Gardenia carotenoid cleavage dioxygenase 4a is an efficient tool for biotechnological production of crocins in green and non‐green plant tissues

西红花酸 生物 番红花 番红花苷 八氢番茄红素合酶 玉米黄质 类胡萝卜素 八氢番茄红素脱氢酶 生物化学 植物烯 染色体体 老茧 红花醛 植物 栀子花 生物合成 叶黄素 质体 基因 叶绿体 番茄红素 替代医学 医学 病理
作者
Xiongjie Zheng,Jianing Mi,Aparna Balakrishna,Kit Xi Liew,Abdugaffor Ablazov,Rachid Sougrat,Salim Al‐Babili
出处
期刊:Plant Biotechnology Journal [Wiley]
卷期号:20 (11): 2202-2216 被引量:30
标识
DOI:10.1111/pbi.13901
摘要

Summary Crocins are beneficial antioxidants and potential chemotherapeutics that give raise, together with picrocrocin, to the colour and taste of saffron, the most expensive spice, respectively. Crocins are formed from crocetin dialdehyde that is produced in Crocus sativus from zeaxanthin by the carotenoid cleavage dioxygenase 2L (CsCCD2L), while GjCCD4a from Gardenia jasminoides , another major source of crocins, converted different carotenoids, including zeaxanthin, into crocetin dialdehyde in bacterio . To establish a biotechnological platform for sustainable production of crocins, we investigated the enzymatic activity of GjCCD4a, in comparison with CsCCD2L, in citrus callus engineered by Agrobacterium‐mediated supertransformation of multi genes and in transiently transformed Nicotiana benthamiana leaves. We demonstrate that co‐expression of GjCCD4a with phytoene synthase and β‐carotene hydroxylase genes is an optimal combination for heterologous production of crocetin, crocins and picrocrocin in citrus callus. By profiling apocarotenoids and using in vitro assays, we show that GjCCD4a cleaved β‐carotene, in planta , and produced crocetin dialdehyde via C 30 β‐apocarotenoid intermediate. GjCCD4a also cleaved C 27 β‐apocarotenoids, providing a new route for C 17 ‐dialdehyde biosynthesis. Callus lines overexpressing GjCCD4a contained higher number of plastoglobuli in chromoplast‐like plastids and increased contents in phytoene, C17:0 fatty acid (FA), and C18:1 cis ‐9 and C22:0 FA esters. GjCCD4a showed a wider substrate specificity and higher efficiency in Nicotiana leaves, leading to the accumulation of up to 1.6 mg/g dry weight crocins. In summary, we established a system for investigating CCD enzymatic activity in planta and an efficient biotechnological platform for crocins production in green and non‐green crop tissues/organs.
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