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新型同源乳酸转运蛋白提高了毕赤酵母重组菌株中甘油合成L-乳酸的产量。

Novel homologous lactate transporter improves L-lactic acid production from glycerol in recombinant strains of Pichia pastoris.

作者信息

de Lima Pollyne Borborema Almeida, Mulder Kelly Cristina Leite, Melo Nadiele Tamires Moreira, Carvalho Lucas Silva, Menino Gisele Soares, Mulinari Eduardo, de Castro Virgilio H, Dos Reis Thaila F, Goldman Gustavo Henrique, Magalhães Beatriz Simas, Parachin Nádia Skorupa

机构信息

Grupo de Engenharia Metabólica Aplicada a Bioprocessos, Instituto de Ciências Biológicas, Universidade de Brasília, Brasília, DF, CEP 70.790-900, Brazil.

Integra Bioprocessos e Análises, Campus Universitário Darcy Ribeiro, Edifício CDT, Sala AT-36/37, Brasília, DF, CEP 70.904-970, Brazil.

出版信息

Microb Cell Fact. 2016 Sep 15;15(1):158. doi: 10.1186/s12934-016-0557-9.

Abstract

BACKGROUND

Crude glycerol is the main byproduct of the biodiesel industry. Although it can have different applications, its purification is costly. Therefore, in this study a biotechnological route has been proposed for further utilization of crude glycerol in the fermentative production of lactic acid. This acid is largely utilized in food, pharmaceutical, textile, and chemical industries, making it the hydroxycarboxylic acid with the highest market potential worldwide. Currently, industrial production of lactic acid is done mainly using sugar as the substrate. Thus here, for the first time, Pichia pastoris has been engineered for heterologous L-lactic acid production using glycerol as a single carbon source. For that, the Bos taurus lactate dehydrogenase gene was introduced into P. pastoris. Moreover, a heterologous and a novel homologous lactate transporter have been evaluated for L-lactic acid production.

RESULTS

Batch fermentation of the P. pastoris X-33 strain producing LDHb allowed for lactic acid production in this yeast. Although P. pastoris is known for its respiratory metabolism, batch fermentations were performed with different oxygenation levels, indicating that lower oxygen availability increased lactic acid production by 20 %, pushing the yeast towards a fermentative metabolism. Furthermore, a newly putative lactate transporter from P. pastoris named PAS has been identified by search similarity with the lactate transporter from Saccharomyces cerevisiae Jen1p. Both heterologous and homologous transporters, Jen1p and PAS, were evaluated in one strain already containing LDH activity. Fed-batch experiments of P. pastoris strains carrying the lactate transporter were performed with the batch phase at aerobic conditions followed by an aerobic oxygen-limited phase where production of lactic acid was favored. The results showed that the strain containing PAS presented the highest lactic acid titer, reaching a yield of approximately 0.7 g/g.

CONCLUSIONS

We showed that P. pastoris has a great potential as a fermentative organism for producing L-lactic acid using glycerol as the carbon source at limited oxygenation conditions (below 0.05 % DO in the bioreactor). The best strain had both the LDHb and the homologous lactate transporter encoding genes expressed, and reached a titer 1.5 times higher than the strain with the S. cerevisiae transporter. Finally, it was also shown that increased lactic acid production was concomitant to reduction of acetic acid formation by half.

摘要

背景

粗甘油是生物柴油行业的主要副产品。尽管它有不同的用途,但其提纯成本高昂。因此,在本研究中,提出了一条生物技术路线,用于粗甘油在发酵生产乳酸中的进一步利用。乳酸在食品、制药、纺织和化工行业有大量应用,使其成为全球市场潜力最大的羟基羧酸。目前,乳酸的工业生产主要以糖为底物。因此,这里首次对巴斯德毕赤酵母进行工程改造,使其能够以甘油作为单一碳源异源生产L-乳酸。为此,将牛乳酸脱氢酶基因导入巴斯德毕赤酵母。此外,还评估了一种异源和一种新型同源乳酸转运体用于L-乳酸的生产。

结果

对表达LDHb的巴斯德毕赤酵母X-33菌株进行分批发酵,该酵母能够生产乳酸。尽管巴斯德毕赤酵母以其呼吸代谢而闻名,但分批发酵在不同的氧合水平下进行,这表明较低的氧利用率使乳酸产量提高了20%,促使酵母转向发酵代谢。此外,通过与酿酒酵母Jen1p乳酸转运体搜索相似性,鉴定出一种来自巴斯德毕赤酵母的新的假定乳酸转运体PAS。在一个已经具有LDH活性的菌株中评估了异源和同源转运体Jen1p和PAS。对携带乳酸转运体的巴斯德毕赤酵母菌株进行补料分批实验,分批阶段在好氧条件下进行,随后是有利于乳酸生产的好氧限氧阶段。结果表明,含有PAS的菌株乳酸滴度最高,产量约为0.7 g/g。

结论

我们表明,在限氧条件下(生物反应器中溶解氧低于0.05%),巴斯德毕赤酵母作为以甘油为碳源生产L-乳酸的发酵生物体具有巨大潜力。最佳菌株同时表达了LDHb和同源乳酸转运体编码基因,其滴度比含有酿酒酵母转运体的菌株高1.5倍。最后,还表明乳酸产量的增加伴随着乙酸形成减少一半。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e0b0/5025603/306d0ed1d402/12934_2016_557_Fig1_HTML.jpg

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