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Lost in Translation: Challenges with Heterologous Expression of Lichen Polyketide Synthases

机译:在翻译中丢失:地衣多酮合酶异源表达的挑战

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The ability to functionally express proteins in hosts is a precondition to an advanced understanding of the biosynthetic pathways that are responsible for producing life's complex molecules. The study of secondary metabolites in lichen- forming fungi has long been hampered by slow growth. This study, reports on heterologous expression trials of four polyketide synthase (PKS) genes from C. uncialis in Aspergillus oryzae NSAR1. Isolation of mRNA and RT-PCR demonstrated that A. oryzae can transcribe all lichen genes and remove introns to produce translationally-coherent mRNA. Transforma- tion of A. oryzae with a codon-optimized PKS did not result in metabolite production, nor did co-expression of a number of accessory genes restore function to any lichen PKS. Genes encoding an orsellinic acid synthase (OAS) from Fusarium sp. and a 6-methylsalicylic acid synthase (6MSAS) from Penicillum sp. were transformed into A. oryzae. Readily detectable amounts of de novo orsellinic acid and 6-methylsalicylic acid biosynthesis were observed in A. oryzae when transformed with these non-lichen PKS genes. However, transformation with functionally homologous PKS genes from C. uncialis produced no detectable product.
机译:在宿主中表达蛋白质功能的能力是对负责产生生命复杂分子的生物合成途径的先进理解的前提。长期生长缓慢地阻碍了地衣形成真菌中二级代谢产物的研究。这项研究,关于曲霉菌NSAR1中的四个聚酮化合物合酶(PKS)基因的异源表达试验的报道。 mRNA和RT-PCR的分离表明,绿曲霉可以转录所有地衣基因并去除内含子以产生翻译的mRNA。用密码子优化的PK对绿曲霉的转化并未导致代谢产物产生,也没有共表达许多辅助基因的功能,将功能恢复到任何地衣PKS。编码镰刀菌的蛋黄酸合酶(OAS)的基因。和6-甲基酸酸合酶(6MSAS),来自Penicillum sp。被转化为绿o。当用这些非酸化PKS基因转化时,在绿曲霉中观察到了易于检测量的从头孔酸和6-甲基白杨酸的生物合成。然而,来自非洲梭菌的功能同源PK基因的转化不会产生可检测的产物。

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