Assessment of optimal growth conditions for biomass and exopolysaccharides production in the thermotolerant cyanobacterium Phormidium sp. ETS-05

DOI: https://doi.org/10.21203/rs.3.rs-2697087/v1

Abstract

Phormidium sp. ETS-05 is one of the target cyanobacteria species conferring anti-inflammatory properties to the therapeutic muds applied by spas of the Euganean Thermal District (Italy) to treat arthro-rheumatic pathologies. The beneficial mud is prepared by spas following a traditional method, called maturation, leading to the growth of a specific microbiota on natural raw clay irrigated by flowing thermal water at 37–47°C for about two months. The effectiveness of the mud is related to heat, to electrolytes and to bioactive molecules synthetized by the microbiota. A clear role in the anti-inflammatory activity of the muds has been demonstrated for the exopolysaccharides, EPS, produced by the entire microbiota and Phormidium sp. ETS-05. Considering the interest in this species, we assessed its optimal growth conditions to obtain the higher EPS production in relation to temperature, light spectra and intensity and nitrogen availability. Biomass and pigments production were also taken in consideration, as other high value compounds can be obtained in parallel with EPS. We found the exposure to a temperature of 45°C under white light at 100 µmol photons m− 2 s− 1 as optimal to reach the higher biomass (1.13 g L− 1) and an average production of 75 mg gDW−1 phycocyanin and of 150 mg gDW−1 EPS for Phormidium sp. ETS-05 cultured in lab-scale photobioreactors for 9 days. Putative genes linked with EPS assembly and export have been also identified in its genome, some of which have been investigated for their expression levels, opening to the possibility of biotechnologically boost EPS production.

1. Introduction

Cyanobacteria are ubiquitous organisms, present in different ecosystems including extreme environments, even characterized by very high temperatures (Harwood and Guschina 2009). To thrive in these habitats, they have developed great adaptability to varying conditions and several mechanisms to cope with different stressors (Kumar et al. 2018), leading to an extremely versatile metabolism. Cyanobacteria are indeed able to synthesize a vast range of primary and secondary metabolites, making them a promising source of bioactive compounds, food and feed supplements, biopolymers, biofuels, biofertilizers, and can also be used for bioremediation, wastewater treatments and CO2 sequestering processes (Patel et al. 2019). Cyanobacteria are considered as promising candidates for use in bioindustrial applications (Ducat et al. 2011) thanks to their low requirements needed for growth (sunlight, CO2, water with few mineral nutrients) and the capability to increase the production of compound of interest changing the growth parameters used.

Among hot environments, volcanic environments, hydrothermal vents, and hot springs are inhabited by thermotolerant, thermophilic, and hyper thermophilic microorganisms (Harwood and Guschina 2009). In hot springs, they commonly create microbial communities forming mats that are composed of primary producers, photoautotrophs (cyanobacteria, purple phototrophs, green phototrophs), and chemolithoautotrophs (Franks and Stolz 2009).

The Euganean Thermal District (Padova, Italy) is an important thermal pole in Europe and is renowned for both thermal water treatments and pelotherapy (i.e. mud therapy). These are performed using natural resources of the territory: thermal water gushing at an average temperature of 75°C and clay collected from local thermal lakes. The efficacy of mud therapies relies on thermal, mechanical, and biochemical factors (Fioravanti et al. 2011) that are both inorganic and organic compounds accumulated by a specific microbiota that grows during mud maturation starting from raw clay bathed with thermal water (Gris et al. 2020). The peculiarity of the Euganean mud lies on the growth of microorganisms during the maturation process, among which cyanobacteria plays a leading role composing up to 30% of the total microbiota (Gris et al. 2020). Anti-inflammatory and antioxidant activity of polysaccharides extracted from the therapeutic mud were recently demonstrated by in vivo tests using zebrafish as model organism (Zampieri et al. 2022). Among cyanobacteria, Phormidium sp. ETS-05 (Ceschi Berrini et al. 2004) hereafter referred as ETS-05, is the most abundant species (41% on average) up to 47°C (Gris et al. 2020). Contribution of ETS-05 to the therapeutic activity of the Euganean mud have been investigated in vitro and in vivo revealing that its exopolysaccharides (EPS), have anti-inflammatory activity (Zampieri et al. 2020).

EPS can be found in high concentration in therapeutic muds, linked to the microbial cell surface or released into the environment, acting as boundary between cells and their surroundings with several purposes: creation of biofilms, establishment of symbiosis, protection against desiccation and UV, nutrients sequestration (Pereira et al. 2009). EPS are characterized by peculiar biological activities (anti-inflammatory, antiviral, antioxidant, antibacterial, immunostimulant) and physico-chemical properties (viscosity, water retention) that make them interesting for several fields: pharmaceutical, nutraceutical, cosmetic, food and agriculture (Laroche 2022).

Mechanism responsible for EPS synthesis and release is relatively conserved throughout bacteria, even though limited information is available for cyanobacteria (Pereira et al. 2013). Three biosynthetic pathways have been described: Wzy-dependent, ABC transporter-dependent, Synthase-dependent. For the first two pathways, two protein families are fundamental: polysaccharide copolymerase (PCP) that are respectively Wzc and KpsE, and outer membrane polysaccharide export (OPX) represented by Wza and KpsD proteins. OPX proteins possess conserved domains: a polysaccharide export sequence (PES or poly_export domain) and a soluble ligand-binding beta-grasp domain (SLBB) (Pereira et al. 2013). In Synthase-dependent pathway, polysaccharides are simultaneously assembled and exported by synthase Alg8 (Pereira et al. 2015). In 2013 was hypothesized a polysaccharide secretion system linked with hormogonia formation and gliding motility in Nostoc punctiforme ATCC 29133 (Risser and Meeks 2013; Khayatan et al. 2015). Hormogonia trichomes are functionally and morphologically diverse from vegetative filaments, being generally involved in dispersal events and shorter (Herdman and Rippka 1988). Hormogonium polysaccharides (HPS) synthesis gene set (hps) was identified, interestingly a set of putative Hps proteins have been associated as members of the Wzy-dependent pathway (Zuniga et al. 2020a).

Different strategies can be applied to induce high EPS synthesis in different strains such as nutrient starvation (N, P, Mg2+, Ca2+) or stresses (high light, temperature, salinity). However, the best condition to increased EPS yield is rather species-specific as was nicely described by Pereira et al. (Pereira et al. 2009) and Laroche (Laroche 2022). Together with EPS, other high value compounds can be simultaneously produced such as water- and lipid-soluble pigments. Phycobiliproteins and in particular phycocyanin (PC) have several bioactive properties: antioxidant, anticancer, anti-inflammatory, anti-diabetes, neuroprotective, anti-obesity (Pagels et al. 2019).

In this study ETS-05 was grown under different conditions. Temperatures (30, 35, 40, 45, 50°C), light spectra (white, blue, green, yellow, red lights), light intensities (20, 50, 75, 100, 125, 150, 200, 400 µmol photons m− 2 s− 1) and nitrogen availability were tested to evaluate both biomass production and compounds of interest synthesis, focusing on EPS and PC. Optimal parameters resulted to be 45°C, 100 µmol photons m− 2 s− 1 of white light and with the presence of the nitrogen source (NaNO3) in the medium. Higher biomass obtained corresponded to 1.13 g L− 1 of biomass in 9 days of cultivation, together with an average of 150 mg gDW−1 of EPS and 75 mg gDW−1 of PC. In addition, genes linked with EPS synthesis have been found through a bioinformatic research in ETS-05 genome. For some of these genes, wza, wzc, a gene coding for a protein involved in polysaccharide export (ps_ex) and a gene related to the HPS synthesis (hrmK), correlation between their expression level and the release of polysaccharides by ETS-05 was verified via Real-Time qPCR analysis.

2. Materials & Methods

2.1 Cyanobacterium strain used and maintenance

Cultures of Phormidium sp. ETS-05 were available in the laboratory as result of previous collaborations with Pietro d’Abano Thermal Studies Center (Ceschi Berrini et al. 2004). Organism was maintained in flasks in a thermostatic chamber at 30°C (± 1°C) and 10 µmol photons m− 2 s− 1 of white light with no photoperiod. Medium for maintenance and growth of the cyanobacterium was BG11 (Rippka et al. 1979). For the nitrogen starvation experiments, BG110 medium was used (Rippka et al. 1979), which lacks nitrate source.

2.2 Experimental settings

Experiments culturing ETS-05 under diverse light spectra were conducted using cell culture flasks. The only source of light was given by stripes of LEDs covered in colored filters and spectra were assessed using LI-COR LI-180 spectrometer (Ecosearch Srl, Italy) (light spectra are presented in Fig. S1). For each light, 30 µmol photons m− 2 s− 1 were obtained. Temperature was maintained constant at 30°C.ETS-05 was exposed to the lights for 9 days starting from inocula cultivated for 10 days in white light and diluted to the starting concentration of 0.2 g/L. Experiments were conducted with 4 biological replicates.

For the subsequent tests, organism was cultivated using the photobioreactor Multi-cultivator MC-1000 OD (Photon Systems Instruments, Czech Republic) system. ETS-05 was pre-adapted to the photobioreactor system. Cultures were grown for 10 days starting from and optical density (OD) at 750 nm of 0.4 at 30°C and 50 µmol photons m− 2 s− 1 of constant light. LEDs spectrum (cold white light) is available in Multi-cultivator MC-1000 OD manual (www.psi.cz). A constant flux of filtered atmospheric air bubbles kept the filament in suspension in the medium. Cells were firstly centrifuged to eliminate residues of released compounds present in the medium that could have altered measurements or growth. Inocula were obtained resuspending the cultures to an OD750nm of 0.2 with a final volume of 80 mL for each tube. Growth curves for testing different temperatures were performed at 50 µmol photons m− 2 s− 1, while light intensities curves were completed at 45°C. 6 biological replicates were performed for each condition tested.

For tests relative to nitrogen starvation, 45°C and 100 µmol photons m− 2 s− 1 were used. Two-step cultivation was performed to boost growth of the organism. After 9 days of growth in BG11, cells were centrifugated and resuspended in either BG11 or BG110. Experiments lasted for additional 9 days and were conducted with 4 biological replicates.

2.3 Growth and biomass quantification

Growth was assessed for 9 days. OD750nm was measured using a spectrophotometer, sampling at 0, 2, 4, 7 and 9 days. Biomass was also assessed as dry weight of 5 mL of culture using 0.45 µm filters. Dry weight was measured at the starting and ending point (day 9) of the experiments.

2.4 In vivo absorption spectra

To assess light absorption features of ETS-05, in vivo spectra were measured. Cells were centrifuged at 3000 g for 5 minutes and pellets were carefully homogenized to disaggregate cells. After resuspending, samples were analyzed at spectrophotometer using quartz cuvettes. According to literature (Gan et al. 2014), opaque sides of cuvettes were crossed by the ray, to correct for scattering.

2.5 Chlorophyll a, carotenoids and phycobiliproteins extraction and quantification

For the extraction of lipophilic pigments, organism was sampled at 0, 2, 4, 7 and 9 days after growth and were centrifuged at 20000 g. Pellet was then resuspended in N, N-dimethylformamide (Sigma-Aldrich, USA) and incubated at 4°C for 24 hours in the dark. Supernatant obtained from centrifugation was then analyzed spectrophotometrically using the absorption spectrum from 350 to 750 nm. Chlorophyll a and carotenoids concentrations were calculated according to the equations from (Moran 1982) for chlorophyll a and (Chamovitz et al. 1993) for carotenoids:

$$\text{C}\text{h}\text{l}\text{o}\text{r}\text{o}\text{p}\text{h}\text{y}\text{l}\text{l} a \left({\mu }\text{g} {\text{m}\text{L}}^{-1}\right)={\text{A}}_{664}\times 11.92$$
$$\text{C}\text{a}\text{r}\text{o}\text{t}\text{e}\text{n}\text{o}\text{i}\text{d}\text{s} \left({\mu }\text{g} {\text{m}\text{L}}^{-1}\right)={\text{A}}_{461}-(0.046\times {\text{A}}_{664})\times 4$$

where A461 A664 are the absorbance values at 461 and 664 nm respectively.

For the extraction of hydrophilic pigments, samples collected at the beginning and at the end (9 days) of the growth curves were centrifuged at 20000 g to remove residual traces of medium. An equal volume of glass beads (150–212 µm) was then added to the pellet with cold phosphate buffer (NaCl 0.15 M, Na2HPO4 0.01 M, pH 9). Cells were disrupted with three cycles of bead beater (3500 OPM, 30 seconds) alternated with 30 seconds in ice. Supernatant obtained after centrifugation (20000 g, 4°C) was collected in a clean tube and the pellet resuspended cold phosphate buffer. This step was repeated until the obtainment of a transparent supernatant. The accumulated supernatant was centrifuged again to eliminate eventual remaining cells or membranes. The whole spectrum was measured at the spectrophotometer from 350 to 750 nm. As reported in (Bennett and Bogorad 1973) for phycocyanin (PC) and allophycocyanin (APC) and in (Kaplan et al. 1986) for phycoerythrocyanin (PEC):

$$\text{P}\text{h}\text{y}\text{c}\text{o}\text{c}\text{y}\text{a}\text{n}\text{i}\text{n} \left(\text{m}\text{g} {\text{m}\text{L}}^{-1}\right)={[\text{A}}_{615}-(0.474\times {\text{A}}_{652})]/5.34$$
$$A\text{l}\text{l}\text{o}\text{p}\text{h}\text{y}\text{c}\text{o}\text{c}\text{y}\text{a}\text{n}\text{i}\text{n} \left(\text{m}\text{g} {\text{m}\text{L}}^{-1}\right)=[{\text{A}}_{652}-\left(0.208\times {\text{A}}_{615}\right)]/5.09$$
$$\text{P}\text{h}\text{y}\text{c}\text{o}\text{e}\text{r}\text{y}\text{t}\text{h}\text{r}\text{o}\text{c}\text{y}\text{a}\text{n}\text{i}\text{n} \left(\text{m}\text{g} {\text{m}\text{L}}^{-1}\right)={\text{A}}_{572}-(0.619\times {\text{A}}_{612})+(0.088\times {\text{A}}_{647})/5.775$$

where A572, A612, A615, A647 and A652 correspond to absorbance values at 572, 612, 615, 647 and 652 nm. Values of Chlorophyll a, carotenoids and phycobiliproteins concentrations were then referred to the biomass expressed as dry wight.

2.6 Exopolysaccharides’ extraction and quantification

EPS were collected at the beginning of the experiment and after 9 days, corresponding to the final point. Method followed is described in (Gris et al. 2017). Quantification was performed using sample, phenol 5% and sulfuric acid in the ratio 1:1:5 according to Dubois method (DuBois et al. 1956). Optical density at 488 nm was measured and EPS concentration was referred to a glucose calibration curve. EPS concentration was correlated to the biomass of the cultures express as dry weight.

2.7 Optical microscopy and Transmission Electron Microscopy (TEM) analyses

ETS-05 exposed to different light intensities were observed through light microscopy (Axiophot, Zeiss, equipped with a Leica EC3 camera) and images were acquired moving in the diagonals of the slides. 10X magnification was used to clearly see the filaments in their whole extension. For each condition, 100 filaments were measured in their length using the software ImageJ (Schneider et al. 2012).

TEM images were acquired for samples at the starting point and cultivated for 9 days at 45°C under 25 or 100 µmol photons m− 2 s− 1 of white light. According to La Rocca et al (La Rocca et al. 2015), cells were centrifugated (10 min, 17000 g) and fixed overnight at 4°C in 3% glutaraldehyde in 0.1 M sodium cacodylate buffer (pH 6.9) and post-fixed for 2 h in 1% osmium tetroxide in the same buffer. The samples were dehydrated in a graded series of ethyl alcohol and propylene oxide and embedded in Araldite. Ultrathin sections (80–100 nm) were cut with an ultramicrotome (Ultracut; Reichert-Jung, Vienna, Austria) and stained with lead citrate and uranyl acetate. Analysis was conducted under a transmission electron microscope (Tecnai G2; FEI, Hillsboro, Oregon) operating at 100 kV.

2.8 Real-Time qPCR analysis and research of genes of interest

Samples collected at the beginning of the experiment and after 2 days were centrifuged at 10000 g and pellets were stored at -20°C. Glass beads (acid-washed, 150–212 µm, Sigma-Aldrich) and TRI Reagent® (Sigma-Aldrich) were added to the frozen pellets and cells were disrupted with 3 cycles of bead beater (10 seconds, 3000 OPM) alternated with store in ice for 30 seconds. Chloroform, isopropanol, and ethanol 75% were subsequently used to complete the extraction. RNA was concentrated and purified using RNA Clean and Concentrator™ (Zymo Research, USA) and cDNA was obtained using RevertAid Reverse Transcriptase (Thermo Fisher Scientific, USA). Real-Time qPCRs were performed in a CFX384 Touch Real-Time PCR Detection System (Bio-Rad Laboratories, USA). Primer sequences are reported in Table S1. Data were normalized to the expression of gyrB to standardize the results by eliminating variation in cDNA quantity and quality. The cycling parameters were 95°C for 10 min, followed by 45 cycles at 95°C, annealing (60°C) and extension for 30 s. No amplification products were observed in negative controls and no primer-dimer formations in the control templates. qPCR results were analyzed using the ΔΔCt method using the Bio-Rad CFX Manager software version 3.1 (Bio-Rad Laboratories). Three biological replicas of the experiments were performed, with technical triplicates for each reaction.

ETS-05 genome was previously submitted as BioProject PRJNA622676 (Gris et al. 2020), available in NCBI (NIH). Nucleotide BLAST and tBLASTn (NIH) were used to search for genes of interest. Operon-mapper (Taboada et al. 2018) was utilized to implement or confirm the annotation described in Gris et al. 2020. Pfam (Mistry et al. 2021) and InterPro (Paysan-Lafosse et al. 2022) were used to identify protein families.

2.9 Statistical analysis

Statistical analyses were performed using GraphPad Prism (9.4.1, GraphPad Software, USA). Ordinary One-way ANOVA with Tukey’s multiple comparison test was used for all experiments. Exception was made for the nitrogen starvation test in which only two groups of data were considered, therefore Two-tailed Unpaired t test was applied. P values are reported in figures or tables. All the graphs were created with GraphPad Prism.

3. Results

3.1 Growth of ETS-05 under different light spectra

Preliminary analysis was conducted exposing the organism to different lights, enriched in the wavelengths of blue, green, yellow, and red and compared to white light spectra. After 9 days of growth, higher biomass production, reported as dry weight, was achieved under white, yellow, and red light (Fig. 1a). Slightly lower values were observed in green light and a drastic impaired growth in blue light, reaching a mean dry weight of only 0.25 g L− 1. No appreciable difference could be seen in the in vivo absorption spectra (Fig. S2), suggesting that the organism did not activate any kind of chromatic acclimation (Hirose et al. 2019; Sanfilippo et al. 2019). Considering chlorophyll a, carotenoids, and phycobiliproteins content (Table 1) lower quantities were obtained when cells were exposed to blue light, while no substantial difference was noted for the other lights. Similar results were obtained also for EPS production (Fig. 1b), with blue light being the less interesting for these compounds production. Excluding blue lights in which not only growth but also production of pigments and EPS were lower, no statistically significant difference was observed between other conditions for the mentioned parameters. Following experiments were therefore conducted using white light.

Table 1

Quantification of biomass as dry weight and of extracted pigments after 9 days of growth of ETS-05 exposed to different light spectra. Concentrations are referred to the dry weight. Higher values are indicated in bold. Means ± standard deviations are reported. APC: allophycocyanin; PC: phycocyanin; PEC: phycoerythrocyanin; Chl a: chlorophyll a; Car: carotenoids
 

Biomass

(g L− 1)

APC

PC

PEC

Chl a

Car

Chl a/Car
 

(mg gDW−1)

White

0.57 ± 0.04

51.8 ± 3.5

118.6 ± 5.3

13.0 ± 2.7

15.1 ± 3.9

2.4 ± 0.6

6.1

Blue

0.25 ± 0.07

19.7 ± 9.5

71.5 ± 24.6

4.9 ± 2.3

12.5 ± 5.4

1.7 ± 0.7

7.3

Green

0.42 ± 0.1

34.1 ± 9.3

133.4 ± 3.7

9.7 ± 1.9

14.0 ± 2.7

2.2 ± 0.6

7.0

Yellow

0.51 ± 0.1

39.3 ± 3.3

97.5 ± 10.2

8.8 ± 3.3

14.1 ± 1.3

2.3 ± 0.2

6.2

Red

0.53 ± 0.04

42.3 ± 12.6

112.7 ± 11.6

10.9 ± 4.7

13.1 ± 3.7

1.9 ± 0.6

6.8

3.2 Assessment of the temperature optimum for growth and production of biomolecules

Temperatures from 30 to 50°C were tested. Biomass growth reported as Log OD750nm (Fig. 2a) and dry weight (Table 2), did not changed between 30, 40 and 45°C. A drastic impairment in growth was observed for the higher temperature tested, 50°C, causing the death of the organisms after 4 days. EPS (Fig. 2b) obtained from the supernatant at the end of the growth curves were quantified and were directly correlated to the temperature. Higher value of 48 mg gDW−1 was reached at 45°C. Phycocyanin, the most abundant pigment produced by ETS-05, was quantified at the end of the experiments. Its concentration increased up to 40°C (222 mg gDW−1), while it lowered by half at 45°C (115 mg gDW−1). 50°C condition was not evaluated at 9 days since no viable cell was present in culture, as can be appreciated by the whitish color of tube 50 in Fig. 2a.

Phycobiliprotein content increased with the temperature, in parallel with the concentrations of chlorophylls and carotenoids (Table 2). Lipid-soluble pigment concentrations increased in time in a similar way among the conditions evaluated (Fig. S3), and no difference was assessed in the Chl a/Car ratio, indicating that these pigments composition is not influenced by the temperatures tested.

ETS-05 can be ascribed to mesophilic or lower thermophilic bacteria having the optimum temperature for growth between 40 and 45°C.

Table 2

Quantification of biomass as dry weight and of extracted pigments after 9 days of growth at the tested temperatures. Concentrations are referred to the dry weight. Higher values are indicated in bold. Means ± standard deviations are reported. APC: allophycocyanin; PC: phycocyanin; PEC: phycoerythrocyanin; Chl a: chlorophyll a; Car: carotenoids

°C

Biomass

(g L− 1)

APC

PC

PEC

Chl a

Car

Chl a/Car

(mg gDW−1)

30

0.93 ± 0.01

48.2 ± 9.1

139.7 ± 16.2

3.8 ± 1.1

12.9 ± 1.1

2.4 ± 0.1

5.7

35

0.92 ± 0.02

56.0 ± 4.5

182.1 ± 13.2

17.1 ± 3.3

15.4 ± 1.4

3.1 ± 0.3

5.4

40

0.94 ± 0.01

52.9 ± 3.7

221.8 ± 9.9

22.5 ± 4.8

22.9 ± 2.3

4.3 ± 0.4

5.3

45

0.95 ± 0.07

38.1 ± 9.2

114.5 ± 18.9

21.2 ± 4.9

19.9 ± 2.6

3.7 ± 0.7

5.4

3.3 Analysis of growth under different light intensities and nutrients

Considering previous results obtained, further experiments were conducted at 45°C, with the aim of gaining the higher biomass together with the higher quantity of EPS in the supernatant. Increasing light intensities were tested from 25 to 400 µmol photons m− 2 s− 1. Lowest and highest light tested both determined a reduction in the growth of the cultures (Fig. 3a). No statistical difference was detected between 50, 75, 100, 125, 150 and 200 µmol photons m− 2 s− 1 for both OD750nm and biomass measured as dry weight (Table 3), with 100 µmol photons m− 2 s− 1 reaching higher values. EPS production (Fig. 3b) increased in parallel with the increasing light, with lights 75 and 100 reaching 3 times (average of 150 mg gDW−1) the EPS produced at 25 and 50 µmol photons m− 2 s− 1 (average of 50 mg gDW−1) while a 5-fold increase was measured for 125, 150 and 150 µmol photons m− 2 s− 1 (average of 250 mg gDW−1). The values reached at 400 µmol photons m− 2 s− 1 (430 mg gDW−1) could have been misrepresented by the presence of cellular polysaccharides released by dead cells. The presence of this substantial quantity of EPS could otherwise represent a response to the stress condition caused by high light. Phycocyanin quantification showed the opposite trend, with augmented production at lower light intensities. Indeed, at 25 µmol photons m− 2 s− 1 higher quantity corresponding to 116 mg gDW−1, drastically dropping to only 14 mg gDW−1 at 25 µmol photons m− 2 s− 1. The difference in pigments content is reflected in the coloration of the cultures from a macroscopic point of view.

Considering all the quantified pigments (Table 3), phycobiliproteins showed the higher variability according to the condition tested. Allophycocyanin aside, which decreased 2 or 4 times from 25 to 400 µmol photons m− 2 s− 1, phycocyanin and phycoerythrocyanin were the most variable, with a 10-fold change, implying the leading role of these molecules in the response to the lights given. Chlorophyll a and carotenoids contents were more stable across the intensities tested, decreasing mainly at 200 and 400 µmol photons m− 2 s− 1. These pigments quantity increased for each light intensity tested for the duration of the experiments in a similar way (Fig. S4), correlating with the increase in time of the optical density. The ratio between these two classes of pigments was lower at the extreme light intensities tested (25 and 400 µmol photons m− 2 s− 1) mostly due to the smaller quantity of chlorophylls.

100 µmol photons m− 2 s− 1 was established as optimal for ETS-05, reaching the higher biomass and both an average phycocyanin and EPS production.

Table 3

Biomass produced and pigment content after 9 days of growth under different light intensities (from 25 to 400 µmol photons m− 2 s− 1. Concentrations of pigments are referred to the dry weight. Higher values are highlighted in bold. Means ± standard deviations are reported. APC: allophycocyanin; PC: phycocyanin; PEC: phycoerythrocyanin; Chl a: chlorophyll a; Car: carotenoids
 

Biomass

(g L− 1)

APC

PC

PEC

Chl a

Car

Chl a/Car
 

(mg gDW−1)

25

0.39 ± 0.16

32.1 ± 3.1

116.7 ± 14.3

12.4 ± 2.1

9.6 ± 0.1

2.3 ± 0.5

4.3

50

0.76 ± 0.14

33.6 ± 1.9

106.7 ± 10.1

20.7 ± 4.1

11.9 ± 1.2

2.8 ± 0.4

4.8

75

0.89 ± 0.38

25.5 ± 2.4

79.7 ± 2.6

15.7 ± 2.8

10.9 ± 0.8

2.1 ± 0.3

5.7

100

1.13 ± 0.32

26.7 ± 3.2

72.5 ± 3.5

16.7 ± 2.6

10.6 ± 0.5

2.2 ± 0.4

5.3

125

0.63 ± 0.10

15.1 ± 2.3

52.3 ± 8.2

3.6 ± 1.3

9.3 ± 0.8

2.1 ± 0.5

4.9

150

0.71 ± 0.10

16.9 ± 2.4

51.3 ± 6.9

3.2 ± 0.2

9.7 ± 1.0

2.1 ± 0.2

4.6

200

0.75 ± 0.06

12.3 ± 3.7

31.9 ± 7.4

2.4 ± 0.5

7.9 ± 2.5

1.8 ± 0.4

4.3

400

0.55 ± 0.11

7.3 ± 1.2

14.2 ± 1.2

0.7 ± 0.1

4.6 ± 0.6

1.6 ± 0.5

3.1

Having determined growth optima for both temperature and light intensity, to boost EPS release different medium composition were tested. Salt exposure led to cells death after 2–4 days even at the lower concentration tested of 0.01 M, indicating that the stress caused was too detrimental for ETS-05.

To assess the effect of nitrogen on EPS production, knowing that ETS-05 is not able to fix atmospheric nitrogen (Ceschi Berrini et al. 2004), BG110 was used. After a preliminary experiment performed using optima parameters found, testing in parallel medium with or without NaNO3, the absence of the nutrient was verified to prevent its growth. A two-step growth was then examined (Fig. S5), using as starting point biomass grown for 9 days in ideal conditions, and refreshed then in the two different media. After 4 days of comparable growth, absence of NaNO3 caused a decline in the biomass. This led to a reduction in both EPS and PC synthesis. Similar results were obtained for all pigments quantified (Table S6). Therefore, cultivation of ETS-05 in absence of the nitrogen source was not improved, considering biomass and more importantly EPS production.

3.4 Light intensity affects filament length and hormogonia formation

To further characterize the response of the ETS-05 to the different lighting conditions, cultures were observed under light microscopy. Cells were observed after 4 days of growth, in the exponential phase. A difference in the aspect of the cultures was observed, with the presence of shorter filaments in lights higher than 100 µmol photons m− 2 s− 1. Trichomes were measured in their length (Fig. S6). At lower light intensities (Fig. 4a), filaments were longer with a mean length of 770 µm at 25 µmol photons m− 2 s− 1 and 580 µm at 50 and 75 µmol photons m− 2 s− 1. ETS-05 in these cases reached even a length of more than 1500 µm. At light intensities higher than 100 µmol photons m− 2 s− 1 mean length resulted of 160 µm, with filaments as short as 10–20 µm (corresponding to 5–10 cells per filament).

For all the intensities analyzed, 40–50% of the trichomes were 100–500 µm long (Fig. 4b). The main difference was visible in the lower and higher range of size considered: for lower light intensities (25, 50 and 75 µmol photons m− 2 s− 1), 40–50% of filaments were longer than 500 µm, while for light intensities higher than 100 µmol photons m− 2 s− 1, 40–50% of them measured less than 100 µm in length. These short filaments could be hormogonia, transient cell forms differentiated from vegetative trichomes hypothesized to be involved in EPS release.

Going deeper in detail of the morphology, the sample grown in low light (25 µmol photons m− 2 s− 1) and the optimal light intensity found (100 µmol photons m− 2 s− 1) were investigated through electron microscopy (Fig. S7). Cells dimension and shape did not change between the two conditions (Fig. S7). No difference was detected in the internal organization: cells are packed with thylakoids that occupy most of the volume, arranged in fascicles. Nothing distinctive was observed comparing ETS-05 at the starting point, and after 9 days of growth.

3.5 Identification of genes linked to EPS assembly and export in ETS-05 genome

Proteins involved in Wzy-dependent and ABC-dependent pathways of other cyanobacterial species (Table S7) were aligned with ETS-05 genome (Table S8). Genes coding for PCP and OPX proteins are numerous and different within the same organism, leading to variability in the percentages of identity and query cover. Identities with OPX proteins (Wza/KpsD) had an average of 46%, while for PCP proteins (Wzc/KpsE) this value lowered to 42%. Considering the Wzy-dependent pathway, higher identities were reached by Wxb, that together with Wzy, are ubiquitously present in cyanobacteria according to (Pereira et al. 2015). Low percentages of identity and query cover were found for Wzx that is less conserved. As for ABC-dependent pathway, high levels of identity were observed for KpsM and KpsF (average of 52%) while KpsC/KpsS, KpsT, KpsU had both minimal identity and query cover values, as expected from the low conservation of the protein among cyanobacteria. No similarity was found for proteins involved in the Synthase-dependent pathway. Other pathways considered were associated with polysaccharide release by hormogonia, or HPS (Tables S9 and S10, sequences are reported in Supplementary File 2). High percentages of identity were observed for all genes investigated (average of 69%), with no significant similarity found only for genes pilA, pilB, hpsB, hpsC, hpsG, hpsH and hpsM. Interestingly, gene clusters found in N. punctiforme are also maintained in ETS-05.

Finally, analyzing annotated genes, other candidates were identified as possibly involved in EPS production (Table S11, sequences are reported in Supplementary File 2). In particular, AHNDPDGK_00533 gene codes for a “periplasmic protein involved in polysaccharide export” and contains a poly-export domain, typical of OPX proteins. Protein coded by gene AHNDPDGK_01089 is annotated by Operon-mapper as “putative polysaccharide export protein wza”, presents a poly-export domain and 4 SLBB domains, typical of OPX protein family. Similar results were obtained for AHNDPDGK_03356, annotated as “protein involved in polysaccharide export” and shortened as ps_ex, with a poly-export domain and 5 SLBB domains.

3.6 Molecular analysis of genes linked with EPS production and hormogonia formation

The involvement of low light and optimal light intensities in EPS release was investigated through gene expression analysis. Genes identified in ETS-05 genome and further analyzed were wzc and wza, both part of the Wzy-dependent pathway, responsible for EPS (Pereira et al. 2013) and HPS (Zuniga et al. 2020a) assembly and release. Gene ps_ex was identified in the genome annotation as mentioned. Finally, hrmK was described in (Zuniga et al. 2020b) as fundamental for hormogonia formation, therefore associated with HPS production. For all genes (Fig. 5), increase in the expression was assessed after 2 days of growth in both 25 and 100 µmol photons m− 2 s− 1. While no difference between low and optimal light was measured for wza, a 2-fold increase was observed for wzc at the optimal light. This result suggests that the protein involved in the assembly of the EPS could play a fundamental role in their production, determining the boost in EPS quantity assessed in higher light intensities, rather than the protein implicated in the release itself. A significant rise in the expression of ps_ex at 100 µmol photons m− 2 s− 1 compared to the initial time point, but not at 25 µmol photons m− 2 s− 1, was measured. A similar result was obtained for hrmK expression, giving another hint in the involvement of hormogonia formation under high light intensities, and possibly the augmented polysaccharide production due to HPS release.

3.7 Bioinformatic analysis of genes responsible for cyanotoxins synthesis

As thoroughly indicated, ETS-05 have been reported to produce diverse compounds of interest. Nonetheless, considering the relevance of the species in the production of the Euganean therapeutic mud, the potential production of cyanotoxins was considered. Genes responsible for the synthesis of most known cyanotoxins were searched in ETS-05 genome (Table S12). Microcystin and cylindrospermopsin (hepatotoxic), saxitoxin (neurotoxic) and lyngbyatoxin (dermatotoxic) (Merel et al. 2013) were not found, suggesting the inability of the strain to produce and release these compounds.

4. Discussion

The importance of ETS-05 in the context of therapeutic muds of the Euganean District led to the interest in analyzing the growth optima of this strain. ETS-05 represents in fact a source of high value compounds and could be exploited to both enrich the presence of the strain in the mud microbiota and to optimize its cultivation with biotechnological purposes. Considering the interest in EPS released by ETS-05, temperature, light spectra, light intensity, and nitrogen availability were evaluated not only to observe the culture response, but also to boost their production. Since EPS are obtained from the supernatant, intracellular high value compound production could be linked to the EPS one. Phycocyanin for instance was considered for its use in several fields (pharmaceutical, food, cosmetic (Saini et al. 2018)).

Effect of light spectra on growth was considered, knowing that red and yellow lights (de Mooij et al. 2016; Toyoshima et al. 2020) are generally more effective. Moreover Baer et al. (Baer et al. 2016) showed the importance to determine the optimized RGB mixture for every species. ETS-05 growth was not drastically influenced by light spectra, other than blue light that determined a drastic reduction in the biomass compared to other lights tested, as described in Synechococcus elongatus with 50 µmol photons m− 2 s− 1 (Ooms et al. 2017) and for Arthrospira platensis comparing red and blue light (Lima et al. 2018). According to Han and collegues (Han et al. 2015), both red and blue monochromatic lights enhanced EPS production in Nostoc flagelliforme, compared to white light exposure. However in our study, ETS-05 did not show improvements in EPS release using other lights rather than white light. Similar results were obtained for Nostoc calcicola RDU-3 with higher growth and polysaccharides release in white light followed by yellow, red, green, and blue lights (Singh and Das 2011). Some cyanobacteria can perform photoacclimation processes called chromatic acclimations (CA), involving he regulation of photosystems I and II and of phycobilisomes (Sanfilippo et al. 2019). Some Phormidium strains have been found, through bioinformatic analysis, to perform CA7, a modulation in the quantity of PEC according to the light spectrum (Hirose et al. 2019). Chromatic acclimation in red and green light was described in Phormidium sp. C86, with more synthesis of PE in green light and of PC in red light (Westermann and Wehrmeyer 1995). Alteration in PE and PC content was also observed in Phormidium autumnale CCAP1462/10 (Palinska et al. 2011). No change in pigmentation was observed in ETS-05, other than a diminished amount of all pigments in blue light, therefore the strain seems not able to perform any known kind of chromatic acclimation.

Thermotolerance of the species, anticipated considering its presence during the mud maturation process up to 47°C (Gris et al. 2020), determined higher biomass to be reached at 45°C. Higher temperature tested of 50°C led nonetheless to death of the organisms at 4 days, after a slight increase in OD750nm in the first days of cultivation. At the optimal temperature for biomass, higher EPS production was also obtained, as tested in cyanobacteria Scytonema tolypothrichoides and Tolypothrix bouteillei (Kvíderová et al. 2019). There was a direct correlation between temperature and EPS release. Same correlation was observed for PC up to 40°C where larger quantities were obtained: 221.8 ± 9.9 mg gDW−1. The content of PC in this condition was up to 21% w wDW−1, similarly to A. platensis (Xie et al. 2015), the most productive source of PC (Nwoba et al. 2019).

ETS-05 optimal light intensity corresponded to 100 µmol photons m− 2 s− 1 reaching a dry weight of 1.13 g L− 1 in 9 days. This was a promising result considering the 1.7 g L− 1 obtained for A. platensis cultivated for 15 days in raceways ponds (Raeisossadati et al. 2019). It is also possible that supplementing CO2 growth of ETS-05 could further increase. At lowest (25 µmol photons m− 2 s− 1) and highest (400 µmol photons m− 2 s− 1) intensities, biomass was reduced to a third or half. Direct correlation between EPS release and light intensity determined higher EPS concentration at 400 µmol photons m− 2 s− 1, indicating in this case the absence of a relationship between DW and EPS optima, as for T. bouteillei (Kvíderová et al. 2019). The positive effect of high light on EPS release was also observed in Cyanobacterium aponinum (Gris et al. 2017), Nostoc sp. (Ge et al. 2014a) and Microcoleus vaginatus (Ge et al. 2014b). Synthesis of phycobiliproteins behaved in the opposite way, with higher concentrations obtained at 25 µmol photons m− 2 s− 1, decreasing up to 10 mg gDW−1 at 400 µmol photons m− 2 s− 1. Chlorophyll a and total carotenoids content remained more or less similar in each intensity tested. There seems to be a trade-off between EPS and PC production, with optima conditions for one being non advantageous for the other.

Interestingly, under low and high light, ETS-05 filaments had different lengths, while other morphological features considered (cells dimension, shape, membrane thickness, internal arrangement) did not changed. We hypothesized that high light exposure stimulates hormogonia formation in ETS-05. Their differentiation can be stimulated or inhibited by environmental factors such as light and nutrients, in a species-specific manner (de Marsac 1994). As mentioned before, hormogonia are involved in the release of exopolysaccharides called HPS (Risser and Meeks 2013), to enhance the gliding motility of these trichomes for dispersal. Part of the quantified EPS in higher light intensities could be therefore correlated with abundance of hormogonia.

Finally, nitrogen depletion was tested since it is known to enhance EPS release in Nostoc sp. BTA97, Anabaena sp. BTA990 (Tiwari et al. 2015) Spirulina sp. (Nicolaus et al. 1999) and Cyanothece sp. 113 (Su et al. 2007). However, it was not observed a positive relation between the absence of this nutrient and EPS production in ETS-05. This condition was indeed too detrimental for growth and synthesis of compound of interest, even in a two-step cultivation system. Ultimately, it is important to notice the species-specific variability that characterize EPS production in cyanobacteria, implying the requirement to verify the best condition for each strain.

Furthermore, from an industrial point of view, using the residual biomass of EPS and hydrophilic pigment extraction as starting material, carotenoids, and lipids (not evaluated in this study) could be obtained. In (Liu et al. 2016) was for example successfully verified an integrated production of triacylglycerols and astaxanthin (as high-value carotenoid) using the microalgae Chlorella zofingiensis. Carotenoids from cyanobacteria can have various applications: anti-inflammatory, antioxidant, antitumor, color enhancer, anti-aging agent for cosmetics (Pagels et al. 2021). Furthermore, chlorophylls present biotechnological applications as food colorant, for cosmetics production and for human health being anti-inflammatory, antioxidant and antitumor agents (da Silva Ferreira and Sant’Anna 2017).

Bioinformatic analysis of putative genes involved in EPS assembly and secretion was performed to understand which mechanisms are carried out in ETS-05. Results highlighted the presence in ETS-05 genome of Wzy-dependent, ABC transporter-dependent (Pereira et al. 2015) and HPS-linked pathways (Zuniga et al. 2020a). Moreover other candidates were highlighted: proteins characterized by poly_export and SLBB domains, that can therefore act as OPX proteins. Real-Time qPCR allowed to verify the involvement of some of these putative genes: wzc (belonging to Wzy-dependent pathway), ps_ex (possibly coding for a OPX protein) and hrmK (probably involved in hormogonia formation), all augmented the expression when ETS-05 was exposed to optimal light, compared to low-light condition and the starting point.

To sum up, wzc, and ps_ex could be promising target genes to overexpress for an additional EPS assembly and release. On the other hand, enhancement of hormogonia formation through hrmK could stimulate HPS release but advantageous effects on biomass achievement should be further investigated.

Ultimately, the potential toxicity of ETS-05 was investigated, resulting in the absence of the genes involved in the synthesis of microcystin, cylindrospermopsin, saxitoxin, and lyngbyatoxin. These findings confirmed the absence of toxicity that was observed with an in vivo co-cultivation of ETS-05 and zebrafish (Danio rerio) larvae (Zampieri et al. 2020).

In this research ETS-05 was studied being the target species of the maturation process for the making of the Euganean therapeutic muds, possessing for this reason an importance in the territory and in the obtainment of this unique product with verified bioactive properties. Moreover, these results showed that ETS-05 could represent an interesting organism for biotechnological applications, considering the limited resources needed for its cultivation and the numerous high value compounds produced. In particular EPS synthesized by this species, which possess a demonstrated anti-inflammatory activity, can reach high yield when modulating the growth conditions. In addition to that, the absence of toxicity of the species is an important factor to consider in the optic of use its high value compounds for animal or human consumption and therapy. Finally, we investigated the involvement of several genes linked to EPS assembly and release by the organism with the hope to shed some light on this process that should gain more interest in the near future. The correlation between these genes’ expression and the condition of growth tested is a promising starting point for further characterizations and possible manipulations of ETS-05 to boost EPS productivity.

Declarations

Funding This work was supported by the Pietro d’Abano Thermal Studies Center (LA_R_EPPR18_01) and intramural grants by the Department of Biology of University of Padua.

Competing interests The authors have no competing interests to declare that are relevant to the content of this article.

Availability of data and material The datasets generated during the current study are available from the corresponding author on reasonable request. Phormidium sp. ETS-05 genome is publicly available in NCBI under the BioProject PRJNA622676.

Code availability Not applicable 

Authors’ contributions Conceptualization: Nicoletta La Rocca, Raffaella Margherita Zampieri; Methodology: Nicoletta La Rocca, Raffaella Margherita Zampieri; Formal analysis and investigation: Raffaella Margherita Zampieri; Writing - original draft preparation: Raffaella Margherita Zampieri; Writing - review and editing: Nicoletta La Rocca, Fabrizio Caldara; Funding acquisition: Nicoletta La Rocca; Resources: Nicoletta La Rocca, Raffaella Margherita Zampieri; Supervision: Nicoletta La Rocca, Fabrizio Caldara

Acknowledgements

The authors wish to acknowledge Dr. Sara Zambolin for the enthusiastic contribution during her master thesis internship.

References

  1. Baer S, Heining M, Schwerna P, Buchholz R, Hübner H (2016) Optimization of spectral light quality for growth and product formation in different microalgae using a continuous photobioreactor. Algal Res 14:109–115. https://doi.org/10.1016/j.algal.2016.01.011
  2. Bennett A, Bogorad L (1973) Complementary chromatic adaptation in a filamentous blue-green alga. J Cell Biol 58(2):419–435. https://doi.org/10.1083/jcb.58.2.419
  3. Ceschi Berrini C, De Appolonia F, Dalla Valle L, Komárek J, Andreoli C (2004) Morphological and molecular characterization of a thermophilic cyanobacterium (Oscillatoriales) from the Euganean Thermal Springs (Padua, Italy). Algological Studies/Archiv für Hydrobiologie, Supplement Volumes 113(August):73–85. https://doi.org/10.1127/1864-1318/2004/0113-0073
  4. Chamovitz D, Sandmann G, Hirschberg J (1993) Molecular and biochemical characterization of herbicide-resistant mutants of cyanobacteria reveals that phytoene desaturation is a rate-limiting step in carotenoid biosynthesis. J Biol Chem 268(23):17348–17353. https://doi.org/10.1016/s0021-9258(19)85341-3
  5. da Silva Ferreira V, Sant’Anna C (2017) Impact of culture conditions on the chlorophyll content of microalgae for biotechnological applications. World J Microbiol Biotechnol 33(1):1–8. https://doi.org/10.1007/s11274-016-2181-6
  6. de Marsac NT (1994) Differentiation of Hormogonia and Relationships with Other Biological Processes. The Molecular Biology of Cyanobacteria, Kluwer Academic Publishers, pp 825–842. https://doi.org/10.1007/0-306-48205-3_28
  7. de Mooij T, de Vries G, Latsos C, Wijffels RH, Janssen M (2016) Impact of light color on photobioreactor productivity. Algal Res 15:32–42. https://doi.org/10.1016/j.algal.2016.01.015
  8. DuBois M, Gilles KA, Hamilton JK, Rebers PA, Smith F (1956) Colorimetric Method for Determination of Sugars and Related Substances. Anal Chem 28(3):350–356. https://doi.org/10.1021/ac60111a017
  9. Ducat DC, Way JC, Silver PA (2011) Engineering cyanobacteria to generate high-value products. Trends Biotechnol 29(2):95–103. https://doi.org/10.1016/j.tibtech.2010.12.003
  10. Fioravanti A, Cantarini L, Guidelli GM, Galeazzi M (2011) Mechanisms of action of spa therapies in rheumatic diseases: What scientific evidence is there? Rheumatol Int 31(1):1–8. https://doi.org/10.1007/s00296-010-1628-6
  11. Franks J, Stolz JF (2009) Flat laminated microbial mat communities. Earth Sci Rev 96(3):163–172. https://doi.org/10.1016/j.earscirev.2008.10.004
  12. Gan F, Zhang S, Rockwell NC, Martin SS, Lagarias JC, Bryant DA (2014) Extensive remodeling of a cyanobacterial photosynthetic apparatus in far-red light. Science (1979) 345(6202):1312–1317. https://doi.org/10.1126/science.1256963
  13. Ge H, Xia L, Zhou X, Zhang D, Hu C (2014a) Effects of light intensity on components and topographical structures of extracellular polysaccharides from the cyanobacteria Nostoc sp. J Microbiol 52(2):179–183. https://doi.org/10.1007/s12275-014-2720-5
  14. Ge H, Zhang J, Zhou X, Xia L, Hu C (2014b) Effects of light intensity on components and topographical structures of extracellular polymeric substances from Microcoleus vaginatus (Cyanophyceae). Phycologia 53(2):167–173. https://doi.org/10.2216/13-163.1
  15. Gris B, Sforza E, Morosinotto T, Bertucco A, la Rocca N (2017) Influence of light and temperature on growth and high-value molecules productivity from Cyanobacterium aponinum. J Appl Phycol. https://doi.org/10.1007/s10811-017-1133-3
  16. Gris B, Treu L, Zampieri RM, Caldara F, Romualdi C, Campanaro S, La Rocca N (2020) Microbiota of the Therapeutic Euganean Thermal Muds with a Focus on the Main Cyanobacteria Species. Microorganisms 8:1–23. https://doi.org/10.3390/microorganisms8101590
  17. Han PP, Shen SG, Wang HY, Sun Y, Dai YJ, Jia SR (2015) Comparative metabolomic analysis of the effects of light quality on polysaccharide production of cyanobacterium Nostoc flagelliforme. Algal Res 9:143–150. https://doi.org/10.1016/j.algal.2015.02.019
  18. Harwood JL, Guschina IA (2009) The versatility of algae and their lipid metabolism. Biochimie 91(6):679–684. https://doi.org/10.1016/j.biochi.2008.11.004
  19. Herdman M, Rippka R (1988) Cellular Differentiation: Hormogonia and Baeocytes. In: Methods in Enzymology. pp 232–242
  20. Hirose Y, Chihong S, Watanabe M, Yonekawa C, Murata K, Ikeuchi M, Eki T (2019) Diverse Chromatic Acclimation Processes Regulating Phycoerythrocyanin and Rod-Shaped Phycobilisome in Cyanobacteria. Mol Plant 12(5):715–725. https://doi.org/10.1016/j.molp.2019.02.010
  21. Kaplan D, Calvert HE, Peters GA (1986) The Azolla-Anabaena azollae Relationship : XII. Nitrogenase Activity and Phycobiliproteins of the Endophyte as a Function of Leaf Age and Cell Type. Plant Physiol 80(4):884–90. https://doi.org/10.1104/pp.80.4.884
  22. Khayatan B, Meeks JC, Risser DD (2015) Evidence that a modified type IV pilus-like system powers gliding motility and polysaccharide secretion in filamentous cyanobacteria. Mol Microbiol 98(6):1021–1036. https://doi.org/10.1111/mmi.13205
  23. Kumar J, Singh D, Tyagi MB, Kumar A (2018) Cyanobacteria: Applications in Biotechnology. Elsevier Inc.
  24. Kvíderová J, Kumar D, Lukavský J, Kaštánek P, Adhikary SP (2019) Estimation of growth and exopolysaccharide production by two soil cyanobacteria, Scytonema tolypothrichoides and Tolypothrix bouteillei as determined by cultivation in irradiance and temperature crossed gradients. Eng Life Sci 19(3):184–195. https://doi.org/10.1002/elsc.201800082
  25. La Rocca N, Sciuto K, Meneghesso A, Moro I, Rascio N, Morosinotto T (2015) Photosynthesis in extreme environments: Responses to different light regimes in the Antarctic alga Koliella antarctica. Physiol Plant 153(4):654–667. https://doi.org/10.1111/ppl.12273
  26. Laroche C (2022) Exopolysaccharides from Microalgae and Cyanobacteria: Diversity of Strains, Production Strategies, and Applications. Mar Drugs 20(5). https://doi.org/10.3390/md20050336
  27. Lima GM, Teixeira PCN, Teixeira CMLL, Filócomo D, Lage CLS (2018) Influence of spectral light quality on the pigment concentrations and biomass productivity of Arthrospira platensis. Algal Res 31(April 2017):157–166. https://doi.org/10.1016/j.algal.2018.02.012
  28. Liu J, Mao X, Zhou W, Guarnieri MT (2016) Simultaneous production of triacylglycerol and high-value carotenoids by the astaxanthin-producing oleaginous green microalga Chlorella zofingiensis. Bioresour Technol 214:319–327. https://doi.org/10.1016/j.biortech.2016.04.112
  29. Merel S, Walker D, Chicana R, Snyder S, Baurès E, Thomas O (2013) State of knowledge and concerns on cyanobacterial blooms and cyanotoxins. Environ Int 59:303–327. https://doi.org/10.1016/j.envint.2013.06.013
  30. Mistry J, Chuguransky S, Williams L, Qureshi M, Salazar GA, Sonnhammer ELL, Tosatto SCE, Paladin L, Raj S, Richardson LJ, Finn RD, Bateman A (2021) Pfam: The protein families database in 2021. Nucleic Acids Res 49:412–419. https://doi.org/10.1093/nar/gkaa913
  31. Moran R (1982) Formulae for Determination of Chlorophyllous Pigments Extracted with N,N -Dimethylformamide . Plant Physiol 69(6):1376–1381. https://doi.org/10.1104/pp.69.6.1376
  32. Nicolaus B, Panico A, Lama L, Romano I, Manca MC, de Giulio A, Gambacorta A (1999) Chemical composition and production of exopolysaccharides from representative members of heterocystous and non-heterocystous cyanobacteria. Phytochemistry 52(4):639–647. https://doi.org/10.1016/S0031-9422(99)00202-2
  33. Nwoba EG, Parlevliet DA, Laird DW, Alameh K, Moheimani NR (2019) Sustainable phycocyanin production from Arthrospira platensis using solar-control thin film coated photobioreactor. Biochem Eng J 141(October 2018):232–238. https://doi.org/10.1016/j.bej.2018.10.024
  34. Ooms MD, Graham PJ, Nguyen B, Sargent EH, Sinton D (2017) Light dilution via wavelength management for efficient high-density photobioreactors. Biotechnol Bioeng 114(6):1160–1169. https://doi.org/10.1002/bit.26261
  35. Pagels F, Guedes AC, Amaro HM, Kijjoa A, Vasconcelos V (2019) Phycobiliproteins from cyanobacteria: Chemistry and biotechnological applications. Biotechnol Adv 37(3):422–443. https://doi.org/10.1016/j.biotechadv.2019.02.010
  36. Pagels F, Vasconcelos V, Guedes AC (2021) Carotenoids from cyanobacteria: Biotechnological potential and optimization strategies. Biomolecules 11(5). https://doi.org/10.3390/biom11050735
  37. Palinska KA, Deventer B, Hariri K, Łotocka M (2011) A taxonomic study on Phormidium-group (cyanobacteria) based on morphology, pigments, RAPD molecular markers and RFLP analysis of the 16S rRNA gene fragment. Fottea 11(1):41–55. https://doi.org/10.5507/fot.2011.006
  38. Patel A, Matsakas L, Rova U, Christakopoulos P (2019) A perspective on biotechnological applications of thermophilic microalgae and cyanobacteria. Bioresour Technol 278(November 2018):424–434. https://doi.org/10.1016/j.biortech.2019.01.063
  39. Paysan-Lafosse T, Blum M, Chuguransky S, Grego T, Pinto BL, Salazar GA, Bileschi ML, Bork P, Bridge A, Colwell L, Gough J, Haft DH, Letunić I, Marchler-Bauer A, Mi H, Natale DA, Orengo CA, Pandurangan AP, Rivoire C, Sigrist CJA, Sillitoe I, Thanki N, Thomas PD, Tosatto SCE, Wu CH, Bateman A (2022) InterPro in 2022. Nucleic Acids Res :1–10. https://doi.org/10.1093/nar/gkac993
  40. Pereira S, Zille A, Micheletti E, Moradas-ferreira P, Philippis R de, Tamagnini P (2009) Complexity of cyanobacterial exopolysaccharides: composition, structures, inducing factors and putative genes involved in their biosynthesis and assembly. FEMS Microbiol Rev 33(5):917–941. https://doi.org/10.1111/j.1574-6976.2009.00183.x
  41. Pereira SB, Mota R, Santos CL, De Philippis R, Tamagnini P (2013) Assembly and export of extracellular polymeric substances (EPS) in cyanobacteria. A phylogenomic approach. Elsevier
  42. Pereira SB, Mota R, Vieira CP, Vieira J, Tamagnini P (2015) Phylum-wide analysis of genes/proteins related to the last steps of assembly and export of extracellular polymeric substances (EPS) in cyanobacteria. Sci Rep 5(July):1–16. https://doi.org/10.1038/srep14835
  43. Raeisossadati M, Moheimani NR, Parlevliet D (2019) Red and blue luminescent solar concentrators for increasing Arthrospira platensis biomass and phycocyanin productivity in outdoor raceway ponds. Bioresour Technol 291(July):121801. https://doi.org/10.1016/j.biortech.2019.121801
  44. Rippka R, Deruelles J, Waterbury JB (1979) Generic assignments, strain histories and properties of pure cultures of cyanobacteria. J Gen Microbiol 111(1):1–61. https://doi.org/10.1099/00221287-111-1-1
  45. Risser DD, Meeks JC (2013) Comparative transcriptomics with a motility-deficient mutant leads to identification of a novel polysaccharide secretion system in Nostoc punctiforme. Mol Microbiol 87(4):884–893. https://doi.org/10.1111/mmi.12138
  46. Saini DK, Pabbi S, Shukla P (2018) Cyanobacterial pigments: Perspectives and biotechnological approaches. Food and Chemical Toxicology 120(April):616–624. https://doi.org/10.1016/j.fct.2018.08.002
  47. Sanfilippo JE, Garczarek L, Partensky F, Kehoe DM (2019) Chromatic acclimation in cyanobacteria: A diverse and widespread process for optimizing photosynthesis. Annu Rev Microbiol 73:407–433. https://doi.org/10.1146/annurev-micro-020518-115738
  48. Schneider CA, Rasband WS, Eliceiri KW (2012) NIH Image to ImageJ: 25 years of image analysis. Nat Methods 9(7):671–675. https://doi.org/10.1038/nmeth.2089
  49. Singh S, Das S (2011) Screening, production, optimization and characterization of cyanobacterial polysaccharide. World J Microbiol Biotechnol 27(9):1971–1980. https://doi.org/10.1007/s11274-011-0657-y
  50. Su C, Chi Z, Lu W (2007) Optimization of medium and cultivation conditions for enhanced exopolysaccharide yield by marine Cyanothece sp. 113. Chin J Oceanol Limnol 25(4):411–417. https://doi.org/10.1007/s00343-007-0411-3
  51. Taboada B, Estrada K, Ciria R, Merino E (2018) Operon-mapper: A web server for precise operon identification in bacterial and archaeal genomes. Bioinformatics 34(23):4118–4120. https://doi.org/10.1093/bioinformatics/bty496
  52. Tiwari ON, Khangembam R, Shamjetshabam M, Sharma AS, Oinam G, Brand JJ (2015) Characterization and Optimization of Bioflocculant Exopolysaccharide Production by Cyanobacteria Nostoc sp. BTA97 and Anabaena sp. BTA990 in Culture Conditions. Appl Biochem Biotechnol 176(7):1950–1963. https://doi.org/10.1007/s12010-015-1691-2
  53. Toyoshima M, Toya Y, Shimizu H (2020) Flux balance analysis of cyanobacteria reveals selective use of photosynthetic electron transport components under different spectral light conditions. Photosynth Res 143(1):31–43. https://doi.org/10.1007/s11120-019-00678-x
  54. Westermann M, Wehrmeyer W (1995) A new type of complementary chromatic adaptation exemplified by Phormidium sp. C86: Changes in the number of peripheral rods and in the stoichiometry of core complexes in phycobilisomes. Arch Microbiol 164(2):132–141. https://doi.org/10.1007/BF02525319
  55. Xie Y, Jin Y, Zeng X, Chen J, Lu Y, Jing K (2015) Fed-batch strategy for enhancing cell growth and C-phycocyanin production of Arthrospira (Spirulina) platensis under phototrophic cultivation. Bioresour Technol 180:281–287. https://doi.org/10.1016/j.biortech.2014.12.073
  56. Zampieri RM, Adessi A, Caldara F, Codato A, Furlan M, Rampazzo C, De Philippis R, La Rocca N, Dalla Valle L (2020) Anti-inflammatory activity of exopolysaccharides from Phormidium sp. ETS05, the most abundant cyanobacterium of the therapeutic euganean thermal muds, using the zebrafish model. Biomolecules 10(4). https://doi.org/10.3390/biom10040582
  57. Zampieri RM, Adessi A, Caldara F, De Philippis R, Dalla Valle L, La Rocca N (2022) In vivo anti-inflammatory and antioxidant effects of microbial polysaccharides extracted from Euganean therapeutic muds. Int J Biol Macromol 209(PB):1710–1719. https://doi.org/10.1016/j.ijbiomac.2022.04.123
  58. Zuniga EG, Boateng KKA, Bui NU, Kurnfuli S, Muthana SM, Risser DD (2020a) Identification of a hormogonium polysaccharide-specific gene set conserved in filamentous cyanobacteria. Mol Microbiol 114(4):597–608. https://doi.org/10.1111/mmi.14566
  59. Zuniga EG, Figueroa NM, Gonzalez A, Pantoja AP, Risser DD (2020b) The hybrid histidine kinase HrmK is an early-acting factor in the hormogonium gene regulatory network. J Bacteriol 202(5). https://doi.org/10.1128/JB.00675-19