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模型木质素单体的酶促芳基-O-甲基-C 标记。

Enzymatic aryl-o-methyl-C labeling of model lignin monomers.

机构信息

Department of Microbiology, and Department of Environmental Medicine, New York University Medical Center, New York, New York 10016.

出版信息

Appl Environ Microbiol. 1986 Jan;51(1):80-3. doi: 10.1128/aem.51.1.80-83.1986.

Abstract

Aryl-O-methyl ethers are abundant in aerobic and anaerobic environments. In particular, lignin is composed of units of this type. Lignin monomers specifically radiolabeled in methoxy, side chain, and ring carbons have been synthesized by chemical procedures and are important in studies of lignin synthesis and degradation, humus formation, and microbial O-demethylation. In this paper attention is drawn to an enzymatic procedure for preparing O-methyl-C-labeled aromatic lignin monomers which has not previously been exploited in microbial ecology and physiology studies and which has several advantages compared with chemical synthesis procedures. O-[methyl-C]vanillic and O-[methyl-C]ferulic acids were prepared with S-[methyl-C]adenosyl-l-methionine as the methyl donor, using commercially obtained porcine liver catechol-O-methyltransferase (EC 2.1.1.6). The specific activity of the methylated products was the same as that of the methyl donor, a maximum of about 58 muCi/mumol, and the yields were 42% (vanillate) and 35% (ferulate). Thus lignin monomers are readily prepared as O-methylated products of the catechol-O-methyltransferase reaction and, with this enzyme method of preparation, would be more widely available than labeled compounds which require chemical synthesis.

摘要

芳基-O-甲基醚在需氧和厌氧环境中都很丰富。特别是木质素由这种类型的单元组成。通过化学程序合成了专门在甲氧基、侧链和环碳原子上进行放射性标记的木质素单体,它们在木质素合成和降解、腐殖质形成和微生物 O-去甲基化的研究中非常重要。本文提请注意一种酶促程序,用于制备 O-甲基-C-标记的芳香木质素单体,该程序以前尚未在微生物生态学和生理学研究中得到利用,并且与化学合成程序相比具有几个优点。使用市售的猪肝儿茶酚-O-甲基转移酶(EC 2.1.1.6),以 S-[甲基-C]腺苷甲硫氨酸作为甲基供体,制备了 O-[甲基-C]香草酸和 O-[甲基-C]阿魏酸。甲基化产物的比活与甲基供体相同,最大约为 58 muCi/mumol,产率分别为 42%(香草酸盐)和 35%(阿魏酸盐)。因此,木质素单体很容易作为儿茶酚-O-甲基转移酶反应的 O-甲基化产物制备,并且与需要化学合成的标记化合物相比,该酶法制备的木质素单体更容易获得。

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本文引用的文献

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Appl Environ Microbiol. 1986 Jan;51(1):84-7. doi: 10.1128/aem.51.1.84-87.1986.
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