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Short-Chain Flavor Ester Synthesis in Organic Media by an E. coli Whole-Cell Biocatalyst Expressing a Newly Characterized Heterologous Lipase

机译:表达新特性的异源脂肪酶的大肠杆菌全细胞生物催化剂在有机介质中合成短链风味酯

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摘要

Short-chain aliphatic esters are small volatile molecules that produce fruity and pleasant aromas and flavors. Most of these esters are artificially produced or extracted from natural sources at high cost. It is, however, possible to ‘naturally’ produce these molecules using biocatalysts such as lipases and esterases. A gene coding for a newly uncovered lipase was isolated from a previous metagenomic study and cloned into E. coli BL21 (DE3) for overexpression using the pET16b plasmid. Using this recombinant strain as a whole-cell biocatalyst, short chain esters were efficiently synthesized by transesterification and esterification reactions in organic media. The recombinant lipase (LipIAF5-2) showed good affinity toward glyceryl trioctanoate and the highest conversion yields were obtained for the transesterification of glyceryl triacetate with methanol. Using a simple cetyl-trimethylammonium bromide pretreatment increased the synthetic activity by a six-fold factor and the whole-cell biocatalyst showed the highest activity at 40°C with a relatively high water content of 10% (w/w). The whole-cell biocatalyst showed excellent tolerance to alcohol and short-chain fatty acid denaturation. Substrate affinity was equally effective with all primary alcohols tested as acyl acceptors, with a slight preference for methanol. The best transesterification conversion of 50 mmol glyceryl triacetate into isoamyl acetate (banana fragrance) provided near 100% yield after 24 hours using 10% biocatalyst loading (w/w) in a fluidized bed reactor, allowing recycling of the biocatalyst up to five times. These results show promising potential for an industrial approach aimed at the biosynthesis of short-chain esters, namely for natural flavor and fragrance production in micro-aqueous media.
机译:短链脂族酯是挥发性小分子,可产生水果和令人愉悦的香气和风味。这些酯中的大多数是人工生产或从天然来源提取的,成本较高。但是,可以使用脂肪酶和酯酶等生物催化剂“天然”产生这些分子。从以前的宏基因组学研究中分离出编码新发现的脂肪酶的基因,并使用pET16b质粒克隆到大肠杆菌BL21(DE3)中进行过表达。使用这种重组菌株作为全细胞生物催化剂,可以通过在有机介质中进行酯交换和酯化反应有效地合成短链酯。重组脂肪酶(LipIAF5-2)对三辛酸甘油酯显示出良好的亲和力,并且三乙酸甘油酯与甲醇的酯交换反应获得最高的转化率。使用简单的十六烷基三甲基溴化铵预处理可将合成活性提高六倍,全细胞生物催化剂在40°C时显示出最高活性,且水含量相对较高,为10%(w / w)。全细胞生物催化剂显示出对醇和短链脂肪酸变性的优异耐受性。底物亲和力与所有作为酰基受体测试的伯醇一样有效,略微偏爱甲醇。 50 mmol三乙酸甘油酯向乙酸异戊酯(香蕉香料)的最佳酯交换反应可在流化床反应器中使用10%生物催化剂负载(w / w)在24小时后提供接近100%的收率,从而使生物催化剂循环使用多达五次。这些结果表明,针对短链酯生物合成的工业方法,即在微水介质中生产天然香料和香精,具有广阔的前景。

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