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Cloning of the pks3 gene of Aurantiochytrium limacinum and functional study of the 3-ketoacyl-ACP reductase and dehydratase enzyme domains

机译:淡金牛卵菌pks3基因的克隆及3-酮酰基-ACP还原酶和脱水酶结构域的功能研究

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摘要

Aurantiochytrium limacinum has received attention because of its abundance of polyunsaturated fatty acids (PUFAs), particularly docosahexaenoic acid (DHA). DHA is synthesized through the polyketide synthase (PKS) pathway in A. limacinum. The related enzymes of the PKS pathway are mainly expressed by three gene clusters, called pks1, pks2 and pks3. In this study, the full-length pks3 gene was obtained by polymerase chain reaction amplification and Genome Walking technology. Based on a domain analysis of the deduced amino acid sequence of the pks3 gene, 3-ketoacyl-ACP reductase (KR) and dehydratase (DH) enzyme domains were identified. Herein, A. limacinum OUC168 was engineered by gene knock-in of KR and DH using the 18S rDNA sequence as the homologous recombination site. Total fatty acid contents and the degree of unsaturation of total fatty acids increased after the kr or dh gene was knocked in. The cloning and functional study of the pks3 gene of A. limacinum establishes a foundation for revealing the DHA synthetic pathway. Gene knock-in of the enzyme domain associated with PKS synthesis has the potential to provide effective recombinant strains with higher DHA content for industrial applications.
机译:由于其丰富的多不饱和脂肪酸(PUFAs),特别是二十二碳六烯酸(DHA),金黄色的金鱼藻受到了关注。 DHA是通过利马曲霉中的聚酮化合物合酶(PKS)途径合成的。 PKS途径的相关酶主要由三个基因簇表达,称为pks1,pks2和pks3。本研究通过聚合酶链反应扩增和Genome Walking技术获得了全长pks3基因。根据对pks3基因推导的氨基酸序列的域分析,确定了3-酮酰基-ACP还原酶(KR)和脱水酶(DH)酶域。在此,使用18S rDNA序列作为同源重组位点,通过KR和DH的基因敲入工程化了青霉菌OUC168。敲除kr或dh基因后,总脂肪酸含量和总脂肪酸的不饱和度增加。南美曲霉pks3基因的克隆和功能研究为揭示DHA合成途径奠定了基础。与PKS合成相关的酶结构域的基因敲入具有为工业应用提供具有更高DHA含量的有效重组菌株的潜力。

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