-homo-Cys with respect to the cosubstrate AdoMet, and followed a sequential bi-bi reaction mechanism, where AdoMet was the first to bind and S-adenosyl-l-homo-Cys was released last. In-gel trypsin digestion of the purified protein yielded several peptides, two of which exhibited strong amino acid sequence homology, upon protein identification, to a number of previously identified Group II plant OMTs. The availability of peptide sequences will allow the design of specific nucleotide probes for future cloning of the gene encoding this novel enzyme for its use in metabolic engineering.
染用麻花头(菊科)主要积累3,3'-二甲基槲皮素,并少量积累3-甲基槲皮素作为中间体。鉴于3-甲基槲皮素在植物中很少大量积累,且其作为在应激条件下积累的抗病毒和抗炎剂具有重要作用,促使我们纯化并鉴定参与其甲基化的酶。黄酮醇3-O-甲基转移酶(3-OMT)通过硫酸铵沉淀以及在Superose-12、Mono-Q和腺苷琼脂糖亲和柱上的连续层析进行部分纯化,其比活性提高了194倍。该酶蛋白对黄酮醇槲皮素3位的甲基化表现出特异性,不过它也利用山奈酚、杨梅素和一些单甲基黄酮醇作为底物。它的最适pH为7.6,pI为6.0,表观分子量为31 kD。以槲皮素为底物、S-腺苷-L-甲硫氨酸(AdoMet)为辅底物时,其K(m)值分别为12和45 μmol。3-OMT不需要Mg(2+),但受到对氯汞苯甲酸的强烈抑制,这表明催化活性需要巯基。相对于辅底物AdoMet,槲皮素甲基化受到S-腺苷-L-高半胱氨酸的竞争性抑制,并且遵循有序的双底物双产物反应机制,其中AdoMet首先结合,S-腺苷-L-高半胱氨酸最后释放。对纯化蛋白进行胶内胰蛋白酶消化产生了几个肽段,其中两个在蛋白质鉴定时与许多先前鉴定的II类植物OMT具有很强的氨基酸序列同源性。肽序列的获得将有助于设计特异性核苷酸探针,以便将来克隆编码这种新酶的基因用于代谢工程。