1. Introduction

Hydrogen peroxide (H₂O₂) has been traditionally linked to toxicity, but it also participates in signaling events by both regulating different physiological processes and activating antioxidant cascades (for reviews, see [1,2,3,4]). Generation and scavenging of H₂O₂ have been a matter of study for many decades, as well as the fluxes of peroxides between different cellular compartments.

Mitochondria is an important source of the production of reactive oxygen species. Both electron transport chain (ETC) components and other mitochondrial enzymes, such as 2-oxoglutarate dehydrogenase, pyruvate dehydrogenase, and the mitochondrial membrane forms of glycerol 3-phosphate dehydrogenase, contribute to the formation, directly or indirectly, of H₂O₂ (for a review, see [5]). When derived from the ETC and from other sources, peroxides are formed after spontaneous or superoxide dismutase-catalyzed dismutation from superoxide radicals. Another important source of H₂O₂ is the family of NADPH oxidases, normally referred to as NOX enzymes. Finally, a wide range of non-mitochondrial proteins, such as cytochrome P450 enzymes or xanthine oxidase, and organelles different from mitochondria, such as the endoplasmic reticulum, can all produce H₂O₂ (for a review, see [6]).

The quantitative contribution of these organelles and proteins to the final steady-state levels of H₂O₂ is unknown. Traditionally the ETC has been considered the main producer of reactive oxygen species, with 5% of the electron accidentally leaking to oxygen from transiently reduced ETC intermediates [7], while other predictions suggest a 0.15% electron leakage [8]. While the analysis of Mn-SOD knockout mice experiments strongly suggested that mitochondrial ROS generation is a physiologically significant process in vivo [9,10], the group of Imlay has proposed, using Escherichia coli, that the contribution of the ETC to H₂O₂ production is not major [11].

Most of the studies estimating mitochondrial H₂O₂ production have been performed in vitro with isolated mitochondria and with the aid of ETC inhibitors. Based on their use, the topology of ROS production has been predicted. It has been demonstrated that inhibition of complex I produces superoxide towards the matrix [12]. Regarding complex III (CIII), it was first proposed that the addition of antimycin A or other inhibitors caused superoxide generation towards the matrix [13]. However, the crystal structure of CIII revealed that the semiquinone, reducing oxygen to superoxide at complex III [14], faces the IMS [15], and indeed ROS are produced at both sides of the inner membrane upon treatment with CIII inhibitors [8,16,17,18]. The specific ETC sites causing mitochondrial ROS production in vivo in the absence of ETC inhibitors are unclear.

Regarding H₂O₂ scavenging, cells have developed efficient systems to metabolize peroxides. They are mainly based, although not exclusively [19], on two types of chemistries: heme-based catalases and thiol-based peroxidases (peroxiredoxins and glutathione peroxidases) [20]. While catalases depend on the heme group to promote peroxide scavenging, peroxidases use their highly reactive thiol groups, which have to be recycled at the expense of the reduced cofactor. The amount, relevance, and localization in different cellular compartments vary depending on the cell type. In fission yeast, we have established that the cytosolic peroxiredoxin Tpx1 is the major H₂O₂ scavenger during physiological growing conditions, and growth of cells lacking Tpx1 on solid plates is halted under aerobic conditions [21]. Tpx1 is a highly abundant typical 2-cysteine peroxiredoxin [22,23], which together with catalase constitutes the main line of defense against H₂O₂ [24]. Using biochemical and mathematical approaches [25], as well as the ultrasensitive H₂O₂ reporter roGFP2-Tpx1.C169S [26], we have determined that the cytosolic concentrations of peroxides that arrest the growth of cells lacking Tpx1 are between 0.1 and 0.3 µM. Catalase is the next barrier of detoxification when the steady-state levels of peroxides are increased in ∆tpx1 cells [24] or when toxic extracellular peroxides are applied to wild-type cultures [26]. The only glutathione peroxidase encoded by the Schizosaccharomyces pombe genome has a minor secondary role when high doses of extracellular peroxides are applied [24].

The final steady-state levels of peroxides will not only depend on synthesis and scavenging but also on subcellular localization. Biological membranes have limited permeability to H₂O₂, and compartment-specific scavenging activities further enhance the gradients across membranes. We have established that the fission yeast cytoplasmic membrane creates a permeability gradient of extracellular-to-intracellular peroxides of 40:1, but scavenging by the peroxiredoxin Tpx1, the main H₂O₂ detoxifier in fission yeast, enhances the gradient up to 300:1 [25].

Different concentrations of peroxides, in a space and time context, will drive physiological events, redox signaling, or toxicity. Measurements of intracellular H₂O₂ based on the use of permeable fluorescent dyes are controversial [27]. More than a decade ago, several groups decided to investigate the use of protein-based reporters to measure intracellular redox potentials and, later on, H₂O₂ levels [28]. The two major families of genetically encoded redox reporters are: the reduction-oxidation sensitive green fluorescent protein (roGFP)-based proteins [28] and HyPer and derivatives, based on the Escherichia coli H₂O₂ sensor OxyR [29]. Both families of probes suffer ratiometric fluorescence changes, which can be easily monitored with fluorescent microscopy, flow cytometry, or fluorescence plate readers. The specificity and sensitivity of roGFP to sense oxidants has been improved in the last years by fusing real H₂O₂ protein sensors, carrying mutations to limit their reduction rates, such as Orp1 or the peroxiredoxins Tsa2∆Cr or Tpx1.C169S [26,30,31]; fluorescence changes of roGFP fused to H₂O₂ sensors or of HyPer are specific for H₂O₂, and other oxidants such as superoxide, oxidized glutathione or other reactive oxygen species are not able to induce them. Regarding HyPer and derivatives, a new family member has been recently reported, HyPer7, which is based on Neisseria meningitidis OxyR [32]; as for the original HyPer, HyPer7 has been tested in mammalian cells, and the sensitivity of this biosensor is much higher than the original HyPer.

We have expressed the most sensitive biosensors of each family, roGFP2-Tpx1.C169S [26] and HyPer7 [32], in the same model system, S. pombe. Both probes are exquisitely sensitive in sensing moderate fluctuations of H₂O₂ induced by environmental interventions, although the former, roGFP2-Tpx1.C169S, is ~5-times more sensitive than HyPer7. This superb sensitivity allows roGFP2-Tpx1.C169S to clearly sense the leakage of H₂O₂ from the mitochondria to the cytosol upon the addition of the electron transport chain inhibitor antimycin A. Thanks to the use of our biosensors, we propose that the concentration of peroxides in the cytosol of wild-type cells is ~3–6 nM, while the steady-state H₂O₂ levels within the mitochondrial matrix are ~0.1–0.15 µM. Importantly, the extent of oxidation of HyPer7 is equilibrated up to ~60% in the matrix and cytosol of cells lacking Tpx1, indicating that scavenging by the peroxiredoxin Tpx1 causes the matrix-to-cytosol peroxide gradient.

2. Materials and Methods

2.1. Fission Yeast Growth Media and Genetic Manipulations

For all the experiments, cells were grown in filtered minimal medium (MM) at 30 °C as described previously [33], supplemented with cysteine in auxotrophic strains. The strains used in this study and their genotypes are provided in Table S1.

2.2. Generation of Plasmids Used in This Study

The plasmids described here express fluorescent reporters under the control of the constitutive sty1 promoter [24], and are episomal with an average of 7–8 plasmid copies per cell [34]. According to previous quantifications of other proteins expressed from the same promoter [25], the intracellular protein concentration arising from these constructs is in the order of 2–10 µM. Plasmids p605 and p407.C169S, allowing the expression of HyPer and roGFP2-Tpx1.C169S, respectively, have been previously described [26]. We cloned a synthetic open reading frame (supplied by IDT Technologies, Coralville, IA, USA) coding for HyPer7 [32] downstream of the sty1 promoter and an HA-coding sequence, yielding plasmid p728 (allowing the expression of HA-HyPer7). We then inserted a PCR-amplified DNA fragment from S. pombe cDNA encoding the mitochondrial targeting signal of Aco1, its 60 N-terminal amino acids, ahead of the HA-coding sequence, yielding plasmid p730 (allowing the expression of MTS-HA-HyPer7). To express catalase in the mitochondrial matrix, we purified an insert from p419 [24], including sty1 promoter-driven ctt1, and cloned it in the ura4 episomal vector pREP.42x, inserting after that the coding sequence for MTS from Aco1, yielding p790.

2.3. Growth of Strains Expressing HyPer or roGFP Derivatives for Fluorescence Determination

For wild-type backgrounds, standard MM-based early stationary phase pre-cultures were diluted in filtered MM to reach an OD₆₀₀ of 1 after 4–5 duplications. For strain Δtrx1, auxotrophic for cysteine, MM aerobic cultures contained 38 µg/mL of cysteine. The fluorescence of 190 µL of these cultures, at an OD₆₀₀ of 1, was directly monitored in 96-well plates in a FLUOstar OMEGA (BMG Labtech, Ortenberg, Germany) as described below.

2.4. In Vivo Measurement of Basal and Induced Oxidation of HyPer and roGFP-Derivatives

HyPer has two excitation maxima at 420 and 500 nm and one emission peak at 516 nm [29], while HyPer7 has two excitation maxima at 400 and 499 nm and one emission peak at 516 [32]. Similarly, roGFP2 exhibits two excitation maxima at 400 nm and 475–490 nm when fluorescence emission is monitored at 510 nm. Either HyPer or roGFP2 oxidation was monitored using a fluorescence plate reader FLUOstar OMEGA (BMG Labtech). In both cases, we used excitation filters of 400–10 and 485BP12, combined with an emission filter of EM520. The experiments were performed as previously described [26]. Briefly, 190 µL of cultures at an OD₆₀₀ of 1 were transferred to a 96-well imagine plate (Krystal Microplate™ 215003, Porvair Sciences) in as many wells as treatments were to be tested. The two excitation wavelengths were recorded, and after 4 cycles of approximately 2 min each, 10 µL of the corresponding treatments were added to accomplish the final concentrations of reagents indicated in Figure 1, Figure 2, Figure 3, Figure 4 and Figure 5. For the antimycin (ANT) treatment, a stock at 10 mM was prepared in DMSO, and it was freshly diluted in H₂O to the final concentration for each experiment. In two wells, final concentrations of 50 mM dithiothreitol (DTT) and 1 mM of H₂O₂ were added as controls of fully reduced (red) and oxidized (ox) (see equation below). For each strain, we grew cultures of the wild-type background 972 and performed the same treatments on the 96-well plates; after recording, we subtracted the fluorescence values of the empty strain to those of the strain expressing the reporter. We determined the degree of sensor oxidation (OxD) as described in the following Equation (1):

(1)$\mathbf{OxD}=\frac{\left(I_{sample 488}\times I_{red 405}\right)-(I_{sample 405}\times I_{red 488})}{(I_{sample 405}\times I_{ox 488})-(I_{sample 405}\times I_{red 488})-\left(I_{sample 488}\times I_{ox 405}\right)+\left(I_{sample 488 }\times I_{red 405}\right)}$

2.5. Statistics

For in vivo fluorescence probe oxidation quantification, OxD, one independent culture of the strain of interest, was grown for each replicate. In all figure panels, values of mean of n = 3 or n = 2 (Figure S5d,e), are shown. For the statistical analysis, an unpaired t-test was performed. In supplementary figures, error bars for all the experiments (standard deviation, S.D.) are represented.

3. Results

3.1. Comparing the Performance of Different H₂O₂ Biosensors in the Same Model System—Expression of HyPer7 in Fission Yeast

To quantitatively monitor the sensitivity of HyPer7 to H₂O₂ fluctuations, we expressed it in the cytosol of S. pombe cells under the control of the constitutive sty1 promoter, as previously described for the original HyPer and for roGFP2-Tpx1.C169S. Moreover, we monitored its oxidation directly in exponentially growing cultures before and after the addition of extracellular peroxides, ranging from 1 to 1000 µM, using a fluorescence plate reader as previously described [26]. As shown in Figure 1 and Figure S1, the lower concentrations of extracellular H₂O₂ triggering statistically significant oxidation of HyPer, HyPer7, or roGFP2-Tpx1.C169S are 100, 5–10, and 1–2 µM, respectively. Therefore, even though HyPer7 is significantly more sensitive than the original HyPer, it does not reach the sensitivity of the peroxiredoxin-based biosensor. Nevertheless, HyPer7 is probably better suited to measure fluctuating waves of peroxides since its reduction is clearly faster than that of roGFP2-Tpx1.C169S.

3.2. HyPer7 Is Reduced by the Thioredoxin System

As shown in Figure 1, HyPer7 is actively recycled by S. pombe’s reducing systems, both before and after oxidation by peroxides. The thioredoxin and the glutaredoxin/glutathione systems maintain thiols in their reduced form in all cell types. To test which of both systems recycles HyPer7 in fission yeast, we expressed the reporter in the cytosol of cells lacking the main cytosolic glutaredoxin (Grx1) and the only glutathione reductase (Pgr1) (Figure 2a and Figure S2), or in cells lacking the cytosolic thioredoxins (Trx1 and Trx3) or the only thioredoxin reductase (Trr1) (Figure 2b). While the absence of Grx1 or Pgr1 has no effect on the basal levels of HyPer7 and do not slow down its reduction after H₂O₂ stress, the individual deletion of trx1 has a long-term impact on the recycling of HyPer7 after stress imposition; as expected, the secondary thioredoxin Trx3 does not have an impact on HyPer7 reduction (Figure 2b). The lack of Trr1 also has a large impact on the reduction kinetics of the probe. We conclude that the thioredoxin system recycles HyPer7 in living cells (Figure 2c); on the contrary, the glutaredoxin-glutathione system recycles roGFP-Tpx1.C169S (Figure S2c), as previously described [26].

Regarding scavenging of cytosolic H₂O₂, we and others have previously demonstrated that catalase (Ctt1 in fission yeast) is required to detoxify high concentrations of applied peroxides, specifically those with an extracellular concentration higher than 0.1 mM. As shown in Figure 2d, when we compare the oxidation of HyPer7 in cells lacking Ctt1 (Figure 2d, ∆ctt1 + HyPer7) and in wild-type cells (Figure 2a, WT + HyPer7), the sensor remains oxidized for longer times at extracellular concentrations ranging from 0.1 to 1 mM, while there are no significant differences at lower concentrations.

3.3. Expression of HyPer7 in the Mitochondria—Steady-State Levels of H₂O₂ in the Matrix

In order to determine the steady-state levels of H₂O₂ in the mitochondrial matrix, and also to study the fluxes of peroxides from the cytosol to the matrix and vice versa, we expressed HyPer7 at the mitochondrial matrix by fusing it to the mitochondrial targeting sequence (MTS) of Aco1, including the amino-terminal 60 amino acids of the matrix-resident protein aconitase 1 [35] (Figure 3a). Upon application of extracellular peroxides, the mitochondrial-targeted biosensor is capable of detecting oxidation, although ~5-times higher doses have to be applied to reach the oxidation levels of the cytosolic probe (compare WT + HyPer7 in Figure 2a with WT + MTS-HyPer7 of Figure 3a). This indicates that while there is a gradient of peroxides of 300:1 between the extracellular milieu and the cytosol, the gradient between the extracellular media and the mitochondrial matrix is 1500:1. Probe recycling after stress imposition is very similar to cytosolic HyPer7, suggesting that the matrix can efficiently reduce HyPer7 (compare Figure 3a with Figure 2a).

Most importantly, the basal level of oxidation of MTS-HyPer7, OxD₀, is also significantly altered, with ~35–40% of the probe being oxidized in a wild-type background (Figure 3a and Figure S3), while cytosolic HyPer7 is fully reduced during unperturbed conditions (see Figure 2a, WT + HyPer7). To rule out the lack of efficient recycling activities for oxidized MTS-HyPer7 in the matrix, we over-expressed catalase in this mitochondrial compartment by fusing it again to the MTS of Aco1. As shown in Figure 3b, the starting oxidation level of MTS-HyPer7 drops down to 0 when Ctt1 is also co-expressed in the matrix, strongly suggesting that the concentration of H₂O₂ in this site of production is significantly higher than in the cytosol. The extent of basal MTS-HyPer7 oxidation, ~35–40% OxD₀, can be used as a non-quantitative readout of steady-state levels of H₂O₂, using cytosolic HyPer7 as a control. In wild-type cells, 50 μM of extracellular peroxides, which according to the 300:1 gradient correspond to ~0.15 μM of intracellular H₂O₂, are able to oxidize the probe up to ~40% (Figure 2a, WT + HyPer7). Therefore, we propose that the steady-state concentration of peroxides in the mitochondrial matrix is in the order of ~0.15 μM.

3.4. Role of the Peroxiredoxin Tpx1 in the Generation of Mitochondria-To-Cytosol H₂O₂ Gradients

Using biochemical approaches [25], as well as the basal oxidation levels of cytosolic roGFP2-Tpx1.C169S as a readout of the steady–state levels of H₂O₂ [26], we demonstrated that cells lacking Tpx1 display toxic concentrations of peroxides in the cytosol in the range of 0.2–0.3 µM. We expressed HyPer7 and MTS-HyPer7 in ∆tpx1 cells (Figure 4 and Figure S4). The OxD₀ for both reporters, cytosolic and mitochondrial, are very similar, ~60% oxidation in both compartments, suggestive of the presence of toxic concentrations of H₂O₂ irrespective of the presence of two membranes between the main site of peroxide production, the matrix, and the cytosol. This suggests that the different H₂O₂ levels in the matrix and the cytosol observed in wild-type cells (compare the OxD₀ of HyPer7 with that of MTS-HyPer7 in wild-type strain; Figure 2a vs. Figure 3a) is caused by the efficient scavenging at the cytosol by the peroxiredoxin Tpx1, and the continuous production of reactive oxygen species at the mitochondria.

3.5. H₂O₂ Mitochondrial Bursts Can Be Detected by Mitochondrial MTS-HyPer7, or by HyPer7 in the Cytosol of Cells Lacking Tpx1

Since the ETC is an important source of H₂O₂ production, and its inhibitors can exacerbate peroxide production, we tested whether cytosolic HyPer7 is able to sense the H₂O₂ produced at and diffused out of the mitochondria. We treated cells with antimycin A (ANT), an inhibitor of CIII, and monitored HyPer7 oxidation in wild-type and ∆tpx1 cells. Contrary to roGFP2-Tpx1.C169S, which is ~five-times more sensitive than HyPer7 to peroxides (see Figure 1) [26], HyPer7 can barely sense the leakage of H₂O₂ from the mitochondria upon addition of the ETC inhibitor ANT in wild-type cells (black lines in Figure 5a and Figure S5). Thus, while ANT treatments cause ~20% oxidation of cytosolic roGFP2-Tpx1.C169S (Figure S5d,e and Figure 5b), less than 5% of cytosolic HyPer7 is oxidized with the same treatments (Figure 5b). On the contrary, cytosolic HyPer7 is clearly oxidized upon ANT treatment in cells lacking the H₂O₂ scavenger Tpx1 (black lines in Figure 5c), confirming that H₂O₂ produced at the mitochondria is rapidly dispersed to the cytosol and degraded by Tpx1 in wild-type cells.

MTS-HyPer7 expressed in wild-type cells, however, can monitor mitochondrial H₂O₂ production: ANT addition causes clear oxidation of this biosensor with very similar kinetics to the oxidation of cytosolic HyPer7 in ∆tpx1 cells (compare black lines in Figure 5c,d).

4. Discussion

Redox biology is in need of reliable methods to measure in vivo fluctuations of H₂O₂. It may be quite easy to quantify large increases, which are normally linked to transient or permanent toxicity. Here, we test and compare two families of peroxide sensors expressed at similar levels in the same model system. By doing so, we demonstrate the advantages of one or the other and reach important conclusions regarding redox biology.

Thus, the peroxiredoxin-based sensor roGFP2-Tpx1.C169S is ~five times more sensitive than HyPer7 in monitoring increases in intracellular peroxides after applying H₂O₂ to the growth media, so that roGFP2-Tpx1.C169S oxidation can be detected upon 1–2 µM of H₂O₂ (Figure 1). The peroxiredoxin-based probe is partially oxidized in the cytosol of wild-type cells, in part due to the recycling of oxidized roGFP2, which depends on the glutaredoxin-glutathione system, but also due to the high sensitivity of peroxides to this probe [26]; HyPer7, on the contrary, is fully reduced during unperturbed conditions. Furthermore, the higher sensitivity of roGFP2-Tpx1.C169S explains why this peroxiredoxin-based probe can unambiguously detect in the cytosol the H₂O₂ produced at the mitochondria after ANT addition [26], but HyPer7 can barely suffer some minor changes (Figure 5b).

The gradient of extracellular-to-intracellular peroxide is, on average, 300:1 [25]. Taking advantage of this knowledge, we can establish that roGFP2-Tpx1.C169S is able to detect intracellular H₂O₂ fluctuations in the low nanomolar (~3–6 nM) range, which is below the level where antioxidant redox signaling and toxicity occur (at least 200–300 nM of intracellular H₂O₂ is required to trigger activation of the pre-toxic Pap1 signaling cascade [25]). Since our probe is based on the natural H₂O₂ S. pombe scavenger Tpx1 [21], we propose that the capacity of this reporter to sense peroxides coincides with the steady-state levels of peroxides in the cytosol of wild-type cells, which are probably below and very close to 3–6 nM (Figure 6).

HyPer7 is, however, a very sensitive reporter, still detecting peroxide fluxes below the concentrations ruling signaling and toxicity events. Furthermore, it is rapidly recycled by the thioredoxin system so that mutants lacking cytosolic thioredoxins show slower reduction kinetics after stress imposition (Figure 2). A similar profile can be detected in cells lacking catalase at high concentrations of peroxides since this enzyme scavenges H₂O₂ ranging from an extracellular concentration of 0.1–1 mM (Figure 2d). In cells lacking Tpx1, for which we predicted an intracellular peroxide concentration of ~0.3 µM [25,26], HyPer7 is partially oxidized to ~60% (Figure 4a).

A remarkable advantage of the use of HyPer7 is that it can be efficiently imported to and recycled inside the mitochondrial matrix (Figure 3a). By doing so, we reach important conclusions about physiological peroxide fluxes and redox biology: (i) when extracellular H₂O₂ is applied, there is an additional peroxide gradient of 5:1 from the cytosol to the matrix, or of 1500:1 from the extracellular milieu to the matrix; (ii) MTS-HyPer7 is ~35–40% oxidized in the matrix of wild-type cells, which is ~half of the basal oxidation of cytosolic HyPer7 in ∆tpx1 cells, with an OxD₀ of ~0.6, or the levels of HyPer7 oxidation accomplished in wild-type cells upon 50 µM extracellular H₂O₂. We propose that the steady-state levels of peroxides in the matrix are ~0.15 µM. Thus, the main site of H₂O₂ production displays ~25–50 times higher levels of peroxides than the cytosol (Figure 6).

Is this gradient caused by active H₂O₂ scavenging in the cytosolic compartment or by the limited permeability of the mitochondrial membranes? We propose that the gradient is caused by the former since HyPer7 and MTS-HyPer7 display similar OxD₀ in cells lacking the peroxiredoxin Tpx1 (Figure 4 and Figure 6). This result suggests that mitochondrial H₂O₂ can diffuse out of the mitochondria, but it is rapidly scavenged by Tpx1 at the cytosol. In fact, this diffusion is rapid, as shown with ANT treatments, and only endogenous Tpx1 or the roGFP2-Tpx1.C169S probe contain a sensitive thiol group (thiol switch) in their cysteine 48 as to detect waves of physiological peroxides [26] (Figure 6). This is an important concept in redox signaling, which reinforces the idea that only a handful of proteins such as peroxiredoxins can sense peroxide waves emanating from the mitochondria and transduce the signal to control cell signaling cascades.

5. Conclusions

We have compared the H₂O₂ reporters HyPer7 and roGFP2-Tpx1.C160S in S. pombe. Most results are outlined in Figure 3a and Figure 6. Thus, the peroxide gradient from the extracellular media to the matrix, 1500:1, is five times higher than that from the extracellular media to the cytosol. Thanks to the use of these reporters, we speculate that the steady-state H₂O₂ level in the matrix is around 0.15 µM, while the concentration in the cytosol is in the low nanomolar range; this gradient is caused by the scavenging activity of the cytosolic peroxiredoxin, Tpx1. Thus, in cells lacking this scavenger, the mitochondria-to-cytosol gradient disappears, with matrix and cytosolic H₂O₂ concentrations being in the order of 0.3 µM. The future use of these reporters in other subcellular compartments (intermembrane space or endoplasmic reticulum) and in different model systems (such as mammalian cells) will be required to generalize all the findings of our work.

Supplementary Materials

The following are available online at https://www.mdpi.com/article/10.3390/antiox10050731/s1, Figures S1–S5—graphs of main figures with error bars; Table S1—Strains used in this study.

Author Contributions

Conceptualization, E.H. and J.A.; Data curation, L.d.C.; Funding acquisition, E.H.; Investigation, L.d.C.; Methodology, L.d.C.; Resources, V.V.P. and V.V.B.; Supervision, E.H.; Writing—original draft, E.H. All authors have read and agreed to the published version of the manuscript.

Funding

This work is supported by the Ministerio de Ciencia, Innovación y Universidades (Spain), PLAN E and FEDER (PGC2018-093920-B-I00 to E.H., PGC2018-097248-B-I00 to J.A. and Redox Biology and Medicine Research Network (Red2018-102576-T) to E.H.), and from the Ministry of Science and Higher Education (Russia) (075-15-2019-1933 to V.V.B.). The Oxidative Stress and Cell Cycle group is also supported by Generalitat de Catalunya (Spain) (2017-SGR-539) and by Unidad de Excelencia María de Maeztu, funded by the AEI (CEX2018-000792-M) (Spain). L.d.C. is recipient of a María de Maeztu predoctoral fellowship from the Ministerio de Economía y Competitividad (Spain).

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

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

Conflicts of Interest

The authors declare no conflict of interest.

Publisher’s Note: MDPI stays neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Figures

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Figure 1. Expression of HyPer (a), HyPer7 (b) and roGFP2-Tpx1.C169S (c) in fission yeast. Wild-type strain HM123. was transformed with plasmids p605, p728, and p407.C169S to express HyPer, HyPer7, and roGFP2-Tpx1.C169S, respectively. The indicated extracellular concentrations of H2O2 were directly added to MM cultures at an OD600 of 1 in 96-well imaging plates, and growth proceeded at 30 °C for the time indicated with shaking. The degree of probe oxidation (amount of probe oxidized per 1) is indicated in the Y-axis (OxD). The minimum concentrations of H2O2 capable of causing probe oxidation are indicated with arrows. For each strain, average data from three biological replicates are shown, with error bars (S.D.) displayed in Figure S1. Graph bars (bottom panels of a–c) represent the average OxD between 10 and 15 min for each treatment. Statistical significance was calculated between the indicated samples with an unpaired Student’s t-test with P-values of 0.05 (*), 0.01 (**), and 0.001 (***); ns, non-significant. (d) Percentage of oxidation of HyPer7 and roGFP2-Tpx1.C169S upon H2O2 treatments. Data from panels b and c are represented as the average of the percentage of oxidation between 10 and 15 min for each treatment, as described in Materials and Methods.

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Figure 2. HyPer7 is recycled by the thioredoxin system. (a,b) Strains HM123 (WT), AD88 (∆pgr1), SG154. (∆trx1), SB469 (∆grx1), SG152 (∆trr1), and MC184 (∆trx3), transformed with plasmid p728 expressing cytosolic HyPer7, were treated or not with H2O2 and oxidation of the reporter was estimated as described in Figure 1. (c) Scheme depicting the role of the thioredoxin system as the electron donor in HyPer7 recycling. (d) Strain EP160 (∆ctt1) transformed with plasmid p728 expressing cytosolic HyPer7 was treated or not with H2O2, and oxidation of the reporter was estimated as described in Figure 1. For each strain, average data from three biological replicates are shown, with error bars (S.D.) displayed in Figure S2.

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Figure 3. Mitochondrial MTS-HyPer7 is partially oxidized in basal conditions. (a) Strain HM123 (WT) transformed with plasmid p730 expressing MTS-HyPer7 targeted to the mitochondrial matrix was treated or not with H2O2, and oxidation of the reporter was estimated as described in Figure 1. The gradients of extracellular-to-cytosol (300:1) and cytosol-to-matrix (5:1) upon addition of H2O2 to the growing media are indicated. (b) Strain PN513 (WT) transformed with plasmids p730 and p790 expressing MTS-HyPer7 and MTS-Ctt1, respectively, in the mitochondrial matrix was treated and analyzed as in Figure 1. For each strain, average data from three biological replicates are shown, with error bars (S.D.) displayed in Figure S3.

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Figure 4. The levels of basal oxidation, OxD0, of HyPer7 and MTS-Hyper7 are very similar in cells lacking Tpx1. Strain SG5 (∆tpx1) transformed with p728 (a) or p730 (b) encoding HyPer7 or MTS-HyPer7, respectively, was grown and analyzed as in Figure 1. Average data from three biological replicates are shown, with error bars (S.D.) displayed in Figure S4.

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Figure 5. Detection of H2O2 produced at the mitochondria upon ANT treatment can be detected by MTS-HyPer7 but not by cytosolic HyPer7 unless the H2O2 scavenger Tpx1 is absent. (a) The indicated concentrations of H2O2 or ANT were directly added to MM cultures of strain HM123 + p728 (WT + HyPer7), and oxidation of the reporter was estimated as described in Figure 1; oxidations upon ANT treatments are represented with solid (10 μM ANT) or dashed (5 μM ANT) black lines. Average data from three biological replicates are shown, with error bars (S.D.) displayed in Figure S5. (b) Percentages of oxidation of the reporters HyPer7 and roGFP2-Tpx1.C169S upon ANT treatment were determined as described in Figure 1d between 45 and 50 min, from experiments of Figure 5a (HyPer7) and Figure S5d (roGFP2-Tpx1.C169S). (c,d) Cultures of strains SG5 + p728 (∆tpx1+ HyPer7), (c) and HM123 + p730 (WT + MTS-HyPer7) (d) were treated and analyzed as in (a).

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Figure 6. Scheme depicting the main finding of the use of the roGFP2-Tpx1.C169S and HyPer7 reporters in the quantification of basal and induced H2O2 levels and inter-compartmental H2O2 gradients. See Discussion for details.