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在产油酵母解脂耶氏酵母中进行蓖麻酸的代谢工程。

Metabolic engineering for ricinoleic acid production in the oleaginous yeast Yarrowia lipolytica.

机构信息

INRA, UMR1319, Micalis, 78352, Jouy-en-Josas, France.

出版信息

Appl Microbiol Biotechnol. 2014 Jan;98(1):251-62. doi: 10.1007/s00253-013-5295-x. Epub 2013 Oct 18.

Abstract

Although there are numerous oleochemical applications for ricinoleic acid (RA) and its derivatives, their production is limited and subject to various safety legislations. In an effort to produce RA from alternative sources, we constructed a genetically modified strain of the oleaginous yeast Yarrowia lipolytica. This strain is unable to perform β-oxidation and is invalidated for the native triacylglycerol (TAG) acyltransferases (Dga1p, Dga2p, and Lro1p) and the ∆12 desaturase (Fad2p). We also expressed the Ricinus communis ∆12 hydroxylase (RcFAH12) under the control of the TEF constitutive promoter in this strain. However, RA constituted only 7% of the total lipids produced by this modified strain. By contrast, expression of the Claviceps purpurea hydroxylase CpFAH12 in this background resulted in a strain able to accumulate RA to 29% of total lipids, and expression of an additional copy of CpFAH12 drove RA accumulation up to 35% of total lipids. The co-expression of the C. purpurea or R. communis type II diacylglycerol acyltransferase (RcDGAT2 or CpDGAT2) had negative effects on RA accumulation in this yeast, with RA levels dropping to below 14% of total lipids. Overexpression of the native Y. lipolytica PDAT acyltransferase (Lro1p) restored both TAG accumulation and RA levels. Thus, we describe the consequences of rerouting lipid metabolism in this yeast so as to develop a cell factory for RA production. The engineered strain is capable of accumulating RA to 43% of its total lipids and over 60 mg/g of cell dry weight; this is the most efficient production of RA described to date.

摘要

尽管蓖麻酸(RA)及其衍生物有许多应用,但它们的产量有限,且受到各种安全法规的限制。为了从替代资源中生产 RA,我们构建了一株产油酵母解脂耶氏酵母的基因修饰株。该菌株无法进行β-氧化,并且其天然三酰基甘油(TAG)酰基转移酶(Dga1p、Dga2p 和 Lro1p)和 ∆12 去饱和酶(Fad2p)失活。我们还在该菌株中,通过 TEF 组成型启动子控制表达了大蓖麻 ∆12 羟化酶(RcFAH12)。然而,该修饰株产生的总脂中只有 7%是 RA。相比之下,在该背景下表达麦角菌羟化酶 CpFAH12 可使菌株积累 RA 至总脂的 29%,而额外表达一个 CpFAH12 拷贝可使 RA 积累至总脂的 35%。在该酵母中,共同表达大蓖麻或麦角菌 II 型二酰基甘油酰基转移酶(RcDGAT2 或 CpDGAT2)对 RA 积累有负面影响,RA 水平降至总脂的 14%以下。过量表达天然的解脂耶氏酵母 PDAT 酰基转移酶(Lro1p)可恢复 TAG 积累和 RA 水平。因此,我们描述了在这种酵母中重新路由脂质代谢的后果,以开发用于 RA 生产的细胞工厂。该工程菌株能够将 RA 积累到其总脂的 43%,超过细胞干重的 60mg/g;这是迄今为止 RA 生产效率最高的报道。

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