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. 2025 Aug 18;15(1):30196.
doi: 10.1038/s41598-025-13271-1.

Bioelectromics of a photosynthetic microalgae assisted microbial fuel cell for wastewater treatment and value added production

Affiliations

Bioelectromics of a photosynthetic microalgae assisted microbial fuel cell for wastewater treatment and value added production

Ankesh Ahirwar et al. Sci Rep. .

Abstract

Power generation and recovery of value-added products using microalgae, Haematococcus lacustris is tested in a dual chamber photosynthetic microalgae-assisted microbial fuel cell (PMA-MFCt1). The microalgal cells in conical flask act as control. The performance was compared to another, test PMA-MFCt2. The control MFC in second test had electrode wires not connected (PMA-MFCnw). The PMA-MFCt1 set had microalgal catholytic media replenished unlike in PMA-MFCt2. A comparative PMA0-MFC, was used without microalgae and only water as catholyte. The results demonstrated maximum power density (PDmax) of 33.76 mW m-2 in PMA-MFCt1, 15.36 mW m-2 in PMA-MFCt2 and 8.05 mW m-2 in PMA0-MFC. The non replenishment of catholytic media in PMA-MFCt2 set resulted in nutrient limitations, poor photosynthesis, and disrupted redox reactions. Further lowest PDmax in PMA0-MFC proves that microalgae are excellent source of free nascent oxygen required for redox reaction. Taxonomic identity of microbes at the anode via 16 S rRNA showed the dominance of catalytic microbes mainly Proteobacteria. The different kinds of carotenoids from microalgae were estimated by UV-Vis and liquid chromatography-mass spectrometry (LC-MS) analysis. The microalgal growth, evaluated in terms of biomass dry weight (DW), was 118 mg L-1, after 40 days of PMA-MFCt1 operation, which was lesser than in control (conical flask) 123 mg L-1. The pigments including total chlorophyll (a + b), and total carotenoids were 699.7 µg g-1 and 224.6 µg g-1, respectively, on day 16. Microalgal performance in PMA-MFCt2 and its control (PMA-MFCnw) was 10% and 32.52% inferior than in PMA-MFCt1 and its control. The continuous replenishment of media in PMA-MFCt1 maintained microalgal cells in continuous state of multiplication and photosynthesis resulting into higher bioelectricity generation and bioproducts than PMA-MFCt2, and PMA-MFCnw.

Keywords: Haematococcus lacustris; Bioelectricity; Carotenoids; Lipids; Metagenomics, microalgae; Microbial fuel cell; Wastewater treatment.

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Conflict of interest statement

Declarations. Competing interests: The authors declare no competing interests.

Figures

Fig. 1
Fig. 1
Average physiochemical parameters intensity changes of five fed batch cycles for 40 days in a PMA-MFCt1, (A) Anode, (B) Cathode, (C) Control, (D) Anode of PMA-MFCt2, PMA-MFCnw, PMA0-MFC and (E) Cathode of PMA-MFCt2, PMA-MFCnw, PMA0-MFC.
Fig. 2
Fig. 2
Polarization curve of reactors (A) PMA-MFCt1, (B) PMA-MFCt2, (C) PMA0-MFC and (D) COD removal of PMA-MFCt1, PMA-MFCt2, PMA-MFCnw, PMA0-MFC.
Fig. 3
Fig. 3
Summary of microbial community profiles in the multilevel Krona function annotation diagram depicting taxonomic hierarchies where each cycle represents taxonomic levels of the bacterial communities in wastewater of PMA-MFCt1 (A) sample of 1st day and (B) sample of day 40 at anodic chamber; (C) Heatmap is representing the abundance of different taxonomic groups of bacteria and the number are representing the percentage of abundance of a particular group on day 1 and day 40.
Fig. 4
Fig. 4
Haematococcus lacustris in cathode of PMA-MFCt1 from day 1 to day 40 (A) Cell count (B); Specific growth and Logistic kinetics with respect to cell count in PMA-MFCt1 and control flask (C) total weight of biomass of control flask and PMA-MFCt1 reactor from day 1 to 40 days, (D) Semi log plot growth kinetics with respect to biomass in PMA-MFCt1 and control flask (E) total lipid percentage and lipid concentration MFC reactor and (F) Chlorophyll ‘a’, ‘b’, ‘a + b’ and total carotenoids in PMA-MFCt1 and Astaxanthin in PMA-MFCt1 and control flask.
Fig. 5
Fig. 5
Astaxanthin and other carotenoids identified by liquid chromatography-mass spectrometry (LC-MS) from Haematococcus lacustris cells at cathode in a PMA-MFCt1 for the presence of, (A) Astaxanthin fragment at RT 3.68 at m/z 279.08 detected in day 1 sample and on day 40, the LCMS showed (B) Halocynthiaxanthin at RT 6.71 min at m/z 233.08; (C) Docosahexaenoic acid (DHA) at 4.36 min at m/z 326; (D) at 7.11 min at m/z 139.08 fragments of fatty acid hexacosanedioic acid, carotenoids neoxanthin and vioxanthin; (E) astaxanthin diester at RT 8.23 m/z 1119.58; (F) Astaxanthin mono esters at retention time (RT) 15.92 min at m/z 579.58 and 596.83 and palmitic acid at 15.92 min at m/z 255.33.

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