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Biochemical and molecular characterization of a novel UDP-glucose : anthocyanin 3 '-O-glucosyltransferase, a key enzyme for blue anthocyanin biosynthesis, from gentian

机译:一种来自龙胆的新型UDP-葡萄糖的生化和分子表征:花青素3'-O-葡萄糖基转移酶,一种用于蓝色花青素生物合成的关键酶

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摘要

Gentian (Gentiana triflora) blue petals predominantly contain an unusually blue and stable anthocyanin, delphinidin 3-O-glucosyl-5-O-(6-O-caffeoyl-glucosyl)-3'-O-(6-O-caffeoyl-glucoside) (gentiodelphin). Glucosylation and the subsequent acylation of the 3'-hydroxy group of the B-ring of anthocyanins are important to the stabilization of and the imparting of bluer color to these anthocyanins. The enzymes and their genes involved in these modifications of the B-ring, however, have not been characterized, purified, or isolated to date. In this study, we purified a UDP-glucose (Glc):anthocyanin 3'-O-glucosyltransferase (3'GT) enzyme to homogeneity from gentian blue petals and isolated a cDNA encoding a 3'GT based on the internal amino acid sequences of the purified 3'GT. The deduced amino acid sequence indicates that 3'GT belongs to the same subfamily as a flavonoid 7-O-glucosyltransferase from Schutellaria baicalensis in the plant glucosyltransferase superfamily. Characterization of the enzymatic properties using the recombinant 3'GT protein revealed that, in contrast to most of flavonoid glucosyltransferases, it has strict substrate specificity: 3'GT specifically glucosylates the 3'-hydroxy group of delphinidin-type anthocyanins containing Glc groups at 3 and 5 positions. The enzyme specifically uses UDP-Glc as the sugar donor. The specificity was confirmed by expression of the 3'GT cDNA in transgenic petunia (Petunia hybrida). This is the first report of the gene isolation of a B-ring-specific glucosyltransferase of anthocyanins, which paves the way to modification of flower color by production of blue anthocyanins.
机译:龙胆草(Gentiana triflora)蓝色花瓣主要包含异常蓝色和稳定的花色苷,飞燕草素3-O-葡萄糖基-5-O-(6-O-咖啡酰基-葡萄糖基)-3'-O-(6-O-咖啡酰基-葡萄糖苷)(gentiodelphin)。花青苷的B环的3'-羟基的糖基化和随后的酰化对于这些花青苷的稳定化和赋予其较蓝的颜色很重要。但是,迄今为止,尚未鉴定,纯化或分离出涉及B环修饰的酶及其基因。在这项研究中,我们从龙胆蓝花瓣中纯化了UDP-葡萄糖(Glc):花青素3'-O-葡萄糖基转移酶(3'GT)酶,使其同质,并基于AFP的内部氨基酸序列分离了编码3'GT的cDNA。纯化的3'GT。推导的氨基酸序列表明,在植物葡糖基转移酶超家族中,3'GT与来自Schutellaria baicalensis的类黄酮7-O-葡糖基转移酶属于同一亚家族。使用重组的3'GT蛋白表征酶学性质表明,与大多数类黄酮葡糖基转移酶相比,它具有严格的底物特异性:3'GT专门对3个含有Glc基团的delphinidin型花色苷的3'-羟基进行糖基化。和5个职位。该酶特别使用UDP-Glc作为糖供体。通过在转基因矮牵牛(Petunia hybrida)中表达3'GT cDNA证实了特异性。这是花色苷B环特异性葡萄糖基转移酶基因分离的第一个报道,它为通过生产蓝色花色苷修饰花色铺平了道路。

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