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首页> 外文期刊>Biochemical Pharmacology >The galloyl moiety of green tea catechins is the critical structural feature to inhibit fatty-acid synthase.
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The galloyl moiety of green tea catechins is the critical structural feature to inhibit fatty-acid synthase.

机译:绿茶儿茶素的没食子酰基部分是抑制脂肪酸合酶的关键结构特征。

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摘要

It has been reported that inhibition of fatty-acid synthase (FAS) is selectively cytotoxic to human cancer cells. Considerable interest has developed in identifying novel inhibitors of this enzyme complex. Our previous work showed that green tea (-)-epigallocatechin gallate can inhibit FAS in vitro. To elucidate the structure-activity relationship of the inhibitory effects of tea polyphenols, we investigated the inhibition kinetics of the major catechins and analogues. Ungallated catechins from green tea do not show obvious inhibition compared with gallated catechins. Another gallated catechin, (-)-epicatechin gallate, was also found as a potent inhibitor of FAS and its inhibition characteristics are similar to (-)-epigallocatechin gallate. Furthermore, the analogues of galloyl moiety without the catechin skeleton such as propyl gallate also showed obvious slow-binding inhibition, whereas the green tea ungallated catechin not. Atomic orbital energy analyses suggest that the positive charge is more distinctly distributed on the carbon atom of ester bond of galloyl moiety of gallate catechins, and that gallated forms are more susceptible for a nucleophilic attack than other catechins. Here we identify the galloyl moiety of green tea catechins as critical in the inactivation of the ketoacyl reductase activity of FAS for the first time.
机译:据报道,抑制脂肪酸合酶(FAS)对人癌细胞具有选择性的细胞毒性。在鉴定该酶复合物的新型抑制剂方面已经引起了相当大的兴趣。我们以前的工作表明,绿茶(-)-表没食子儿茶素没食子酸酯可以在体外抑制FAS。为了阐明茶多酚的抑制作用的构效关系,我们研究了主要儿茶素和类似物的抑制动力学。与没食子儿茶素相比,来自绿茶的未没食子儿茶素没有明显的抑制作用。还发现了另一种没食子儿茶素,(-)-表儿茶素没食子酸酯,作为FAS的有效抑制剂,其抑制特性类似于没食子酸(-)-表没食子儿茶素。此外,没有儿茶素骨架的没食子酰基部分的类似物,如没食子酸丙酯也显示出明显的缓慢结合抑制作用,而绿茶未加盖儿茶素则没有。原子轨道能量分析表明,正电荷在没食子儿茶素的没食子酸部分的没食子酸酯部分的酯键的碳原子上更明显地分布,并且没食子酸形式比其他儿茶素更容易发生亲核攻击。在这里,我们首次确定了绿茶儿茶素的没食子酰基部分对于FAS的酮酰基还原酶活性的失活至关重要。

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