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Scientific Reports volume 13, Article number: 7249 (2023 ) Cite this article Ered Supplier
l -Lactate is a major waste compound in cultured animal cells. To develop a sustainable animal cell culture system, we aimed to study the consumption of l -lactate using a photosynthetic microorganism. As genes involved in l -lactate utilization were not found in most cyanobacteria and microalgae, we introduced the NAD-independent l -lactate dehydrogenase gene from Escherichia coli (lldD) into Synechococcus sp. PCC 7002. The lldD-expressing strain consumed l -lactate added to basal medium. This consumption was accelerated by expression of a lactate permease gene from E. coli (lldP) and an increase in culture temperature. Intracellular levels of acetyl-CoA, citrate, 2-oxoglutarate, succinate, and malate, and extracellular levels of 2-oxoglutarate, succinate, and malate, increased during l -lactate utilization, suggesting that the metabolic flux from l -lactate was distributed toward the tricarboxylic acid cycle. This study provides a perspective on l -lactate treatment by photosynthetic microorganisms, which would increase the feasibility of animal cell culture industries.
Shanshan Zhang, Jiahui Sun, … Xuefeng Lu
Jake N. Gonzales, Tanner R. Treece, … Shota Atsumi
Elizabeth C. Hann, Sean Overa, … Robert E. Jinkerson
Cultured animal cells are valuable in industries such as biopharmaceutical production1,2. Cultured meat production has also been studied, in which only edible parts are produced by cultured animal cells3,4. To produce nutrients for animal cells (e.g. sugars and amino acids), photosynthetic microorganisms (i.e. prokaryotic cyanobacteria and eukaryotic microalgae) have been recently studied because of their high ability to produce biomass from atmospheric CO25. Mouse C2C12 myoblasts and primary bovine myoblasts have been successfully cultured using cell extracts from Chlorella vulgaris, Chlorococcum littorale, and Arthrospira platensis as nutrients6,7. Thus, by treating waste compounds from animal cells (such as ammonium and l -lactate) using a photosynthetic microorganism, a sustainable animal cell culture system, that is, a circular cell culture (CCC) system, can be developed8 (Fig. 1). Consumption of ammonium in the culture waste of C2C12 cells has already been achieved through the cultivation of C. vulgaris and C. littorale9. The potential application of the CCC system was previously shown using C. littorale, RL34 hepatocytes, and C2C12 myoblasts as producers of nutrients, growth factors, and muscles, respectively8. However, l -lactate consumption by photosynthetic microorganisms has not yet been investigated. l -Lactate is a major waste compound in cultured animal cells, and its accumulation in medium causes cytotoxic effects by changing the pH and osmolarity10. Therefore, l -lactate removal is a ubiquitous requirement in industries that utilize cultured animal cells and is necessary for optimal functioning of the CCC system.
Scheme of circular cell culture (CCC).
Cyanobacteria such as Synechococcus sp. PCC 7002 and Synechocystis sp. PCC 6803 harbor d -lactate dehydrogenase (d -LDH; EC 1.1.1.28) as an enzyme involved in lactate metabolism and can produce d -lactate11,12 (Fig. 2). The genetically engineered strains of PCC 6803 into which NAD-dependent l -lactate dehydrogenase (l -nLDH, EC 1.1.1.27) has been introduced can also produce l -lactate13. However, the ability of microalgae and cyanobacteria to consume l -/d -lactate remains unclear. Several heterotrophic bacteria, such as Escherichia coli, Corynebacterium glutamicum, and Pseudomonas aeruginosa, can utilize l -lactate with the help of NAD-independent l -lactate dehydrogenase (l -iLDH, EC 1.1.2.3), which catalyzes the conversion of l -lactate into pyruvate14,15,16. For example, E. coli harbors the lactate operon, which is composed of the lldD (l -iLDH) and lldP (lactate permease) genes for l -lactate utilization as well as the lldR (regulatory protein) gene14.
Enzymes involved in l -lactate metabolism.
The present study aimed to develop a method for l -lactate consumption using a photosynthetic microorganism. Most cyanobacteria and microalgae do not possess genes for l -lactate metabolism and cannot utilize l -lactate. Therefore, the ability for l -lactate utilization was added to PCC 7002 by heterogeneous expression of the lldD and lldP genes from E. coli. The distribution of metabolic flux derived from l -lactate was determined through metabolome analysis. This study provides a perspective on l -lactate treatment by photosynthetic microorganisms and establishes a method to develop cyanobacteria with the ability to utilize l -lactate. These findings will be valuable to industries using animal cell cultures and would increase the feasibility of the CCC system.
l -Lactate has cytotoxic effects on animal cells10. In the present study, C2C12 cells were examined, and addition of l -lactate higher than 20 mM significantly decreased cell viability (Supplementary Fig. 1). To achieve a sustainable CCC system8 (Fig. 1), we aimed to develop a method for l -lactate consumption using a photosynthetic microorganism. The conservation of genes involved in l -lactate metabolism was first investigated in silico to examine the l -lactate utilization ability of photosynthetic microorganisms in nature (Fig. 2). In this investigation, cyanobacteria and microalgae harboring l -iLDH (EC 1.1.2.3), l -lactate oxidase (LOX, EC 1.1.3.2), or lactate 2-monoxygenase (LMO, EC 1.13.12.4) genes were identified using the Kyoto Encyclopedia of Genes and Genomes (KEGG) database17. l -iLDH and LOX convert l -lactate into pyruvate, and LMO converts l -lactate into acetate18. In contrast, l -nLDH (EC 1.1.1.27) synthesizes l -lactate from pyruvate reversibly or irreversibly19. Therefore, cyanobacteria and microalgae harboring LOX and LMO genes were not found. In addition, the l -iLDH gene is absent in most cyanobacteria and microalgae, except Aureococcus anophagefferens20, Crocosphaera watsonii21, Trichodesmium erythraeum22, and Rivularia sp.23, among which A. anophagefferens and T. erythraeum are known to cause harmful algal blooms. Thus, the present study found that l -lactate utilization genes are absent in most cyanobacteria and microalgae.
To experimentally examine the l -lactate utilization ability, several cyanobacteria and microalgae, i.e. Synechococcus sp. PCC 700224, Anabaena sp. PCC 712025, Arthrospira platensis NIES-3926, Chlamydomonas sp. KOR127, and Pavlova sp. OPMS 3054328, were cultured phototrophically in the presence of l -lactate. The growth of these cyanobacteria and microalgae, except for PCC 7120, was not suppressed by 20 mM l -lactate, which is nearly equivalent to the culture waste of animal cells. However, lactate concentration in the medium did not change during cultivation (Supplementary Fig. 2). These results suggest that few cyanobacteria and microalgae species in nature can utilize l -lactate. Therefore, genetic engineering should be a suitable approach for creating photosynthetic microorganisms capable of utilizing l -lactate.
To develop photosynthetic microorganisms capable of l -lactate utilization, this study introduced heterogenous genes into the marine cyanobacterium PCC 7002, which is tolerant to salinity of animal medium. Because several heterotrophic bacteria can grow using l -lactate due to l -iLDH14,15,16, the present study employed l -iLDH encoded by the E. coli lldD gene. The lldP gene encoding lactate permease was previously shown to improve d -lactate export in cyanobacteria such as PCC 7002 and Synechococcus elongatus PCC 794212,29,30. This study employed the lldP gene to enhance l -lactate uptake. The lldD and lldP genes were expressed in PCC 7002 cells using the constitutive trc promoter (Fig. 3A). These genetic elements were introduced into the ldhA gene site encoding d -LDH to prevent d -lactate synthesis from pyruvate by the native enzyme. Integration and complete segregation were confirmed using PCR (Supplementary Fig. 3).
Evaluation of the lldD/lldP-expressing cyanobacteria. (A) Genetic elements for l -lactate utilization. The ldhA (d-lactate dehydrogenase) gene in the pAQ7 plasmid of Synechococcus sp. PCC 7002 was replaced with the gentamicin resistance cassette (GmR) and codon-optimized NAD-independent l-lactate dehydrogenase (lldD) and lactate permease (lldP) genes from Escherichia coli. The lldD and lldP genes were constitutively expressed in the trc promoter region. The black boxes indicate homologous sequences used to introduce these genetic elements into the ldhA gene site. (B,C) Comparison of the lldD/lldP-expressing strains. Cyanobacteria were phototrophically cultured in the presence of 20 mM l -lactate, and the dry cell weight (DCW)-based biomass concentrations (B) and lactate concentration in the medium (C) were investigated. (D,E) Influence of temperature on l -lactate utilization. The cyanobacteria expressing both lldD and lldP were phototrophically cultured in the presence of 20 mM l -lactate at 30–40 °C, and DCW-based biomass concentrations (D) and lactate concentration in the medium (E) were investigated. Error bars indicate standard deviation of three replicate experiments.
To evaluate the l -lactate utilization ability, PCC 7002 and the recombinant strains were phototrophically cultured in the presence of 20 mM l -lactate. During the early stage of cultivation, the recombinant strains showed more enhanced cell growth than PCC 7002 (Fig. 3B). l -lactate concentration in the medium significantly decreased in the lldD-expressing strain, while it remained unchanged in PCC 7002 (Fig. 3C). Additional introduction of the lldP gene enhanced l -lactate consumption by the lldD-expressing strain, and as a result, 20 mM (1.8 g·L−1) of l -lactate was completely consumed in 9 days. Thus, the l -lactate utilization ability was successfully added to PCC 7002 using the lldD/lldP genes. These results indicate that both LldD and LldP proteins were functional in cyanobacteria and that lldP can contribute to l -lactate import.
To accelerate l -lactate consumption, the culture temperature of the lldD/lldP-expressing strain was examined. During the initial 4 days, biomass concentration was not significantly different at 30–40 °C (Fig. 3D). In contrast, higher temperatures resulted in higher l -lactate consumption, and 20 mM l -lactate was completely consumed in 7 days at 35–40 °C (Fig. 3E). This result indicates that l -lactate utilization by the lldD/lldP-expressing strain can be enhanced by elevated temperatures probably because this temperature range is suitable for these E. coli enzymes. Thus, we established a method to develop cyanobacteria with the l -lactate utilization ability. Addition of a functional l -iLDH would also be valuable in adding l -lactate utilization ability to microalgae.
In lldD/lldP-expressing cells, pyruvate synthesized by LldD is converted to other metabolites by intrinsic enzymes. To elucidate the distribution of the metabolic flux derived from l -lactate, metabolome analysis of lldD/lldP-expressing cells cultured in the absence and presence of l -lactate was performed. Lactate, pyruvate, and acetyl-CoA (AcCoA) accumulated in cells when supplemented with l -lactate (Fig. 4A). In addition, several metabolites of the tricarboxylic acid (TCA) cycle, that is, citrate, 2-oxoglutarate (2-OG), succinate, and malate, accumulated in the presence of l -lactate. These results indicate that the metabolic flux from l -lactate was largely distributed to the TCA cycle.
Metabolome analysis during l -lactate utilization. The lldD/lldP-expressing strain was phototrophically cultured in the absence and presence of 20 mM l -lactate at 30 °C for 7 days. (A) Intracellular metabolites in lldD/lldP-expressing cells. The solid and dotted lines represent single and multiple enzymatic steps, respectively. (B) Extracellularly released metabolites from lldD/lldP-expressing cells. Error bars indicate the standard deviation of three replicate experiments (*P < 0.05, **P < 0.01, Welch’s t test). 2-OG 2-oxoglutarate, 2-PGA 2-phosphoglyceric acid, 3-PGA 3-phosphoglyceric acid, AcCoA acetyl-CoA, CBB cycle Calvin–Benson–Bassham cycle, DCW dry cell weight, F6P fructose 6-phosphate, PEP phosphoenolpyruvate. Ru5P ribulose-5-phosphate, RuBP ribulose-1,5-bisphosphate, TCA cycle tricarboxylic acid cycle.
A significant intracellular accumulation of these metabolites should trigger their releases from lldD/lldP-expressing cells during l -lactate utilization. By analyzing the metabolites in the culture supernatant, we found that several metabolites increased extracellularly when supplemented with l -lactate (Fig. 4B). Extracellular levels of pyruvate, 2-OG, succinate, and malate in the lldD/lldP-expressing strain when supplemented with 20 mM l -lactate were 2,021.1, 496.7, 300.6, and 53.3 μM, respectively. The accumulation of intracellular metabolites by l -lactate utilization likely caused a significant release of these organic acids. A similar phenomenon, with elevated release of organic acids such as pyruvate and 2-OG, has been reported in glycogen-deficient cyanobacterial mutants31,32,33. Because 2-OG can be converted into glutamine, which is an essential and abundant amino acid in the medium for mammalian cell cultures34, the lldD/lldP-expressing strain may also be valuable for producing amino acids in animal cells.
To examine whether the photosynthetic activity of lldD/lldP-expressing cells was affected by l -lactate utilization, the cells were analyzed in the presence and absence of l -lactate. First, O2 evolution was analyzed on day 3 when the cells performed biomass production and l -lactate utilization (Fig. 3). The apparent O2 evolution rate measured under light conditions significantly decreased in the presence of l -lactate (Fig. 5A). The O2 consumption rate was measured in the dark and was found to be significantly increased when l -lactate was supplied to the medium. This might be due to the enhanced metabolic flux of the TCA cycle during l -lactate utilization (Fig. 4A) as the TCA cycle is the dominant source of NAD(P)H for respiratory electron transport35. The net photosynthetic O2 evolution rate was calculated by subtracting the O2 consumption rate from the apparent O2 evolution rate and was found to be almost the same in the presence or absence of l -lactate.
Photosynthetic activity during l -lactate utilization. lldD/lldP-expressing cells were phototrophically cultured in the absence and presence of 20 mM l -lactate at 30 °C for 3 days and then subjected to analyses of photosynthetic activity. (A) Oxygen evolution rate. The photosynthetic O2 evolution rate was calculated by subtracting the O2 consumption rate (dark) from the apparent O2 evolution rate (light). (B) 13C fraction of metabolites in the Calvin–Benson–Bassham (CBB) cycle. Newly synthesized metabolites from CO2 were 13C-labeled by incubating the cells with NaH13CO3 as the carbon source. Error bars indicate the standard deviation of three replicate experiments (*P < 0.05, **P < 0.01, Welch’s t test). 3-PGA 3-phosphoglyceric acid, DCW dried cell weight, Ru5P ribulose-5-phosphate, RuBP ribulose-1,5-bisphosphate.
To further examine photosynthetic activity, the CO2 fixation activity of lldD/lldP-expressing cells was analyzed by in vivo 13C labeling experiments. NaH13CO3 was added to the medium on day 3 to supply the lldD/lldP-expressing cells with 13CO2. After incubation for 0–20 min, the 13C fraction of metabolites in the Calvin–Benson–Bassham (CBB) cycle, which conducts photosynthetic CO2 fixation by ribulose 1,5-bisphosphate carboxylase/oxygenase (Rubisco), was analyzed. The de novo synthesis of 3-phosphoglyceric acid (3-PGA), ribulose-5-phosphate (Ru5P), and ribulose-1,5-bisphosphate (RuBP) from CO2 occurred even in the presence of l -lactate, although the 13C fraction of 3-PGA was slightly decreased (Fig. 5B). These results reveal that photosynthesis in the lldD/lldP-expressing cells continued even during l -lactate utilization. In the presence of l -lactate, the de novo synthesis of Ru5P was not changed (Fig. 5B), while its accumulation significantly increased (Fig. 4A). These results are contrasting but not necessarily conflicting because these experiments analyzed for distinct metabolic parameters at different time points. The higher growth rate of l -lactate-assimilating cyanobacteria than that of PCC 7002 (Fig. 3B) might be due to the simultaneous utilization of CO2 and l -lactate as carbon sources. Thus, this study established a method to consume l -lactate in animal cell cultures using photosynthetic cyanobacteria expressing the heterogenous lldD and lldP genes. The findings of this study will contribute to the development of a sustainable CCC system for the animal cell culture industry.
Cyanobacterium Synechococcus sp. PCC 7002 and the recombinant strains were phototrophically cultured in double-deck flasks on a BR-40LF bioshaker (TAITEC, Aichi, Japan). The upper stage of the flasks was supplemented with 70 mL of Medium A2 (8.30 × 10–3 M tris(hydroxymethyl)aminomethane, 1.76 × 10–2 M NaNO3, 3.10 × 10–1 M NaCl, 2.00 × 10–2 M MgSO4·7H2O, 2.50 × 10–3 M CaCl2·2H2O, 3.70 × 10–4 M KH2PO4, 8.10 × 10–3 M KCl, 8.90 × 10–5 M Na2EDTA·2H2O, 3.00 × 10–5 M FeCl3·6H2O, 5.50 × 10–4 M H3BO3, 2.20 × 10–5 M MnCl2·4H2O, 2.30 × 10–6 M ZnCl2, 2.10 × 10–7 M Na2MoO4·2H2O, 1.20 × 10–8 M CuSO4·5H2O, 5.10 × 10–8 M CoCl2·6H2O, and 3.00 × 10–9 M vitamin B12), containing 40 mg·L−1 gentamicin when necessary. To investigate l -lactate utilization, 20 mM l -lactate (Sigma-Aldrich, St. Louis, MO, USA) and 20 mM NaOH were added to the medium. The lower stage of the flasks was supplemented with 50 mL of 2 M K2CO3/KHCO3 solution, which adjusted the CO2 gas concentration to 2% (v/v). Cells were inoculated at an optical density of 750 nm (OD750) = 0.1 and cultured under continuous illumination with white fluorescent lamps at 100 µmol photons·m−2·s−1 at 30 °C with rotary shaking at 100 rpm24.
The pUC118-based vectors, harboring the trc promoter and homology arms for the ldhA gene (SYNPCC7002_G0164) in the pAQ7 plasmid of Synechococcus sp., were used to introduce the lldD and lldP genes from E. coli via homologous recombination. The codon-optimized genes of LldD (NP_418062.1) and LldP (NP_418060.1) were prepared by the Genscript gene synthesis service and cloned into the vector using the In-Fusion HD Cloning Kit (Takara Bio USA, Inc., Mountain View, CA, USA). PCC 7002 was transformed as previously described24. Integration and complete segregation were confirmed by PCR using the specific primer pair 5′-AGACATTTCCCACAGACCACATCAAATTA-3′ and 5′-GGATCAATTTACGTCTTTGTTGGCGCA-3′.
Each culture was centrifuged at 8000×g for 5 min. The supernatant was filtered using a Shim-pack SPR-Pb column (Shimadzu, Kyoto, Japan) and analyzed using a high-performance liquid chromatography system (Shimadzu) equipped with an Aminex HPX-87H column (Bio-Rad Laboratories, Hercules, CA, USA). l -Lactate (Sigma-Aldrich) was used as the quantitative standard to determine the lactate concentration using a calibration curve.
To prepare intracellular metabolites, a culture broth containing cells equivalent to 5 mg dry weight was mixed with four times the volume of 32.5% (v/v) methanol pre-cooled at − 30 °C. The mixture was centrifuged at 8000×g for 3 min at 4 °C. After complete removal of the supernatant, the cells were washed with 20 mM ammonium carbonate once and immediately resuspended in 1 mL of pre-cooled methanol containing 37.5 μM l -methionine sulfone and 37.5 μM piperazine-1,4-bis(2-ethanesulfonic acid) (PIPES) as internal standards. The cell suspension (500 μL) was added to 200 μL ultrapure water and 500 μL chloroform pre-cooled at 4 °C and then vigorously mixed using vortexing for 30 s. After centrifugation at 14,000×g for 5 min at 4 °C, the aqueous layer was collected and filtered using an Amicon Ultra-0.5 Centrifugal Filter Unit UFC5003BK (Merck Millipore, Burlington, MA, USA) by centrifugation at 14,000×g at 4 °C. The sample (300 μL) was dried under vacuum using a centrifugal evaporator CEV-3100 (EYELA, Tokyo, Japan) and resuspended in 20 µL of ultrapure water. To prepare extracellular metabolites, the culture was centrifuged at 8000×g for 5 min. The supernatant (500 μL) was mixed with 500 μL chloroform pre-cooled at 4 °C by vortexing. After centrifugation at 14,000×g for 5 min at 4 °C, the upper layer was collected and filtered using UFC5003BK (Merck Millipore) as described above. Next, 400 μM l -methionine sulfone and 400 μM PIPES were added as internal standards. The intracellular and extracellular samples were subjected to capillary electrophoresis time-of-flight mass spectrometry (CE-TOFMS) using a G7100 CE and G6224AA liquid chromatography-mass selective detector (LC/MSD) TOF system (Agilent Technologies, Santa Clara, CA, USA)24.
Cells were cultivated for 3 days under the conditions described above. To analyze the O2 evolution rate, cultured cells were harvested, centrifuged at 8000×g for 5 min, and resuspended in fresh Medium A2 with or without 20 mM l -lactate to adjust the cell density to OD750 = 5.0. The O2 concentration in the cell suspension was measured using an oxygen electrode (Hansatech, King’s Lynn, UK). During the measurements, the cell suspension was maintained at 30 °C and mixed using a magnetically controlled microstirrer. The O2 consumption rate of the cells was determined by measuring the O2 concentration in the dark, while the apparent O2 evolution rate was determined under illumination with a red LED light (200 μmol photons·m−2·s−1). The photosynthetic O2 evolution rate was calculated by subtracting the O2 consumption rate from the apparent O2 evolution rate24.
To investigate carbon fixation from CO2, in vivo 13C labeling of metabolites in the CBB cycle was performed. After 3 d of cultivation, the cell culture was added to 25 mM NaH13CO3 as a carbon source and incubated under illumination with white fluorescent lamps (100 μmol photons·m−2·s−1). After labeling for 0–20 min, the intracellular metabolites were analyzed as described above24. The ratio of 13C in the total carbon (13C fraction) of the metabolite was determined based on the shifts between the 12C and 13C mass spectra.
Data in this study are represented as mean ± standard deviation of three replicate experiments. Statistical significance was determined by Welch’s t test.
The data supporting the findings of this study are available from the corresponding author upon reasonable request.
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We thank Ms. Aya Narita and Ms. Mami Matsuda for their technical assistance. This study was financially supported by the Cabinet Office, Government of Japan, Moonshot Research and Development Program.
Engineering Biology Research Center, Kobe University, 1-1 Rokkodai, Nada, Kobe, 657-8501, Japan
Yuichi Kato, Kosuke Inabe, Akihiko Kondo & Tomohisa Hasunuma
Graduate School of Science, Technology and Innovation, Kobe University, 1-1 Rokkodai, Nada, Kobe, 657-8501, Japan
Yuichi Kato, Akihiko Kondo & Tomohisa Hasunuma
Institute of Advanced Biomedical Engineering and Science, TWIns, Tokyo Women’s Medical University, 8-1 Kawada, Shinjuku, Tokyo, 162-8666, Japan
Yuji Haraguchi & Tatsuya Shimizu
Department of Chemical Science and Engineering, Graduate School of Engineering, Kobe University, 1-1 Rokkodai, Nada, Kobe, 657-8501, Japan
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Y.K.: Conceptualization, investigation, methodology, writing–original draft. K.I.: Investigation. Y.H.: Conceptualization, writing–review and editing. T.S.: Conceptualization, project administration. A.K.: Supervision. T.H.: Project administration, writing–review and editing.
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Kato, Y., Inabe, K., Haraguchi, Y. et al. l -Lactate treatment by photosynthetic cyanobacteria expressing heterogeneous l -lactate dehydrogenase. Sci Rep 13, 7249 (2023). https://doi.org/10.1038/s41598-023-34289-3
DOI: https://doi.org/10.1038/s41598-023-34289-3
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