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An Ocean Acidification Acclimatised Green Tide Alga Is Robust to Changes of Seawater Carbon Chemistry but Vulnerable to Light Stress

  • Guang Gao ,

    Contributed equally to this work with: Guang Gao, Yameng Liu

    Affiliation Marine Resources Development Institute of Jiangsu, Huaihai Institute of Technology, Lianyungang, China

  • Yameng Liu ,

    Contributed equally to this work with: Guang Gao, Yameng Liu

    Affiliation Marine Resources Development Institute of Jiangsu, Huaihai Institute of Technology, Lianyungang, China

  • Xinshu Li,

    Affiliation Marine Resources Development Institute of Jiangsu, Huaihai Institute of Technology, Lianyungang, China

  • Zhihua Feng,

    Affiliation Marine Resources Development Institute of Jiangsu, Huaihai Institute of Technology, Lianyungang, China

  • Juntian Xu

    jtxu@hhit.edu.cn

    Affiliation Marine Resources Development Institute of Jiangsu, Huaihai Institute of Technology, Lianyungang, China

Abstract

Ulva is the dominant genus in the green tide events and is considered to have efficient CO2 concentrating mechanisms (CCMs). However, little is understood regarding the impacts of ocean acidification on the CCMs of Ulva and the consequences of thalli’s acclimation to ocean acidification in terms of responding to environmental factors. Here, we grew a cosmopolitan green alga, Ulva linza at ambient (LC) and elevated (HC) CO2 levels and investigated the alteration of CCMs in U. linza grown at HC and its responses to the changed seawater carbon chemistry and light intensity. The inhibitors experiment for photosynthetic inorganic carbon utilization demonstrated that acidic compartments, extracellular carbonic anhydrase (CA) and intracellular CA worked together in the thalli grown at LC and the acquisition of exogenous carbon source in the thalli could be attributed to the collaboration of acidic compartments and extracellular CA. Contrastingly, when U. linza was grown at HC, extracellular CA was completely inhibited, acidic compartments and intracellular CA were also down-regulated to different extents and thus the acquisition of exogenous carbon source solely relied on acidic compartments. The down-regulated CCMs in U. linza did not affect its responses to changes of seawater carbon chemistry but led to a decrease of net photosynthetic rate when thalli were exposed to increased light intensity. This decrease could be attributed to photodamage caused by the combination of the saved energy due to the down-regulated CCMs and high light intensity. Our findings suggest future ocean acidification might impose depressing effects on green tide events when combined with increased light exposure.

Introduction

Due largely to burning fossil fuel and change of net land use, the carbon dioxide level in the air has increased by 40% since 1750 [1]. Meanwhile, the ocean—as a sink of carbon—has absorbed about 30% of the emitted anthropogenic carbon dioxide, leading to ocean acidification (OA) [1]. The pH of surface seawater has decreased by 0.1 since the beginning of the industrial era, corresponding to an increase of 26% in hydrogen ion concentration. A global increase in OA for all representative concentration pathway (RCP) scenarios is projected by Earth System Models, in which the corresponding decrease in surface ocean pH by the end of this century is in the range of 0.06 to 0.07 for RCP2.6, 0.14 to 0.15 for RCP4.5, 0.20 to 0.21 for RCP6.0, and 0.30 to 0.32 for RCP8.5 [1]. Such an increase in OA would also affect the stability or the baseline of carbonate chemistry in coastal waters, where most of the macroalgae inhabit. Furthermore, coastal waters are more susceptible to acidification than the pelagic ocean due to eutrophication and following microbial respiration [2].

The concentration of CO2 in seawater is vital for algal photosynthesis since ribulose-1, 5-bisphosphate carboxylase/oxygenase (Rubisco) can also catalyse ribulose-1, 5-bisphosphate with oxygen (O2) in a process called photorespiration if the ratio of CO2 to O2 is low [3]. Although the concentration of dissolved inorganic carbon (DIC) is very high (about approximately 2 mmol L-1) in seawater, its predominant form is HCO3-, and CO2 accounts for less than 1% of it. Rubisco has a relatively low affinity for CO2 and is consequently less than half saturated under current CO2 levels for most algal species [4,5]. Accordingly, most algae including macroalgae have evolved CO2 concentrating mechanisms (CCMs), which can promote the internal CO2 concentrations to the levels significantly higher than extracellular concentrations. On the other hand, a few red and green macroalgae do not have any CCMs at the Rubisco active site and acquire Ci solely by CO2 diffusion from the external environment [5,6]. Therefore, the influence of ocean acidification and a changed seawater carbonate system on macroalgae may be species specific.

Species that can actively use bicarbonate seem unlikely to show stimulation of photosynthesis or growth with an increase in atmospheric CO2 levels since increased atmospheric CO2 will result in a small proportional change in HCO3- compared to CO2 and CO32- concentrations in seawater [7]. On the other hand, species relying on CO2 uptake by passive diffusion might benefit more than those that can take up CO2 actively with an active CCM. For instance, increasing atmospheric CO2 concentrations have been demonstrated to enhance the growth of the red algae Porphyra yezoensis grown at 15°C and 300 μmol photons m-2 s-1 light level [8], Gracilaria sp. grown at 20°C and 300 μmol photons m-2 s-1 light level [9], Lomentaria articulata grown at 10°C and 40 μmol photons m-2 s-1 light level [6], Hizikia fusiforme grown at 20°C and 120 μmol photons m-2 s-1 light level [10], and Neosiphonia harveyi grown at both 10°C and 17.5°C with the light level of 100–150 μmol photons m-2 s-1 [11]. On the other hand, negative effects of increased CO2 on photosynthesis in Ulva spp. cultured at 25°C and 200 μmol photons m-2 s-1 light level [12], as well as growth in Gracilaria tenuistipitata cultured at 25°C and 200 μmol photons m-2 s-1 light level [13], P. leucostica cultured at 15°C and 60 μmol photons m-2 s-1 light level [14], P. linearis cultured at 15°C and 100 μmol photons m-2 s-1 light level [15] and Fucus vesiculosus cultured at 10°C and 70–100 μmol photons m-2 s-1 light level [16] were observed. In addition, a pCO2 level of 750 μatm had no significant effect on the growth of 14 macroalgae species from three major divisions, i.e. Chlorophyta, Rhodophyta and Phaeophyta [17]. Recent research demonstrated that U. rigida grown at 13°C and 50 μmol photons m-2 s-1 light level [18] and giant kelp Macrocystis pyrifera grown at 12°C and 110 μmol photons m-2 s-1 light level [19] were also insensitive to ocean acidification (~1220 μatm pCO2).

Ulva, a cosmopolitan genus which is common in tide-pools, has been gaining significant interest due to its potential value in animal feed [20,21], human food [22,23], biofuel [24,25] as well as the delivery of crucial ecosystem services such as wastewater bioremediation [26,27] and CO2 removal [28,29]. Meanwhile, Ulva is the only genus contributing to reported green tide events [30,31]. A powerful CO2 concentrating mechanism (CCM) for algae is helpful to outcompete other species, particularly when CO2 is limited. U. lactuca has very efficient CCMs, including a HCO3- dehydration mechanism and a HCO3- uptake mechanism [32,33]. U. prolifera also has a high pH compensation point of 10.56, suggesting that thalli can utilise HCO3- for photosynthesis [34]. However, little has been known about the CCMs in U. linza, a causative species of green tide [35,36], or the impacts of ocean acidification on CCMs in U. linza. Ocean acidification caused by increasing pCO2 can usually down-regulate algal CCMs and the saved CCMs-related energy expenditure facilitates growth [37,38]. On the other hand, the saved energy from down-regulated CCMs could harm photosynthesis and growth of phytoplankton when cells were exposed to increased light intensity [37]. Based on the previous studies, we hypothesise that ocean acidification will down-regulate the CCMs in U. linza and this down-regulation will not affect its effective response to seawater carbon chemistry but increase its sensitivity to high light (Fig 1).

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Fig 1. Physiological responses of ocean acidification acclimatised U. linza to changes of seawater carbon chemistry and light exposure.

The blue-dotted and the red-solid symbols represent down- and up-regulated metabolic pathways respectively. PSI: Photosystem I; PSII: Photosystem II; Fd: ferredoxin; Fp: flavoprotein; OEC: oxygen- evolving complex; NPQ: non-photochemical quenching; CA: carbonic anhydrase.

https://doi.org/10.1371/journal.pone.0169040.g001

Materials and Methods

Materials and culture conditions

Thalli of U. linza were collected from the coastal water of Lianyungang (119.3°E, 34.5°N), Jiangsu province of China in April 2013. No specific permission is required for the collection as Ulva is a nuisance in China. The natural temperature and salinity in the seawater were 12°C and 31 respectively. The thalli were transported to the lab in a cooling box (4–6°C) within one hour and then washed gently with 0.2 μm filtered seawater to remove any sediment, epiphytes or small grazers. The thalli were cultured in 500 mL conical flasks, aerated with ambient (LC, 390 μatm) and elevated (HC, 1000 μatm) CO2 levels. The culture densities for LC and HC treatments were controlled below 0.1g L-1 in order to maintain the pH variation less than 0.05. Media were made from natural seawater with the addition of 60 μM NaNO3 and 8 μM KH2PO4. The concentrations of nitrate and phosphate in natural seawater were 20 and 2 μM respectively and the artificial addition of nitrate and phosphate was to avoid the limit of nutrients during the laboratory culture. The light conditions were set as 100 μmol photons m-2 s-1 (light/dark 12:12 h) and the temperature was set as 12°C, in accordance with where U. linza was found in its natural conditions. The increased biomass was removed and the culture medium was renewed every 48 h. To avoid the effect of cutting on thalli’s physiological performances, the removal was conducted by taking out some individual randomly rather than cutting off every individual in the flasks. The culture lasted three weeks and five replicates were conducted under each treatment. According to Eggert [39], the acclimation of seaweeds to environment can take place over the period of hours to days. Therefore, three weeks should be enough for thalli to acclimatise to the condition of ocean acidification.

Carbonate chemistry parameters

The pCO2 in seawater was maintained by bubbling ambient air (390 μatm) and CO2 enriched air (1000 μatm), and the latter was achieved by a CO2 plant chamber (HP1000 G-D, Wuhan Ruihua Instrument & Equipment Ltd, China) with the variation of CO2 less than 5%. The seawater pH in flasks was recorded with a pH meter (pH 700, Eutech Instruments, Singapore) and total alkalinity (TA) was measured by titrations. Other carbonate system parameters, which were not directly measured, were calculated via CO2SYS [40], using the equilibrium constants of K1 and K2 for carbonic acid dissociation [41].

Measurements of photosynthetic oxygen evolution

The net photosynthetic rate of U. linza was measured by a Clark-type oxygen electrode (YSI Model 5300, USA). The thalli were prepared for about 1-cm-long segments with scissors, and the cutting damage was minimised by incubating the segments in cultured seawater for about 1 h. Approximately 0.015 g of harvested fresh weight algae was transferred to the oxygen electrode cuvette which containing 8 ml reaction medium, and the medium was stirred. The irradiance and temperature were maintained as the same as that in the growth condition. The measurement was finished within five minutes and the pH did not vary over this period. CA inhibitors (Sigma), acetazolamide (AZ) and 6-ethoxyzolamide (EZ) were used to study the mechanism of DIC acquisition via carbonic anhydrase (CA), and their final concentrations were both 200 μM. The buffer Tris, with a final concentration of 20 mM, was also used to test whether or not the extracellular acidic compartments present in the green macroalga (Fig 1).

To investigate the responses of U. linza grown under LC and HC to various pH and light levels, the net photosynthetic rates of thalli were also measured at different pH (7.0, 7.8, 8.2, 9.0 and 10.0) and light levels (LL, 100 μmol photons m-2 s-1; HL, 600 μmol photons m-2 s-1). The light level of 600 μmol photons m-2 s-1 was set as high light because it is the saturation light intensity for photosynthesis in U. linza, which was revealed in a preliminary experiment.

Measurement of growth

The relative growth rate (RGR) of U. linza was estimated after the thalli had acclimated to the CO2 levels for three weeks as follows: RGR = (lnNt − lnN0) / t × 100, where N0 is the initial fresh weight, Nt is the final fresh weight, and t is the number of culture days.

Chlorophyll fluorescence measurements

Chlorophyll fluorescence parameters of U. linza grown under LC and HC were measured with a pulse modulation fluorometer (Water PAM, Walz). After dark adaption for 15 minutes, the induction curves of the thalli were carried out for determining the chlorophyll fluorescence parameters. The relative electron transport rate (rETR) and non-photosythetic quenching (NPQ) can be obtained from the induction curve. rETR, was calculated according to Genty et al. (1989). NPQ, was attained as fellows: NPQ = (Fm − Fm’) / Fm’, Fm and Fm’ are the maximal fluorescence levels from algae after dark adaptation and in light respectively. The actinic light levels in the induction curves were set at 100 and 600 μmol photons m-2 s-1.

Determination of photosynthetic pigments

Approximately 100 mg fresh weight of thalli was extracted with 10 mL of absolute methanol at 4°C for 24 h in darkness. The contents of Chl a and Chl b were estimated according to Wellburn [42].

Statistical analysis

The data were presented as the means ± standard deviation (SD) of five replicates and analysed using the software SPSS v.21. The data under every treatment conformed to a normal distribution (Shapiro-Wilk, P > 0.05) and the variances could be considered equal (Levene’s test, P > 0.05). Independent samples t-tests were conducted to compare the seawater carbonate parameters, relative growth rate, Chl a, and Chl b between LC and HC. One-way ANOVAs were conducted to assess the differences in the net photosynthetic rate between inhibitors at LC and HC. Three-way ANOVA was conducted to investigate the effects of culture CO2, media pH, and light on net photosynthetic rate of U. linza. Two-way ANOVAs were conducted to assess the effect of culture CO2 and light on rETR and NPQ. Tukey HSD was conducted for post hoc investigation. The 95% confidence level was used in all analyses.

Results

Changes of seawater carbonate chemistry caused by ocean acidification

The effects of ocean acidification on seawater carbonate parameters were observed (Table 1). Projected ocean acidification decreased pH by 0.34 unit (Independent samples t-test, t = 29.242, df = 8, P < 0.001), CO32- by 50.43% (Independent samples t-test, t = 25.308, df = 8, P < 0.001) but increased pCO2 by 143.87% (Independent samples t-test, t = -22.777, df = 8, P < 0.001), DIC by 7.47% (Independent samples t-test, t = -6.023, df = 8, P < 0.001), HCO3- by 9.94% (Independent samples t-test, t = -7.771, df = 8, P < 0.001), CO2 by 143.87% (Independent samples t-test, t = -22.779, df = 8, P < 0.001), with an insignificant effect on TA (Independent samples t-test, t = -1.369, df = 8, P = 0.208).

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Table 1. Parameters of the seawater carbonate system at LC and HC.

Measurements and estimation of the parameters are described in Materials and Methods. Data are the means ± SD (n = 5). LC, the low pCO2 condition, HC, the high pCO2 condition, DIC = dissolved inorganic carbon, TA = total alkalinity. The unit of pCO2 is μatm and all other parameters’ unit is μmol kg-1.Different superscript letters indicate significant differences between two conditions (P < 0.05).

https://doi.org/10.1371/journal.pone.0169040.t001

Effects of elevated CO2 on CCMs and growth

The net photosynthetic rate of U. linza grown under LC was altered when inhibitors were added (Fig 2; ANOVA, F = 47.109, df = 3, 16, P < 0.001). It was reduced to 32.44 ± 4.40 μmol O2 g-1 FW h-1 from 63.87 ± 12.23 μmol O2 g-1 FW h-1 (Control) with the addition of Tris for thalli grown at LC (Tukey HSD, P < 0.001), which amounts to an inhibition rate of 49.21%. The net photosynthetic rate of U. linza grown at LC decreased to 47.10 ± 2.84 μmol O2 g-1 FW h-1 when AZ was added, indicating an inhibition rate of 26.26% (Tukey HSD, P = 0.005). Compared to Tris and AZ, EZ displayed a higher inhibition rate (75.19%) (Tukey HSD, P = 0.306), with the photosynthetic rate decreasing to 15.85 ± 1.20 μmol O2 g-1 FW h-1. The pattern varied for U. linza grown under HC. There was no significant difference in the net photosynthetic rate between the treatments of AZ (49.22 ± 6.87 μmol O2 g-1 FW h-1) and control (59.13 ± 15.04 μmol O2 g-1 FW h-1) (Tukey HSD, P > 0.05). Tris (Tukey HSD, P = 0.005) and EZ (Tukey HSD, P = 0.001) still had inhibitory effects on the net photosynthetic rate, with the inhibition rates of 37.00% and 47.03% respectively. But the difference in the net photosynthetic rate between Tris (37.25 ± 3.79 μmol O2 g-1 FW h-1) and EZ (31.32 ± 3.58 μmol O2 g-1 FW h-1) was insignificant (Tukey HSD, P = 0.705). HC did not increase the net photosynthetic rates of U. linza except under the addition of EZ (an increase of 97.64%, Independent samples t-test, t = -9.160, df = 8, P < 0.001). The effect of elevated CO2 on growth of U. linza was also examined (Fig 3). The RGR of thalli grown at LC was 12.56 ± 3.13% and the HC increased it to 18.31 ± 2.42% (Independent samples t-test, t = -3.250, df = 8, P = 0.012).

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Fig 2. Net photosynthetic rate of U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels and measured under different treatments (Control, added with Tris, AZ, and EZ).

Different superscript letters indicate significant differences between treatments within one culture condition (P < 0.05, one-way ANOVA and Tukey HSD test) and the lowercase and capital letters represent the comparisons at LC and HC, respectively. Asterisks indicate significant differences between culture conditions (P < 0.05, Independent samples t-tests).

https://doi.org/10.1371/journal.pone.0169040.g002

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Fig 3. Relative growth rate of U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels.

Different superscript letters indicate significant differences between culture conditions (P < 0.05, Independent samples t-tests).

https://doi.org/10.1371/journal.pone.0169040.g003

Responses to seawater carbon chemistry and light

The responses of U. linza grown at LC and HC to seawater carbon chemistry and light levels were investigated (Fig 4). There were no interactive effects of CO2, light, and seawater carbon chemistry but any two of them interacted on the net photosynthetic rate of U. linza (Table 2). For instance, HC did not affect the net photosynthetic rate of U. linza at LL but it significantly reduced net photosynthetic rate at HL, regardless of the seawater carbon chemistry conditions. Similarly, the differences in net photosynthetic rate between seawater carbon chemistry conditions at LL were insignificant but lower pH (or higher CO2) decreased net photosynthetic rate at HL.

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Fig 4. Changes of net photosynthetic rates of U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels measured at different pH and light (LL, 100 μmol photons m-2 s-1; HL, 600 μmol photons m-2 s-1) conditions.

https://doi.org/10.1371/journal.pone.0169040.g004

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Table 2. Three-way analysis of variance of the responses of the net photosynthetic rate in U. linza grown under LC and HC to various light and seawater pH levels.

LC, the low pCO2 condition, HC, the high pCO2 condition.

https://doi.org/10.1371/journal.pone.0169040.t002

rETR and NPQ

There was an interactive effect on rETR between CO2 and light, and both also had main effects (Table 3). The rETR were 15.97 ± 0.90 μmol e- m-2 s-1 (LC) and 19.50 ± 0.91 μmol e- m-2 s-1 (HC) at LL and HL increased them to 70.28 ± 1.40 μmol e- m-2 s-1 (LC) and 95.59 ± 2.82 μmol e- m-2 s-1 (HC), respectively (Fig 5). HC increased rETR by 18.12% at LL and the stimulating effect (26.48%) was more significant at HL. CO2 and light also had an interactive effect on NPQ (Table 4). For instance, HC increased NPQ by 28.60% at LL while it was 37.82% at HL, indicating that the stimulating effect of CO2 increases with light (Fig 6). HL increased NPQ regardless of CO2.

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Fig 5. rETR of U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels and measured at different light conditions (LL, 100 μmol photons m-2 s-1; HL, 600 μmol photons m-2 s-1).

https://doi.org/10.1371/journal.pone.0169040.g005

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Fig 6. NPQ of U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels and measured at different light conditions (LL, 100 μmol photons m-2 s-1; HL, 600 μmol photons m-2 s-1).

https://doi.org/10.1371/journal.pone.0169040.g006

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Table 3. Two-way analysis of variance of the effects of CO2 and light on rETR in U. linza.

https://doi.org/10.1371/journal.pone.0169040.t003

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Table 4. Two-way analysis of variance of the effects of CO2 and light on NPQ in U. linza.

https://doi.org/10.1371/journal.pone.0169040.t004

Photosynthetic pigments.

The contents of Chl a and Chl b in U. linza grown at LC were 680.91 ± 65.81 μg g-1 FW and 507.06 ± 55.21 μg g-1 FW respectively and they decreased to 434.05 ±105.93 μg g-1 FW (Independent samples t-test, t = 4.426, df = 8, P = 0.002) and 318.67 ± 67.87 μg g-1 FW (Independent samples t-test, t = 4.815, df = 8, P = 0.001) in U. linza grown at HC (Fig 7).

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Fig 7. Contents of Chl a and Chl b in U. linza grown at ambient (LC; 390 μatm) and elevated (HC; 1000 μatm) CO2 levels.

Different superscript letters indicate significant differences between culture conditions (P < 0.05, Independent samples t-tests).

https://doi.org/10.1371/journal.pone.0169040.g007

Discussion

Ocean acidification changes CCMs

The inhibiting effect of Tris buffer on net photosynthetic rate of U. linza grown at LC implies that the thalli possess the acidic compartments as one of CCMs pathways. This is the first report of acidic compartments existing in cell wall of Ulva species, although it has been found in other macrophytes, such as Ruppia cirrhosa [43], Zostera marina [44], Z. noltii [45] and Laminaria saccharina [46]. Acidic compartments are created by excreting protons outside of the plasma membrane and thus CO2 concentration in the zones is enhanced above its level in the medium, which can speed up the diffusion of CO2 into the cell either through the cell membrane proper or via proteinaceous pores [46,47]. The Tris buffer is considered to act as a proton dissipating system facilitating the H+ diffusion out of the acidic compartments [46,48], which consequently increases the pH within acid compartments and weakens the function of acidic compartments as the CCMs pathway. The addition of AZ and EZ also reduced net photosynthetic rate of U. linza grown at LC, suggesting both extracellular CA and intercellular CA function in the CCMs of U. linza. Tris, AZ, and EZ inhibited the net photosynthetic rate of thalli grown at LC, which means that acidic compartments, external and internal CA work together in the thalli grown in natural seawater medium and the acquisition of exogenous carbon in the thalli may be achieved by the collaboration of acidic compartments and external CA.

After U. linza was cultured at HC for three weeks, the addition of Tris still inhibited net photosynthetic rate although the inhibition rate decreased from 49.21% at LC to 37.00%, indicating a little down-regulation of acidic compartments. In contrast, no significant difference in net photosynthetic rate of U. linza grown under HC was found when AZ was added, which suggests that the function of extracelluar CA should be completely switched off at HC. Mercado et al. [46] demonstrated that acidic compartments must feature external CA activity in Laminaria saccharina since the acidic compartments per se played a minor role when external CA was completely inhibited, but our study suggests that external CA is not essential for the acidic compartments in U. linza. When EZ is added, the net photosynthetic rate in U. linza at HC was reduced by 47.03%, lower than the decrease of 75.19% at LC, indicating intercellular CA was also down-regulated at HC. It is worth noticing that the net photosynthetic rate at HC was 97.64% higher than that at LC when EZ was added. This indicates that diffusion of CO2 plays a more important role at HC since the acquisition of exogenous carbon is mostly based on the diffusion of CO2 in seawater medium when activity of CA is inhibited. The acidic compartment at HC should contribute to the higher net photosynthetic rate under the treatment of EZ, and higher rETR at HC may supply additional ATP to maintain the operation of acidic compartment, considering energy is needed to run the proton pump in the acidic compartment. Although ocean acidification down-regulated CCMs and altered pathways of CCMs in U. linza, it did not increase or decrease the net photosynthetic rate. Neutral effects of elevated CO2 on photosynthesis were also found in phytoplankton assemblages [49] and macroalgae U. prolifera [38]. One possible reason is that photorespiration is also reduced along with the down-regulated CCMs at elevated CO2 conditions [50,51].

Ocean acidification increases growth

The growth at HC was enhanced compared to LC (Fig 2), albeit the net photosynthetic rate in U. linza grown at HC did not increase. The enhancement of Ulva growth at HC might be attributed to the saved energy due to down-regulated CCMs, e.g., reduced synthesis of CA, which can benefit other metabolisms and biosynthesis. For example, high CO2 increased activity of nitrate reductase in U. rigida [52,53], brown seaweed Hizikia fusiforme [10], and calcifying rhodophyte Corallina officinalis [54]. Accordingly, the nitrogen assimilation in plants was enhanced at high CO2 conditions [10,52,53]. In addition to the saved energy from down-regulated CCMs, content of pigments (Chl a and Chl b) at HC was also decreased. Energy saved from the ‘pigment economy’ can also flow to other metabolisms and biosynthesis and hence enhance growth. The increased growth at HC was also reported in another green tidal alga, U. prolifera [38]. The similar physiological responses of the two main green tidal species to high CO2 level indicate that future ocean acidification might lead to more severe green tides when the light level is low.

Responses of ocean acidification acclimatised thalli to seawater carbon chemistry and light

Under LL, the net photosynthetic rate of U. linza grown at LC was not affected by pH and even at the pH 10 where [CO2] was zero and [HCO3-] was below 10% (Fig 5), the net photosynthetic rate was still comparable to the values at other pH conditions. We presume that the robust CCMs at various pH conditions must be involved in two or more pathways for the acquisition of exogenous carbon. Our findings show that Tris, AZ and EZ all significantly decreased the net photosynthetic rate of U. linza (Fig 4), that is, acidic compartments, internal and external CA were all the functional elements in the CCMs. The robust CCMs of U. linza may partially explain its ecological success as it does experience pH perturbations in the field, which is lower pH at night due to respiration and higher pH in the daytime due to photosynthesis. When green tides break out, the seawater is covered with extensive Ulva thalli which could lead to a dramatic increase of pH, efficient CCMs at higher pH support continuous growth of Ulva and thus the development of green tides. High CO2 acclimatised U. linza still showed consistent net photosynthetic rate at various pH. As discussed above, ocean acidification altered the pathways of CCMs in U. linza, but it seems not to alter the capability of U. linza to respond to changes of seawater carbon chemistry, which could be attributed to its diverse pathways of CCMs and differential responses of pathways of CCMs to ocean acidulation.

On the other hand, the net photosynthetic rate in high CO2-cultured U. linza was reduced compared to the low CO2-cultured plant when they were exposed to high light intensity. When rETR and NPQ were examined, both of them were enhanced at HC and this trend was more significant at HCHL. NPQ is an important photoprotective process that can dissipate excess energy, and avoid or reduce formation of reactive oxygen species produced by excessive light. U. linza grown under HC showed increased NPQ (28.60%) when exposed to LL, suggesting that the down-regulated CCMs at HC may lead to the need to dissipate excess energy even at a light intensity of 100 μmol photons m-2 s-1. When thalli were exposed to 600 μmol photons m-2 s-1, HC-grown U. linza presented an increase of 37.82% in NPQ, indicating more severe light stress. Despite increased thermal dissipation (NPQ), high light still reduced the net photosynthetic rate of U. linza grown at HC, which may imply the protective activity is not enough to fully avoid the photodamage caused by excessive light. The increased NPQ and reduced net photosynthetic rate at HCHL was also documented in phytoplankton assemblages [37] and U. prolifera [38]. This assumption of thalli grown at HC suffering more severe light stress is also supported by the alteration of light-capture pigments. High CO2-grown Ulva had lower Chl a and Chl b contents. This decline in photosynthetic pigments could avoid over-excitation of the electron transport and be a sign of light sufficient in thalli grown at HC. Such a “pigment economy” phenomenon at elevated CO2 conditions seems to be a general rule in plants since it has been also found in U. prolifera [38], U. rigida [53], unicellular chlorophyte Dunaliella viridis [55], cyanobacterium Spirulina platensis [56], and trees [57]. In addition, highest pH of 10 dramatically reduced net photosynthetic rate when thalli were exposed to HL no matter U. linza was grown under LC or HC, indicating U. linza can maintain consistent net photosynthetic rate at various seawater carbon chemistry conditions when expose to LL but when light was enhanced, the increased requirement for CO2 was beyond the capacity of CCMs.

Conclusions

Our study, for the first time, provided experimental data regarding the robustness of the ocean acidification acclimatised green tide algae to changes of seawater carbon chemistry and vulnerability to light stress and proposed a possible mechanism. Ocean acidification changed the CCMs of U. linza, in which the function of external CA was switched off, the proportion of internal CA was reduced, but the importance of acidic compartments and diffusion of CO2 was advanced, which may explain why ocean acidification did not affect the efficient response of the plant to various seawater carbon chemistry. The saved energy from the down-regulated CCMs may lead to increased vulnerability of the plant to high light. Future ocean surfaces might receive rising solar radiation with the compulsory implementation of air quality measures in industrialised countries and thus the decline in anthropogenic aerosol emissions [58]. From this point of view, future ocean acidification might have a depressing effect on Ulva and consequently Ulva cultivation or green tides.

Supporting Information

Acknowledgments

This study was supported by the National Natural Science Foundation of China (No. 41476097), the Natural Science Foundation of Jiangsu Province (No. BK20161295) and Priority Academic Program Development of Jiangsu Higher Education Institutions. We sincerely thank Dr Serena Lim for contributing to the improvement of this manuscript.

Author Contributions

  1. Conceptualization: JX GG YL.
  2. Data curation: GG JX YL.
  3. Formal analysis: GG YL JX.
  4. Funding acquisition: JX.
  5. Investigation: YL JX GG XL ZF.
  6. Methodology: JX YL.
  7. Project administration: JX.
  8. Resources: JX XL.
  9. Supervision: JX.
  10. Validation: XJ YL GG.
  11. Writing – original draft: GG JX YL.
  12. Writing – review & editing: GG JX.

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