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利用生长素介导的蛋白耗竭进行萜类化合物生产酵母的代谢工程。

Auxin-mediated protein depletion for metabolic engineering in terpene-producing yeast.

机构信息

Australian Institute for Bioengineering and Nanotechnology (AIBN), the University of Queensland, Brisbane, QLD, Australia.

School of Chemistry and Molecular Biosciences (SCMB), the University of Queensland, Brisbane, QLD, Australia.

出版信息

Nat Commun. 2021 Feb 16;12(1):1051. doi: 10.1038/s41467-021-21313-1.

Abstract

In metabolic engineering, loss-of-function experiments are used to understand and optimise metabolism. A conditional gene inactivation tool is required when gene deletion is lethal or detrimental to growth. Here, we exploit auxin-inducible protein degradation as a metabolic engineering approach in yeast. We demonstrate its effectiveness using terpenoid production. First, we target an essential prenyl-pyrophosphate metabolism protein, farnesyl pyrophosphate synthase (Erg20p). Degradation successfully redirects metabolic flux toward monoterpene (C10) production. Second, depleting hexokinase-2, a key protein in glucose signalling transduction, lifts glucose repression and boosts production of sesquiterpene (C15) nerolidol to 3.5 g L in flask cultivation. Third, depleting acetyl-CoA carboxylase (Acc1p), another essential protein, delivers growth arrest without diminishing production capacity in nerolidol-producing yeast, providing a strategy to decouple growth and production. These studies demonstrate auxin-mediated protein degradation as an advanced tool for metabolic engineering. It also has potential for broader metabolic perturbation studies to better understand metabolism.

摘要

在代谢工程中,失活功能实验被用于理解和优化代谢。当基因缺失对生长具有致死性或有害时,需要使用条件基因失活工具。在这里,我们利用生长素诱导的蛋白降解作为酵母中的代谢工程方法。我们使用萜类生产来证明其有效性。首先,我们针对必需的 prenyl-pyrophosphate 代谢蛋白,法呢基焦磷酸合酶(Erg20p)。降解成功地将代谢通量重新导向单萜(C10)生产。其次,耗尽葡萄糖信号转导中的关键蛋白六磷酸激酶-2(hexokinase-2),解除葡萄糖抑制作用,并将倍半萜(C15)橙花叔醇的产量提高到 3.5g/L 在摇瓶培养中。第三,耗尽另一种必需蛋白乙酰辅酶 A 羧化酶(Acc1p)会导致生长停滞,但不会降低橙花叔醇生产酵母的生产能力,为生长和生产解耦提供了一种策略。这些研究表明,生长素介导的蛋白降解是代谢工程的一种先进工具。它也有可能用于更广泛的代谢扰动研究,以更好地理解代谢。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/effc/7886869/a7b634264ecf/41467_2021_21313_Fig1_HTML.jpg

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