胞外游离脂肪酸的产率与胞外酰基- acp合成酶及s层蛋白的基因破坏。

Kamonchanock Eungrasamee, Peter Lindblad, Saowarath Jantaro
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引用次数: 3

摘要

背景:基于已知的对过量游离脂肪酸(FFA)产物的代谢反应,蓝细菌Synechocystis sp. PCC 6803优先通过FFA回收过程回收并将其隐藏到培养基中。具有良好生长和高度分泌FFA能力的工程蓝藻被认为是生物燃料生产和可持续生物技术的最佳资源。在本研究中,为了达到更高的FFA分泌目标,我们成功构建了Synechocystis sp. PCC 6803突变体,破坏与FFA循环反应相关的基因(aas基因编码酰基酰基载体蛋白合成酶)和表层蛋白(sll1951编码)。结果:3株聚胞孢子菌(Synechocystis sp. PCC 6803)工程菌株,包括2株缺乏aas (KA)和sll1951 (KS)的单突变体和1株同时缺乏aas和sll1951 (KAS)的双突变体,其分泌的FFAs显著高于野生型(WT)。除菌株KS外,细胞在缺氮、bg11 -半氮和BG11-N条件下分泌的游离脂肪酸均有一定的增加。在BG11-N条件下,菌株KAS在第10天显著分泌FFAs产物达40%w/DCW或238.1 mg/L, PHB含量微量。出乎意料的是,s层破坏的菌株KS在BG11-N生长培养基中存活的时间更长。菌株KS通过积累更大的糖原库和更低的FFA产量来显著适应BG11-N环境,而菌株KA则倾向于更高的PHB和细胞内脂质积累,并适度分泌FFA。结论:聚囊藻(Synechocystis sp. PCC 6803)的aas和sll1951基因突变显著提高了分泌游离脂肪酸的产量,特别是在氮剥夺条件下。
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Enhanced productivity of extracellular free fatty acids by gene disruptions of acyl-ACP synthetase and S-layer protein in Synechocystis sp. PCC 6803.

Background: Based on known metabolic response to excess free fatty acid (FFA) products, cyanobacterium Synechocystis sp. PCC 6803 preferentially both recycles via FFA recycling process and secrets them into medium. Engineered cyanobacteria with well growth and highly secreted FFA capability are considered best resources for biofuel production and sustainable biotechnology. In this study, to achieve the higher FFA secretion goal, we successfully constructs Synechocystis sp. PCC 6803 mutants disrupting genes related to FFA recycling reaction (aas gene encoding acyl-acyl carrier protein synthetase), and surface layer protein (encoded by sll1951).

Results: Three Synechocystis sp. PCC 6803 engineered strains, including two single mutants lacking aas (KA) and sll1951 (KS), and one double mutant lacking both aas and sll1951 (KAS), significantly secreted FFAs higher than that of wild type (WT). Certain increase of secreted FFAs was noted when cells were exposed to nitrogen-deficient conditions, BG11-half N and BG11-N conditions, with the exception of strain KS. Under BG11-N condition at day 10, strain KAS strikingly secreted FFAs products up to 40%w/DCW or 238.1 mg/L, with trace amounts of PHB. Unexpectedly, strain KS, with S-layer disruption, appeared to have endured longer in BG11-N growth medium. This strain KS significantly acclimated to the BG11-N environment by accumulating a greater glycogen pool with lower FFA production, whereas strain KA favored higher PHB and intracellular lipid accumulations with moderate FFA secretion.

Conclusions: Mutations of both aas and sll1951 genes in Synechocystis sp. PCC 6803 significantly improved the productivity of secreted FFAs, especially under nitrogen deprivation.

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