Lignocellulosic ethanol production by starch-base industrial yeast under PEG detoxification

Liu, Xiumei; Xu, Wei; Mao, Liaoyuan; Zhang, Chao; Yan, Peifang; Xu, Zhanwei; Zhang, Z. Conrad

doi:10.1038/srep20361

Cited by 30 publications

(13 citation statements)

References 44 publications

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“…The low μ max values in the present study may be due to the cell growth inhibition by ethanol and/or inhibitory compounds generated during PRs pretreatment. It has been reported that the presence in the fermentation medium of phenolics at 2.0 g/L negatively affects both cell viability of S. cerevisiae and ethanol production (Liu et al, 2016). In the present study, the initial concentration of phenolic compounds was about 2.0 g/L and remained almost constant during fermentation of S. cerevisiae .…”

Section: Resultsmentioning

confidence: 99%

Bioconversion of pomegranate residues into biofuels and bioactive lipids

Dourou¹,

Economou

Aggeli

et al. 2021

Preprint

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Pomegranate residues (PRs) (i.e. the solid residues remaining after juice extraction), generated currently in abundance in Greece, contain a variety of carbon sources and therefore can be regarded as a potential feedstock for chemical and biotechnological processes rather than as waste materials. In the current project, the polysaccharides contained in PRs were extracted and hydrolyzed in a one-step process without the use of chemical reagents and the resulting broth was used as substrate in biotechnological applications, including ethanol and single cell oil (SCO) production. The yeasts Meyerozyma guilliermondii, Scheffersomyces coipomoensis, Sugiyamaella paludigena and especially Saccharomyces cerevisiae, were able to efficiently convert PR derived reducing sugars into bioethanol. Ethanol production under anaerobic conditions ranged from 3.6 to 12.5 g/L. In addition, the oleaginous yeasts Lipomyces lipofer and Yarrowia lipolytica as well as M. guilliermondii, S. coipomoensis and S. paludigena were tested for their ability to accumulate lipids suitable as feedstock for biodiesel production. Lipids were accumulated at concentrations up to 18% and were rich in palmitic acid (C16:0) and oleic acid (C18:1). Finally, the oleaginous fungus Cunnichamella echinulata was cultivated on PR based solid substrates for γ-linolenic acid (GLA) production. The fermented bio-products (i.e. fermented substrate plus fungal mycelia) contained up to 4.8 mg GLA/g of dry weight. Phenolic removal (up to 30%) was achieved by several of the above mentioned microorganisms, including C. echinulata, L. lipofer, M. guilliermondii, S. paludigena and Y. lipolytica. We conclude that PRs can be used as a raw material for microbial growth, ethanol and SCO production, which is of economic and environmental importance.

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Section: Resultsmentioning

confidence: 99%

Bioconversion of pomegranate residues into biofuels and bioactive lipids

Dourou¹,

Economou

Aggeli

et al. 2021

Preprint

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“…Additionally, it is possible to observe that 28.99% of the reducing sugars present in the medium were not consumed. Although the pretreatment processes of the lignocellulosic biomass employed in this work are widely used strategies, they have the disadvantage of generating toxic compounds to fermenting organisms, such as phenolic compounds, guaiacol, levulinic acid, furfural and 5-hydroxymethyl furfural (Varanasi et al, 2013;Liu et al, 2016). The presence of such substances may have inhibited the activity of S. cerevisiae, making it impossible to deplete the substrate offered, since the samples were not detoxified to remove these substances.…”

Section: Discussionmentioning

confidence: 99%

Evaluation of buriti endocarp as lignocellulosic substrate for second generation ethanol production

Rodrigues

Araújo

Rocha

et al. 2018

Preprint

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The production of lignocellulosic ethanol is one of the most promising alternatives to fossil fuels, however, this technology still faces many challenges related to the viability of the alcohol in the market. In this paper the endocarp of buriti fruit was assessed for ethanol production. The whole fruit was characterized physically and chemically and its endocarp submitted to acid and alkaline pre-treatments, which were optimized through the use of surface response methodology for removal of hemicellulose and lignin, respectively. Abstract 16 The production of lignocellulosic ethanol is one of the most promising alternatives to fossil fuels, 17 however, this technology still faces many challenges related to the viability of the alcohol in the 18 market. In this paper the endocarp of buriti fruit was assessed for ethanol production. The whole 19 fruit was characterized physically and chemically and its endocarp submitted to acid and alkaline 20 pre-treatments, which were optimized through the use of surface response methodology for 21 removal of hemicellulose and lignin, respectively. Hemicellulose content was reduced by 88% 22 after acid pretreatment. Alkaline pre-treatment reduced the lignin content in the recovered 23 biomass from 11.8% to 4.2% and increased the concentration of the cellulosic fraction to 88.5%. 24 The pre-treated biomass was saccharified by the action of cellulolytic enzymes and, in the 25 optimized condition, was able to produce 110 g of glucose per L of hydrolyzate. Alcoholic 26 fermentation of the enzymatic hydrolyzate bio-catalized by Saccharomyces cerevisiae resulted in 27 a fermented medium with 4.3% ethanol and Y P/S of 0.33 . The current configuration of global economic advance has created a growing demand for 33 energy resources to support its maintenance. Additionally, the growth of the human population 34 on the planet, the depletion of fossil fuels and the growing concerns about human impacts on the 35 environment have encouraged the search for renewable sources to the development of green 36 energy production (Singh, Nigam & Murphy, 2011; Sarkar et al., 2012). In this context, 37 lignocellulosic biomasses are a promising feedstock for the production of liquid biofuels, 38 alternative to petroleum based fuels (Cherubini & Ulgiati, 2010). 39The technology for the production of second generation (2G) bioethanol, or 40 lignocellulosic ethanol, has evolved in the last decades and functioning industrial plants already 41 exist in some parts of the world, nevertheless, this biofuel still faces the challenge of feedstock 42 access, supply chain infrastructure, and price competitiveness with the petroleum industry (UNCTAD, 43 2016). 44Lignocellulosic ethanol can be obtained from the fermentation of hexoses and pentoses 45 derived from the polysaccharides that constitute the plants cell wall and require additional 46 operations to those normally used to produce first generation ethanol (Mielenz, 2001). Lignin 47 removal and hemicellulose hydrolysis, followed by cellulose saccharif...

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“…It is possible to observe in the fermentation experiment with Saccharomyces cerevisiae that 28.99% of the reducing sugars present in the medium were not consumed. The pretreatment processes of lignocellulosic biomasses employed in this work are widely used strategies; however, they have the disadvantage of generating toxic compounds to fermenting organisms, such as phenolic compounds, guaiacol, levulinic acid, furfural and 5-hydroxymethylfurfural ( Varanasi et al, 2013 ; Liu et al, 2016 ). Although the pre-treated endocarp was rinsed with distillate water before enzymatic scarification, Zhang et al (2010) indicate that this method is not efficient for total removal of toxic compounds impregnated in the biomass.…”

Section: Discussionmentioning

confidence: 99%

Evaluation of buriti endocarp as lignocellulosic substrate for second generation ethanol production

Rodrigues

Araújo

Rocha

et al. 2018

PeerJ

View full text Add to dashboard Cite

The production of lignocellulosic ethanol is one of the most promising alternatives to fossil fuels; however, this technology still faces many challenges related to the viability of the lignocellulosic alcohol in the market. In this paper the endocarp of buriti fruit was assessed for ethanol production. The fruit endocarp was characterized physically and chemically. Acid and alkaline pre-treatments were optimized by surface response methodology for removal of hemicellulose and lignin from the biomass. Hemicellulose content was reduced by 88% after acid pretreatment. Alkaline pre-treatment reduced the lignin content in the recovered biomass from 11.8% to 4.2% and increased the concentration of the cellulosic fraction to 88.5%. The pre-treated biomass was saccharified by the action of cellulolytic enzymes and, under optimized conditions, was able to produce 110 g of glucose per L of hydrolyzate. Alcoholic fermentation of the enzymatic hydrolyzate performed by Saccharomyces cerevisiae resulted in a fermented medium with 4.3% ethanol and a yield of product per substrate (YP/S) of 0.33.

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Lignocellulosic ethanol production by starch-base industrial yeast under PEG detoxification

Cited by 30 publications

References 44 publications

Bioconversion of pomegranate residues into biofuels and bioactive lipids

Bioconversion of pomegranate residues into biofuels and bioactive lipids

Evaluation of buriti endocarp as lignocellulosic substrate for second generation ethanol production

Evaluation of buriti endocarp as lignocellulosic substrate for second generation ethanol production

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