Mol. Cells 2016; 39(1): 46-52
Published online January 25, 2016
https://doi.org/10.14348/molcells.2016.2328
© The Korean Society for Molecular and Cellular Biology
Correspondence to : *Correspondence: t.dick@dkfz.de
It is increasingly apparent that nature evolved peroxiredoxins not only as H2O2 scavengers but also as highly sensitive H2O2 sensors and signal transducers. Here we ask whether the H2O2 sensing role of Prx can be exploited to develop probes that allow to monitor intracellular H2O2 levels with unprecedented sensitivity. Indeed, simple gel shift assays visualizing the oxidation of endogenous 2-Cys peroxiredoxins have already been used to detect subtle changes in intracellular H2O2 concentration. The challenge however is to create a genetically encoded probe that offers real-time measurements of H2O2 levels in intact cells via the Prx oxidation state. We discuss potential design strategies for Prx-based probes based on either the redox-sensitive fluorophore roGFP or the conformation-sensitive fluorophore cpYFP. Furthermore, we outline the structural and chemical complexities which need to be addressed when using Prx as a sensing moiety for H2O2 probes. We suggest experimental strategies to investigate the influence of these complexities on probe behavior. In doing so, we hope to stimulate the development of Prx-based probes which may spearhead the further study of cellular H2O2 homeostasis and Prx signaling.
Keywords biosensor, genetically encoded fluorescent probes, hydrogen peroxide, peroxiredoxin
Nature evolved specialized proteins to respond to increased intracellular hydrogen peroxide (H2O2). These proteins typically remove H2O2 by either dismutation or reduction (Winterbourn, 2013). Some of these proteins additionally serve as H2O2 sensors and signal transmitters to inform the cell about changes in intracellular H2O2 levels (Delaunay et al., 2002; Rhee et al., 2012; Sobotta et al., 2015). In principle, it should be possible to use these H2O2-sensing proteins as research tools, namely to exploit them as biosensors for the real-time observation of H2O2 in living cells.
Indeed, the two existing genetically encoded H2O2 probes, HyPer and roGFP2-Orp1, are based on OxyR and Orp1, respectively (Bilan and Belousov, 2015; Schwarzlander et al., 2015). OxyR is a H2O2-sensing transcription factor from bacteria and Orp1 is a member of the glutathione peroxidase family from yeast. Both proteins have a rate constant for the reaction with H2O2 of approximately 105 M?1s?1 (Aslund et al., 1999). However, peroxiredoxins have a significantly higher reactivity towards H2O2 which can be as high as 107 ? 108 M?1 s?1 (Rhee and Woo, 2011). This potentially makes them superior H2O2 sensors. Indeed, a side by side comparison between endogenous Prx2 and ectopic roGFP2-Orp1 in mammalian cells showed that Prx2 is many times more sensitive than Orp1 (Sobotta et al., 2013). Nevertheless, little has been done to develop biosensors based on Prx. In the following we will address the question of whether such probes can be developed.
It is interesting to note that endogenous 2-Cys peroxiredoxins have already been utilized as H2O2 reporters, albeit in a biochemical way that imposes many restrictions (Cox et al., 2010; Poynton and Hampton, 2014). Oxidation of 2-Cys peroxiredoxins yields covalent dimers which can be visualized by non-reducing SDS-PAGE and Prx-specific immunoblotting. The Prx dimerization assay is capable of detecting increases in intracellular H2O2 levels associated with physiologically relevant signaling events (Cox et al., 2008; Kumar et al., 2009). Moreover, subcellular information can be obtained by analyzing peroxiredoxins expressed in different organelles (e.g. Prx1 in the cytosol and Prx3 in the mitochondrial). However, the approach is limited in scope (Cox et al., 2008; Kumar et al., 2009), as it doesn’t allow real-time monitoring of the Prx redox state in intact cells. Cell need to be lysed, which inevitably causes unwanted oxidation of peroxiredoxins, unless intact cells are pretreated with sufficient amounts of alkylating agents prior to cell lysis. Finding the best conditions for preserving the endogenous Prx redox state and excluding artifacts is not always a trivial task (Cox et al., 2010; Poynton and Hampton, 2014; Sobotta et al., 2013). Thus, the challenge is to develop genetically encoded probes which do not suffer from these limitations and can be monitored in living cells (Bilan and Belousov, 2015; Schwarzlander et al., 2015).
Genetically encoded Prx-based H2O2 probes will necessarily consist of (at least) two moieties. The first moiety is the Prxs domain and the second a fluorescent reporter protein. In currently used genetically encoded redox probes the fluorescent reporter is either circularly permutated yellow fluorescent protein (cpYFP) or redox-sensitive green fluorescent protein (roGFP) (Fig. 1). The cpYFP reporter responds to a structural perturbation, whereas the roGFP reporter responds to the oxidation of its cysteine pair to a disulfide bridge (Bilan and Belousov, 2015; Schwarzlander et al., 2015). Another potential strategy is the use of a F?rster resonance energy transfer (FRET) pair of two fluorescent proteins to sense structural changes imposed by the oxidation of the peroxiredoxin (Barranco-Medina et al., 2009). Thus, based on existing probes at least three different designs can be envisaged.
The key requirement for a roGFP-based Prx probe is the ability of the peroxiredoxin to mediate oxidation of the roGFP cysteine pair. Recently, it was found that the human 2-Cys peroxiredoxin Prx2 acts as a transmitter of oxidizing equivalents towards the transcription factor STAT3 (Sobotta et al., 2015). Thus, it is conceivable that 2-Cys peroxiredoxins can also transmit oxidation to other proteins, including roGFP (Figs. 2A and 2B). Obviously, various Prx-roGFP or roGFP-Prx fusion proteins would need to be tested and optimized empirically to identify those in which the oxidizing equivalents are transmitted most efficiently to the roGFP moiety.
When using cpYFP as reporter moiety, Prx oxidation must provoke a conformational change that can be sensed by the cpYFP fluorophore. Peroxiredoxins undergo a local unfolding transition upon reaction with H2O2 (Hall et al., 2011). However, it is not obvious if and how this limited structural change could be transferred to the cpYFP moiety. Alternatively, a cpYFP domain could be positioned to respond to the decamer to dimer transition, which accompanies oxidation of typical 2-Cys peroxiredoxins (Barranco-Medina et al., 2009). Perhaps a cpYFP moiety that is placed between two Prx domains would sense decamer dissociation. Yet another strategy is a fusion protein in which cpYFP is sandwiched between a Prx and a thioredoxin (Trx) domain, the latter lacking its resolving cysteine (Figs. 2C and 2D). The reasoning behind this design is that the mutant Trx domain will covalently trap the oxidized Prx domain thus causing a structural change that is sensed by the cpYFP moiety. This strategy was used previously to generate a methionine sulfoxide sensitive probe in which cpYFP is inserted between a methionine sulfoxide reductase domain and a mutant Trx domain (Tarrago et al., 2015). A major disadvantage of utilizing circular permutated fluorescent proteins (cpFPs) like cpYFP is their intrinsic pH sensitivity and the requirement to use stringent pH controls in each experiment (Bilan and Belousov, 2015). However, a potential advantage is that cpFPs of different color can be used to create spectral probe variants (Ermakova et al., 2014; Zhao et al., 2011).
The use of FRET to investigate 2-Cys peroxiredoxin behavior has already been reported (Muthuramalingam et al., 2009; Seidel et al., 2010). The authors used two (single-step FRET) or three (two-step FRET) Prx-fluorescent protein (FP) pairs to monitor the decamer dissociation upon peroxiredoxin oxidation. Although these Prx-FP fusions showed potential as cellular H2O2 biosensors, no further developments in this direction have been reported.
The envisaged Prx-based biosensors promise to achieve much higher sensitivity than the current generation of genetically encoded H2O2 sensors (Ezerina et al., 2014). However, peroxiredoxins exhibit rather complex biochemical and structural behavior (Rhee and Woo, 2011; Perkins et al., 2015). This may complicate or compromise their utilization as H2O2 sensors. In the following we discuss these complexities and how they may affect probe behavior. For simplicity, we focus our discussion on roGFP-Prx fusion proteins, but most considerations equally apply to the other design strategies.
First of all, fusion to a fluorescent protein might already influence Prx behavior. Previously, the presence of an N- or C-terminal tag was found to influence peroxidase activity, chaperone holdase activity, hyperoxidation sensitivity or oligomeric structure of several Prxs (Cao et al., 2007; Konig et al., 2013; Koo et al., 2002; Noichri et al., 2015; Randall et al., 2014; Sayed and Williams, 2004; Seo et al., 2009). Thus, each potential Prx-based probe should be functionally characterized and compared to the unfused Prx.
Many Prxs not only react with H2O2, but also show reactivity towards organic peroxides and peroxinitrite (Perkins et al., 2014). For example, human Prx5 and
The oligomeric state of different peroxiredoxins can vary from monomers to decamers/docecamers and may change upon oxidation (Barranco-Medina et al., 2009; Hall et al., 2011). In principle, a probe should have a simple design, and thus a monomeric Prx may be preferred as a sensing moiety. However, only a few peroxiredoxins are monomeric. The majority forms dimers and higher oligomeric structures. A typical 2-Cys peroxiredoxin fused to a fluorescent reporter would need to dimerize to be active. This situation raises several questions: Does a probe based on a typical 2-Cys Prx only form probe-probe dimers, or does it also form heterodimers with endogenous Prx molecules? Does the probe form decamers, or is decamerization prevented by the fused reporter protein? If it does form decamers, does it form probe homo-decamers or mixed hetero-decamers with endogenous peroxiredoxins? Furthermore, is decamerization required for the probe to function? Mutations at the A-type interface, either stabilizing or destabilizing decamerization, may be used to investigate this question. For example, Parsonage et al. showed that substitution of Thr77 of
The inactivation of peroxiredoxins by hyperoxidation has been observed under physiological circumstances (Nelson et al., 2013; Perkins et al., 2014). If a Prx-based probe turns out to be susceptible to hyperoxidation, it may under certain conditions report false results. Fortunately, not all Prx are highly sensitive to hyperoxidation. Bacterial Prxs are in general more robust, whereas some eukaryotic Prxs, including human Prx2, are remarkably sensitive (Nelson et al., 2013; Wood et al., 2003). Thus, bacterial Prxs may be preferable over eukaryotic Prxs when designing a Prx-based probe. Nevertheless, an intrinsically sensitive Prx could be modified to decrease its hyperoxidation sensitivity. Several factors have been described to influence hyperoxidation sensitivity, including two distinct sequence motifs: a GGLG and a C-terminal YF motif (Wood et al., 2003). It has been shown that alteration of these motifs and their surrounding residues modulate hyperoxidation sensitivity (Sayed and Williams, 2004; Wang et al., 2012). One possibility to decrease hyperoxidation sensitivity is the truncation of the C-terminus (Koo et al., 2002; Randall et al., 2014; Sayed and Williams, 2004; Seo et al., 2009). This strategy could be used to increase the robustness of hyperoxidation-sensitive peroxiredoxins, making them more suitable as a sensing moiety for a probe. In any case, the hyperoxidation sensitivity of any Prx-based probe should be determined experimentally since unambiguous predictors of hyperoxidation sensitivity are lacking (Perkins et al., 2014). Immunoblotting with hyperoxidation specific antibodies allows to determine hyperoxidation of Prx-based probes (Fig. 3A).
Peroxiredoxins are subject to various post-translational modifications which influence their peroxidase activity or other properties. For instance, phosphorylation of Thr90 in human Prx1 and Thr89 in Prx2 attenuates peroxidase activity and promotes chaperone holdase activity whereas Ser32 phosphorylation of Prx1 is reported to increase peroxidase activity (Chae et al., 2012; Chang et al., 2002; Jang et al., 2006; Qu et al., 2007; Zykova et al., 2010). N-terminal acetylation of human Prx2 was found to influence hyperoxidation sensitivity (Seo et al., 2009). Thus, it is conceivable that a Prx-based probe can also undergo post-translational modifications under certain conditions. Such modifications may alter the probe response and lead to the misinterpretation of measurements. For those residues already known to be potentially modified, corresponding probe point mutants (e.g. preventing or mimicking phosphorylation) can be created and studied in parallel. Alternatively or additionally, a probe based on a heterologous Prx may be employed, thus decreasing the probability of its post-translational modification in the host system.
A dynamic (i.e. reversible) probe offers the possibility to monitor transient elevations in H2O2. Since the reaction with the peroxide is an irreversible reaction, probe reduction depends on cellular reducing systems (Figs. 1 and 2). Thus, a Prx-based probe is a dual-specificity sensor in the sense that it responds not only to changes in peroxide levels, but also to changes in the activity of the relevant reducing system. The reducing system to which the probe responds will depend on the design of the probe (Fig. 2). If the probe uses a typical 2-Cys Prx moiety, it will likely be reduced by the Trx system, unless the Prx moiety is intentionally altered to avoid reduction by thioredoxin (e.g. by mutation of the resolving cysteine). Designing a Prx-based probe to respond to a particular reducing system may be useful in order to limit or adjust the total H2O2 turnover of the probe. The latter determines how much H2O2 is consumed by the probe inside cells (see next paragraph). In any case, it will be important to characterize in detail how a given Prx-based probe is reduced inside cells. This can be achieved by using selective deletion/silencing of reducing systems inside cells and can additionally be studied in vitro with recombinant proteins.
In principle, the ectopic expression of any H2O2-consuming probe may perturb cellular H2O2 homeostasis (Schwarzlander et al., 2015). The impact of a Prx-based probe on endogenous H2O2 levels will depend on two factors, namely the probe’s expression level and its H2O2 turnover. The latter depends on both the rate of probe oxidation and the rate of probe reduction. Under most conditions, the endogenous peroxidase activity of the cell is highly efficient, not least due to the high reactivity and abundance of endogenous Prxs (Rhee et al., 2012). Thus, it can be expected that ectopic expression of a Prx-based probe at levels not higher than that of endogenous Prxs will not lead to a major impact on endogenous H2O2 homeostasis. Nevertheless, the impact of expressing a H2O2-consuming probe will need to be determined experimentally. A simple and coarse approach would be to follow growth and survival of cells exposed to a range of H2O2 concentrations in the absence or presence of ectopic probe expression. If probe expression does not enhance the overall H2O2 scavenging capacity, the rate and extent of recovery will not be different from cells lacking probe expression (Fig. 3B). However, this experiment does not directly investigate the impact of probe expression on endogenous H2O2 levels and cellular adaptations could obscure the interpretation. More sophisticated experiments to directly investigate the contribution of a Prx-based probe to cellular H2O2 scavenging could be envisaged along the following lines: a non-fluorescent mutant of the probe (i.e. a mutant with identical expression, but lacking a mature fluorophore) is expressed in the cytosol and a fluorescent version of the same or alternative probe is expressed in the mitochondrial matrix. A bolus of H2O2 is given from outside the cell and the amount of H2O2 reaching the mitochondrial matrix is monitored by the mitochondrially targeted probe. This reveals if and how much the cytosolic probe (which is made non-fluorescent in order not to interfere with measurement of the mitochondrial probe) contributes to H2O2 scavenging (Fig. 3C). An alternative approach makes use of the wide distribution of probe expression levels within a cell population upon transient transfection (which reaches from barely detectable expression to very strong overexpression) (Barata and Dick, 2013; Schwarzlander et al., 2015). Any ratiometric probe (like the cpYFP and roGFP based probes) that does not influence its own measurement (i.e. endogenous H2O2 levels) is expected to yield a perfectly straight line on a scatter plot that relates the fluorescent emission intensities at the two excitation wavelengths. Any deviation of this linearity at higher fluorescence intensities (i.e. higher expression levels) would indicate an impact of the probe on H2O2 levels. These assays should also allow screening for probe variants with minimal impact on endogenous H2O2 homeostasis.
Chaperon holdase activity is a well-known non-peroxidase function of 2-Cys peroxiredoxins (Rhee and Woo, 2011). The gain of chaperone activity seems to be tightly linked to the loss of peroxidase activity through hyperoxidation or heat stress. It is conceivable that a 2-Cys Prx-based probe introduces additional chaperone activity to the cell, especially if the Prx is sensitive to hyperoxidation. However, the reporter moiety might sterically hinder the chaperone activity. Indeed, the N-terminus of peroxiredoxins is crucial for the binding of client proteins and an N-terminal tag was found to abolish the chaperone activity (Teixeira et al., 2015). The intrinsic chaperone activity of a recombinant Prx-based probe may be determined with commonly used
In summary, despite the many complexities that need to be addressed, peroxiredoxins promise to become the foundation of the next generation of genetically encoded H2O2 biosensors.
Mol. Cells 2016; 39(1): 46-52
Published online January 31, 2016 https://doi.org/10.14348/molcells.2016.2328
Copyright © The Korean Society for Molecular and Cellular Biology.
Koen Van Laer, and Tobias P. Dick*
Division of Redox Regulation, DKFZ?ZMBH Alliance, German Cancer Research Center, Heidelberg, Germany
Correspondence to:*Correspondence: t.dick@dkfz.de
It is increasingly apparent that nature evolved peroxiredoxins not only as H2O2 scavengers but also as highly sensitive H2O2 sensors and signal transducers. Here we ask whether the H2O2 sensing role of Prx can be exploited to develop probes that allow to monitor intracellular H2O2 levels with unprecedented sensitivity. Indeed, simple gel shift assays visualizing the oxidation of endogenous 2-Cys peroxiredoxins have already been used to detect subtle changes in intracellular H2O2 concentration. The challenge however is to create a genetically encoded probe that offers real-time measurements of H2O2 levels in intact cells via the Prx oxidation state. We discuss potential design strategies for Prx-based probes based on either the redox-sensitive fluorophore roGFP or the conformation-sensitive fluorophore cpYFP. Furthermore, we outline the structural and chemical complexities which need to be addressed when using Prx as a sensing moiety for H2O2 probes. We suggest experimental strategies to investigate the influence of these complexities on probe behavior. In doing so, we hope to stimulate the development of Prx-based probes which may spearhead the further study of cellular H2O2 homeostasis and Prx signaling.
Keywords: biosensor, genetically encoded fluorescent probes, hydrogen peroxide, peroxiredoxin
Nature evolved specialized proteins to respond to increased intracellular hydrogen peroxide (H2O2). These proteins typically remove H2O2 by either dismutation or reduction (Winterbourn, 2013). Some of these proteins additionally serve as H2O2 sensors and signal transmitters to inform the cell about changes in intracellular H2O2 levels (Delaunay et al., 2002; Rhee et al., 2012; Sobotta et al., 2015). In principle, it should be possible to use these H2O2-sensing proteins as research tools, namely to exploit them as biosensors for the real-time observation of H2O2 in living cells.
Indeed, the two existing genetically encoded H2O2 probes, HyPer and roGFP2-Orp1, are based on OxyR and Orp1, respectively (Bilan and Belousov, 2015; Schwarzlander et al., 2015). OxyR is a H2O2-sensing transcription factor from bacteria and Orp1 is a member of the glutathione peroxidase family from yeast. Both proteins have a rate constant for the reaction with H2O2 of approximately 105 M?1s?1 (Aslund et al., 1999). However, peroxiredoxins have a significantly higher reactivity towards H2O2 which can be as high as 107 ? 108 M?1 s?1 (Rhee and Woo, 2011). This potentially makes them superior H2O2 sensors. Indeed, a side by side comparison between endogenous Prx2 and ectopic roGFP2-Orp1 in mammalian cells showed that Prx2 is many times more sensitive than Orp1 (Sobotta et al., 2013). Nevertheless, little has been done to develop biosensors based on Prx. In the following we will address the question of whether such probes can be developed.
It is interesting to note that endogenous 2-Cys peroxiredoxins have already been utilized as H2O2 reporters, albeit in a biochemical way that imposes many restrictions (Cox et al., 2010; Poynton and Hampton, 2014). Oxidation of 2-Cys peroxiredoxins yields covalent dimers which can be visualized by non-reducing SDS-PAGE and Prx-specific immunoblotting. The Prx dimerization assay is capable of detecting increases in intracellular H2O2 levels associated with physiologically relevant signaling events (Cox et al., 2008; Kumar et al., 2009). Moreover, subcellular information can be obtained by analyzing peroxiredoxins expressed in different organelles (e.g. Prx1 in the cytosol and Prx3 in the mitochondrial). However, the approach is limited in scope (Cox et al., 2008; Kumar et al., 2009), as it doesn’t allow real-time monitoring of the Prx redox state in intact cells. Cell need to be lysed, which inevitably causes unwanted oxidation of peroxiredoxins, unless intact cells are pretreated with sufficient amounts of alkylating agents prior to cell lysis. Finding the best conditions for preserving the endogenous Prx redox state and excluding artifacts is not always a trivial task (Cox et al., 2010; Poynton and Hampton, 2014; Sobotta et al., 2013). Thus, the challenge is to develop genetically encoded probes which do not suffer from these limitations and can be monitored in living cells (Bilan and Belousov, 2015; Schwarzlander et al., 2015).
Genetically encoded Prx-based H2O2 probes will necessarily consist of (at least) two moieties. The first moiety is the Prxs domain and the second a fluorescent reporter protein. In currently used genetically encoded redox probes the fluorescent reporter is either circularly permutated yellow fluorescent protein (cpYFP) or redox-sensitive green fluorescent protein (roGFP) (Fig. 1). The cpYFP reporter responds to a structural perturbation, whereas the roGFP reporter responds to the oxidation of its cysteine pair to a disulfide bridge (Bilan and Belousov, 2015; Schwarzlander et al., 2015). Another potential strategy is the use of a F?rster resonance energy transfer (FRET) pair of two fluorescent proteins to sense structural changes imposed by the oxidation of the peroxiredoxin (Barranco-Medina et al., 2009). Thus, based on existing probes at least three different designs can be envisaged.
The key requirement for a roGFP-based Prx probe is the ability of the peroxiredoxin to mediate oxidation of the roGFP cysteine pair. Recently, it was found that the human 2-Cys peroxiredoxin Prx2 acts as a transmitter of oxidizing equivalents towards the transcription factor STAT3 (Sobotta et al., 2015). Thus, it is conceivable that 2-Cys peroxiredoxins can also transmit oxidation to other proteins, including roGFP (Figs. 2A and 2B). Obviously, various Prx-roGFP or roGFP-Prx fusion proteins would need to be tested and optimized empirically to identify those in which the oxidizing equivalents are transmitted most efficiently to the roGFP moiety.
When using cpYFP as reporter moiety, Prx oxidation must provoke a conformational change that can be sensed by the cpYFP fluorophore. Peroxiredoxins undergo a local unfolding transition upon reaction with H2O2 (Hall et al., 2011). However, it is not obvious if and how this limited structural change could be transferred to the cpYFP moiety. Alternatively, a cpYFP domain could be positioned to respond to the decamer to dimer transition, which accompanies oxidation of typical 2-Cys peroxiredoxins (Barranco-Medina et al., 2009). Perhaps a cpYFP moiety that is placed between two Prx domains would sense decamer dissociation. Yet another strategy is a fusion protein in which cpYFP is sandwiched between a Prx and a thioredoxin (Trx) domain, the latter lacking its resolving cysteine (Figs. 2C and 2D). The reasoning behind this design is that the mutant Trx domain will covalently trap the oxidized Prx domain thus causing a structural change that is sensed by the cpYFP moiety. This strategy was used previously to generate a methionine sulfoxide sensitive probe in which cpYFP is inserted between a methionine sulfoxide reductase domain and a mutant Trx domain (Tarrago et al., 2015). A major disadvantage of utilizing circular permutated fluorescent proteins (cpFPs) like cpYFP is their intrinsic pH sensitivity and the requirement to use stringent pH controls in each experiment (Bilan and Belousov, 2015). However, a potential advantage is that cpFPs of different color can be used to create spectral probe variants (Ermakova et al., 2014; Zhao et al., 2011).
The use of FRET to investigate 2-Cys peroxiredoxin behavior has already been reported (Muthuramalingam et al., 2009; Seidel et al., 2010). The authors used two (single-step FRET) or three (two-step FRET) Prx-fluorescent protein (FP) pairs to monitor the decamer dissociation upon peroxiredoxin oxidation. Although these Prx-FP fusions showed potential as cellular H2O2 biosensors, no further developments in this direction have been reported.
The envisaged Prx-based biosensors promise to achieve much higher sensitivity than the current generation of genetically encoded H2O2 sensors (Ezerina et al., 2014). However, peroxiredoxins exhibit rather complex biochemical and structural behavior (Rhee and Woo, 2011; Perkins et al., 2015). This may complicate or compromise their utilization as H2O2 sensors. In the following we discuss these complexities and how they may affect probe behavior. For simplicity, we focus our discussion on roGFP-Prx fusion proteins, but most considerations equally apply to the other design strategies.
First of all, fusion to a fluorescent protein might already influence Prx behavior. Previously, the presence of an N- or C-terminal tag was found to influence peroxidase activity, chaperone holdase activity, hyperoxidation sensitivity or oligomeric structure of several Prxs (Cao et al., 2007; Konig et al., 2013; Koo et al., 2002; Noichri et al., 2015; Randall et al., 2014; Sayed and Williams, 2004; Seo et al., 2009). Thus, each potential Prx-based probe should be functionally characterized and compared to the unfused Prx.
Many Prxs not only react with H2O2, but also show reactivity towards organic peroxides and peroxinitrite (Perkins et al., 2014). For example, human Prx5 and
The oligomeric state of different peroxiredoxins can vary from monomers to decamers/docecamers and may change upon oxidation (Barranco-Medina et al., 2009; Hall et al., 2011). In principle, a probe should have a simple design, and thus a monomeric Prx may be preferred as a sensing moiety. However, only a few peroxiredoxins are monomeric. The majority forms dimers and higher oligomeric structures. A typical 2-Cys peroxiredoxin fused to a fluorescent reporter would need to dimerize to be active. This situation raises several questions: Does a probe based on a typical 2-Cys Prx only form probe-probe dimers, or does it also form heterodimers with endogenous Prx molecules? Does the probe form decamers, or is decamerization prevented by the fused reporter protein? If it does form decamers, does it form probe homo-decamers or mixed hetero-decamers with endogenous peroxiredoxins? Furthermore, is decamerization required for the probe to function? Mutations at the A-type interface, either stabilizing or destabilizing decamerization, may be used to investigate this question. For example, Parsonage et al. showed that substitution of Thr77 of
The inactivation of peroxiredoxins by hyperoxidation has been observed under physiological circumstances (Nelson et al., 2013; Perkins et al., 2014). If a Prx-based probe turns out to be susceptible to hyperoxidation, it may under certain conditions report false results. Fortunately, not all Prx are highly sensitive to hyperoxidation. Bacterial Prxs are in general more robust, whereas some eukaryotic Prxs, including human Prx2, are remarkably sensitive (Nelson et al., 2013; Wood et al., 2003). Thus, bacterial Prxs may be preferable over eukaryotic Prxs when designing a Prx-based probe. Nevertheless, an intrinsically sensitive Prx could be modified to decrease its hyperoxidation sensitivity. Several factors have been described to influence hyperoxidation sensitivity, including two distinct sequence motifs: a GGLG and a C-terminal YF motif (Wood et al., 2003). It has been shown that alteration of these motifs and their surrounding residues modulate hyperoxidation sensitivity (Sayed and Williams, 2004; Wang et al., 2012). One possibility to decrease hyperoxidation sensitivity is the truncation of the C-terminus (Koo et al., 2002; Randall et al., 2014; Sayed and Williams, 2004; Seo et al., 2009). This strategy could be used to increase the robustness of hyperoxidation-sensitive peroxiredoxins, making them more suitable as a sensing moiety for a probe. In any case, the hyperoxidation sensitivity of any Prx-based probe should be determined experimentally since unambiguous predictors of hyperoxidation sensitivity are lacking (Perkins et al., 2014). Immunoblotting with hyperoxidation specific antibodies allows to determine hyperoxidation of Prx-based probes (Fig. 3A).
Peroxiredoxins are subject to various post-translational modifications which influence their peroxidase activity or other properties. For instance, phosphorylation of Thr90 in human Prx1 and Thr89 in Prx2 attenuates peroxidase activity and promotes chaperone holdase activity whereas Ser32 phosphorylation of Prx1 is reported to increase peroxidase activity (Chae et al., 2012; Chang et al., 2002; Jang et al., 2006; Qu et al., 2007; Zykova et al., 2010). N-terminal acetylation of human Prx2 was found to influence hyperoxidation sensitivity (Seo et al., 2009). Thus, it is conceivable that a Prx-based probe can also undergo post-translational modifications under certain conditions. Such modifications may alter the probe response and lead to the misinterpretation of measurements. For those residues already known to be potentially modified, corresponding probe point mutants (e.g. preventing or mimicking phosphorylation) can be created and studied in parallel. Alternatively or additionally, a probe based on a heterologous Prx may be employed, thus decreasing the probability of its post-translational modification in the host system.
A dynamic (i.e. reversible) probe offers the possibility to monitor transient elevations in H2O2. Since the reaction with the peroxide is an irreversible reaction, probe reduction depends on cellular reducing systems (Figs. 1 and 2). Thus, a Prx-based probe is a dual-specificity sensor in the sense that it responds not only to changes in peroxide levels, but also to changes in the activity of the relevant reducing system. The reducing system to which the probe responds will depend on the design of the probe (Fig. 2). If the probe uses a typical 2-Cys Prx moiety, it will likely be reduced by the Trx system, unless the Prx moiety is intentionally altered to avoid reduction by thioredoxin (e.g. by mutation of the resolving cysteine). Designing a Prx-based probe to respond to a particular reducing system may be useful in order to limit or adjust the total H2O2 turnover of the probe. The latter determines how much H2O2 is consumed by the probe inside cells (see next paragraph). In any case, it will be important to characterize in detail how a given Prx-based probe is reduced inside cells. This can be achieved by using selective deletion/silencing of reducing systems inside cells and can additionally be studied in vitro with recombinant proteins.
In principle, the ectopic expression of any H2O2-consuming probe may perturb cellular H2O2 homeostasis (Schwarzlander et al., 2015). The impact of a Prx-based probe on endogenous H2O2 levels will depend on two factors, namely the probe’s expression level and its H2O2 turnover. The latter depends on both the rate of probe oxidation and the rate of probe reduction. Under most conditions, the endogenous peroxidase activity of the cell is highly efficient, not least due to the high reactivity and abundance of endogenous Prxs (Rhee et al., 2012). Thus, it can be expected that ectopic expression of a Prx-based probe at levels not higher than that of endogenous Prxs will not lead to a major impact on endogenous H2O2 homeostasis. Nevertheless, the impact of expressing a H2O2-consuming probe will need to be determined experimentally. A simple and coarse approach would be to follow growth and survival of cells exposed to a range of H2O2 concentrations in the absence or presence of ectopic probe expression. If probe expression does not enhance the overall H2O2 scavenging capacity, the rate and extent of recovery will not be different from cells lacking probe expression (Fig. 3B). However, this experiment does not directly investigate the impact of probe expression on endogenous H2O2 levels and cellular adaptations could obscure the interpretation. More sophisticated experiments to directly investigate the contribution of a Prx-based probe to cellular H2O2 scavenging could be envisaged along the following lines: a non-fluorescent mutant of the probe (i.e. a mutant with identical expression, but lacking a mature fluorophore) is expressed in the cytosol and a fluorescent version of the same or alternative probe is expressed in the mitochondrial matrix. A bolus of H2O2 is given from outside the cell and the amount of H2O2 reaching the mitochondrial matrix is monitored by the mitochondrially targeted probe. This reveals if and how much the cytosolic probe (which is made non-fluorescent in order not to interfere with measurement of the mitochondrial probe) contributes to H2O2 scavenging (Fig. 3C). An alternative approach makes use of the wide distribution of probe expression levels within a cell population upon transient transfection (which reaches from barely detectable expression to very strong overexpression) (Barata and Dick, 2013; Schwarzlander et al., 2015). Any ratiometric probe (like the cpYFP and roGFP based probes) that does not influence its own measurement (i.e. endogenous H2O2 levels) is expected to yield a perfectly straight line on a scatter plot that relates the fluorescent emission intensities at the two excitation wavelengths. Any deviation of this linearity at higher fluorescence intensities (i.e. higher expression levels) would indicate an impact of the probe on H2O2 levels. These assays should also allow screening for probe variants with minimal impact on endogenous H2O2 homeostasis.
Chaperon holdase activity is a well-known non-peroxidase function of 2-Cys peroxiredoxins (Rhee and Woo, 2011). The gain of chaperone activity seems to be tightly linked to the loss of peroxidase activity through hyperoxidation or heat stress. It is conceivable that a 2-Cys Prx-based probe introduces additional chaperone activity to the cell, especially if the Prx is sensitive to hyperoxidation. However, the reporter moiety might sterically hinder the chaperone activity. Indeed, the N-terminus of peroxiredoxins is crucial for the binding of client proteins and an N-terminal tag was found to abolish the chaperone activity (Teixeira et al., 2015). The intrinsic chaperone activity of a recombinant Prx-based probe may be determined with commonly used
In summary, despite the many complexities that need to be addressed, peroxiredoxins promise to become the foundation of the next generation of genetically encoded H2O2 biosensors.
Sue Goo Rhee
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