Bioethanol production from sugarcane molasses by co-fermentation of Saccharomyces cerevisiae isolate TA2 and Wickerhamomyces anomalus isolate HCJ2F-19

Hawaz, Estifanos; Tafesse, Mesfin; Tesfaye, Anteneh; Kiros, Solomon; Beyene, Dereje; Kebede, Gessesse; Boekhout, Teun; Groenwald, Marizeth; Theelen, Bart; Degefe, Ayantu; Degu, Sisay; Admasu, Alene; Hunde, Biru; Muleta, Diriba

doi:10.1186/s13213-024-01757-8

Bioethanol production from sugarcane molasses by co-fermentation of Saccharomyces cerevisiae isolate TA2 and Wickerhamomyces anomalus isolate HCJ2F-19

detalle del documento

IDENTIFICACIÓN

doi:10.1186/s13213-024-01757-8...

Autor

Hawaz, Estifanos Tafesse, Mesfin Tesfaye, Anteneh Kiros, Solomon Beyene, Dereje Kebede, Gessesse Boekhout, Teun Groenwald, Marizeth Theelen, Bart Degefe, Ayantu Degu, Sisay Admasu, Alene Hunde, Biru Muleta, Diriba

Langue

Editor

BioMed Central

Categoría

Mycology

Año

2024

fecha de cotización

10/4/2024

Palabras clave

co-fermentation optimization bioethanol sugarcane molasses ethanol yield stress tolerance statistical optimization g^−1 h^−1 conditions using respectively 5 g production productivity ethanol isolate yield bioethanol molasses anomalus l^−1 0 co-fermentation

Métrico

Resumen

Purpose Co-culturing is a widely used method to improve bioethanol production from biomass enriched in fermentable sugars.

This study aims to produce bioethanol from sugarcane molasses by simultaneous co-fermentation of S. cerevisiae isolate TA2 and W. anomalus isolate HCJ2F-19.

Methods Response surface methodology (RSM) based on the central composite design (CCD) was employed to optimize fermentation conditions, including mixing rate (110–150 rpm), temperature (25–35 °C), molasses concentration (25–35 ^obrix), and incubation time (36–72 h).

The ethanol concentration was analyzed using HPLC equipped with a UV detector.

Results The monoculture S. cerevisiae isolate TA2 produced 17.2 g.L^−1 of ethanol, 0.33 g.g^−1 of ethanol yield, and 0.36 g.L^−1.

h^−1 of productivity compared to W. anomalus isolate HCJ2F that produced 14.5 g.L^−1, 0.30 g.g^−1 and 0.28 g.L^−1.

h^−1 ethanol, ethanol yield, and productivity under laboratory conditions, respectively.

In comparison to single cultures of S. cerevisiae TA2 and W. anomalus HCJ2F, the co-fermentation using both isolates showed an increased ethanol yield of 29% and 53% compared to the single species fermentations, respectively.

The results showed that the growth of W. anomalus HCJ2F-19 and S. cerevisiae TA2 was not influenced by each other during the co-fermentation process.

The one variable at a time optimization (OVAT) analysis resulted in an ethanol concentration of 26.5 g.L^−1 with a specific yield and productivity of 0.46 g.g^−1, 0.55 g.L^−1.

h^−1, respectively, at pH 5.5, 25 ^obrix, 48 h, 150 rpm, 30 °C, 60:40 inoculum ratio, and 10% overall inoculum size.

The maximum ethanol concentration of 35.5 g.L^−1 was obtained by co-fermentation using the RSM-CCD tool at 30 ^obrix, 30 °C, 54 h, and 130 rpm.

Conclusion The results suggested that the co-fermentation of S. cerevisiae isolate TA2 and W. anomalus isolate HCJ2F improves bioethanol production from sugar cane molasses under optimum fermentation conditions.

Hawaz, Estifanos,Tafesse, Mesfin,Tesfaye, Anteneh,Kiros, Solomon,Beyene, Dereje,Kebede, Gessesse,Boekhout, Teun,Groenwald, Marizeth,Theelen, Bart,Degefe, Ayantu,Degu, Sisay,Admasu, Alene,Hunde, Biru,Muleta, Diriba, 2024, Bioethanol production from sugarcane molasses by co-fermentation of Saccharomyces cerevisiae isolate TA2 and Wickerhamomyces anomalus isolate HCJ2F-19, BioMed Central