Next Article in Journal
Chromosome and Genome Diversity in the Genus Trifolium (Fabaceae)
Next Article in Special Issue
The Potential of Cold Plasma and Electromagnetic Field as Stimulators of Natural Sweeteners Biosynthesis in Stevia rebaudiana Bertoni
Previous Article in Journal
Bioactive Essential Oils from Cuban Plants: An Inspiration to Drug Development
Previous Article in Special Issue
Increase of Productivity and Neutralization of Pathological Processes in Plants of Grain and Fruit Crops with the Help of Aqueous Solutions Activated by Plasma of High-Frequency Glow Discharge
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Plants
Volume 10
Issue 11
10.3390/plants10112516
plants-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles thumb_up
...
Endorse textsms
...
Comment
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Plasma-Activated Water Triggers Rapid and Sustained Cytosolic Ca2+ Elevations in Arabidopsis thaliana

by
Enrico Cortese
1,
Alessio G. Settimi
2,
Silvia Pettenuzzo
3,4,5,
Luca Cappellin
5,
Alessandro Galenda
6,
Alessia Famengo
6,
Manuele Dabalà
2,
Vanni Antoni
7 and
Lorella Navazio
1,8,*
1
Department of Biology, University of Padova, Via U. Bassi 58/B, 35131 Padova, Italy
2
Department of Industrial Engineering, University of Padova, Via F. Marzolo 9, 35131 Padova, Italy
3
Center Agriculture Food Environment (C3A), University of Trento, Via E. Mach 1, 38010 San Michele all’Adige, Italy
4
Research and Innovation Centre, Edmund Mach Foundation, Via E. Mach 1, 38010 San Michele all’Adige, Italy
5
Department of Chemical Sciences, University of Padova, Via F. Marzolo 1, 35131 Padova, Italy
6
CNR Institute of Condensed Matter Chemistry and Technologies for Energy (ICMATE), Corso Stati Uniti 4, 35127 Padova, Italy
7
Consorzio RFX, Corso Stati Uniti 4, 35127 Padova, Italy
8
Botanical Garden, University of Padova, Via Orto Botanico 15, 35123 Padova, Italy
*
Author to whom correspondence should be addressed.
Plants 2021, 10(11), 2516; https://doi.org/10.3390/plants10112516
Submission received: 29 October 2021 / Revised: 12 November 2021 / Accepted: 16 November 2021 / Published: 19 November 2021
(This article belongs to the Special Issue Effects of Non-thermal Plasma Treatment on Plant Physiological and Biochemical Processes)
Browse Figures
Versions Notes

Abstract

:
Increasing evidence indicates that water activated by plasma discharge, termed as plasma-activated water (PAW), can promote plant growth and enhance plant defence responses. Nevertheless, the signalling pathways activated in plants in response to PAW are still largely unknown. In this work, we analysed the potential involvement of calcium as an intracellular messenger in the transduction of PAW by plants. To this aim, Arabidopsis thaliana (Arabidopsis) seedlings stably expressing the bioluminescent Ca2+ reporter aequorin in the cytosol were challenged with PAW generated by a plasma torch. Ca2+ measurement assays demonstrated the induction by PAW of rapid and sustained cytosolic Ca2+ elevations in Arabidopsis seedlings. The dynamics of the recorded Ca2+ signals were found to depend upon different parameters, such as the operational conditions of the torch, PAW storage, and dilution. The separate administration of nitrate, nitrite, and hydrogen peroxide at the same doses as those measured in the PAW did not trigger any detectable Ca2+ changes, suggesting that the unique mixture of different reactive chemical species contained in the PAW is responsible for the specific Ca2+ signatures. Unveiling the signalling mechanisms underlying plant perception of PAW may allow to finely tune its generation for applications in agriculture, with potential advantages in the perspective of a more sustainable agriculture.

Graphical Abstract

1. Introduction

Cold atmospheric plasmas are weakly ionized gases that can be generated in ambient air. At a relatively low consumption of energy, they constitute a unique delivery system of a rich family of short- and long-lived chemicals, such as reactive oxygen (ROS) and nitrogen (RNS) species, called RONS when grouped together. Cold plasmas have already proven effective in medicine applications such as in regenerative medicine for blood coagulation and dental treatment, as well as in sanitizing surfaces and medical tools, and further applications, such as anti-cancer treatments, are under investigation [1]. When interacting with a liquid, cold plasmas can generate further new chemical species, as in the case of the so-called plasma-activated water (PAW). The nature and concentration of the RONS generated depend on the sources and gases used for plasma generation, on the chemical environment, and can be modulated by varying parameters such as voltage, distance between the liquid and the plasma, exposure time, and type of electrodes used. In the generated PAW short-living species such as hydroxyl- (OH), superoxide- (O2•−), nitric oxide- (NO) radicals, and ozone (O3) are formed and further react, yielding nitric oxide (NO), nitrate (NO3) and nitrite (NO2), peroxynitrite (ONOO), and hydrogen peroxide (H2O2) [2].
The complex chemistry occurring during the PAW generation has recently attracted a great deal of interest due to a variety of applications in agriculture and in the food sector [2,3,4,5]. In plant biology, cold plasma and PAW have been shown to increase the seed germination rate, even under osmotic and saline stresses, as well as to promote plant growth [6,7,8,9,10,11]. Moreover, PAW irrigation of tomato plants has been reported to induce defence gene expression [12,13] and accumulation of the defence hormones salicylic acid and jasmonic acid [12,14]. A differential expression of genes involved in the main plant defence pathways was also confirmed in PAW-treated periwinkle and grapevine plants [15]. These studies suggest that PAW can play beneficial roles in agriculture by promoting plant growth and pre-alerting plant defence prior to a potential subsequent attack by pathogens, a phenomenon defined as “priming” [8,16]. PAW may, therefore, represent an attractive eco-friendly alternative to pesticides, whose administration in bulk quantities represent a matter of growing concern for their impact on the environment. Nevertheless, studies addressing the signalling pathways activated in plants in response to PAW have been lacking so far.
In this work, we investigated the signalling mechanisms underpinning the effects played by PAW on plants. In particular, we evaluated the potential involvement of calcium in the plant perception and transduction of the mixture of molecules contained in PAW. Calcium is a universal signalling element involved in a wide range of physiological processes in all living organisms [17]. In plants, Ca2+ serves as an intracellular messenger of primary importance in many different signal transduction pathways [18]. A plethora of abiotic stimuli, such as touch/wind [19,20], salinity, drought [21,22,23], oxidative stress [24], and cold/heat stress [25,26,27,28,29,30,31], as well as biotic stimuli in pathogenic and beneficial plant-microbe interactions [32,33], have been shown to evoke in plants specific spatio-temporal Ca2+ signals, which are further transduced by Ca2+ sensor proteins into transcriptional and metabolic responses [34,35,36]. Notably, Ca2+-based signalling circuits are well conserved along the green lineages, from algae to embryophytes [30,37].
To test the effect of PAW on the induction of transient changes in the cytosolic concentration of the ion ([Ca2+]cyt), we used as an experimental system a transgenic line of the model plant Arabidopsis thaliana (Arabidopsis) stably expressing the genetically encoded Ca2+ indicator aequorin in the cytosol. The obtained results showed that Arabidopsis perception of PAW generated by two different plasma torches is mediated by rapid and sustained cytosolic Ca2+ elevations. Further studies are needed in the future to address conserved and unique features of Ca2+-mediated sensing mechanisms of PAW in phylogenetically distant plant species, as well as in plants of economic interest. A better understanding of the biochemical and molecular bases of plant perception of PAW may allow to finely tune the chemical composition of PAW for an optimal application in agriculture.

2. Results

2.1. Generation of PAW by Plasma Torch

During the course of this work two plasma torches (torch #1 and torch #2) were used, both consisting of a non-transferred arc generated through a narrow nozzle less than 1 cm wide, so that a relatively high-power plasma could be generated and concentrated in a relatively narrow surface. To produce PAW, samples of 50 mL deionized H2O were treated for different time intervals, ranging from 1 to 10 min, with the torch at a distance of 1 to 10 cm from the H2O surface, in a cooling bath of ice and salt. Operational parameters of the plasma torch were set to operate in a range of power 450–1800 W and with a pressure from 1 to 3 bar. Upon generation, PAW was quickly fractionated in small single-use aliquots and immediately frozen in liquid N2.

2.2. PAW Triggers a Cytosolic Ca2+ Increase in Aequorin-Expressing Arabidopsis thaliana Seedlings

To evaluate the potential involvement of Ca2+ signalling in the perception of PAW by plants, an Arabidopsis line stably expressing the bioluminescent Ca2+ indicator aequorin in the cytosol was used [38,39,40]. Ca2+ measurement assays were carried out in 7-day-old transgenic Arabidopsis intact seedlings, which were challenged with PAW generated by the above-described plasma torch settings. Plant treatment with PAW induced rapid and sustained cytosolic Ca2+ increases (Figure 1a), whose magnitude was found to correlate with the duration of the exposure of H2O to plasma (Figure 1b). No [Ca2+]cyt changes were observed in control samples, in which deionized H2O (without activation by plasma) was applied to seedlings (Figure 1a). These data demonstrate that PAW sensing by plants occurs through intracellular Ca2+ changes, characterized by a specific signature.

2.3. The Dynamics of the Elicited Ca2+ Signals Depend on PAW Features

We next investigated the potential dependence of PAW-induced Ca2+ signals on the characteristics of PAW. It is known that the production of plasma-induced chemistry and, in particular, RONS generated within the aqueous medium depends on the plasma source and on several parameters, among which is power [41]. Operating the plasma torch at different power regimes, ranging from 450 to 1800 W, was found to affect the amplitude of the recorded Ca2+ changes (Figure 2a,b), confirming a key role played by the modulation of the energy transferred to the pressurized gas during the generation of the cold plasma.
Ca2+ signals with progressively reduced magnitude were triggered by increasing ratios of PAW dilution (Figure 3a,b), demonstrating a dose-dependent effect in the PAW-induced intracellular Ca2+ changes triggered in Arabidopsis seedlings.

2.4. Effects of Different Temperature and Time Intervals of PAW Storage on Cytosolic Ca2+ Changes

An additional factor that was taken into consideration was the effect of different temperature and time intervals of PAW storage. Upon production, PAW was kept at different temperatures (−80 °C, 4 °C, and room temperature [RT]) for increasing time intervals, ranging from the immediate use up to 3 months. Figure 4 shows that PAW stored at −80 °C retains unvaried inducing activity on [Ca2+]cyt elevations for at least 3 months. On the other hand, storage at either 4 °C or RT was found to severely affect PAW properties, resulting in greatly reduced Ca2+ signals already after 1 day from PAW production (Figure 4).

2.5. PAW Induces a Long-Lasting Cytosolic Ca2+ Elevation, but Not Cell Death

Ca2+ measurement assays demonstrated that the [Ca2+]cyt elevation evoked by PAW appeared long-lasting, with sustained Ca2+ levels as high as ~1 µM after 1 h (Figure 5a). Nevertheless, viability assays carried out in Arabidopsis suspension-cultured cells [39] by the Evans blue test demonstrated the lack of cytotoxic effects by the PAW treatment. Indeed, no significant increase in cell death was found either at 1 h or even 48 h after PAW administration, in comparison with control samples (Figure 5b).

2.6. The Peculiar Chemical Environment Generated by Activation of H2O by Plasma Discharge Accounts for the Specific PAW-Induced Ca2+ Signature

Chemical analyses performed by ion chromatography allowed the detection and quantification of nitrate (NO3) and nitrite/nitrous acid (NO2/HNO2) in the PAW (Figure 6a,b). The content in ammonium (NH4+), measured by ion chromatography, as well as the content of hydrogen peroxide (H2O2), measured through spectrophotometric analysis of TiIV/H2O2 adduct, resulted under the detection limit of the assays [42]. Additional analyses performed by the ferrous oxidation in xylenol orange (FOX1) method [43] provided a quantification of H2O2 content at 0.59 ± 0.02 mg/L (Figure 6b).
Notably, the separate administration of the single chemical components (H2O2, NO2, and NO3), at the same concentrations as those measured in the PAW, did not trigger detectable Ca2+ response in transgenic Arabidopsis seedlings (Figure 7). No differences were observed when NO2 and NO3 were provided as either K+ salts or Na+ salts (Figure 7). These results indicate that the unique mixture of the different chemical species found in the PAW is responsible for the induced Ca2+ signature.
Measurements of pH and conductivity of PAW demonstrated that the exposure of deionized H2O to cold plasma resulted in remarkable changes of its chemical properties. Figure S1 shows a decrease in pH from about 5.5 in deionized H2O to about 3.0 (in PAW generated by 5 min exposure to plasma torch #1 operating at 900 W). The extent of the pH drop was found to depend on the time interval of plasma discharge (Figure S1a), torch power (Figure S1c), and PAW dilution (Figure S1e). Likewise, the conductivity of deionized H2O was found to be affected by the plasma discharge, with significantly higher values in PAW obtained through increasing time intervals of exposure to plasma (Figure S1b), increasing torch powers (Figure S1d), and PAW concentration (Figure S1f).
To check if the low pH could be responsible for the observed PAW-induced Ca2+ elevations, aequorin-expressing Arabidopsis seedlings were challenged with deionized H2O that had been previously acidified to the same pH as PAW at 1:4 dilution (from pH 5.5 to pH 3.5). The pH change alone was found to only slightly perturb the resting level of cytosolic Ca2+ (Figure 8a); therefore, the low pH-induced integrated [Ca2+]cyt change could not account for the remarkably higher Ca2+ signal induced by PAW (Figure 8b). This result further confirms that the peculiar chemical environment generated in the PAW by plasma discharge is the ultimate responsible factor for the specific PAW-induced Ca2+ signature. In agreement with these data, no significant changes in the PAW pH were found as a consequence of PAW storage at different temperatures for different time intervals (Figure S2).

2.7. The Plant Ca2+ Response to PAW Depends on the Total Energy Transferred to the H2O during Plasma Discharge

Further experiments were carried out with an additional plasma torch (torch #2) operating in a different range of power and gas pressure (see Materials and Methods). Administration of the PAW generated by this plasma source to Arabidopsis seedlings resulted in the induction of a cytosolic Ca2+ increase that closely mirrored the one generated by the first plasma torch (Figure 9a). Spectrophotometric analyses also confirmed, in this case, the presence of nitrate and nitrite in the PAW. Figure 9b shows the UV-Vis spectrum of the obtained PAW. The main absorption in the range 190–250 nm is ascribed to nitrite, nitrate, and hydrogen peroxide. In the 270–420 nm interval, the structured band typical of acidic NO2 is present at 354 nm, while the maximum of the nitrate absorption reported at 300 nm is not visible due to the lower concentration of NO3 species [44]. It must be noted that with this alternative torch, an exposure of the H2O to plasma lasting only 90 s was found to be sufficient to induce a Ca2+ increase in comparatively similar intensity to the one generated by 5 min exposure with the first torch (Figure 1). Indeed, the magnitude of the evoked plant Ca2+ response was found to depend on the overall power of the torch, which is the critical factor determining the energy transferred to the H2O during plasma discharge.

3. Discussion

In the last few years there has been a surge of papers in the field of cold plasma technology. Several studies have addressed the effects of the administration of PAW to plants, concerning the promotion of growth and development [5,8,16], as well as the induction of defence responses (see [5,9,14,16] for reviews).
In this work we focused our attention on the elucidation of the mechanisms underlying PAW perception by plants. By using an Arabidopsis line stably expressing the bioluminescent Ca2+ reporter aequorin in the cytosol, we demonstrated that PAW evokes rapid and sustained cytosolic Ca2+ elevations, characterized by specific signatures, that were found to depend upon several parameters, such as: (a) operational conditions of the torches used to generate PAW; (b) time interval of H2O exposure to plasma; (c) dose of PAW administered to plants; and (d) temperature and time interval of PAW storage. In particular, the magnitude of the recorded Ca2+ signals, measured as integral of the overall PAW-induced Ca2+ increases, was found to depend on the torch power, determining the energy transferred to the water during PAW generation. This was also confirmed by the use of a different torch as plasma generating device. The consistency of the results using two torches operating at different operational parameters and with different nozzle geometries has, therefore, confirmed the key role of the transferred energy to determine the Ca2+ signal evolution.
The involvement of Ca2+ signalling in the transduction mechanisms triggered by PAW in plants could somehow be anticipated, because PAW is known to contain a mixture of ROS and RNS. In the literature, a tight link between ROS and Ca2+ has been firmly highlighted [45,46]. Moreover, the involvement of Ca2+ also in nitrate sensing is increasingly emerging [47,48]. However, it must be noted that the treatment of Arabidopsis seedlings with the same doses of H2O2, nitrate, and nitrite as those measured in the PAW did not result in detectable Ca2+ changes. Indeed, the concentrations of H2O2 and nitrate commonly reported as capable of inducing cytosolic Ca2+ elevations are much higher, i.e., in the millimolar range [24,47]. These data suggest that the induction of the PAW-induced Ca2+ signature may be attributable to a complex “cocktail” of different reactive chemical species contained in the PAW, rather than to a single component (such as H2O2 or nitrate).
The PAW-induced cytosolic Ca2+ signature is characterized by a fast, immediate increase in [Ca2+]cyt up to 10–25 times the resting level of the ion; notably, the Ca2+ change was found to reach, after about 10 min, a plateau that is maintained for additional 20 min, before slowly decreasing. Continuous monitoring of Ca2+ showed that even after 1 h the Ca2+ elevation did not dissipate completely. However, cell viability assays demonstrated the lack of cytotoxic effects of PAW in our experimental set up. An intriguing possibility is that the unique dynamics of the PAW-activated Ca2+ signals, i.e., a sustained, long-lasting Ca2+ elevation, may be a crucial determinant of the induced “priming” condition, consisting in the activation of defence gene expression and antioxidant activities that bolster plant resistance to subsequent pathogen attacks. The lack of return of [Ca2+]cyt back to pre-stimulus resting values (about 100 nM) may lead to a state of plant alert in which the plant gets more prepared to face subsequent battles [49]. Future research will be directed at unravelling whether PAW-induced Ca2+ signalling underlies only plant self-defence responses or also plant growth promoting effects.
Ca2+ measurement assays performed by challenging transgenic Arabidopsis seedlings with PAWs stored for different time intervals at different temperatures demonstrate that only PAW quickly frozen in liquid N2 upon production and then stored at −80 °C retained the ability to induce a Ca2+-mediated response in plants, whereas the Ca2+-inducing activity of PAW stored at 4 °C or room temperature rapidly decreased over time. It has previously been reported that only PAW stored at −80 °C maintained an unvaried bactericidal activity against S. aureus, providing important cues for optimal applications in disinfection and food preservation [50]. Our results confirm those observations about the dependence of the physico-chemical properties of PAW on temperature storage, by extending the range of PAW activities to Ca2+-mediated responses elicited in plants. The obtained data highlight the necessity for either cryopreservation or generation of the PAW ready-to-use and in situ, in order to allow an effective and quick administration to plants upon production.
In summary, in this work we provided evidence that Ca2+ acts as an intracellular messenger in the signalling pathway triggered by PAW in Arabidopsis. Our data indicate the possibility to use aequorin-based Ca2+ measurements as a rapid and reliable assay to rapidly monitor early plant responses to PAW. Establishing a sound scientific ground will provide the key elements to develop tools and treatments aimed to improve plant growth and resistance to pathogens, in order to increase crop yield in a sustainable and eco-friendly way.

4. Materials and Methods

4.1. Plant Material and Growth Conditions

An Arabidopsis thaliana ecotype Columbia (Col-0) transgenic line (Cyt_YA) stably expressing in the cytosol the bioluminescent Ca2+ reporter aequorin fused to yellow fluorescent protein (YFP) [38,39,40] was used in this study. Seeds were surface-sterilized and sown on half-strength Murashige and Skoog medium (½ MS) (Duchefa Biochemie, Haarlem, The Netherlands) supplemented with 1.5% (w/v) sucrose, 0.8% (w/v) agar. Seedlings were grown for 7 days under a 16/8 h light/dark photoperiod at 21 °C. In some experiments, cell suspension cultures derived from the Cyt-YA line [39] were used. They were maintained and subcultured weekly in MS medium containing 0.5% (w/v) sucrose, 0.5 µg/mL 2,4-dichlorophenoxiacetic acid (2,4-D), and 0.25 µg/mL 6-benzylaminopurine (BAP) (Merck, Darmstadt, Germany), supplemented with 10 µg/mL kanamycin as selective agent, as recently described [51].

4.2. Generation of PAW

PAW was generated by exposing deionized H2O at room temperature to the cold plasma obtained by two different plasma torches operating in a range of power 450–2700 W and with pressure from 1 to 3 bar. Torch #1 was a single rotating FLUME Jet RD1004 with an FG 1001 plasma generator (Plasmatreat, Elgin, IL, USA), that worked with an excitation frequency between 16 and 20 kHz and generated a plasma with a maximum power of 2.7 kW (Voltage = 230 V, Current = 12 A). Torch #2 was an AcXys ULS series atmospheric pressure cold plasma (AcXys Technologies, Saint-Martin-le-Vinoux, France) fed with purified air; plasma nozzle ϕ = 5 mm. Initial tests were performed varying the H2O amount, the distance of the nozzle from the H2O surface (from 1 to 10 cm), and the treatment time (from 1 to 10 min). H2O was kept in beakers immersed in an ice and salt cooling bath, in order to keep the H2O temperature increase within 40 °C for the longer treatments and the maximum power. Taking the pH as a target reference (i.e., 3.0), it has been found that the best compromise between temperature rise and pH change was, for torch #1, with the nozzle at 1.5 cm from the H2O surface and with treatment duration between 3 and 5 min. Concerning torch #2, the target pH was achieved with the nozzle at 10 cm from the H2O surface and 90 s of treatment time. Therefore, most of the results reported in this paper refer to 50 mL deionized H2O with its surface exposed at 1.5 cm from the torch nozzle with the standard protocol parameters set at about 900 W for 5 min concerning torch #1 and 10 cm from torch to H2O surface at 800 W for 90 s concerning torch #2. After generation, PAW was divided in single-use aliquots (1 mL for Ca2+ measurement purposes, 5 mL for pH and conductivity measurements or 25 mL for chemical analyses), immediately cryogenically frozen through immersion in liquid N2, and then stored at −80 °C. For long-term storage tests, some PAW aliquots were kept also at 4 °C or room temperature.

4.3. Chemical Analyses of PAW

Nitrite and nitrate in PAW were quantified by Dionex ICS-6000 SP ion chromatography on a Dionex IonPac ASIP-4 μm column 2 × 250 mm (Thermo Fisher Scientific, Waltham, MA, USA). Ammonium concentration was determined by Dionex Easion ion chromatography equipped with a Dionex IonPac CS12A RFIC column 4 × 250 mm (Thermo Fisher Scientific). PAW conductivity and pH were measured with electrode-based instruments, Cond7+ (XS Instruments, Carpi, Italy) and pH METER BasiC 20 (Crison, Alella, Spain), respectively.
H2O2 content in PAW was measured by spectrophotometric analysis of TiIV/H2O2 adduct as described by [52]. Briefly, 0.5 mL of titanium (IV) oxysulfate solution was added to 1 mL of the sample and diluted with 8.5 mL deionized H2O. Spectrophotometric analysis of the peroxidic complex [Ti(O2)OH(H2O)3]+aq was then carried out measuring the absorption at 409 nm with a double beam spectrometer Varian Cary 100 Bio (Varian, Palo Alto, CA, USA), using a solution containing 0.5 mL of TiOSO4 and 9.5 mL of deionized H2O as reference. H2O2 content in PAW was also determined through the FOX1 method [43]. The assay is based on a colorimetric reaction caused by the peroxide-mediated oxidation of Fe2+ followed by the reaction of Fe3+ with xylenol orange. A total of 50 μL of diluted PAW samples (consisting in 10 μL of PAW and 40 μL of H2O) were added to 950 μL of assay solution (0.25 mM ammonium ferrous sulfate, 25 mM H2SO4, 0.1 mM xylenol orange, and 100 mM sorbitol) and the absorbance at 560 nm was detected after 1 h incubation.
UV-Vis absorbance was measured immediately after the production of PAW by torch #2 using a double-beam UV-Vis spectrophotometer UV-2600 (Shimadzu, Kyoto, Japan) on quartz cuvettes with standard optical path of 10 mm. The spectra were recorded from 190 to 450 nm with a spectral resolution of 1 nm and a scan speed of 480 nm/min.

4.4. Aequorin-Based Ca2+ Measurement Assays

Transgenic Arabidopsis seedlings (7-day-old) were incubated overnight in the dark with 5 µM coelenterazine (Prolume, Pinetop, AZ, USA) to reconstitute the functional aequorin probe. Prior to the start of the experiment, each seedling was gently rinsed and placed in 250 µL deionized H2O inside the chamber of a custom-made luminometer (ET Enterprises Ltd., Uxbridge, UK), in close proximity to a low-noise photomultiplier, with a built-in amplifier discriminator. The output was captured using a photon-counting board. After 100 s, 250 µL of either PAW (tested at various dilutions) or deionized H2O (that has not been exposed to plasma; used as control) were injected. In some experiments, Arabidopsis seedlings were challenged with H2O2, NO2, and NO3 at the same concentrations as those measured in the PAW. NO2 and NO3 were administered as either Na+ or K+ salts (Merck). At the end of the experiment, 500 µL of a solution containing 1 M CaCl2, 30% (v/v) ethanol was added to completely discharge the remaining Ca2+ probe, allowing for the conversion of the collected light signal into [Ca2+]cyt by means of a built-in algorithm based on the calibration curve of aequorin [53]. Integrated [Ca2+]cyt values were obtained as the sum of each instantaneous [Ca2+]cyt value for the entire duration of the experiment.

4.5. Cell Viability Assay

Cell viability was determined by the Evans blue method [54]. Briefly, Arabidopsis cell suspension cultures obtained from the transgenic line [39] were kept in control conditions or treated at mid-exponential phase (4 days) with PAW (diluted 1:4) for either 1 h or 48 h. After 15 min incubation with 0.05% (w/v) Evans blue (Merck), excess and unbound dye was removed by extensive washing with H2O. The dye bound to dead cells was solubilized in 1% (w/v) SDS, 50% (v/v) methanol for 30 min at 55 °C. The percentage of cell death was assessed by measuring the absorbance at 600 nm. As positive control (100% cell death), cells were incubated for 10 min at 100 °C.

Supplementary Materials

The following are available online at https://www.mdpi.com/article/10.3390/plants10112516/s1: Figure S1, effects of different plasma exposure time intervals, torch power and PAW dilution on pH and conductivity of PAWs; Figure S2, effect of time interval and temperature of PAW storage on pH.

Author Contributions

Conceptualization, L.N. and V.A.; methodology, L.N., E.C., V.A., M.D., L.C., A.G. and A.F.; software, E.C.; validation, E.C., A.G.S., S.P. and L.C.; formal analysis, E.C.; investigation, E.C., A.G.S., S.P., L.C., A.G. and A.F.; resources, V.A., M.D., L.C., A.F. and L.N.; data curation, E.C., L.C., A.G. and V.A.; writing—original draft preparation, L.N. and E.C.; writing—review and editing, L.N., E.C., V.A., L.C, A.G., A.F. and M.D.; visualization, E.C.; supervision, L.N. and V.A.; project administration, L.N.; funding acquisition, L.N. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by the University of Padova, Italy, PRID 2018 (prot. BIRD180317) and DOR 2018–2021 to L.N.; L.C. acknowledges funding from P-DiSC#02BIRD2019-UNIPD. E.C. is the recipient of a post-doctoral grant from the Department of Biology, University of Padova, Italy (MIUR Excellence Department Project 2018).

Data Availability Statement

The data presented in this study are available on request from the corresponding author.

Acknowledgments

We thank U. Vothknecht (Bonn, Germany) for kindly providing A. thaliana transgenic seeds (Cyt-YA) expressing cytosolic aequorin. We also acknowledge the Plant Genome Editing Facility of the Department of Biology, University of Padova, for support with in vitro and in vivo plant growth.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. Kaushik, N.K.; Ghimire, B.; Li, Y.; Adhikari, M.; Veerana, M.; Kaushik, N.; Jha, N.; Adhikari, B.; Lee, S.J.; Masur, K.; et al. Biological and medical applications of plasma-activated media, water and solutions. Biol. Chem. 2018, 400, 39–62. [Google Scholar] [CrossRef] [PubMed]
  2. Thirumdas, R.; Kothakota, A.; Annapure, U.; Siliveru, K.; Blundell, R.; Gatt, R.; Valdramidis, V.P. Plasma activated water (PAW): Chemistry, physico-chemical properties, applications in food and agriculture. Trends Food Sci. Technol. 2018, 77, 21–31. [Google Scholar] [CrossRef]
  3. Bourke, P.; Ziuzina, D.; Boehm, D.; Cullen, P.J.; Keener, K. The potential of cold plasma for safe and sustainable food production. Trends Biotechnol. 2018, 36, 615–626. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  4. Herianto, S.; Hou, C.Y.; Lin, C.M.; Chen, H.L. Nonthermal plasma-activated water: A comprehensive review of this new tool for enhanced food safety and quality. Compr. Rev. Food Sci. Food Saf. 2021, 20, 583–626. [Google Scholar] [CrossRef]
  5. Guo, D.; Liu, H.; Zhou, L.; Xie, J.; He, C. Plasma-activated water production and its application in agriculture. J. Sci. Food Agric. 2021, 101, 4891–4899. [Google Scholar] [CrossRef] [PubMed]
  6. Bafoil, M.; Jemmat, A.; Martinez, Y.; Merbahi, N.; Eichwald, O.; Dunand, C.; Yousfi, M. Effects of low temperature plasmas and plasma activated waters on Arabidopsis thaliana germination and growth. PLoS ONE 2018, 13, e0195512. [Google Scholar] [CrossRef] [PubMed]
  7. Bafoil, M.; Le Ru, A.; Merbahi, N.; Eichwald, O.; Dunand, C.; Yousfi, M. New insights of low-temperature plasma effects on germination of three genotypes of Arabidopsis thaliana seeds under osmotic and saline stresses. Sci. Rep. 2019, 9, 8649. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  8. Adhikari, B.; Adhikari, M.; Park, G. The effects of plasma on plant growth, development, and sustainability. Appl. Sci. 2020, 10, 6045. [Google Scholar] [CrossRef]
  9. Song, J.S.; Kim, S.B.; Ryu, S.; Oh, J.; Kim, D.S. Emerging plasma technology that alleviates crop stress during the early growth stages of plants: A review. Front. Plant Sci. 2020, 11, 988. [Google Scholar] [CrossRef] [PubMed]
  10. Starič, P.; Vogel-Mikuš, K.; Mozetič, M.; Junkar, I. Effects of nonthermal plasma on morphology, genetics and physiology of seeds: A review. Plants 2020, 9, 1736. [Google Scholar] [CrossRef]
  11. Šerá, B.; Scholtz, V.; Jirešová, J.; Khun, J.; Julák, J.; Šerý, M. Effects of non-thermal plasma treatment on seed germination and early growth of leguminous plants—A review. Plants 2021, 10, 1616. [Google Scholar] [CrossRef]
  12. Adhikari, B.; Adhikari, M.; Ghimire, B.; Park, G.; Choi, E.H. Cold atmospheric plasma-activated water irrigation induces defense hormone and gene expression in tomato seedlings. Sci. Rep. 2019, 9, 16080. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  13. Perez, S.M.; Biondi, E.; Laurita, R.; Proto, M.; Sarti, F.; Gherardi, M.; Bertaccini, A.; Colombo, V. Plasma activated water as resistance inducer against bacterial leaf spot of tomato. PLoS ONE 2019, 14, e0217788. [Google Scholar] [CrossRef] [PubMed]
  14. Adhikari, B.; Pangomm, K.; Veerana, M.; Mitra, S.; Park, G. Plant disease control by non-thermal atmospheric-pressure plasma. Front. Plant Sci. 2020, 11, 77. [Google Scholar] [CrossRef] [PubMed]
  15. Zambon, Y.; Contaldo, N.; Laurita, R.; Várallyay, E.; Canel, A.; Gherardi, M.; Colombo, V.; Bertaccini, A. Plasma activated water triggers plant defence responses. Sci. Rep. 2020, 10, 19211. [Google Scholar] [CrossRef] [PubMed]
  16. Holubová, L.; Kyzek, S.; Ďurovcová, I.; Fabová, J.; Horváthová, E.; Ševčovičová, A.; Gálová, E. Non-thermal plasma—A new green priming agent for plants? Int. J. Mol. Sci. 2020, 21, 9466. [Google Scholar] [CrossRef] [PubMed]
  17. Berridge, M.J.; Lipp, P.; Bootman, M.D. The versatility and universality of calcium signalling. Nat. Rev. Mol. Cell. Biol. 2000, 1, 11–21. [Google Scholar] [CrossRef]
  18. Sanders, D.; Pelloux, J.; Brownlee, C.; Harper, J.F. Calcium at the crossroads of signaling. Plant Cell 2002, 14 (Suppl. 1), S401–S417. [Google Scholar] [CrossRef] [Green Version]
  19. Knight, M.R.; Campbell, A.K.; Smith, S.M.; Trewavas, A.J. Transgenic plant aequorin reports the effects of touch and cold-shock and elicitors on cytoplasmic calcium. Nature 1991, 352, 524–526. [Google Scholar] [CrossRef] [PubMed]
  20. Knight, M.R.; Smith, S.M.; Trewavas, A.J. Wind-induced plant motion immediately increases cytosolic calcium. Proc. Natl. Acad. Sci. USA 1992, 89, 4967–4971. [Google Scholar] [CrossRef] [Green Version]
  21. Knight, H.; Trewavas, A.J.; Knight, M.R. Calcium signalling in Arabidopsis thaliana responding to drought and salinity. Plant J. 1997, 5, 1067–1078. [Google Scholar] [CrossRef] [PubMed]
  22. Sun, J.; Wang, M.J.; Ding, M.Q.; Deng, S.R.; Liu, M.Q.; Lu, C.F.; Zhou, X.Y.; Shen, X.; Zheng, X.J.; Zhang, Z.K.; et al. H2O2 and cytosolic Ca2+ signals triggered by the PM H+-coupled transport system mediate K+/Na+ homeostasis in NaCl-stressed Populus euphratica cells. Plant Cell Environ. 2010, 33, 943–958. [Google Scholar] [CrossRef] [PubMed]
  23. Chen, S.; Wang, X.; Jia, H.; Li, F.; Ma, Y.; Liesche, J.; Liao, M.; Ding, X.; Liu, C.; Chen, Y.; et al. Persulfidation-induced structural change in SnRK2.6 establishes intramolecular interaction between phosphorylation and persulfidation. Mol. Plant 2021, 14, 1814–1830. [Google Scholar] [CrossRef]
  24. Rentel, M.C.; Knight, M.R. Oxidative stress-induced calcium signaling in Arabidopsis. Plant Physiol. 2004, 135, 1471–1479. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  25. Knight, H.; Trewavas, A.J.; Knight, M.R. Cold calcium signaling in Arabidopsis involves two cellular pools and a change in calcium signature after acclimation. Plant Cell 1996, 8, 489–503. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  26. Gong, M.; van der Luit, A.H.; Knight, M.R.; Trewavas, A.J. Heat-shock-induced changes in intracellular Ca2+ level in tobacco seedlings in relation to thermotolerance. Plant Physiol. 1998, 116, 429–437. [Google Scholar] [CrossRef] [Green Version]
  27. Saidi, Y.; Finka, A.; Muriset, M.; Bromberg, Z.; Weiss, Y.G.; Maathuis, F.J.; Goloubinoff, P. The heat shock response in moss plants is regulated by specific calcium-permeable channels in the plasma membrane. Plant Cell 2009, 21, 2829–2843. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  28. Finka, A.; Cuendet, A.F.; Maathuis, F.J.; Saidi, Y.; Goloubinoff, P. Plasma membrane cyclic nucleotide gated calcium channels control land plant thermal sensing and acquired thermotolerance. Plant Cell 2012, 24, 3333–3348. [Google Scholar] [CrossRef] [Green Version]
  29. Lenzoni, G.; Knight, M.R. Increases in absolute temperature stimulate free calcium concentration elevations in the chloroplast. Plant Cell Physiol. 2019, 60, 538–548. [Google Scholar] [CrossRef] [PubMed]
  30. de Vries, J.; de Vries, S.; Curtis, B.A.; Zhou, H.; Penny, S.; Feussner, K.; Pinto, D.M.; Steinert, M.; Cohen, A.M.; von Schwartzenberg, K.; et al. Heat stress response in the closest algal relatives of land plants reveals conserved stress signaling circuits. Plant J. 2020, 103, 1025–1048. [Google Scholar] [CrossRef]
  31. Liu, Q.; Ding, Y.; Shi, Y.; Ma, L.; Wang, Y.; Song, C.; Wilkins, K.A.; Davies, J.M.; Knight, H.; Knight, M.R.; et al. The calcium transporter ANNEXIN1 mediates cold-induced calcium signaling and freezing tolerance in plants. EMBO J. 2021, 40, e104559. [Google Scholar] [CrossRef]
  32. Zipfel, C.; Oldroyd, G. Plant signalling in symbiosis and immunity. Nature 2017, 543, 328–336. [Google Scholar] [CrossRef]
  33. Aldon, D.; Mbengue, M.; Mazars, C.; Galaud, J. Calcium signalling in plant biotic interactions. Int. J. Mol. Sci. 2018, 19, 665. [Google Scholar] [CrossRef] [Green Version]
  34. Dodd, A.N.; Kudla, J.; Sanders, D. The language of calcium signaling. Annu. Rev. Plant Biol. 2010, 61, 593–620. [Google Scholar] [CrossRef]
  35. Costa, A.; Navazio, L.; Szabo, I. The contribution of organelles to plant intracellular calcium signalling. J. Exp. Bot. 2018, 69, 4175–4193. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  36. Kudla, J.; Becker, D.; Grill, E.; Hedrich, R.; Hippler, M.; Kummer, U.; Parniske, M.; Romeis, T.; Schumacher, K. Advances and current challenges in calcium signaling. New Phytol. 2018, 218, 414–431. [Google Scholar] [CrossRef]
  37. Edel, K.H.; Marchadier, E.; Brownlee, C.; Kudla, J.; Hetherington, A.M. The evolution of calcium-based signalling in plants. Curr. Biol. 2017, 27, R667–R679. [Google Scholar] [CrossRef] [PubMed]
  38. Mehlmer, N.; Parvin, N.; Hurst, C.H.; Knight, M.R.; Teige, M.; Vothknecht, U.C. A toolset of aequorin expression vectors for in planta studies of subcellular calcium concentrations in Arabidopsis thaliana. J. Exp. Bot. 2012, 63, 1751–1761. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  39. Sello, S.; Perotto, J.; Carraretto, L.; Szabò, I.; Vothknecht, U.C.; Navazio, L. Dissecting stimulus-specific Ca2+ signals in amyloplasts and chloroplasts of Arabidopsis thaliana cell suspension cultures. J. Exp. Bot. 2016, 67, 3965–3974. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  40. Sello, S.; Moscatiello, R.; Mehlmer, N.; Leonardelli, M.; Carraretto, L.; Cortese, E.; Zanella, F.G.; Baldan, B.; Szabò, I.; Vothknecht, U.C.; et al. Chloroplast Ca2+ fluxes into and across thylakoids revealed by thylakoid-targeted aequorin probes. Plant Physiol. 2018, 177, 38–51. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  41. Zhou, R.; Zhou, R.; Wang, P.; Xian, Y.; Mai-Prochnow, A.; Lu, X.; Cullen, P.J.; Ostrikov, K.; Bazaka, K. Plasma activated water (PAW): Generation, origin of reactive species and biological applications. J. Phys. D Appl. Phys. 2020, 53, 303001. [Google Scholar] [CrossRef]
  42. Judée, F.; Simon, S.; Bailly, C.; Dufour, T. Plasma-activation of tap water using DBD for agronomy applications: Identification and quantification of long lifetime chemical species and production/consumption mechanisms. Water Res. 2018, 133, 47–59. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  43. Wolff, S.P. [18] Ferrous ion oxidation in presence of ferric ion indicator xylenol orange for measurement of hydroperoxides. Method Enzymol. 1994, 233, 182–189. [Google Scholar] [CrossRef]
  44. Brisset, J.L.; Pawlat, J. Chemical effects of air plasma species on aqueous solutes in direct and delayed exposure modes: Discharge, post-discharge and plasma activated water. Plasma Chem. Plasma Process. 2016, 36, 355–381. [Google Scholar] [CrossRef]
  45. Gilroy, S.; Suzuki, N.; Miller, G.; Choi, W.G.; Toyota, M.; Devireddy, A.R.; Mittler, R. A tidal wave of signals: Calcium and ROS at the forefront of rapid systemic signaling. Trends Plant Sci. 2014, 19, 623–630. [Google Scholar] [CrossRef] [PubMed]
  46. Marcec, M.J.; Gilroy, S.; Poovaiah, B.W.; Tanaka, K. Mutual interplay of Ca2+ and ROS signaling in plant immune response. Plant Sci. 2019, 283, 343–354. [Google Scholar] [CrossRef] [PubMed]
  47. Riveras, E.; Alvarez, J.M.; Vidal, E.A.; Oses, C.; Vega, A.; Gutiérrez, R.A. The calcium ion is a second messenger in the nitrate signaling pathway of Arabidopsis. Plant Physiol. 2015, 169, 1397–1404. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  48. Wang, X.; Feng, C.; Tian, L.; Hou, C.; Tian, W.; Hu, B.; Zhang, Q.; Ren, Z.; Niu, Q.; Song, J.; et al. A transceptor–channel complex couples nitrate sensing to calcium signaling in Arabidopsis. Mol. Plant. 2021, 14, 774–786. [Google Scholar] [CrossRef] [PubMed]
  49. Prime-A-Plant Group; Conrath, U.; Beckers, G.J.; Flors, V.; García-Agustín, P.; Jakab, G.; Mauch, F.; Newman, M.A.; Pieterse, C.M.; Poinssot, B.; et al. Priming: Getting ready for battle. Mol. Plant Microbe Interact. 2006, 19, 1062–1071. [Google Scholar] [CrossRef] [Green Version]
  50. Shen, J.; Tian, Y.; Li, Y.; Ma, R.; Zhang, Q.; Zhang, J.; Fang, J. Bactericidal effects against S. aureus and physicochemical properties of plasma activated water stored at different temperatures. Sci. Rep. 2016, 6, 28505. [Google Scholar] [CrossRef] [Green Version]
  51. Cortese, E.; Carraretto, L.; Baldan, B.; Navazio, L. Arabidopsis photosynthetic and heterotrophic cell suspension cultures. Methods Mol. Biol. 2021, 2200, 167–185. [Google Scholar] [CrossRef] [PubMed]
  52. Sandri, F.; Danieli, M.; Zecca, M.; Centomo, P. Comparing catalysts of the direct synthesis of hydrogen peroxide in organic solvent: Is the measure of the product an issue? Chem. Cat. Chem. 2021, 13, 2653–2663. [Google Scholar] [CrossRef]
  53. Brini, M.; Marsault, R.; Bastianutto, C.; Alvarez, J.; Pozzan, T.; Rizzuto, R. Transfected aequorin in the measurement of cytosolic Ca2+ concentration ([Ca2+]c). A critical evaluation. J. Biol. Chem. 1995, 270, 9896–9903. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  54. Baker, C.J.; Mock, N.M. An improved method for monitoring cell-death in cell-suspension and leaf disc assays using evans blue. Plant Cell Tissue Organ Cult. 1994, 39, 7–12. [Google Scholar] [CrossRef]
Plants 10 02516 g001 550
Figure 1. Monitoring of changes in cytosolic Ca2+ concentration ([Ca2+]cyt) induced by plasma-activated water (PAW) in Arabidopsis thaliana (Arabidopsis). Ca2+ measurement assays were conducted in Arabidopsis seedlings stably expressing aequorin in the cytosol. Seven-day-old intact seedlings were challenged with 1:2 dilutions of different PAWs, obtained by exposing deionized H2O to cold plasma (generated at 900 W power, torch #1) for different time intervals: 1 min (green), 3 min (light blue), 5 min (blue), or 10 min (dark blue). Untreated deionized H2O was administered to control samples (grey). (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 1. Monitoring of changes in cytosolic Ca2+ concentration ([Ca2+]cyt) induced by plasma-activated water (PAW) in Arabidopsis thaliana (Arabidopsis). Ca2+ measurement assays were conducted in Arabidopsis seedlings stably expressing aequorin in the cytosol. Seven-day-old intact seedlings were challenged with 1:2 dilutions of different PAWs, obtained by exposing deionized H2O to cold plasma (generated at 900 W power, torch #1) for different time intervals: 1 min (green), 3 min (light blue), 5 min (blue), or 10 min (dark blue). Untreated deionized H2O was administered to control samples (grey). (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g001
Plants 10 02516 g002 550
Figure 2. Dependence of the PAW-induced [Ca2+]cyt elevation dynamics on the power of the plasma torch used to generate PAW. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:2 dilutions of different PAWs, obtained after 5 min exposure of deionized H2O to cold plasma generated under various torch #1 power conditions: 450 W (pale blue), 900 W (blue), and 1800 W (dark blue). (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 2. Dependence of the PAW-induced [Ca2+]cyt elevation dynamics on the power of the plasma torch used to generate PAW. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:2 dilutions of different PAWs, obtained after 5 min exposure of deionized H2O to cold plasma generated under various torch #1 power conditions: 450 W (pale blue), 900 W (blue), and 1800 W (dark blue). (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g002
Plants 10 02516 g003 550
Figure 3. Concentration dependence of PAW-induced [Ca2+]cyt increases. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with progressive dilutions of PAW (lighter colours indicate more diluted PAWs) generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min are shown. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 3. Concentration dependence of PAW-induced [Ca2+]cyt increases. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with progressive dilutions of PAW (lighter colours indicate more diluted PAWs) generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. (a) Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min are shown. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g003
Plants 10 02516 g004 550
Figure 4. (a) Effects of different temperatures and time intervals of PAW storage on PAW-induced [Ca2+]cyt increases. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:4 dilutions of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. Upon production, PAW was stored at different temperatures prior to plant treatment: −80 °C (blue), 4 °C (purple), and room temperature (RT) (pink) for various time intervals (ranging from 0 days up to 3 months), as indicated on top of the panels. Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. Arrowheads indicate the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min are shown. Key: d, days; w, weeks; and m, months. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 4. (a) Effects of different temperatures and time intervals of PAW storage on PAW-induced [Ca2+]cyt increases. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:4 dilutions of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. Upon production, PAW was stored at different temperatures prior to plant treatment: −80 °C (blue), 4 °C (purple), and room temperature (RT) (pink) for various time intervals (ranging from 0 days up to 3 months), as indicated on top of the panels. Data are the means (solid lines) ± SE (shading) of six seedlings derived from three independent growth replicates. Arrowheads indicate the time of stimulus application (at 100 s); (b) statistical analyses of integrated [Ca2+]cyt dynamics over 30 min are shown. Key: d, days; w, weeks; and m, months. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g004
Plants 10 02516 g005 550
Figure 5. The long-lasting [Ca2+]cyt elevation induced by PAW is not cytotoxic. (a) Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowhead) seedlings were challenged with a 1:4 dilution of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. Changes in [Ca2+]cyt were continuously recorded for 1 h. Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates; (b) viability of Arabidopsis cell suspension cultures treated with PAW (1:4 diluted) for either 1 h or 48 h (blue bars). Control cells were incubated with cell culture medium only (white bars). The 100% value corresponds to cells treated for 10 min at 100 °C (black bars). Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 5. The long-lasting [Ca2+]cyt elevation induced by PAW is not cytotoxic. (a) Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowhead) seedlings were challenged with a 1:4 dilution of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power. Changes in [Ca2+]cyt were continuously recorded for 1 h. Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates; (b) viability of Arabidopsis cell suspension cultures treated with PAW (1:4 diluted) for either 1 h or 48 h (blue bars). Control cells were incubated with cell culture medium only (white bars). The 100% value corresponds to cells treated for 10 min at 100 °C (black bars). Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g005
Plants 10 02516 g006 550
Figure 6. Chemical analyses for the detection of reactive oxygen and nitrogen species (RONS) in PAW. (a) Undiluted PAW (blue) generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power was analysed by ion chromatography. Deionized H2O (grey) was used as a control. NO2 (pink) and NO3 (purple) solutions were used as standards. Representative traces are shown. (b) Determination of H2O2 (green), NO2 (yellow), and NO3 (red) concentrations in PAW generated in six different batches.
Figure 6. Chemical analyses for the detection of reactive oxygen and nitrogen species (RONS) in PAW. (a) Undiluted PAW (blue) generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power was analysed by ion chromatography. Deionized H2O (grey) was used as a control. NO2 (pink) and NO3 (purple) solutions were used as standards. Representative traces are shown. (b) Determination of H2O2 (green), NO2 (yellow), and NO3 (red) concentrations in PAW generated in six different batches.
Plants 10 02516 g006
Plants 10 02516 g007 550
Figure 7. Monitoring of [Ca2+]cyt in response to hydrogen peroxide, nitrite, and nitrate at the same doses as those measured in the PAW at 1:2 dilution. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowheads) seedlings were challenged separately with: (a) 8.7 µM H2O2 (green trace); (b) 520.1 µM NO2 (provided as K+ salt, yellow trace; provided as Na+ salt, orange trace); (c) 264.2 µM NO3 (provided as K+ salt, red trace; provided as Na+ salt, brown trace); and (d) a solution (mix) containing all the above chemicals (with NO2 and NO3 provided as K+ salt, grey trace; with NO2_and NO3 provided as Na+ salt, black trace). Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates.
Figure 7. Monitoring of [Ca2+]cyt in response to hydrogen peroxide, nitrite, and nitrate at the same doses as those measured in the PAW at 1:2 dilution. Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowheads) seedlings were challenged separately with: (a) 8.7 µM H2O2 (green trace); (b) 520.1 µM NO2 (provided as K+ salt, yellow trace; provided as Na+ salt, orange trace); (c) 264.2 µM NO3 (provided as K+ salt, red trace; provided as Na+ salt, brown trace); and (d) a solution (mix) containing all the above chemicals (with NO2 and NO3 provided as K+ salt, grey trace; with NO2_and NO3 provided as Na+ salt, black trace). Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates.
Plants 10 02516 g007
Plants 10 02516 g008 550
Figure 8. Comparison between the [Ca2+]cyt responses induced by PAW and by an acidified H2O. Ca2+ assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:4 dilution of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power (blue) or deionized H2O acidified to the same pH as PAW at 1:4 dilution (pH 3.5) (black). Untreated deionized H2O (pH 5.5) was administered to control samples (grey). (a) Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s). (b) Statistical analyses of integrated [Ca2+]cyt dynamics over 60 min are shown. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Figure 8. Comparison between the [Ca2+]cyt responses induced by PAW and by an acidified H2O. Ca2+ assays were conducted in aequorin-expressing Arabidopsis seedlings. Seedlings were challenged with 1:4 dilution of PAW generated by exposing deionized H2O to cold plasma for 5 min at 900 W torch #1 power (blue) or deionized H2O acidified to the same pH as PAW at 1:4 dilution (pH 3.5) (black). Untreated deionized H2O (pH 5.5) was administered to control samples (grey). (a) Data are the means (solid lines) ± SE (shading) of six different seedlings derived from three independent growth replicates. The arrowhead indicates the time of stimulus application (at 100 s). (b) Statistical analyses of integrated [Ca2+]cyt dynamics over 60 min are shown. Bars labelled with different letters differ significantly (p < 0.05, Student’s t test).
Plants 10 02516 g008
Plants 10 02516 g009 550
Figure 9. Monitoring of [Ca2+]cyt in Arabidopsis seedlings challenged with PAW generated by an alternative plasma torch. (a) Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowhead) seedlings were challenged with 1:2 dilution of a PAW, obtained after 90 s exposure of deionized H2O to cold plasma generated by a different plasma torch (torch #2). Data are the means (solid lines) ± SE (shading) of three independent experiments. (b) Spectrophotometric UV-Vis analyses of the generated PAW, showing the characteristic spectrum of absorbance of nitrite, nitrate, and hydrogen peroxide. In the inset, a magnification of the region between 270 and 420 nm, highlighting the five-fingers band of NO2 around 354 nm, is shown.
Figure 9. Monitoring of [Ca2+]cyt in Arabidopsis seedlings challenged with PAW generated by an alternative plasma torch. (a) Ca2+ measurement assays were conducted in aequorin-expressing Arabidopsis seedlings. At 100 s (arrowhead) seedlings were challenged with 1:2 dilution of a PAW, obtained after 90 s exposure of deionized H2O to cold plasma generated by a different plasma torch (torch #2). Data are the means (solid lines) ± SE (shading) of three independent experiments. (b) Spectrophotometric UV-Vis analyses of the generated PAW, showing the characteristic spectrum of absorbance of nitrite, nitrate, and hydrogen peroxide. In the inset, a magnification of the region between 270 and 420 nm, highlighting the five-fingers band of NO2 around 354 nm, is shown.
Plants 10 02516 g009
Publisher’s Note: MDPI stays neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Share and Cite

MDPI and ACS Style

Cortese, E.; Settimi, A.G.; Pettenuzzo, S.; Cappellin, L.; Galenda, A.; Famengo, A.; Dabalà, M.; Antoni, V.; Navazio, L. Plasma-Activated Water Triggers Rapid and Sustained Cytosolic Ca2+ Elevations in Arabidopsis thaliana. Plants 2021, 10, 2516. https://doi.org/10.3390/plants10112516

AMA Style

Cortese E, Settimi AG, Pettenuzzo S, Cappellin L, Galenda A, Famengo A, Dabalà M, Antoni V, Navazio L. Plasma-Activated Water Triggers Rapid and Sustained Cytosolic Ca2+ Elevations in Arabidopsis thaliana. Plants. 2021; 10(11):2516. https://doi.org/10.3390/plants10112516

Chicago/Turabian Style

Cortese, Enrico, Alessio G. Settimi, Silvia Pettenuzzo, Luca Cappellin, Alessandro Galenda, Alessia Famengo, Manuele Dabalà, Vanni Antoni, and Lorella Navazio. 2021. "Plasma-Activated Water Triggers Rapid and Sustained Cytosolic Ca2+ Elevations in Arabidopsis thaliana" Plants 10, no. 11: 2516. https://doi.org/10.3390/plants10112516

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop