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. 2024 Aug 23;14(1):19578.
doi: 10.1038/s41598-024-70377-8.

A serum-free culture medium production system by co-culture combining growth factor-secreting cells and L-lactate-assimilating cyanobacteria for sustainable cultured meat production

Shanga Chu  1   2 Yuji Haraguchi  2 Toru Asahi  1   3   4 Yuichi Kato  5   6 Akihiko Kondo  5   6   7 Tomohisa Hasunuma  5   6   7 Tatsuya Shimizu  8
Affiliations

A serum-free culture medium production system by co-culture combining growth factor-secreting cells and L-lactate-assimilating cyanobacteria for sustainable cultured meat production

Shanga Chu et al. Sci Rep. .

Abstract

Large-scale production of cultured meat requires bulk culture medium containing growth-promoting proteins from animal serum. However, animal serum for mammalian cell culture is associated with high costs, ethical concerns, and contamination risks. Owing to its growth factor content, conditioned medium from rat liver epithelial RL34 cells can replace animal serum for myoblast proliferation. More seeded cells and longer culture periods are thought to yield higher growth factor levels, resulting in more effective muscle cell proliferation. However, RL34 cells can deplete nutrients and release harmful metabolites into the culture medium over time, potentially causing growth inhibition and apoptosis. This issue highlights the need for waste clearance during condition medium production. To address this issue, we introduced a lactate permease gene (lldP) and an L-lactate-to-pyruvate conversion enzyme gene (lldD) to generate a recombinant L-lactate-assimilating cyanobacterium Synechococcus sp. KC0110 strain. Transwell co-culture of this strain with RL34 cells exhibited a marked reduction in the levels of harmful metabolites, lactate and ammonium, while maintaining higher concentrations of glucose, pyruvate, and pyruvate-derived amino acids than those seen with RL34 cell monocultures. The co-culture medium supported myoblast proliferation without medium dilution or additional nutrients, which was attributed to the waste clearance and nutrient replenishment effects of the KC0110 strain. This culture system holds potential for the production of low-cost, and animal-free cultured meat.

Keywords: l-lactate-assimilating cyanobacterium; Co-culture; Cultured meat; Mammalian cell cultures; RL34 cells; Serum replacement.

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Conflict of interest statement

Tokyo Women’s Medical University has received research funds from IntegriCulture Inc. The part of this manuscript describing the technique for culturing mammalian cells using culture supernatants is the subject of the following patent application: patent applicant (Tokyo Women’s Medical University and IntegriCulture, Inc.), name of inventors (T. Shimizu, Y. Haraguchi), application number (PCT/JP2023/019786), status of application (pending). The part of this manuscript describing the technique for L-lactate-assimilating cyanobacteria is the subject of the following patent application: patent applicant (Kobe University and Tokyo Women’s Medical University), name of inventors (T. Hasunuma, Y. Kato, A. Kondo, T. Shimizu, Y. Haraguchi), application number (PCT/JP2022/044962), status of application (Granted in Japan). S. Chu, and T. Asahi, declare no financial competing interests.

Figures

Figure 1
Figure 1
Evaluation of C2C12 cell proliferation following the addition of RL34 cell culture medium: (ae) or 50:50 v/v% of DMEM-diluted RL34 cell culture medium: (fj). (a,f) Fold change of C2C12 cell density relative to the initial cell density (a: 4.5 ± 0.70 × 104 cells/well; f: 4.8 ± 0.84 × 104 cells/well in 12-well plates) after culture with 1 mL of DMEM or serum-free RL34 medium for 2 days (a: n = 4; f: n = 3). The darker color of columns indicates higher seeding density of RL34 cells; 0.25 × 106 (light pink), 1.0 × 106 (pink), and 4.0 × 106 (crimson) cells/well in 6-well plate. (be), (gj) Time-dependent changes in (b,g) glucose; (c,h) lactate; (d,i) ammonium; (e,j) LDH content of RL34 culture medium and 50:50 v/v% of DMEM-diluted RL34 cell culture medium (4.0 × 106 cells/well in 6-well plate, (be): n = 4, (gj): n = 3). Data represent the mean ± SD; ***p < 0.001; **p < 0.01; *p < 0.05.
Figure 2
Figure 2
Comparing RL34 monoculture vs. RL34 and KC0110 strain transwell co-culture. The gray columns stand for RL34 monoculture (seeding density of 4.0 × 106 cells/well in 6-well plate for 3 days), and the green columns stand for RL34 and KC0110 strain transwell co-culture. The darker the green color of the column stands for the higher seeding density of KC0110; optical density at 750 nm (OD750) 1.0 (light green), 2.0 (green), 4.0 (dark green) cultured with 4.0 × 106 RL34 cells/well in 6-well plate for 3 days. (a) Fold change of RL34 cell density relative to the initial cell density (4.5 ± 0.50 × 106 cells/well in 6-well plates) co-cultured with KC0110 for 3 days (n = 4). (b) Change of OD750 to the initial cell density (Low: 0.97 ± 0.058; Mid: 2.0 ± 0.017; High: 4.0 ± 0.015) of KC0110 co-cultured with RL34 for 3 days (n = 3). (cg) Metabolite content of co-culture medium (seeding density of 4.0 × 106 RL34 cells/well with OD750 2.0 KC0110 in 6-well plate for 3 days) compared to monoculture medium (seeding density of 4.0 × 106 RL34 cells/well without KC0110 in the 6-well plate for 3 days); (c) lactate; (d) ammonium; (e) glucose; (f) pyruvate and (g) LDH (n = 6). (h) 20 amino acids composition (n = 5); (i) total amount of 20 amino acids (n = 5). Data represent the mean ± SD; ****p < 0.0001; ***p < 0.001; **p < 0.01; *p < 0.05; ns not significant.
Figure 3
Figure 3
Evaluation of the proliferation of C2C12 cells in RL34 and KC0110 co-culture medium (sup.). (a) Fold change of C2C12 cell density relative to the initial cell density (4.1 ± 0.62 × 104 cells/well in 12-well plates) following culture in different media (1 mL per well, respectively) for 2 days (n = 3); DMEM (white); RL34 monoculture medium (gray, seeding density of 4.0 × 106 cells/well in 6-well plate for 3 days); RL34 and KC0110 co-culture medium (light green, OD750 1.0; green, OD750 2.0; dark green, OD750 4.0 KC0110 with 4.0 × 106 RL34 cells/well in 6-well plate for 3 days). **p < 0.01; ns not significant. (b) Immunofluorescence staining for phalloidin (red) together with nucleus (blue) and MyoD (green) in C2C12 cells cultured in DMEM, RL34 monoculture medium, or RL34 and KC0110 (OD750 2.0) co-culture medium (scale bar: 200 µm). Data represent the mean ± SD; **p < 0.01; ns not significant.
Figure 4
Figure 4
Schematic diagram of the experiments (a) Evaluation of C2C12 cell proliferation following the addition of RL34 cell culture medium. (b) Evaluation of C2C12 cell proliferation following the addition of 50:50 v/v% DMEM-diluted RL34 cell culture medium. (c) Evaluation of C2C12 cell proliferation in RL34 and Synechococcus sp. KC0110 strain co-culture medium.
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