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咖啡因生物合成中的关键酶N-7甲基转移酶的分离。

Separation of the N-7 methyltransferase, the key enzyme in caffeine biosynthesis.

作者信息

Mösli Waldhauser S S, Gillies F M, Crozier A, Baumann T W

机构信息

Institute of Plant Biology, University of Zürich, Switzerland.

出版信息

Phytochemistry. 1997 Aug;45(7):1407-14. doi: 10.1016/s0031-9422(97)00187-8.

Abstract

Caffeine biosynthesis comprises sequential methylations at N-7, N-3 and N-1 of the xanthine ring catalysed by S-adenosyl-L-methionine (SAM)-dependent methyltransferase activities that, to date, have not been resolved. Enzyme extracts were prepared from young, emerging coffee leaflets and following anion exchange chromatography, chromatofocusing facilitated the clear separation of the N-7-methyltransferase from the N-3- and N-1-methyltransferase activities. All three N-methyltransferases co-eluted when analysed by gel filtration chromatography and their native molecular mass was ca 67 kDa. Photoaffinity labelling with [methyl-3H]SAM followed by SDS-PAGE of a chromatofocusing-purified preparation containing only N-7-methyltransferase activity demonstrated the presence of a single labelled band of 40 kDa. Similar analysis of a gel filtration purified preparation containing all three N-methyltransferase activities revealed the presence of three labelled bands at 49, 43 and 40 kDa. It remains to be determined whether the 49 and 43 kDa bands are associated with the N-3 and N-1-methyltransferases or whether they are unrelated SAM-dependent methyltransferases or other SAM-binding proteins.

摘要

咖啡因生物合成包括在黄嘌呤环的N-7、N-3和N-1处依次进行甲基化,这一过程由依赖S-腺苷-L-甲硫氨酸(SAM)的甲基转移酶活性催化,迄今为止,这些活性尚未得到解析。从幼嫩的、正在生长的咖啡小叶中制备酶提取物,经过阴离子交换色谱后,聚焦色谱法有助于将N-7-甲基转移酶与N-3-和N-1-甲基转移酶活性清晰分离。当通过凝胶过滤色谱分析时,所有三种N-甲基转移酶共同洗脱,其天然分子量约为67 kDa。用[甲基-³H]SAM进行光亲和标记,然后对仅含有N-7-甲基转移酶活性的聚焦色谱纯化制剂进行SDS-PAGE分析,结果显示存在一条40 kDa的单一标记带。对含有所有三种N-甲基转移酶活性的凝胶过滤纯化制剂进行类似分析,结果显示在49、43和40 kDa处存在三条标记带。49 kDa和43 kDa的条带是否与N-3和N-1-甲基转移酶相关,或者它们是否是无关的依赖SAM的甲基转移酶或其他SAM结合蛋白,仍有待确定。

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