#PAGE_PARAMS# #ADS_HEAD_SCRIPTS# #MICRODATA#

The monothiol glutaredoxin GrxD is essential for sensing iron starvation in Aspergillus fumigatus


Authors: Matthias Misslinger aff001;  Mareike Thea Scheven aff002;  Peter Hortschansky aff002;  Manuel Sánchez López-Berges aff001;  Katharina Heiss aff001;  Nicola Beckmann aff001;  Thomas Heigl aff001;  Martin Hermann aff004;  Thomas Krüger aff002;  Olaf Kniemeyer aff002;  Axel A. Brakhage aff002;  Hubertus Haas aff001
Authors place of work: Institute of Molecular Biology, Biocenter, Medical University of Innsbruck, Innsbruck, Austria aff001;  Department of Molecular and Applied Microbiology, Leibniz Institute for Natural Product Research and Infection Biology—Hans Knöll Institute (HKI), Jena, Germany aff002;  Institute of Microbiology, Friedrich Schiller University Jena, Jena, Germany aff003;  Department of Anaesthesiology and Critical Care Medicine, Medical University of Innsbruck, Innsbruck, Austria aff004
Published in the journal: The monothiol glutaredoxin GrxD is essential for sensing iron starvation in Aspergillus fumigatus. PLoS Genet 15(9): e32767. doi:10.1371/journal.pgen.1008379
Category: Research Article
doi: https://doi.org/10.1371/journal.pgen.1008379

Summary

Efficient adaptation to iron starvation is an essential virulence determinant of the most common human mold pathogen, Aspergillus fumigatus. Here, we demonstrate that the cytosolic monothiol glutaredoxin GrxD plays an essential role in iron sensing in this fungus. Our studies revealed that (i) GrxD is essential for growth; (ii) expression of the encoding gene, grxD, is repressed by the transcription factor SreA in iron replete conditions and upregulated during iron starvation; (iii) during iron starvation but not iron sufficiency, GrxD displays predominant nuclear localization; (iv) downregulation of grxD expression results in de-repression of genes involved in iron-dependent pathways and repression of genes involved in iron acquisition during iron starvation, but did not significantly affect these genes during iron sufficiency; (v) GrxD displays protein-protein interaction with components of the cytosolic iron-sulfur cluster biosynthetic machinery, indicating a role in this process, and with the transcription factors SreA and HapX, which mediate iron regulation of iron acquisition and iron-dependent pathways; (vi) UV-Vis spectra of recombinant HapX or the complex of HapX and GrxD indicate coordination of iron-sulfur clusters; (vii) the cysteine required for iron-sulfur cluster coordination in GrxD is in vitro dispensable for interaction with HapX; and (viii) there is a GrxD-independent mechanism for sensing iron sufficiency by HapX; (ix) inactivation of SreA suppresses the lethal effect caused by GrxD inactivation. Taken together, this study demonstrates that GrxD is crucial for iron homeostasis in A. fumigatus.

Keywords:

Biology and life sciences – Genetics – Gene expression – Biochemistry – Organisms – Eukaryota – Physical sciences – Chemistry – Research and analysis methods – Animal studies – Experimental organism systems – Model organisms – proteins – DNA-binding proteins – Fungi – Yeast – Saccharomyces – Saccharomyces cerevisiae – Molecular biology – Yeast and fungal models – Mycology – Gene regulation – Molecular biology techniques – Medicine and health sciences – Chemical compounds – Microbiology – Medical microbiology – Microbial pathogens – Pathology and laboratory medicine – Pathogens – Fungal molds – Aspergillus – Aspergillus fumigatus – Schizosaccharomyces – Schizosaccharomyces pombe – Fungal pathogens – Transcription factors – Regulatory proteins – Amino acids – Sulfur containing amino acids – Cysteine – Protein interactions – Molecular biology assays and analysis techniques – Gene expression and vector techniques – Hyperexpression techniques – Organic compounds – Carbohydrates – Monosaccharides – Xylose – Organic chemistry

Introduction

Iron is an essential trace element for almost all organisms in all kingdoms of life. On the other hand, iron excess is toxic. Therefore, to maintain cell homeostasis, the balance between iron uptake and iron consumption has to be tightly regulated.

Previous studies have shown that iron homeostasis in the pathogenic mold Aspergillus fumigatus is mainly regulated by two transcription factors, SreA, the repressor of siderophore biosynthesis and reductive iron assimilation [1], and HapX, which is a repressor of iron-consuming pathways and activator of iron acquisition [2]. Moreover, HapX is essential for adaptation to iron excess. When iron concentrations increase, HapX changes its function from a repressor to an activator of iron-consuming and detoxifying pathways to avoid iron toxicity. Consequently, HapX is crucial for adaptation to both iron starvation (-Fe) and high iron concentrations (hFe), i.e. lack of this regulator causes growth defects under -Fe as well as hFe [3]. Notably, both the -Fe and hFe functions of HapX require the HapB/HapC/HapE CCAAT-binding complex (CBC) as a DNA binding platform [4].

SreA and HapX are interconnected in a feedback-loop [5]: Expression of sreA is repressed by HapX during -Fe [2] and, in turn, hapX expression is repressed by SreA under iron sufficiency/excess [1]. Moreover, HapX induces sreA expression in response to iron.

Fungal iron sensing has been studied most intensively so far in the yeasts Saccharomyces cerevisiae and Schizosaccharomyces pombe [6,7]. Remarkably, there is little similarity with respect to transcriptional iron regulation between S. cerevisiae and A. fumigatus. Despite the fact that both, HapX and SreA are conserved in most ascomycetes, S. cerevisiae lacks classical homologs of SreA and HapX. In this yeast, adaptation to iron starvation is mainly mediated by two paralogous transcription factors, termed Aft1 and Aft2 [810]. Adaptation to hFe by transcriptional activation iron detoxification is mediated by the bZIP transcription factor Yap5 [11]. Nevertheless, S. cerevisiae Yap5 and HapX show similarities. Both transcription factors are essential for iron detoxification by activation of vacuolar iron deposition. Moreover, they share a highly conserved cysteine-rich region (CRR) that is crucial for this function and which has been shown to coordinate a [2Fe-2S] cluster in Yap5 [3,12]. In contrast to HapX, however, Yap5 has no function during iron starvation. S. pombe employs a homolog of SreA, termed Fep1 [13] and a regulator displaying similarity with HapX, termed Php4 [14]. Similar to HapX, Php4 acts as repressor of iron-consuming functions during iron starvation, but in contrast to HapX it is not involved in activation of iron detoxification. Taken together, S. cerevisiae, S. pombe and A. fumigatus show significant differences with regard to the employed iron-regulatory transcription factors and the molecular mechanisms of iron sensing in A. fumigatus are largely uncharacterized.

In both S. cerevisiae and S. pombe, the cytosolic monothiol glutaredoxins Grx3/4 respectively Grx4 have been shown to be involved in iron sensing [15,16] and coordination and transport of [2Fe-2S] clusters. These proteins contain a thioredoxin (Trx)-like domain, for which a canonical reductase activity has been excluded [17], and a glutaredoxin (Grx) domain comprising a highly conserved CGFS motif. Coordination of [2Fe-2S] clusters is performed via the cysteine residue of the CGFS motif and two glutathione residues, which leads to dimerization of these monothiol glutaredoxins [1820].

In the current study, we characterized the role of the cytosolic monothiol glutaredoxin of A. fumigatus (Afu2g14960), designated GrxD. We demonstrate that GrxD is essential for iron sensing by the iron-responsive transcription factors HapX and SreA, particularly for signaling iron starvation conditions. The study revealed both similarities and differences to iron sensing in other fungal species.

Results

GrxD is essential for A. fumigatus

Protein BLAST searches identified the A. fumigatus homolog, termed GrxD, of S. cerevisiae Grx3/4 and S. pombe Grx4, respectively. Alignment of GrxD homologs demonstrated high conservation, even between distantly related species (Figs 1 and S1). Compared to the Trx-like domain, the Grx domain shows significantly higher conservation including the [2Fe-2S] cluster coordinating CGFS motif.

Fig. 1.

Alignment of GrxD homologs from A. fumigatus, S. cerevisiae, and S. pombe.

<h2>Alignment of GrxD homologs from <i>A</i>. <i>fumigatus</i>, <i>S</i>. <i>cerevisiae</i>, and <i>S</i>. <i>pombe</i>.</h2>

Trx-like and Grx domains are highlighted in blue and yellow, respectively. The strictly conserved monothiol glutaredoxin specific CGFS motif and the conserved single cysteine residue in the Trx domain are framed. Identical amino acids in all three proteins are marked by asterisks. Amino acids, which are absent in truncated protein versions GrxDΔ19 or GrxDVenusΔTrx, are indicated by bars in green or purple, respectively.

To investigate GrxD function in A. fumigatus, we aimed to delete the grxD gene via replacement by a hygromycin resistance-conferring cassette (hph) (S2 Fig). Several attempts were unsuccessful, indicating that grxD is an essential gene, which we proved by heterokaryon rescue [21]. In short, this technique is based on the fact that A. fumigatus cells contain multiple nuclei. The fungal transformation procedure usually targets only the genome of one nucleus leading to heterokaryosity, in our case grxD+hph- (wt; containing grxD but lacking hph) nuclei and grxD-hph+ (ΔgrxD; lacking grxD but containing hph conferring hygromycin resistance) nuclei, which was proven by Southern blot analysis (Fig 2A). During conidiation, nuclei are separated since conidia contain only a single nucleus. Conidia of eight heterokaryotic transformants were able to grow under non-selective conditions but not in the presence on hygromycin (Fig 2A), demonstrating the inability of ΔgrxD (grxD-hph+) conidia to grow; i.e. grxD is an essential gene.

Fig. 2.

GrxD is essential, influences iron-dependent growth and SreA inactivation suppresses the lethal effect of GrxD inactivation.

<h2>GrxD is essential, influences iron-dependent growth and SreA inactivation suppresses the lethal effect of GrxD inactivation.</h2>

Strains were grown for 48 h at 37°C in minimal medium, with exception of F, where complex medium was used. In general, media contained 1% glucose with exception of media containing 1% xylose, which leads to maximal activation of the PxylP promoter. -Fe, +Fe, hFe media contained no, 0.03 mM and 10 mM iron, respectively. BPS media contained 0.2 mM of the ferrous-iron specific chelator bathophenanthroline disulfonate to generate iron starvation in complex media. (A) Heterokaryon rescue: Exemplary Southern blot analysis showing heterokaryosity of two independent transformants because of the presence of wt as well as ΔgrxD alleles; eight independent heterokaryotic transformants were able to grow under non-selective conditions but failed to grow in the presence of hygromycin indicating essentiality of grxD. (B) Schematic overview of generated strains for PxylP-mediated conditional expression of grxD variants indicating truncations and Venus-tagging (C) PxylP-mediated downregulation of full-length GrxD (PxylP:grxD) and full-length Venus-tagged GrxD (PxylP:grxDvenus) decreased growth during -Fe. Overexpression decreased growth during hFe (D) PxylP-mediated downregulation of N-terminal truncation of GrxD (PxylP:grxDΔ19) and, even more pronounced, truncation of the Trx domain (PxylP:grxDvenusΔtrx) blocked growth during iron starvation, which was rescued by iron supplementation. A spontaneous suppressor mutation (PxylP:grxDΔ19sup) as well as inactivation of SreA (PxylP:grxDΔ19/ΔsreA) rescued the growth defect of downregulation of N-terminal truncated GrxD (PxylP:grxDΔ19) during -Fe and +Fe. (E) C-terminal Venus-tagging (PxylP:grxDvenus) did not affect the function of GrxD. (F) Inactivation of SreA (ΔgrxD/ΔsreA) suppressed lethality of lack of GrxD (ΔgrxD).

Due to the lethality of grxD deletion, we generated strains, in which grxD is under the control of the xylose-inducible xylP promoter (PxylP, [22]). These strains were generated without and with C-terminal tagging of GrxD with the yellow fluorescent protein derivative Venus, yielding strains PxylP:grxD and PxylP:grxDvenus, respectively (Fig 2B). PxylP displays xylose concentration-dependent activation. Without xylose supplementation, activity of this promoter is very low, i.e. expression of essential genes under this promoter in A. fumigatus led to the inability to grow [23]. Although we proved that grxD is essential (Fig 2A), strains PxylP:grxD and PxylP:grxDvenus were able to grow without xylose-induction on solid minimal medium (Fig 2C). This indicates that very low expression is sufficient to support growth. Nevertheless, we observed growth deficiencies under iron starvation, which were ameliorated with increasing iron concentrations (Fig 2C), which indicates a role of GrxD in iron homeostasis. Overexpression of grxD with and without venus-tagging decreased growth under excess iron, but not under iron starvation or iron replete conditions (Fig 2C), indicating that a surplus of GrxD impedes adaptation to high iron conditions.

The Trx domain is not essential for growth

To further analyze GrxD function, we generated A. fumigatus mutants producing PxylP-driven GrxD variants lacking either the 19 N-terminal amino acids (strain PxylP:grxDΔ19) or the whole Trx domain (PxylP:grxDvenusΔtrx, Fig 1), whereby in the latter strain GrxD was C-terminally tagged with Venus (Fig 2B). Under non-inducing conditions (without xylose), truncation of 19 N-terminal amino acids or truncation of the complete Trx domain, respectively, blocked growth during iron starvation and iron sufficiency (Fig 2D). Growth of both mutant strains was rescued by xylose supplementation, whereby the strain expressing the Trx domain lacking GrxD required higher xylose supplementation indicating lower activity. Important to note, C-terminal tagging with Venus did not affect function of GrxD, at least judged by growth ability (Fig 2E).

The fact that, in contrast to strains PxylP:grxD and PxylP:grxDvenus, strains PxylP:grxDΔ19 and PxylP:grxDvenusΔtrx were unable to grow in -Fe conditions under non-induced conditions indicates that truncation of the N-terminal 19 amino acids or, even more pronounced, the truncation of the Trx domain decreases activity of GrxD. This might be due to decreased protein stability or hampered function. Nevertheless, under xylose-inducing conditions, all strains were able to grow under all conditions, which indicates that in contrast to the whole GrxD protein, the Trx domain is not essential for growth, at least when overexpressed. Consequently, the Grx domain is likely essential for growth.

Iron supplementation partially rescues GrxD deficiency

As shown above, N-terminal truncated GrxD versions (PxylP:grxDΔ19 and PxylP:grxDvenusΔtrx) were not able to grow at non-inducing conditions during iron starvation or iron sufficiency (Fig 2D). However, high iron supplementation partially rescued the growth of these strains at non-inducing conditions (Fig 2D). These data indicate that GrxD is involved in iron homeostasis with an important role especially during iron starvation. This is in agreement with decreased growth of strains with down-regulated GrxD, without and with C-terminal Venus-tagging, under iron starvation but not iron sufficiency and iron excess (Fig 2C).

Inactivation of SreA suppresses the lethality caused by lack of GrxD

Occasionally, cultivation of PxylP:grxDΔ19 conidia on plates resulted in suppressor mutants. We characterized one of these mutant strains, termed PxylP:grxDΔ19sup, in more detail. In contrast to PxylP:grxDΔ19, PxylP:grxDΔ19sup was able to grow without xylose-induction under iron starvation and iron sufficiency (Fig 2D). Under 0.1% xylose-inducing conditions, PxylP:grxDΔ19sup displayed a similar radial growth under iron starvation but decreased growth under iron sufficiency and high iron conditions compared to PxylP:grxDΔ19 (Fig 2D). These results indicated that the suppressor mutation present in this strain leads to a defect in adaptation to iron excess.

Northern analysis revealed an additional sreA transcript as well as de-repression of hapX and mirB (encoding a siderophore transporter) during iron sufficiency in strain PxylP:grxDΔ19sup compared to PxylP:grxDΔ19 (S3A Fig). These results suggested that the suppressor mutation affects the function of SreA, which has previously been shown to repress transcription of these two genes [1]. PCR amplification analyses of the sreA locus (S3B and S3F Fig) followed by rapid amplification of cDNA ends (3´-RACE) and nucleotide sequencing (S3C and S3D Fig) revealed that the suppressor mutation caused a chromosomal rearrangement (S3E Fig), which results in truncation of SreA within the DNA-binding region.

To independently confirm the genetic interaction between grxD and sreA, the sreA gene was deleted in a PxylP:grxDΔ19 background. This mutant, PxylP:grxDΔ19/Δ sreA, displayed the same growth pattern as PxylP:grxDΔ19sup (Fig 2D), which affirms that sreA loss-of-function rescues the growth defect caused by down-regulation of grxD during iron starvation and sufficiency.

To analyze whether inactivation of SreA rescues growth only in response to downregulation of GrxD (PxylP:grxDΔ19/ΔsreA at non-inducing conditions) or also complete lack of GrxD, we aimed to delete the grxD gene in a ΔsreA background. In contrast to wt background (see above), this approach was successful. Compared to wt, the ΔgrxD/ΔsreA strain displayed severely decreased radial growth under iron starvation, iron sufficiency and iron excess, but it was viable (Fig 2F).

SreA is the repressor of iron uptake and SreA inactivation results in increased iron acquisition [1]. Consequently, the identified genetic interaction between grxD and sreA, together with the rescue of growth of the PxylP:grxDΔ19 strain under non-inducing conditions by high iron supplementation (Fig 2D), indicate that lack of GrxD results in iron shortage, possibly caused by the requirement of GrxD for sensing iron starvation.

Iron starvation increases grxD expression and promotes nuclear localization

To monitor endogenous and PxylP-controlled grxD expression, we performed Northern analysis. In wt grxD transcript levels decreased with increasing iron supplementation (Fig 3A). In PxylP:grxDΔ19, grxD expression was highly induced under xylose-induced conditions and decreased below detection limit upon xylose withdrawal demonstrating functionality of PxylP-mediated conditional grxD expression (Fig 3A).

Fig. 3.

Expression of grxD is regulated by iron availability and controlled by xylose when expressed under control of the PxylP promoter.

<h2>Expression of <i>grxD</i> is regulated by iron availability and controlled by xylose when expressed under control of the <i>PxylP</i> promoter.</h2>

(A) For Northern analysis, RNA from wt and PxylP:grxDΔ19 was isolated after growth for 20 h at 25°C in inducing conditions and subsequent growth under non-inducing conditions at -Fe, +Fe and hFe for 20 h at 37°C. As a control, inducing conditions were maintained (0.1% xylose). (B,C) For Western blot analysis, grxDvenus, PxylP:grxDvenus and PxylP:grxDvenusΔtrx were harvested after growth for 16h at -Fe, +Fe or hFe with the indicated xylose concentrations. Loading of equal protein amounts was confirmed by Coomassie staining; Venus-tagged GrxD or variants thereof were detected with a mouse α-GFP antibody. Western blot analysis of GrxDvenusΔtrx under non-inducing conditions is only shown for hFe as this is the only condition in which PxylP:grxDvenusΔtrx is able to grow. For quantification of Northern and Western blot data (Tables), images were analyzed using ImageJ. Northern blot signals were first normalized to the respective rRNA and subsequently to the reference strain, whereby genes repressed by iron (mirB, hapX, grxD) were normalized to the reference strain grown under iron starvation, while genes induced by iron (sreA, cccA) were normalized to the reference strain grown under iron sufficiency. GrxDvenus protein levels were first normalized to total protein and subsequently to the reference strain grown under iron starvation.

In agreement with wt grxD transcript levels, Western blot analysis demonstrated that Venus-tagged GrxD (GrxDVenus) protein levels decreased with increasing iron availability when grxD was expressed from the endogenous promoter (strain grxDvenus; Fig 3B). Under control of the PxylP promoter, the protein level of Venus-tagged full-length GrxD (GrxDVenus, strain PxylP:grxDvenus) was highly decreased under non-inducing compared to inducing conditions (Fig 3C). Interestingly, hFe conditions slightly decreased the GrxDVenus protein level under xylose-inducing conditions, which indicates an influence of iron on xylP promoter activity or on the grxD transcript stability.

To analyze protein levels of the GrxD variant lacking the 19 N-terminal amino acids (GrxDΔ19), we generated a strain in which C-terminally Venus-tagged GrxDΔ19 is under the control of the xylP promoter (strain PxylP:grxDvenusΔ19). This strain showed identical growth compared to the untagged version PxylP:grxDΔ19 (S4 Fig). Compared to GrxDVenus, the protein levels of the Venus-tagged GrxD variants lacking the 19 N-terminal amino acids (GrxDVenusΔ19, strain PxylP:grxDvenusΔ19) or the Trx domain (GrxDVenusΔTrx, strain PxylP:grxDvenusΔtrx) were slightly decreased under inducing conditions. Remarkably, under steady-state, non-inducing, high iron conditions (Fig 3C), truncation of the 19 N-terminal amino acid residues (GrxVenusΔ19) decreased the protein level compared to GrxDVenus although not as much as truncation of the entire Trx domain (GrxVenusΔTrx). Due to the use of the same promoter, these data indicate higher protein stability of GrxDVenus compared to the truncated versions. These results most likely provide the explanation for the lack of growth of strains PxylP:grxDvenusΔ19 and PxylP:grxDvenusΔtrx during iron starvation and sufficiency under non-inducing conditions (Figs 2D and S4) in contrast to strain PxylP:grxDvenus (Fig 2C).

Subcellular localization of Venus-tagged GrxD was determined by fluorescence. To visualize the nucleus, we expressed a gene encoding histone H2A tagged with monomeric red fluorescence protein (H2AmRFP) in recipient strains PxylP:grxDvenus and PxylP:grxDvenusΔtrx (yielding strains PxylP:grxDvenus/H2AmRFP and PxylP:grxDvenusΔtrx/H2AmRFP).

Fluorescence microscopy with these strains revealed that GrxDVenus and GrxDVenusΔTrx displayed predominant nuclear localization during iron starvation but not iron sufficiency (Fig 4). During iron sufficiency, we did not observe organelle-specific accumulation of GrxDVenus. The nuclear localization indicates a regulatory role of GrxD at least during iron starvation. Noteworthy, it has been demonstrated previously that HapX also accumulates in the nucleus during iron starvation [3].

Fig. 4.

GrxDVenus and GrxDVenusΔTrx are enriched in the nucleus during iron starvation.

<h2>GrxD<sup>Venus</sup> and GrxD<sup>VenusΔTrx</sup> are enriched in the nucleus during iron starvation.</h2>

For fluorescent microscopy, strains (A) PxylP:grxDvenus/H2AmRFP and (B) PxylP:grxDvenusΔtrx/H2AmRFP were grown for 18h with 0.05% xylose under iron starvation (-Fe) or iron sufficiency (+Fe). The mRFP-tagged histone H2A served to visualize nuclei.

GrxD associates with the iron responsive transcription factors HapX and SreA as well as with components of the cytosolic iron-sulfur protein assembly (CIA) pathway

To identify GrxD-interacting proteins, A. fumigatus strains wt, PxylP:grxDvenus and PxylP:grxDvenusΔtrx were cultivated under iron starvation (-Fe), sufficiency (0.03 mM Fe) and excess (5 mM Fe) and the corresponding crude cell extracts were subjected to GFP-Trap affinity purification [24]. Here, wt served as a negative control to distinguish specifically interacting proteins from false positive bound ones. Effective enrichment of GrxDVenus and GrxDVenusΔTrx proteins was validated by SDS-PAGE and silver staining as well as Western blot analysis (S5 Fig). Eluates from three independent biological GFP-Trap replicates were subsequently analyzed by nLC-MS/MS. For visualization of the specific enrichment of GrxD-interacting proteins, label-free quantification (LFQ) abundances of the most enriched proteins identified in PxylP:grxDvenus and PxylP:grxDvenusΔtrx GFP-Trap eluates were plotted against their LFQ abundances in wt control eluates (Fig 5 and Tables 1 and S1).

Fig. 5.

Scatterplot visualization of specifically enriched proteins interacting with Venus tagged GrxD (GrxDVenus) and GrxD lacking its Trx domain (GrxDVenusΔTrx).

<h2>Scatterplot visualization of specifically enriched proteins interacting with Venus tagged GrxD (GrxD<sup>Venus</sup>) and GrxD lacking its Trx domain (GrxD<sup>VenusΔTrx</sup>).</h2>

Absolute label-free quantification (LFQ) abundances of proteins were determined by nLC-MS/MS analysis after GFP-Trap affinity purification from A. fumigatus PxylP:grxDvenus (A-C) and PxylP:grxDvenusΔtrx (D-F) mycelial extracts and plotted against their LFQ abundances in wt GFP-Trap eluates. Each dot represents the mean value of three biological replicates. Mycelia were grown under iron starvation (-Fe), sufficiency (0.03 mM Fe), and excess (5 mM Fe) at 37°C for 22 h. Expression of grxDvenus and grxDvenusΔtrx under control of PxylP was induced by addition of 1% (w/v) xylose. Specifically co-purified proteins are indicated by green dots. Bait proteins GrxDVenus and GrxDVenusΔTrx are marked as red dots.

Tab. 1.

List of the most enriched proteins by GFP-Trap affinity purification using GrxDVenus and GrxDVenusΔTrx as bait proteins.

<h2>List of the most enriched proteins by GFP-Trap affinity purification using GrxD<sup>Venus</sup> and GrxD<sup>VenusΔTrx</sup> as bait proteins.</h2>

GFP-Trap eluates from A. fumigatus wt mycelial extracts were used as control. Proteins with LFQ abundances higher than 5x107 that were enriched more than 4-fold (log2) versus wt controls in at least one iron supply condition are presented. Nbp35 and Mms19 are included, but are enriched less than 4-fold (log2). nd, ortholog not determined.

We identified HapX as one of the most highly enriched proteins by GrxDVenus GFP-Trap under iron limitation (Fig 5A). HapX was also detected in iron sufficient and high-iron conditions (Fig 5B and 5C), however, with lower abundance, most likely due to its low protein level under these conditions [3]. Inversely, SreA was preferentially co-purified under iron sufficiency and excess (Fig 5B and 5C), again reflecting the expression pattern of SreA [1]. These data indicate that GrxD constitutively interacts with HapX irrespective of the cellular iron status and at least under iron sufficiency and iron excess also with SreA; possibly, GrxD interacts also constitutively with SreA—the missing detection of the interaction during iron starvation might be due to the low expression of sreA during this condition [1].

In addition, proteins that are part of the cytosolic iron-sulfur protein assembly (CIA) machinery, namely Nbp35 (Afu2g15960), Dre2 (AFUB_008090) and Mms19 (Afu8g05370), were enriched with high abundance under standard and excess iron levels (Fig 5B and 5C). The CIA machinery was investigated extensively in the model organism S. cerevisiae. These studies showed that the monothiol glutaredoxins Grx3 and Grx4 play an indispensable role for cytosolic iron-sulfur (FeS) cluster biogenesis. An early step in cytosolic [4Fe-4S] cluster assembly involves Nbp35 forming a hetero-tetrameric scaffold complex with Cfd1 on which a [4Fe-4S] cluster is bound transiently [25,26]. Dre2 belongs to the CIA electron transfer complex and is needed for formation of the [4Fe-4S] cluster on Nbp35 [27,28]. Mms19 is part of the CIA targeting complex consisting of Cia1, Cia2 and Mms19, which, together with Nar1 transfers the [4Fe-4S] cluster to target apoproteins [29,30].

The precise site of requirement of monothiol glutaredoxins in the cytosolic FeS protein biogenesis has not been determined yet. In yeast, Grx3/4 is required for FeS cluster assembly on Dre2 and Nar1 [19]. How GrxD is exactly involved in the CIA of A. fumigatus remains to be elucidated. Nevertheless, these data underline the specificity of the approach.

Grx4 protein interaction studies in S. pombe demonstrated that the Trx domain is essential for a stable protein interaction with both the iron regulators Fep1 (SreA ortholog) [31] and Php4 (HapX ortholog) [32]. Therefore, we were interested whether the GrxD Trx domain is necessary for all of the detected GrxD protein interactions in A. fumigatus. To address this topic, we analyzed our quantitative GrxDVenus and GrxDVenusΔTrx GFP-Trap co-purification data for selected interaction partners in detail (Fig 6). The GrxD Trx domain appeared to be dispensable for GrxD-HapX complex formation irrespective of the iron supplementation (Fig 6B). In contrast, the GrxD Trx domain was essential for GrxD-SreA protein interaction (Fig 6C) indicated by a severely decreased SreA LFQ abundance in the absence of the Trx domain. Likewise, GrxDVenusΔTrx pull-down enrichment of the CIA proteins Dre2, Nbp35 and Mms19 was less effective (Fig 6D–6F).

Fig. 6.

The GrxD Trx domain is crucial for protein interaction of GrxD with SreA (C), Bol3 (I), and the CIA proteins Dre2 (D), Nbp35 (E) and Mms19 (F), but not for interaction with HapX (B), CmtA (G) and Bol1 (H). PxylP-driven production of GrxDVenus and GrxDVenusΔTrx facilitated trapping of both bait proteins independent from iron supplementation (A).

Unexpectedly, we identified the putative copper metallothionein CmtA (encoded by Afu4g04318) as an interaction partner of GrxD, preferably under iron excess conditions (Fig 6G). A recent study regarding cmtA regulation and CmtA protein function in A. fumigatus [33] revealed that cmtA expression is not regulated by copper availability and that CmtA is not required for copper detoxification. Consistently, the cmtA ortholog in A. nidulans (AN7011), termed MtlA, was found to be dispensable for copper ion tolerance [34]. Our GFP-Trap pull-down results may suggest that a GrxD-CmtA complex is involved in iron detoxification and/or transport, however this hypothesis has to be verified by future experiments.

Furthermore, our data suggested an interaction of GrxD with two putative BolA family proteins, Bol1 (Afu7g01520) and Bol3 (Afu6g12490). The Trx domain was dispensable for GrxD-Bol1 interaction, but GrxD-Bol3 interaction was dependent on its presence (Fig 6H and 6I). However, both A. fumigatus proteins contain an N-terminal mitochondrial targeting sequence, suggesting that these proteins are localized in mitochondria. In support, homologs of A. fumigatus Bol1 and Bol3 from other Aspergillus species also contain N-terminal mitochondrial targeting sequences. In agreement, fluorescent microscopy of a strain (PgpdA:bol1venus) expressing Bol1 C-terminally tagged with Venus (Bol1Venus) suggested that Bol1 is mainly localized in mitochondria (S6 Fig). It has been demonstrated previously that the homologous S. cerevisiae BolA proteins Bol1 and Bol3 form complexes with mitochondrial Grx5, which lacks a Trx domain [35]. As GrxD is localized in the cytosol and nucleus, the interaction with both mitochondrial Bol1 and Bol3 proteins in vivo appears unlikely. One possible explanation for their detected GrxD interaction is the artificial mixture of the proteins when cellular compartments are disrupted during sample preparation. A similar phenomenon has been observed in S. cerevisiae for interaction of Grx3/4 with Bol1, respectively Bol3 [36], which are both localized in mitochondria [35]. Nevertheless, we can neither exclude that a minor fraction of Bol1 is localized in the cytosol nor that Bol3 is exclusively or partially localized in the cytosol and that GrxD indeed interacts with these BolA-like proteins in vivo as described in other organisms [15,31,37,38].

To exemplary confirm GFP trap affinity purification results, we performed co-immunoprecipitation (co-IP) with subsequent Western blot detection (S7 Fig). HapX or SreA, respectively, was immunoprecipitated and purified from PxylP:grxDvenus and PxylP:grxDvenusΔtrx whole cell lysates using rabbit α-HapX, or rabbit α-SreA antibodies covalently linked to Protein-A-Sepharose. Western blot analysis demonstrated co-IP of GrxDVenus with both HapX and SreA (S7 Fig). These experiments confirmed that GrxDVenus interacts with both HapX and SreA, while truncation of the Trx domain GrxDVenusΔTrx blocks interaction with SreA but not with HapX.

Co-expression of GrxD and HapX promotes complex formation

For in vitro co-purification experiments, A. fumigatus GrxD was fused with a C-terminal His-tag (GrxDHis6) and bicistronically co-expressed in Escherichia coli with a polypeptide representing the A. fumigatus HapX C-terminus (HapX161-491) that contains all four cysteine-rich regions (CRR; Fig 7A). To investigate the interaction between both proteins, GrxDHis6 was enriched from crude cell extract via its His-tag using a Ni-Sepharose column. Consequently, co-purification of HapX161-491 requires binding to GrxDHis6. After initial Ni-chelate chromatography, we observed that GrxDHis6 and HapX161-491 were co-enriched (Fig 7B). The GrxD His-tag was subsequently removed by tobacco etch virus (TEV) protease treatment and the GrxD-HapX161-491 complex stability was further analyzed by preparative size exclusion chromatography (SEC). Two major peaks appeared during SEC and their apparent molecular masses were estimated based on the elution volumes of protein calibration standards. For peak 1, a molecular mass of 152.9 kDa (Fig 7B) approximately corresponding to a heterotetrameric complex consisting of two HapX161-491 and two GrxD subunits (theoretical mass: 130.4 kDa) was calculated. For peak 2, a molecular mass of 27.7 kDa corresponding to a theoretical molecular mass of a GrxD monomer (29.75 kDa) was determined. Additionally, UV-Vis spectra (250–550 nm) were recorded for peak 1 and 2 (Fig 7C). The reddish-brown color of the GrxD-HapX161-491 complex (peak 1) as well as the absorption maxima at 322 and 415 nm indicated the incorporation of a [2Fe-2S] ligand, as spectra of [2Fe-2S] proteins are typically more complex than those of [4Fe-4S] proteins, which display only one characteristic peak around 400–420 nm [39]. In contrast, GrxD separated in excess from the GrxD-HapX161-491 complex (peak 2) appeared colorless and displayed no absorption at 322 and 415 nm (Fig 7C). We hypothesized that the reddish-brown color of the GrxD-HapX161-491 complex is mainly derived from binding of an FeS ligand by HapX161-491 CRR. This was supported by SEC purification of HapX161-491 in the absence of GrxD, which yielded a reddish-brown colored SEC fraction displaying a UV-Vis spectrum almost identical to that of the GrxD-HapX161-491 complex (Fig 7D and 7E). These data strongly indicate that HapX is able to coordinate FeS cluster(s) without GrxD.

Fig. 7.

Neither the GrxD Trx domain nor the presence of conserved cysteine residues of GrxD and HapX are required for their in vitro protein-protein interaction in E. coli.

<h2>Neither the GrxD Trx domain nor the presence of conserved cysteine residues of GrxD and HapX are required for their <i>in vitro</i> protein-protein interaction in <i>E</i>. <i>coli</i>.</h2>

(A) Schematic illustration of the co-purified HapX and GrxD polypeptides. The four cysteine-rich regions of HapX161-491 are marked in yellow and the C-terminal region, which is essential for low-iron adaptation is shown in turquoise. GrxD thioredoxin (Trx) and glutaredoxin (Grx) domains are marked as grey and pink boxes, respectively. Proteins were enriched from E. coli cell lysates by Ni-chelate affinity chromatography via the His-tag of GrxD. The His-tag was subsequently removed by TEV protease treatment and proteins were further purified by size exclusion chromatography (SEC). (B) SEC A280 and A415 elution profiles of GrxD-HapX161-491 co-purification and Coomassie-staining of collected protein fractions after separation by SDS-PAGE. Peak 1 contained the GrxD-HapX161-491 protein complex with an apparent molecular mass of 152.9 kDa, which corresponds to a complex of two GrxD and two HapX161-491 subunits. Peak 2 represented the excess GrxD monomer with an apparent molecular mass of 27.7 kDa. (C) The GrxD-HapX161-491 complex (SEC peak1) was reddish-brown colored and the corresponding UV-Vis spectrum displayed absorption maxima at 322 and 415 nm, indicating the incorporation of FeS cluster(s), whereas the GrxD fraction (SEC peak 2) was colorless and lacked absorption maxima at 322 and 415 nm. (D) SEC A280 and A415 elution profiles and the corresponding (E) UV-Vis spectrum of HapX161-491 purified in the absence of GrxD indicating the incorporation of FeS cluster(s) by AfuHapX161-491 independent of GrxD. (F) The SEC A280 and A415 elution profiles of GrxDΔTrx-HapX161-491 and (G) GrxDC191A-HapX161-491 co-purifications indicated that the GrxD Trx domain as well as the GrxD cysteine 191, respectively, are not essential for GrxD-HapX161-491 protein interaction. (H) Mutation of HapX161-491 C203 to A as well as (I) exchange of C277 to A in the HapX CRR-A and B did not abolish complex formation with GrxD in vitro.

To analyze the in vitro GrxD-HapX161-491 protein-protein interaction in more detail, two GrxDHis6 mutants were constructed, co-produced with HapX161-491 and purified from E. coli crude cell extracts. Based on the results of the in vivo co-purification experiments, the Trx domain was deleted first. Consistent with our in vivo data, removal of the GrxD Trx domain had no impact on GrxDΔTrx-HapX161-491 protein interaction in vitro (Fig 7F). In a second step, GrxD cysteine (C) residue 191 was mutated to alanine (A). GrxD C191 is part of the CGFS active site motif in the Grx domain, which is highly conserved and known to be important for iron sensing through binding of a [2Fe-2S] cluster in S. cerevisiae [19,40] and S. pombe [32,41]. In S. pombe, the CGFS site’s cysteine is required for iron-dependent Grx4-Php4 complex formation [32]. In this study, mutation of the GrxD C191 to A did not influence binding to the HapX161-491 CRR in E. coli (Fig 7G).

HapX harbors four CRR, which might participate in iron sensing. As reported previously [3], CRR-A and B (Fig 7A) are crucial for adaptation to iron excess. In particular, the mutation of C 203 to A in CRR-A or exchange of C277 to A in CRR-B rendered A. fumigatus more susceptible to iron overload. C277 is part of the CRR-B C277GFCSDGTPCIC motif, which is reminiscent to the CGFCNDNTTCVC [2Fe-2S] cluster binding site in S. cerevisiae Yap5 [12]. To elucidate the impact of both C203 and C277 on GrxD-HapX161-491 complex formation, we targeted C203 and C277 by site-directed mutagenesis and replaced them by alanine. Neither HapX161-491 C203A exchange nor C277A substitution affected binding of the respective HapX versions to GrxD (Fig 7H and 7I). In summary, we conclude that the Trx domain and residue C191 of GrxD as well as residues C203 and C277 in HapX are not required for in vitro complex formation between GrxD and HapX.

GrxD is required for induction of iron acquisition and repression of iron inducible genes under iron starvation: Functions involving SreA and HapX

As gene deletion was not possible in wt cells, we developed a protein depletion strategy to investigate the effects of GrxD deficiency. We avoided to use strain ΔgrxD/ΔsreA as it was not possible to measure effects of GrxD deficiency on SreA in this strain and as growth of this mutant was severely impaired. To study the effects of GrxD depletion on iron regulation, we employed PxylP:grxDΔ19, which allowed to decrease grxD expression to a lethal amount without xylose induction, while growth was fully rescued with a moderate (0.1%) concentration of xylose (see above, Fig 2).

To analyze the effect of GrxD depletion on iron regulation, we performed Northern analysis of iron regulated genes during iron starvation and sufficiency. For GrxD depletion, PxylP:grxDΔ19 was grown under inducing conditions for 20 h at 25°C and subsequently grown for another 20h at 37°C without xylose to repress grxD expression. This method was used previously to investigate essential genes [23]. During iron starvation, GrxD depletion decreased transcript levels of hapX and mirB, which were upregulated during iron starvation in wt (Fig 8A and 8B). On the other hand, GrxD depletion increased transcript levels of sreA (Fig 8A and 8B) and cccA (Fig 8B), which are downregulated during iron starvation in wt. During iron sufficiency, GrxD depletion did not significantly affect transcript levels of these genes. These data emphasize that GrxD is involved in iron regulation and is important for adaptation to iron starvation rather than iron sufficiency.

Fig. 8.

GrxD depletion blocks adaptation to iron starvation, but not adaptation to iron sufficiency/excess.

<h2>GrxD depletion blocks adaptation to iron starvation, but not adaptation to iron sufficiency/excess.</h2>

(A) Conidia were germinated with 0.1% xylose (inducing) for 20 h at 25°C. Subsequently spores were washed and cultivated for another 20 h at 37°C without xylose (repressing) to deplete GrxD in PxylP:grxDΔ19 strains (indicated as Δ19). (B) After growth under iron starvation and depletion of GrxD, 0.03 mM iron was added for 30 min (sFe) to monitor short-term iron response. Similar to wt, iron responsive genes cccA and sreA were induced in a GrxD-depleted strain, indicating that GrxD is mainly required for sensing of iron starvation. (C) sFe response in ΔsreAgrxD showed that also gene-deletion of grxD does not abolish induction of cccA, which indicates a GrxD independent function of HapX. Quantification (Tables) was done as described in Fig 3.

Repression of sreA and cccA during iron starvation has previously been shown to depend exclusively on HapX [2,3]. Therefore, the de-repression of these genes found upon GrxD depletion indicates that GrxD is required for signaling iron starvation to HapX. To test whether the effects on mirB are linked to SreA or HapX, we also depleted GrxD in strains lacking SreA (strain PxylP:grxDΔ19/ΔsreA). It has been shown previously that sreA is downregulated in wt during iron starvation and lack of SreA results in de-repression of iron-uptake genes (mirB, hapX) during iron sufficiency [1]. Deletion of sreA in PxylP:grxDΔ19 increased expression of mirB upon GrxD depletion, albeit not to wt level. This indicated that GrxD is required to inactivate the repressing function of SreA under iron starvation. The absence of full induction in GrxD depleted PxylP:grxDΔ19/ΔsreA compared to the appropriate reference (ΔsreA) indicates that GrxD is not only required to inactivate SreA-mediated repression of mirB, but also for the induction of mirB expression, likely via activation of HapX inducing function.

Interestingly, grxD was also de-repressed during iron sufficiency in a SreA deficient strain (Fig 8A), suggesting that SreA is a repressor of grxD transcription during iron sufficiency. In agreement, MEME analysis [42] of grxD promoter regions of 20 different Aspergillus species identified the highly conserved motif 5´-ATCWGATAA-3´ (S8 Fig), which was previously shown to be the consensus motif for DNA-binding by SreA [1]. This regulatory pattern is similar to that in S. pombe, since grx4 transcript levels are about 2-fold elevated in iron-starved cells [43], but contrasts the situation in S. cerevisiae because grx4 is here under control of Yap5, which activates grx4 gene expression in iron excess conditions [44].

Previously, HapX was shown to be essential for transcriptional short-term induction of iron-consuming genes [3]. To investigate whether this induction depends on GrxD, we shifted GrxD-depleted cells from iron starvation to iron sufficiency (Fig 8B). Such a shift causes extensive transcriptional rearrangements including repression of iron uptake (mainly via SreA, [1]) and induction of iron-consuming genes (mainly via HapX, [3]). Remarkably, GrxD depletion did not completely block induction of sreA and cccA in this set-up indicating independence of GrxD.

To prove that this induction is not mediated by remaining GrxD protein levels upon GrxD depletion, Northern blot analysis was performed using strain ΔgrxD/ΔsreA, which lacks GrxD and SreA. The shift from iron starvation to iron sufficiency still induced cccA in this mutant, although the response was decreased compared to wt (Fig 8C). cccA is exclusively regulated by HapX [3] and therefore its induction during sFe proves that GrxD is, at least partially, dispensable for HapX function during iron excess. The most likely explanation for the decreased response is the transcriptional downregulation of iron acquisition mechanisms during iron starvation in GrxD-lacking cells (see above), which decreases iron uptake in the iron shift.

In summary, these data indicate that GrxD is required during iron starvation conditions to activate HapX iron starvation function (i.e. repression of iron-consuming genes and induction of iron uptake) and to inactivate SreA function (i.e. repression of iron uptake), but not for iron sensing by HapX under iron excess.

Cysteine 191 is essential for iron sensing

FeS clusters in GrxD homologs are coordinated by C191 in the CGFS motif located in the Grx domain (Fig 1). To analyze the function of this cysteine residue in A. fumigatus iron-regulation, we overexpressed C-terminal venus-tagged grxD-variants (targeted to the pksP locus and expressed under control of the strong constitutive PgpdA promoter of glyceraldehyde-3-phosphate dehydrogenase encoding gene) using PxylP:grxDΔ19 as recipient strain (Fig 9A). This strategy allowed for growth during induction with xylose regardless of the functionality of the pksP-targeted grxD-variant due to grxDΔ19 expression of the endogenous PxylP-controlled grxD gene. Without xylose induction, only the pksP-located version is expressed allowing phenotypical characterization of the pksP-targeted grxD variant.

Fig. 9.

GrxD cysteine residue 191 plays a crucial role in adaptation to iron starvation.

<h2>GrxD cysteine residue 191 plays a crucial role in adaptation to iron starvation.</h2>

(A) Schematic view of strains allowing overexpression (PgpdA promoter) of grxD variants integrated into the pksP locus of strain PxylP:grxDΔ19 (1, 2, 3) as well as strains allowing PgrxD- (4) and PxylP-controlled (5, 6) expression of grxD variants from the endogenous locus (B) Growth of strains 1, 2 and 3 under non-inducing conditions (0% xylose) indicating that C191A conversion is lethal, while C191S conversion enables growth under iron sufficiency but not iron starvation. (C) Overexpression of endogenous grxD was replaced by PxylP-driven grxD C191S variant. Overexpression of GrxD carrying a C191S change (strain 5, 1% xylose) rescued growth under high iron supply but only poorly under iron starvation. (D) Northern analysis demonstrating that GrxD and particularly cysteine residue 191 plays a crucial role in transcriptional adaptation to iron starvation. RNA was isolated from grxDvenus (4), PxylP:grxDvenus (5) and PxylP:grxDvenusC191S (6) after 19h of growth with xylose induction (1%) under iron starvation (-Fe), iron sufficiency (+Fe) and an additional shift for 15 min from iron starvation to iron sufficiency (sFe). Quantification (Tables) was done as described in Fig 3.

Overexpression of grxDC191A was unable to rescue the growth defect caused by lack of GrxD (non-inducing conditions) during iron starvation and iron sufficiency, demonstrating that replacement of cysteine residue 191 by alanine blocks GrxD function (Fig 9B). In contrast, expression of grxDvenusC191S was able to rescue the lack of GrxD during iron sufficiency but not iron starvation (Fig 9B). Similarly, serine can partially compensate for the function of this cysteine residue in the S. cerevisiae GrxD homolog [19,45]. Endogenous (wt) GrxD protein levels are highest under iron starvation (Fig 3B), indicating a higher GrxD requirement under iron starvation, which might explain the lack of compensation by GrxDVenusC191S under this condition. Alternatively, C191 might be particularly important for adaptation to iron starvation. Interestingly, under xylose-inducing conditions (leading to expression of grxDΔ19) overexpression of grxDC191A or grxDC191S decreased growth particularly during iron starvation indicating a dominant negative effect of these GrxD variants.

As overexpression of grxDvenusC191S was partially able to compensate downregulation of grxDΔ19, we generated a mutant strain expressing exclusively PxylP-driven grxDvenusC191S (Fig 9A). Indeed, overexpression (xylose-induction) of grxDvenusC191S also enabled growth in this set-up in an iron supply-dependent manner: wt-like (or even better than wt) growth during high iron conditions, decreased growth during iron sufficiency but only poor growth during iron starvation (Fig 9C), as observed above in PxylP:grxDΔ19/PgpdA:grxDvenusC191S (Fig 9B).

Northern analysis revealed that overexpression of either grxDvenus or grxDvenusC191S increased expression of hapX during iron starvation (Fig 9D). As hapX expression is mainly regulated by SreA repression, these data indicate that overexpression of either grxDvenus or grxDvenusC191S inactivates SreA. In agreement, GrxD deficiency constitutively activated SreA (Fig 8A). Remarkably, overexpression of grxDvenusC191S but not grxDvenus decreased expression of mirB during iron starvation (Fig 9D). This result resembles GrxD deficiency (Fig 8B) and indicates that the residual function of GrxDVenusC191S is not sufficient to maintain the iron-regulatory function under iron starvation. As mirB expression requires not only inactivation of SreA (and SreA is highly inactivated as judged by the hapX expression) but also induction by HapX, these findings indicate that GrxDVenusC191S fails to activate HapX in contrast to GrxDVenus. In contrast to iron starvation, overexpression of grxDvenusC191S or grxDvenus had no significant effect on these genes during iron sufficiency (Fig 9D). Taken together, these data underline the importance of GrxD for sensing of iron starvation.

As shown previously [23] and above (Fig 8B), a short-term shift from iron starvation to iron sufficiency upregulates sreA and cccA. This response was previously shown to be mediated by HapX [3] and does not require GrxD as shown here (Fig 8B and 8C). Remarkably, however, this regulation was blocked by overexpression of GrxDVenus but not GrxDVenusC191S (Fig 9D). As GrxD dimers are capable of [2Fe-2S] cluster coordination, these data might indicate that GrxDVenus but not GrxDVenusC191S competes with HapX for [2Fe-2S] and thereby blocks activation of the high-iron function of HapX. In agreement, a grxDvenus overexpressing strain displayed severe growth deficiencies at excess iron conditions (Fig 2C). The observed difference between GrxDVenus and GrxDVenusC191S in these experiments is most likely based on the decreased [2Fe-2S] binding affinity of GrxDVenusC191S compared to GrxDVenus.

Discussion

Recently, we have shown that iron sensing in A. fumigatus depends on a signal from mitochondrial (ISC) but not on cytosolic (CIA) iron-sulfur cluster biosynthesis and on glutathione biosynthesis [23]. Here we demonstrate that A. fumigatus monothiol glutaredoxin GrxD is required to activate HapX-mediated adaptation to iron starvation as well as for inactivation of SreA during iron starvation. Thereby GrxD acts as sensor for iron starvation, most likely by modulating the signal for iron availability, which is generated by ISC.

GrxD homologs have previously been shown to be involved in iron sensing in the ascomycetous yeast species S. cerevisiae, S. pombe and the basidiomycetous yeast species Cryptococcus neoformans [15,19,46,47]. Yet, these fungal species and the filamentous ascomycete A. fumigatus display significant differences with respect to transcriptional iron regulators and the role of the GrxD homologs.

S. cerevisiae employs two paralogs, Grx3/4, which are essential for growth dependent on the genetic background [19]; in S. pombe, mutants lacking Grx4 are viable only under microaerophilic conditions [43,46]; in C. neoformans, deletion of the entire Grx4 gene but not truncation of the Grx domain is lethal [47]. Here we demonstrate that in A. fumigatus GrxD is essential for growth, whereby the cysteine residue in the Grx domain plays a crucial role, while the Trx domain is dispensable for growth, at least when the Grx domain is overexpressed. As shown for Grx4 in S. cerevisiae [19], GrxD has most likely also a dual function in A. fumigatus: a regulatory role in iron sensing as well as in transport of [2Fe-2S] clusters in cellular metabolism. Moreover, Grx3/4 have been suggested to be involved in stress resistance in S. cerevisiae via affecting actin dynamics and Sir2 glutathionylation [48,49].

In agreement, co-IP approaches revealed physical interaction of GrxD not only with the iron regulators SreA and HapX, but also with CIA components. Likewise, physical interaction of Arabidopsis thaliana GrxD homolog GRXS17 and CIA components has been observed previously [50]. Lethality of lack of GrxD might be a synergistic effect of its dual roles. The fact that we found that lack of SreA suppresses the lethal effect of lack of GrxD and that high iron supplementation suppresses the growth defect caused by GrxD downregulation indicates however that the role in iron sensing is the major reason for its essentiality under standard conditions. Our in vivo approaches indicated that the Trx domain of GrxD is required for interaction with SreA but not HapX. In agreement, in vitro studies with recombinant proteins revealed that neither the Trx domain nor the cysteine residue in CGFS motif in the Grx domain, which is essential for the [2Fe-2S] cluster coordination, are required for physical interaction of GrxD with HapX. Moreover, cysteine residues, which have previously been shown to be essential for in vivo function of HapX under high-iron conditions [3], were found to be dispensable for physical interaction of GrxD with HapX.

The paralogous S. cerevisiae transcription factors mediating adaptation to iron starvation, Aft1/2, are conserved exclusively in closely related Saccharomycotina and do not display any similarity to HapX or SreA. In S. cerevisiae, lack of Grx3/4 results in constitutive activation of Aft1/2 irrespective of the iron status. Thus, Grx3/4 is required for inactivation of Aft1/2 during iron sufficiency [15], i.e. sensing of iron sufficiency. The S. cerevisiae transcription factor mediating adaption to iron excess, Yap5 shows similarities to HapX, but has no function during iron starvation [11]. This indicates that HapX homologs have evolved in a modular manner, whereby A. fumigatus HapX combines protein modules and respective functions for adaption to iron excess from S. cerevisiae Yap5 and functions for adaption to iron starvation from S. pombe Php4 (see below). Similar to Yap5, HapX contains two cysteine-rich regions (CRR), which are crucial for high iron functions [3], whereby one of these contains a perfectly conserved CGFC motif, which was shown to be essential for Yap5 function and [2Fe-2S] cluster coordination [12]. We found in the current study that recombinant HapX displays a reddish-brown color and a UV-Vis spectrum indicative of [2Fe-2S] coordination. Together with our previous observation that activation of the HapX high-iron function depends on ISC but not CIA, our data indicate that HapX senses high iron conditions via [2Fe-2S] coordination similar to Yap5. Remarkably, [2Fe-2S] coordination by Yap5 was shown to be independent of Grx3/4 [12]. Similarly, we also observed that GrxD is dispensable for the activation of the HapX high-iron function in A. fumigatus (Figs 8B and 8C and 10).

The transcription factors maintaining iron homeostasis in S. pombe are termed Fep1 and Php4 [13,51]. Fep1 is a homolog of SreA and shares the same function. The HapX homolog Php4 lacks a bZIP-type DNA-binding region but, similar to HapX, interacts with the Php2/Php3/Php5 CBC via its N-terminal CBC-binding domain resulting in repression of iron-consuming pathways under iron starvation [51]. However, in contrast to HapX, Php4 appears to lack a function in activation of iron acquisition during iron starvation and is not involved in adaptation to iron excess. In agreement, the CRR that are conserved and essential for high-iron functions in S. cerevisiae Yap5 and A. fumigatus HapX are not conserved in Php4. In S. pombe, lack of Grx4 caused constitutive activation of the repressing functions of both Php4 and Fep1 [46], i.e. it caused repression of iron acquisition during iron starvation via Fep1 and repression of iron-consuming pathways during iron sufficiency via Php4 and, therefore, deleterious effects during both iron starvation and sufficiency. This finding contrasts the situation in A. fumigatus, in which lack of GrxD caused regulatory defects only during iron starvation. Thus, GrxD appears to modulate the activity of SreA in A. fumigatus in a similar way as Grx4 affects Fep1 in S. pombe (Fig 10). In contrast to Php4 in S. pombe, however, lack of GrxD did not trigger constitutive HapX iron starvation functions. On the contrary, GrxD depletion impaired HapX mediated adaptation to iron starvation (Fig 10), which indicates significant mechanistic differences in the mode of action of the monothiol glutaredoxin in regulation of S. pombe Php4 and A. fumigatus HapX. In S. pombe, Php4 and Grx4 form a heterodimer, irrespective of the cellular iron status via the Trx domain of Grx4 [32]. During iron sufficiency Php4 and Grx4 are suggested to coordinate a [2Fe-2S] cluster with GSH as additional ligand [16], which causes export from the nucleus to block Php4 activity. In contrast to Php4, HapX appears to coordinate [2Fe-2S] clusters also without GrxD, similar to S. cerevisiae Yap5 (see above). Unlike S. pombe Php4, A. fumigatus HapX also has a function in high-iron conditions and therefore it is unlikely that inactivation of HapX iron-starvation functions (repression of iron-consuming pathways, activation of iron acquisition) involves export of HapX from the nucleus, which could explain evolution of mechanistic differences in modulation of activity of Php4 and HapX.

Fig. 10.

Proposed model for the regulatory function of A. fumigatus GrxD in iron regulation mediated by SreA and HapX.

<h2>Proposed model for the regulatory function of <i>A</i>. <i>fumigatus</i> GrxD in iron regulation mediated by SreA and HapX.</h2>

The two iron-responsive transcription factors SreA and HapX are connected by a negative transcriptional feedback loop. HapX represses sreA during iron deprivation (upper panel) and SreA represses expression of hapX during iron sufficiency (lower panel). In -Fe conditions, HapX represses genes involved in iron-dependent pathways to save iron and activates iron acquisition. Both HapX functions require the HapB/HapC/HapE complex (CCAAT-binding complex) as DNA-binding scaffold, and as shown in this study the monothiol glutaredoxin GrxD that simultaneously activates the HapX iron-starvation function and disables the repressor function of SreA at the post-translational level. Under iron-replete conditions, SreA represses iron acquisition as well as expression of the GrxD-encoding gene. The latter SreA mode of action represents a novel negative feedback-loop between GrxD and SreA, in which SreA represses its own inhibitor because the repressor function of SreA requires FeS cluster incorporation. Notably, GrxD is dispensable for the HapX iron detoxification function as HapX is able to sense iron levels independent of GrxD by FeS cluster incorporation.

C. neoformans employs homologs of A. fumigatus SreA and HapX, termed Cir1 and HapX, respectively [52,53]. In contrast to A. fumigatus SreA, however, Cir1 is also involved in adaptation to iron starvation, e.g. activation of iron acquisition. Recently, the GrxD homologue Grx4 was demonstrated to be essential for activation of Cir1 functions via physical interaction, i.e. lack of GrxD phenocopied lack of Cir1 [47]. This differs from the situation in A. fumigatus, in which lack of GrxD renders SreA constitutively active.

Taken together, the role of GrxD homologs in iron sensing has been demonstrated in different fungal species. In all these species, GrxD homologs display physical interaction with the employed iron regulators. However, these transcription factors show in part significant differences in protein domains and mode of action. These differences are most likely the reason for the different regulatory consequences of lack of GrxD in the analyzed species. Moreover, GrxD homologs show different regulatory patterns in different fungal species. In S. cerevisiae, expression of the Grx3/4-encoding genes is upregulated during iron sufficiency compared to iron starvation, which is mediated by Yap5 [44]. In contrast, in S. pombe and C. neoformans, Grx4 is upregulated during iron starvation compared to iron sufficiency [43,47]. In these species, Grx4 is preferentially located in the nucleus. C. neoformans, Grx4, however, shows increased nuclear localization under iron starvation compared to iron sufficiency [46,47]. For A. fumigatus GrxD we found a similar expression and localization pattern as in C. neoformans. Moreover, we discovered a negative feedback-loop between GrxD and SreA: GrxD is required to repress the function of SreA during iron starvation, while SreA transcriptionally represses expression of the GrxD encoding gene during iron sufficiency (Fig 10).

Iron sensing by S. cerevisiae Aft1/2 and S. pombe Fep1 has been shown to involve not only a GrxD homolog but also a cytosolic BolA2-like protein, termed Fra2. In both organisms Fra2 deficiency resembles Grx3/4 or Grx4 deficiency, i.e. a constitutive increase of iron uptake in S. cerevisiae and constitutive repression of iron uptake in S. pombe [54,55]. Similar to S. cerevisiae and S. pombe [56], the genome of A. fumigatus and other Aspergillus species encodes two BolA-like proteins containing mitochondrial targeting sequences. However, in contrast to S. cerevisiae and S. pombe, Aspergillus spp. appear to lack a cytosolic BolA2-like protein (although dual localization cannot be excluded) indicating another possible difference in the iron sensing apparatus in these molds.

An intriguing question is of course how GrxD mechanistically modulates the function of SreA and HapX. For S. pombe it has been suggested that GrxD signals iron starvation to Fep1 by removing iron, not [2Fe-2S], bound by Fep1 [46]. Later on, it was shown that Fep1 coordinates a [2Fe-2S] cluster, not iron, by a highly conserved CRR [57]. Nevertheless, GrxD-mediated removal of [2Fe-2S] clusters bound by SreA and HapX appears to be a conceivable mode of action for signaling iron starvation. Such a model is supported by the fact that overexpression of grxD impaired adaptation to iron sufficiency, i.e it blocked short-term induction of cccA expression, which depends exclusively on HapX [3]. This effect was not seen when the [2Fe-2S] cluster coordinating cysteine residue in the CGFS motif of GrxD was replaced by a serine residue, which decreases the affinity for the [2Fe-2S] cluster [19]. These data might suggest that in this set-up GrxD competes for [2Fe-2S] clusters with HapX, which impairs iron sensing by HapX. Moreover, this cysteine to serine exchange also impaired transcriptional adaptation to iron starvation, i.e. high-affinity [2Fe-2S] binding by GrxD is crucial for sensing iron starvation. The severe growth defect of downregulation of GrxD in A. fumigatus is likely a combination of deficiencies in iron sensing and [2Fe-2S] transport. Alternative to GrxD-mediated removal of [2Fe-2S] clusters bound by SreA and HapX, GrxD might signal iron starvation in complexes with HapX and SreA by inducing conformational changes upon [2Fe-2S] cluster coordination. Thus, the cytosolic monothiol glutaredoxin GrxD is involved in iron sensing in A. fumigatus as shown previously for other fungal species. However, our studies revealed significant differences in the mode of action of GrxD and the consequences of the lack of GrxD in this mold, which underlines a remarkable plasticity in iron sensing in fungi.

The virulence defect of A. fumigatus mutants lacking siderophore biosynthesis [5860] or HapX [2], as well as the transcriptional upregulation of iron acquisition pathways [61] in murine infection models indicate that A. fumigatus faces iron starvation in vivo. Moreover, plasma was recently shown to inhibit growth of A. fumigatus as long as transferrin was not iron saturated, i.e., in the absence of”non-transferrin bound iron” [62]. In line with A. fumigatus facing iron starvation during growth in plasma we found that GrxD localizes to the nucleus during growth in plasma (S9 Fig) similar to growth during iron starvation in minimal medium (Fig 4). In contrast, supplementation of plasma with high amounts of iron blocked the predominant nuclear localization (S9 Fig) similar to growth under iron sufficiency in minimal medium (Fig 4). Taken together, these data implicate that GrxD plays a role in adaptation to iron starvation during infection. In this regard noteworthy, lack of the Grx domain in the GrxD ortholog renders of C. neoformans avirulent in a murine infection model [47]. Moreover, the essential role of GrxD for viability of A. fumigatus underlines the importance of iron metabolism and homeostasis.

Material and methods

Strains oligonucleotides and growth conditions

Strains used in this study are listed in S2 Table. Oligonucleotides used in this study are listed in S3 Table. Growth assays were performed in Aspergillus minimal medium (1% (w/v) glucose, 20 mM glutamine, salt solution and iron-free trace elements according to [63] and Aspergillus complex medium (2% (w/v) glucose, 0.2% (w/v) peptone, 0.1% (w/v) yeast extract, 0.1% (w/v) casamino acids, salt solution and iron-free trace elements according to [63]. Iron (FeSO4) was added separately as indicated in the respective figures. However, -Fe, +Fe and sFe stands for iron starvation (no iron), 0.03 mM iron, and shift to 0.03 mM iron after precedent iron starvation, respectively. PxylP-driven genes are repressed unless xylose (w/v) is added to the medium, which is indicated in the respective Figures. For solid growth, the medium was solidified with 1.8% (w/v) agarose.

GrxD protein depletion

In phase one, 108 spores of strains of interest were shaken in 50 ml minimal medium +Fe at 25°C with 0.1% (w/v) xylose (inducing conditions to enable GrxDΔ19 production and thereby growth) for 20 h. Germlings were centrifuged and washed once with water to remove iron and xylose before being re-suspended in 100 ml minimal medium containing no xylose. To deplete already produced GrxDΔ19 in phase two, growth was continued for 20 h at 37°C. During phase two, the growth conditions were -Fe, +Fe or sFe. Controls were treated the same way.

Microscopy

For microscopy in minimal medium, strains were grown in well chamber slides (Ibidi) with 2 x 104 spores/well (final concentration 105/ml) for 18h at 37°C with 0.05% (w/v) xylose under iron starvation (-Fe) or iron sufficiency (+Fe). Growth in these chamber slides was hardly sufficient to generate iron starvation after 18h. To increase iron starvation, -Fe media contained 0.5 mM of the ferrous-iron chelator bathophenanthroline disulfonic acid (BPS). For growth in human blood plasma, spores were inoculated in plasma without or with spiking with 0.1 mM iron to override iron starvation. Spore inoculation and incubation was identical to microscopy with minimal medium. Human plasma was obtained from the bloodbank of Medical University Innsbruck and treated as described previously [62].

Mycelia were examined with a spinning-disc confocal microscopic system (Ultra VIEW VoX; PerkinElmer, Waltham, MA) that was connected to a Zeiss AxioObserver Z1 inverted microscope (Zeiss, Oberkochen, Germany). Images were acquired with Volocity software (PerkinElmer) with a 63x oil immersion objective with a numerical aperture of 1.4. The laser wavelengths used for excitation of Venus and mRFP were 488 and 561 nm, respectively

Generation of mutant strains

A schematic overview for the generation of all mutant strains is given in S2 Fig.

PxylP:grxD and PxylP:grxDvenus

To simultaneously exchange the endogenous promoter of grxD and include a Venus-tag, a plasmid containing grxD 5’-region, hph, PxylP, grxD (including 3’-region) and pUC19 backbone was generated. Parts of this plasmid were amplified with primers oKM11-16 and pMMHL15 [23] or A. fumigatus wt gDNA as template and finally assembled with NEBuilder (New England Biolabs) in pUC19 yielding plasmid pKM1. Subsequently pKM1 was linearized with oKM26 and oKM27 to integrate the venus-tag (amplified with oKM28 and oKM29 from phapXVENUS-hph [3]) via seamless cloning (NEBuilder; New England Biolabs) yielding pKM1+venus. The insert of pKM1+venus was amplified with primers oKM11 and oKM16 and transformed into a wt recipient strain via homologous recombination. Thereby endogenous grxD was exchanged. As two possibilities for homologous recombination at the grxD locus were available (S2 Fig), we received two types of transformants, PxylP:grxD and PxylP:grxDvenus.

PxylP:grxDvenusΔtrx

Site-directed mutagenesis (Q5 Site-Directed Mutagenesis Kit; New England Biolabs) was performed with pKM1+venus (see above) and primers oMM182 and oMM184 yielding pMMHL43. The insert was amplified with oKM11 and oKM16 and transformed into a wt recipient strain yielding strain PxylP:grxDvenusΔtrx via homologous recombination at the grxD locus. Thereby endogenous grxD was exchanged.

PxylP:grxDvenus/H2AmRFP and PxylP:grxDvenusΔtrx/H2AmRFP

To integrate mRFP-tagged histone H2A driven by constitutive gpdA promoter, a plasmid containing fragment PgpdA:mRFP:H2A, a phleomycin resistance cassette (ble), a pksP homologous site and pUC19 backbone was generated. Subunits of this plasmid were amplified with primers oMM189-194 and plasmid pME3173 [64], A. fumigatus wt gDNA or pAN8-1 [65], respectively, as template and finally assembled with NEBuilder (New England Biolabs) in pUC19 yielding plasmid pMMHL44. The plasmid was linearized with BamHI and integrated into the pksP locus of recipient strains (PxylP:grxDvenus or PxylP:grxDvenusΔtrx) via homologous recombination at the pksP locus. This gene encodes for a polyketide synthase, which is involved in conidial pigmentation [66]. Disruption of pksP allows for fast screening of positive integrations, as ΔpksP strains produce white conidia.

ΔsreA

To delete sreA, a plasmid containing sreA 5’-region, a pyrithiamine resistance cassette (ptrA), sreA 3’-region and pUC19 backbone was generated. Subunits of this plasmid were amplified with primers oMM164-169 and A. fumigatus wt gDNA or pSK275 (syn. pME3024 [67]) as template and finally assembled with NEBuilder (New England Biolabs) in pUC19 yielding plasmid pMMHL38. The insert of pMMHL38 was amplified with oMM164 and oMM169 and transformed into a wt recipient strain. Thereby sreA was deleted via homologous recombination.

grxDvenus

venus-tagging of grxD was performed by employing CRISPR technology as described previously [68]. We used the hygromycin resistance-mediating AMA-plasmid pFC332 and grxD targeting sequence AGGCTCCTGCCAGCGCTTGA as protospacer sequence, yielding pMMHL49. A repair template was amplified with oKM15 and oKM16 from pKM1+venus (see above). The repair template and pMMHL49 were together transformed into a wt recipient strain. This procedure caused cleavage at the grxD locus by CRISPR and integration of the repair template via homologous recombination. By subsequent growth on non-selective media the CRISPR plasmid was lost yielding grxDvenus, a marker-free strain, in which endogenous grxD is tagged with venus without further manipulation of the grxD locus.

PxylP:grxDΔ19 and PxylP:grxDΔ19sup

The 5’-region of grxD was amplified with primers oAfgrx4-oe1 and oAfgrx4-oe2 and digested with AvrII (fragment A). Truncated grxD was amplified with primers oAfgrx4-oe4 and oAfgrx4-oe5 and digested with NcoI. The PxylP sequence was liberated from plasmid pxylPp [69] by digestion with NotI and NcoI. Both, truncated grxD and PxylP were ligated via their NotI overhang, the fragment was amplified with primers oAfgrx4-oe6 and oAfgrx4-oe7 and digested with XbaI (fragment B). The hygromycin resistance cassette was released from plasmid pAN7-1 by digestion with XbaI and AvrII (fragment C). Fragments A, B and C were ligated via AvrII and XbaI overhangs. The resulting fragment was amplified with primers oAfgrx4-oe3 and Afgrx4-oe8 and integrated into a wt recipient strain via homologous recombination at the grxD locus yielding PxylP:grxDΔ19. Thereby endogenous grxD was exchanged. As grxD is essential (see Results) growth under non-inducing conditions (no xylose) was inhibited. However, streaking out >108 spores on non-inducing agar plates yielded colonies. At least one of these, designated as PxylP:grxDΔ19sup, harbored a mutation suppressing the lethal effect caused by grxD deficiency.

PxylP:grxDvenusΔ19

A construct containing grxD 5’-region, hph, PxylP and the 19 aa truncated version of grxD as 3’-homologous region was amplified from strain PxylP:grxDΔ19 gDNA with primers oAfgrx4-1 and oAfgrx4-oe5 and transformed into grxDvenus as recipient strain via homologous recombination.

PxylP:grxDΔ19/ΔsreA and PxylP:grxDΔ19/ΔhapX

To inactivate sreA or hapX in a PxylP:grxDΔ19 background, the knockout constructs were amplified from ΔsreA or ΔhapX gDNA with primers oMM164 and oMM169 or oAfhapX-1 and oAfhapX-2, respectively, and transformed into a PxylP:grxDΔ19 recipient strain via homologous recombination yielding strains PxylP:grxDΔ19/ΔsreA and PxylP:grxDΔ19/ΔhapX.

Heterokaryon rescue and generation of ΔgrxD/ΔsreA

To inactivate grxD, a plasmid containing grxD 5’-region, hph, grxD 3’-region and pUC19 backbone was generated. Subunits of this plasmid were amplified with primers oMM301-306 and A. fumigatus wt gDNA or pAN7-1 [70] as template and finally assembled with NEBuilder (New England Biolabs) in pUC19 yielding plasmid pMMHL61. The insert of pMMHL61 was amplified with oMM301 and oMM306 and transformed into wt as recipient strain. This procedure yielded heterokaryotic transformants, containing two different nuclei (grxD+hph-; wt; containing grxD but lacking hph and grxD-hph+; ΔgrxD; lacking grxD but containing hph) as described in Results. The amplified cassette was also transformed into ΔsreA as recipient strain. Thereby grxD was deleted via homologous recombination.

PxylP:grxDΔ19/PgpdA:grxDvenus, PxylP:grxDΔ19/PgpdA:grxDvenusC191A and PxylP:grxDΔ19/PgpdA:grxDvenusC191S

To rescue grxD deficiency, a plasmid was generated containing pksP and PgpdA:grxD:venus in backbone PgpdA-lacZ-trpCT-pJET1.2 [71]. The pksP fragment was amplified with oAf-pksP1-f and oAf-pksP2-r and integrated into the HindIII site of PgpdA-lacZ-trpCT-pJET1.2 yielding pMMHL6. Subsequently, pMMHL6 was partially amplified with oMM156_HL6fwd and oMM157_HL6rev and assembled with grxD:venus amplified from pKM1+venus with primers oMM158_grxDfwd and oMM159_venus_rev using NEBuilder (New England Biolabs). The resulting plasmid pMMHL37 was used for site-directed mutagenesis (Q5 Site-Directed Mutagenesis Kit; New England Biolabs) with primers oMM313 and oMM314 or oMM314 and oMM315 to generate pMMHL63 or pMMHL64, respectively. pMMHL37, pMMHL63 and pMMHL64 were linearized with FseI and transformed into PxylP:grxDΔ19 as recipient strain to obtain strains PxylP:grxDΔ19/PgpdA:grxDvenus, PxylP:grxDΔ19/PgpdA:grxDvenusC191A and PxylP:grxDΔ19/PgpdA:grxDvenusC191S via homologous recombination in locus pksP.

PxylP:grxDvenusC191S

To exchange endogenous grxD by a PxylP-driven grxD version in which cysteine 191 is replaced by serine, pKM1+venus was used for site directed mutagenesis (Q5 Site-Directed Mutagenesis Kit; New England Biolabs) with primers oMM313 and oMM314 yielding pMMHL65. The insert was amplified with oKM11 and oKM16 and transformed into a wt recipient strain yielding strain PxylP:grxDvenusC191S via homologous recombination in locus grxD. Thereby endogenous grxD was exchanged.

PgpdA:bol1venus

To constitutively express venus tagged bol1 from the pksP locus, a plasmid was generated consisting of PgpdA-driven bol1 followed by venus assembled in pMMHL37 as backbone. Therefore, bol1 was amplified with primers oMM358 and oMM359 from A. fumigatus wt gDNA and assembled with linearized pMMHL37 (linearized with primers oMM356 and oMM357) in a NEBuilder (New England Biolabs) reaction yielding the final plasmid pMMHL83. This plasmid was subsequently linearized with FseI and integrated into locus pksP via homologous recombination.

Nucleic acid isolation, Northern analysis, Southern analysis

RNA was isolated using TRI Reagents (Sigma) according to the manufacturer’s manual. 10 μg of RNA was used for electrophoresis on 2.2 M formaldehyde agarose gels and subsequently blotted onto Amersham Hybond-N Membranes (ThermoFisher). Transcripts of interest were detected with DIG-labeled probes amplified by PCR.

DNA was isolated by PCI extraction and isopropanol precipitation. To confirm the gene-specific restriction pattern of the genetic manipulations, DNA was digested with restriction enzymes specific for the respective gene. The resulting restriction fragments were separated on an agarose gel and transferred to Amersham Hybond-N Membranes (ThermoFisher) by capillary blotting with NaOH. Signals for correct integration were detected with DIG-labeled probes amplified by PCR.

Rabbit polyclonal antisera against HapX and SreA

Rabbits were immunized with polypeptides corresponding to the amino acid residues of HapX161-491 and SreA308-546. Sequences were PCR-amplified as NdeI-NotI fragments from cDNA and inserted into a pET-21b(+) vector (Novagen) to obtain polypeptides with a C-terminal 6x-His tag. The resulting plasmids were introduced into E. coli Rosetta BL21 cells (Novagen), designed to enhance the expression of eukaryotic proteins that contain codons rarely used in E. coli. Expression was induced for 4 h at 37°C with 0.1 mM isopropyl-β-D-thiogalactopyranoside (IPTG). Proteins were purified from cleared lysates by incubation, 2 h at 4°C, with 0.5 ml of Ni-NTA Agarose Resin (Qiagen). Beads were washed repeatedly with phosphate buffer saline (PBS) containing 75 mM imidazole followed by PBS with 100 mM imidazole before proteins were eluted with 500 mM imidazole. Imidazole was removed by extensive dialysis against PBS. Protein material was lyophilized and used to immunize rabbits (by Davids Biotechnologie GmbH, Regensburg, Germany). The specificity of the obtained antibodies was tested by Western analysis (S10 Fig).

Western analysis (HapX, SreA, GrxDVenus, GrxDVenusΔ19, GrxDVenusΔTrx)

Proteins were extracted using a reported procedure [72] involving solubilization from lyophilized mycelial biomass with NaOH, followed by their precipitation with trichloroacetic acid (TCA). Aliquots were resolved in 10–12% (w/v) SDS-polycrylamide gels and transferred to nitrocellulose membranes. Western blots were reacted with rabbit α-HapX or rabbit α-SreA antiserum (1:20,000), mouse α-GFP antibody (1:10,000; Roche, 11814460001) mouse α‐Tub antibody (1:10,000; Sigma, T6199) as primary antibodies and with peroxidase coupled antibodies as secondary antibodies (1:10,000; anti-Rabbit; Sigma, A1949 or 1:10,000; anti-Mouse; Sigma, A4416). Proteins were detected using Amersham Biosciences ECL.

Co-IP assays

Covalent coupling of rabbit α-HapX respectively rabbit α-SreA antibodies (antiserum) to Protein-A-Sepharose (GE Healthcare) was performed according to [73]. For the negative control IgGs contained in preserum were covalently linked to Protein-A-Sepharose. In short: 1 ml of Protein-A-Sepharose slurry (50%) was mixed with 0.5 ml (anti)serum and treated with 20 mM dimethylpimelidate in 0.2 M Na-tetraborate. The reaction was stopped with 0.2 M ethanolamine. Immunoprecipitation assays were performed according to [74]. Mycelia were grown for 16 h in minimal medium containing 0.1% xylose and no iron supplementation for HapX immunoprecipitation, or 0.03 mM iron for SreA immunoprecipitation. For protein extracts, 40 mg of mycelia were grinded and dissolved in 1 ml protein extraction buffer containing 20 mM Tris-HCl pH 8, 110 mM KCl, 10% (v/v) glycerol, 0.1% (v/v) Triton X-100, 1μl BitNuclease (Biotool) and protease inhibitor (cOmplete ULTRA EDTA-free, Roche). Extracts were mixed with 50 μl of covalently linked rabbit α-HapX, rabbit α-SreA or rabbit preserum beads and incubated for 3h at 4°C in a rotating wheel. Subsequently the beads were washed three times (10 min at 4°C in a rotating wheel) with chilled protein extraction buffer and increasing salt concentrations (110 mM, 500 mM and 750 mM KCl). Bound proteins were eluted in 40 μl of Laemmli sample buffer at 95°C. Twenty microliters of aliquots were resolved in 10% SDS-polyacrylamide gels and transferred to nitrocellulose for Venus detection. Venus tagged GrxD or GrxDΔTrx was detected with mouse α-GFP (1:10,000; Roche, 11814460001) and α‐Tubulin was detected with mouse α‐Tub (1:10,000; Sigma, T6199) as primary antibody and with a peroxidase-coupled secondary antibody (1:10,000; anti-Mouse IgG; Sigma, A4416). HapX respectively SreA were detected with rabbit α-HapX or rabbit α-SreA antisera (1:20,000). To avoid the detection of rabbit IgGs, which were used for the co-IP, a conformation specific anti-Rabbit IgG antibody (1:1000; Cell Signaling Technology, L27A9) was used in combination with a peroxidase-coupled anti-Mouse IgG secondary antibody (1:10,000; Sigma, A4416). For the detection Amersham Biosciences ECL was used.

RACE

3’ RACE was performed using FirstChoice RLM-RACE Kit (ThermoFisher). Total RNA from PxylP:grxDΔ19sup was reverse transcribed with the oligo-dT containing primer 3' RACE Adapter. The resulting cDNA was used for Touchdown PCR with sreA (5’-UTR)-specific forward primer oKM31 and adapter-specific reverse primer 3’ RACE Outer Primer. To increase specificity, the resulting PCR product(s) were amplified in a second PCR with nested primers oKM30 and 3’ RACE Inner Primer. This procedure yielded a fragment (~900bp) which was isolated and sequenced (S3 Fig).

GFP-Trap immunoprecipitation of GrxDVenus and GrxDVenusΔTrx fusion proteins

A. fumigatus mycelia were harvested in Stop buffer [75] at 4°C after growth for 22 h and freeze-dried. Protein extraction was performed according to a modified procedure from [75] using HK buffer for total protein extraction. All steps were carried out at 4°C in the cold room. In short, 100 mg of mycelium powder was dissolved in 1 ml HK buffer, centrifuged twice at 20,187 x g for 15 min and 500 μl of the supernatant was incubated with GFP-Trap agarose beads (ChromoTek) for 1 h. The beads were washed twice in HK buffer without IGPAL, twice in wash buffer (25 mM Tris/HCl pH 7.5, 500 mM NaCl, 5 mM EDTA and 15 mM EGTA) and once in ultrapure water. Proteins were eluted in 10% (v/v) acetonitrile and 5% (v/v) acetic acid and used for nLC-MS/MS measurement, Western blot detection and silver staining.

nLC-MS/MS measurement

In-solution digest

Dried GFP-Trap eluates were solubilized in 50 μl 50 mM NH4HCO3 in 50:50 (v/v) trifluoroethanol (TFE)/water. After heat denaturation (90°C, 10 min) the proteins were reduced for 1 h at 55°C by addition of TCEP (tris(2-carboxyethyl)phosphine) at a final concentration of 8 mM. Further carbamidomethylation was performed for 45 min at 32°C in 15 mM chloroacetamide. Subsequently the samples were evaporated in a vacuum concentrator (Eppendorf) to a residual volume of approximately 5 μl. Finally, the volume was set to 30 μl with 50 mM NH4HCO3 and proteins were digested overnight (18 h, 37°C) with a Trypsin/LysC mixture (Promega) at a protein to protease ratio of 25:1. Peptides were dried in vacuum concentrator and re-solubilized in 20 μl of 0.05% TFA in H2O/acetonitrile 98/2 (v/v) and filtered through spin filters. The filtrate was transferred to HPLC vials and injected into the LC-MS/MS instrument. Each sample was measured in triplicate (3 analytical replicates).

LC-MS/MS analysis

LC-MS/MS analysis was carried out on an Ultimate 3000 nano (n) RSLC system coupled to a QExactive Plus mass spectrometer (both Thermo Fisher Scientific, Waltham, MA, USA). Peptides were trapped for 5 min on an Acclaim Pep Map 100 column (2 cm x 75 μm, 3 μm) at 5 μl/min followed by gradient elution separation on an Acclaim Pep Map RSLC column (50 cm x 75 μm, 2μm). Eluent A (0.1% (v/v) formic acid in water) was mixed with eluent B (0.1% (v/v) formic acid in 90/10 acetonitrile/water) as follows: 0 min at 4% B, 6 min at 6% B, 14 min at 10% B, 20 min at 14% B, 35 min at 20% B, 42 min at 26% B, 46 min at 32% B, 52 min at 42% B, 55 min at 50% B, 58min at 65% B, 60–64.9 min at 96% B, 65–90 min at 4% B. Positively charged ions were generated at 2.2 kV using a stainless steel emitter and a Nanospray Flex Ion Source (Thermo Fisher Scientific). The QExactive Plus was operated in Full MS / data-dependent MS2 (Top10) mode. Precursor ions were monitored at m/z 300–1500 at a resolution of 70,000 FWHM (full width at half maximum) using a maximum injection time (ITmax) of 120 ms and an AGC (automatic gain control) target of 1e6. Precursor ions with a charge state of z = 2–5 were filtered at an isolation width of m/z 1.6 amu for HCD fragmentation at 30% normalized collision energy (NCE). MS2 ions were scanned at 17,500 FWHM (ITmax = 120 ms, AGC = 2e5). Dynamic exclusion of precursor ions was set to 20 s. The LC-MS/MS instrument was controlled by QExactive Plus Tune 2.9 and Xcalibur 3.0 with DCMS Link.

Protein database search

Tandem mass spectra were searched against the Aspergillus Genome Database (AspGD) of Aspergillus fumigatus Af293 (http://www.aspergillusgenome.org/download/sequence/A_fumigatus_ Af293/current/A_fumigatus_Af293_current_orf_trans_all.fasta.gz; 2018/09/18) and the protein sequence of Dre2 (AFUB_008090; the Dre2 ortholog is not present in the Af293 gene annotation) as well as further modified protein sequences (e.g. Venus-tag) using Proteome Discoverer (PD) 2.2 (Thermo) and the algorithms of Sequest HT (version of PD2.2) and MS Amanda 2.0. Two missed cleavages were allowed for the tryptic digestion. The precursor mass tolerance was set to 10 ppm and the fragment mass tolerance was set to 0.02 Da. Modifications were defined as dynamic oxidation of Met, acetylation of Ser, phosphorylation of Ser, Thr, and Tyr and ubiquitination (GG) of Lys as well as static Cys carbamidomethylation. At least two peptides per protein and a strict false discovery rate (FDR) < 1% were required for positive protein hits. The Percolator node of PD2.2 and a reverse decoy database was used for q-value validation of spectral matches. Only rank 1 proteins and peptides of the top scored proteins were counted. The Minora algorithm of PD2.2 was applied for relative label-free quantification. GFP-Trap eluates from wt A. fumigatus mycelial extracts were used for quantification of nonspecifically co-purified proteins.

Silver staining and Western blot detection of proteins after GFP-Trap

Proteins were separated by SDS-PAGE using NuPAGE 4–12% (w/v) Bis-Tris gradient gels (Invitrogen). Silver staining was performed using the SilverQuest Silver Staining Kit (Invitrogen) according to the manufacturer’s protocol. For Western detection, proteins were transferred onto a PVDF membrane using the iBlot 2 dry blotting system (Invitrogen). The membrane was blocked in 3% (w/v) bovine serum albumin (BSA) dissolved in 1x PBST (137 mM NaCl, 2.7 mM KCl, 10 mM Na2HPO4, 2 mM KH2PO4, 0.05% (v/v) Tween 20). As primary antibody rabbit α-GFP (abcam, ab290) was used, followed by secondary antibody HRP-conjugated anti-Rabbit IgG (ICL) incubation. The membrane was developed using the 1-Step Ultra TMB-Blotting chromogenic substrate (Thermo Scientific).

Expression and purification of recombinant GrxD and HapX161-491 proteins from E. coli

For individual expression and protein purification, synthetic genes coding for full-length GrxD and HapX amino acids 161–491 (cysteine-rich C-terminus) were cloned into the NdeI and BamHI sites of the pET-MCN vector pnEA/vH [76] producing C-terminally His6-tagged GrxD (pnEA/vH-GrxD) and HapX161-491 (pnEA/vH-HapX161-491) fused to a TEV cleavage site. For co-expression, the synthetic gene coding for HapX161-491 was initially cloned into the NdeI and BamHI sites of the pET-MCN vector pnCS producing untagged HapX161-491 (pnCS-HapX161-491). Subsequently, the BglII/XbaI fragment from pnCS-HapX161-491 was subcloned into the BglII and SpeI sites of pnEA/vH-GrxD generating a bicistronic expression cassette. Site-directed mutagenesis was performed with the QuikChange II site-directed mutagenesis kit (Agilent) according to the manufacturer’s protocol. Primers used for mutagenesis are listed in S3 Table.

E. coli BL21(DE3) cells (New England Biolabs) were transformed with the respective plasmid for autoinduction in Overnight Express Instant TB medium (Novagen). Wet biomass was harvested by centrifugation (10,543 x g) and the cell paste was stored at -80°C. Frozen bacterial cells were resuspended in lysis buffer (50 mM HEPES pH 8.0, 300 mM NaCl, 2 mM glutathione, 10 mM imidazole, 1 mM AEBSF) and disrupted at 1000 bar using a high-pressure homogenizer (Avestin Emulsiflex C5). Cell debris were removed by centrifugation (48,384 x g), the pH was adjusted to 8.0 and the supernatant clarified by filtration through a 1.2 μm membrane. His6-tagged proteins were then purified by Ni-chelate affinity chromatography using a 20 ml Ni-Sepharose FF column (GE Healthcare) and proteins were eluted with 500 mM imidazole. Fractions containing either HapX161-491-His6 or the HapX161-491/GrxD-His6 complex were digested with TEV protease for 4 h at room temperature and loaded onto a Superdex 200 prep grade 26/60 size exclusion chromatography column (GE Healthcare) that was equilibrated with 25 mM HEPES pH 7.5, 150 mM NaCl, 2 mM glutathione. UV-Vis absorption spectra were recorded in the range from 250 to 550 nm with a JASCO V-630 spectrophotometer.

Supporting information

S1 Fig [a]
Phylogenetic conservation of GrxD.

S2 Fig [tiff]
Schemes of genetic manipulations of . .

S3 Fig [a]
Chromosomal rearrangement within the coding region suppresses lethality of lack of .

S4 Fig [hfe]
Strain : phenocopies strain :.

S5 Fig [tif]
Silver staining and α-GFP Western blot analysis of GFP-Trap affinity purification eluates from . wt, : and : crude cell extracts.

S6 Fig [tmrm]
Bol localizes to mitochondria.

S7 Fig [ip]
GrxD interacts with both HapX and SreA; truncation of the Trx domain impairs interaction with SreA but not with HapX.

S8 Fig [tif]
The promoter contains a highly conserved putative SreA binding motif.

S9 Fig [tiff]
GrxD is enriched in the nucleus during growth in plasma without iron supplementation.

S10 Fig [a]
Rabbit polyclonal antisera against HapX and SreA.

S1 Table [xlsx]
Absolute label-free quantification (LFQ) abundances of proteins identified by nLC-MS/MS analysis after GFP-Trap affinity purification from . wild type, : and : mycelial extracts.

S2 Table [aa]
Strains used in this study.

S3 Table [docx]
Oligonucleotides used in this study.


Zdroje

1. Schrettl M, Kim HS, Eisendle M, Kragl C, Nierman WC, Heinekamp T, et al. SreA-mediated iron regulation in Aspergillus fumigatus. Mol Microbiol 2008;70:27–43. doi: 10.1111/j.1365-2958.2008.06376.x 18721228

2. Schrettl M, Beckmann N, Varga J, Heinekamp T, Jacobsen ID, Jöchl C, et al. HapX-mediated adaption to iron starvation is crucial for virulence of Aspergillus fumigatus. PLoS Pathog 2010;6:e1001124. doi: 10.1371/journal.ppat.1001124 20941352

3. Gsaller F, Hortschansky P, Beattie SR, Klammer V, Tuppatsch K, Lechner BE, et al. The Janus transcription factor HapX controls fungal adaptation to both iron starvation and iron excess. EMBO J 2014;33:2261–76. doi: 10.15252/embj.201489468 25092765

4. Hortschansky P, Haas H, Huber EM, Groll M, Brakhage AA. The CCAAT-binding complex (CBC) in Aspergillus species. Biochim Biophys Acta—Gene Regul Mech 2017;1860:560–70. doi: 10.1016/j.bbagrm.2016.11.008 27939757

5. Schrettl M, Haas H. Iron homeostasis-Achilles’ heel of Aspergillus fumigatus? Curr Opin Microbiol 2011;14:400–5. doi: 10.1016/j.mib.2011.06.002 21724450

6. Outten CE, Albetel A-N. Iron sensing and regulation in Saccharomyces cerevisiae: Ironing out the mechanistic details. Curr Opin Microbiol 2013;16:662–8. doi: 10.1016/j.mib.2013.07.020 23962819

7. Brault A, Mourer T, Labbé S. Molecular basis of the regulation of iron homeostasis in fission and filamentous yeasts. IUBMB Life 2015;67:801–15. doi: 10.1002/iub.1441 26472434

8. Yamaguchi-Iwai Y, Dancis A, Klausner RD. AFT1: a mediator of iron regulated transcriptional control in Saccharomyces cerevisiae. EMBO J 1995;14:1231–9. 7720713

9. Yamaguchi-Iwai Y, Stearman R, Dancis A, Klausner RD. Iron-regulated DNA binding by the AFT1 protein controls the iron regulon in yeast. EMBO J 1996;15:3377–84. 8670839

10. Yun CW, Ferea T, Rashford J, Ardon O, Brown PO, Botstein D, et al. Desferrioxamine-mediated iron uptake in Saccharomyces cerevisiae. Evidence for two pathways of iron uptake. J Biol Chem 2000;275:10709–15. doi: 10.1074/jbc.275.14.10709 10744769

11. Li L, Bagley D, Ward DM, Kaplan J. Yap5 is an iron-responsive transcriptional activator that regulates vacuolar iron storage in yeast. Mol Cell Biol 2008;28:1326–37. doi: 10.1128/MCB.01219-07 18070921

12. Rietzschel N, Pierik AJ, Bill E, Lill R, Mühlenhoff U. The Basic Leucine Zipper Stress Response Regulator Yap5 Senses High-Iron Conditions by Coordination of [2Fe-2S] Clusters. Mol Cell Biol 2015;35:370–8. doi: 10.1128/MCB.01033-14 25368382

13. Pelletier B, Beaudoin J, Mukai Y, Labbé S. Fep1, an Iron Sensor Regulating Iron Transporter Gene Expression in Schizosaccharomyces pombe. J Biol Chem 2002;277:22950–8. doi: 10.1074/jbc.M202682200 11956219

14. Mercier A, Watt S, Bähler J, Labbé S, Bahler J, Labbe S. Key Function for the CCAAT-Binding Factor Php4 To Regulate Gene Expression in Response to Iron Deficiency in Fission Yeast. Eukaryot Cell 2008;7:493–508. doi: 10.1128/EC.00446-07 18223116

15. Poor CB, Wegner S V, Li H, Dlouhy AC, Schuermann JP, Sanishvili R, et al. Molecular mechanism and structure of the Saccharomyces cerevisiae iron regulator Aft2. Proc Natl Acad Sci U S A 2014;111:4043–8. doi: 10.1073/pnas.1318869111 24591629

16. Dlouhy AC, Beaudoin J, Labbé S, Outten CE. Schizosaccharomyces pombe Grx4 regulates the transcriptional repressor Php4 via [2Fe–2S] cluster binding. Metallomics 2017;9:1096–105. doi: 10.1039/c7mt00144d 28725905

17. Chi C-B, Tang Y, Zhang J, Dai Y-N, Abdalla M, Chen Y, et al. Structural and biochemical insights into the multiple functions of yeast Grx3. J Mol Biol 2018. doi: 10.1016/j.jmb.2018.02.024 29524511

18. Herrero E, Ros J, Tamarit J, Bellí G. Glutaredoxins in fungi. Photosynth Res 2006;89:127–40. doi: 10.1007/s11120-006-9079-3 16915356

19. Mühlenhoff U, Molik S, Godoy JR, Uzarska M a., Richter N, Seubert A, et al. Cytosolic monothiol glutaredoxins function in intracellular iron sensing and trafficking via their bound iron-sulfur cluster. Cell Metab 2010;12:373–85. doi: 10.1016/j.cmet.2010.08.001 20889129

20. Lillig CH, Berndt C. Glutaredoxins in Thiol/Disulfide Exchange. Antioxid Redox Signal 2013;18:1654–65. doi: 10.1089/ars.2012.5007 23231445

21. Osmani AH, Oakley BR, Osmani SA. Identification and analysis of essential Aspergillus nidulans genes using the heterokaryon rescue technique. Nat Protoc 2006;1:2517–26. doi: 10.1038/nprot.2006.406 17406500

22. Zadra I, Abt B, Parson W, Haas H. xylP promoter-based expression system and its use for antisense downregulation of the Penicillium chrysogenum nitrogen regulator NRE. Appl Environ Microbiol 2000;66:4810–6. doi: 10.1128/aem.66.11.4810-4816.2000 11055928

23. Misslinger M, Lechner BE, Bacher K, Haas H. Iron-sensing is governed by mitochondrial, not by cytosolic iron-sulfur cluster biogenesis in Aspergillus fumigatus. Metallomics 2018;10:1687–700. doi: 10.1039/c8mt00263k 30395137

24. Rothbauer U, Zolghadr K, Muyldermans S, Schepers A, Cardoso MC, Leonhardt H. A Versatile Nanotrap for Biochemical and Functional Studies with Fluorescent Fusion Proteins. Mol Cell Proteomics 2008;7:282–9. doi: 10.1074/mcp.M700342-MCP200 17951627

25. Netz DJA, Pierik AJ, Stümpfig M, Mühlenhoff U, Lill R. The Cfd1-Nbp35 complex acts as a scaffold for iron-sulfur protein assembly in the yeast cytosol. Nat Chem Biol 2007;3:278–86. doi: 10.1038/nchembio872 17401378

26. Netz DJA, Pierik AJ, Stümpfig M, Bill E, Sharma AK, Pallesen LJ, et al. A bridging [4Fe-4S] cluster and nucleotide binding are essential for function of the Cfd1-Nbp35 complex as a scaffold in iron-sulfur protein maturation. J Biol Chem 2012;287:12365–78. doi: 10.1074/jbc.M111.328914 22362766

27. Zhang Y, Lyver ER, Nakamaru-Ogiso E, Yoon H, Amutha B, Lee D-WD-W, et al. Dre2, a conserved eukaryotic Fe/S cluster protein, functions in cytosolic Fe/S protein biogenesis. Mol Cell Biol 2008;28:5569–82. doi: 10.1128/MCB.00642-08 18625724

28. Netz DJA, Stümpfig M, Doré C, Mühlenhoff U, Pierik AJ, Lill R. Tah18 transfers electrons to Dre2 in cytosolic iron-sulfur protein biogenesis. Nat Chem Biol 2010;6:758–65. doi: 10.1038/nchembio.432 20802492

29. Stehling O, Vashisht A a, Mascarenhas J, Jonsson ZO, Sharma T, Netz DJ a, et al. Metabolism and Genomic Integrity 2012;337:195–9. doi: 10.1126/science.1219723.MMS19

30. Balk J, Pierik AJ, Netz DJA, Mühlenhoff U, Lill R. The hydrogenase-like Nar1p is essential for maturation of cytosolic and nuclear iron-sulphur proteins. EMBO J 2004;23:2105–15. doi: 10.1038/sj.emboj.7600216 15103330

31. Jbel M, Mercier A, Labbé S. Grx4 monothiol glutaredoxin is required for iron limitation-dependent inhibition of fep1. Eukaryot Cell 2011;10:629–45. doi: 10.1128/EC.00015-11 21421748

32. Vachon P, Mercier A, Jbel M, Labbé S. The monothiol glutaredoxin Grx4 exerts an iron-dependent inhibitory effect on Php4 function. Eukaryot Cell 2012;11:806–19. doi: 10.1128/EC.00060-12 22523368

33. Wiemann P, Perevitsky A, Lim FY, Shadkchan Y, Knox BP, Landero Figueora JA, et al. Aspergillus fumigatus Copper Export Machinery and Reactive Oxygen Intermediate Defense Counter Host Copper-Mediated Oxidative Antimicrobial Offense. Cell Rep 2017;19:1008–21. doi: 10.1016/j.celrep.2017.04.019 28467895

34. Zhou S, Narukami T, Masuo S, Shimizu M, Fujita T, Doi Y, et al. NO-inducible nitrosothionein mediates NO removal in tandem with thioredoxin. Nat Chem Biol 2013;9:657–63. doi: 10.1038/nchembio.1316 23955366

35. Uzarska MA, Nasta V, Weiler BD, Spantgar F, Ciofi-Baffoni S, Saviello MR, et al. Mitochondrial Bol1 and Bol3 function as assembly factors for specific iron-sulfur proteins. Elife 2016;5:e16673. doi: 10.7554/eLife.16673 27532772

36. Yu H, Braun P, Yildirim MA, Lemmens I, Venkatesan K, Sahalie J, et al. High-Quality Binary Protein Interaction Map of the Yeast Interactome Network. Science (80-) 2008;322:104–10. doi: 10.1126/science.1158684 18719252

37. Rey P, Taupin-Broggini M, Couturier J, Vignols F, Rouhier N. Is There a Role for Glutaredoxins and BOLAs in the Perception of the Cellular Iron Status in Plants? Front Plant Sci 2019;10:712. doi: 10.3389/fpls.2019.00712 31231405

38. Li H, Mapolelo DT, Randeniya S, Johnson MK, Outten CE. Human glutaredoxin 3 forms [2Fe-2S]-bridged complexes with human BolA2. Biochemistry 2012;51:1687–96. doi: 10.1021/bi2019089 22309771

39. Freibert SA, Weiler BD, Bill E, Pierik AJ, Mühlenhoff U, Lill R. Biochemical Reconstitution and Spectroscopic Analysis of Iron–Sulfur Proteins. Methods Enzymol., vol. 599, 2018, p. 197–226. doi: 10.1016/bs.mie.2017.11.034 29746240

40. Ojeda L, Keller G, Muhlenhoff U, Rutherford JC, Lill R, Winge DR. Role of glutaredoxin-3 and glutaredoxin-4 in the iron regulation of the Aft1 transcriptional activator in Saccharomyces cerevisiae. J Biol Chem 2006;281:17661–9. doi: 10.1074/jbc.M602165200 16648636

41. Kim K-D, Kim H-JJ, Lee K-C, Roe J-H. Multi-domain CGFS-type glutaredoxin Grx4 regulates iron homeostasis via direct interaction with a repressor Fep1 in fission yeast. Biochem Biophys Res Commun 2011;408:609–14. doi: 10.1016/j.bbrc.2011.04.069 21531205

42. Bailey TL, Boden M, Buske FA, Frith M, Grant CE, Clementi L, et al. MEME SUITE: tools for motif discovery and searching. Nucleic Acids Res 2009;37:W202–8. doi: 10.1093/nar/gkp335 19458158

43. Mercier A, Labbé S. Both Php4 Function and Subcellular Localization Are Regulated by Iron via a Multistep Mechanism Involving the Glutaredoxin Grx4 and the Exportin Crm1. J Biol Chem 2009;284:20249–62. doi: 10.1074/jbc.M109.009563 19502236

44. Pimentel C, Vicente C, Menezes RA, Caetano S, Carreto L, Rodrigues-Pousada C. The role of the Yap5 transcription factor in remodeling gene expression in response to Fe bioavailability. PLoS One 2012;7:e37434. doi: 10.1371/journal.pone.0037434 22616008

45. Johnson DC, Dean DR, Smith AD, Johnson MK. Structure, Function, and Formation of Biological Iron-Sulfur Clusters. Annu Rev Biochem 2005;74:247–81. doi: 10.1146/annurev.biochem.74.082803.133518 15952888

46. Encinar del Dedo J, Gabrielli N, Carmona M, Ayté J, Hidalgo E. A Cascade of Iron-Containing Proteins Governs the Genetic Iron Starvation Response to Promote Iron Uptake and Inhibit Iron Storage in Fission Yeast. PLOS Genet 2015;11:e1005106. doi: 10.1371/journal.pgen.1005106 25806539

47. Attarian R, Hu G, Sánchez-León E, Caza M, Croll D, Do E, et al. The Monothiol Glutaredoxin Grx4 Regulates Iron Homeostasis and Virulence in Cryptococcus neoformans. MBio 2018;9:e02377–18. doi: 10.1128/mBio.02377-18 30514787

48. Pujol-Carrion N, De La Torre-Ruiz MA. Glutaredoxins Grx4 and Grx3 of Saccharomyces cerevisiae play a role in actin dynamics through their trx domains, which contributes to oxidative stress resistance. Appl Environ Microbiol 2010;76:7826–35. doi: 10.1128/AEM.01755-10 20889785

49. Vall-llaura N, Reverter-Branchat G, Vived C, Weertman N, Rodríguez-Colman MJ, Cabiscol E. Reversible glutathionylation of Sir2 by monothiol glutaredoxins Grx3/4 regulates stress resistance. Free Radic Biol Med 2016;96:45–56. doi: 10.1016/j.freeradbiomed.2016.04.008 27085841

50. Inigo S, Nagels Durand A, Ritter A, Le Gall S, Termathe M, Klassen R, et al. Glutaredoxin GRXS17 Associates with the Cytosolic Iron-Sulfur Cluster Assembly Pathway. Plant Physiol 2016;172:858–73. doi: 10.1104/pp.16.00261 27503603

51. Mercier A, Pelletier B, Labbe S. A transcription factor cascade involving Fep1 and the CCAAT-binding factor Php4 regulates gene expression in response to iron deficiency in the fission yeast Schizosaccharomyces pombe. Eukaryot Cell 2006;5:1866–81. doi: 10.1128/EC.00199-06 16963626

52. Jung WH, Sham A, White R, Kronstad JW. Iron Regulation of the Major Virulence Factors in the AIDS-Associated Pathogen Cryptococcus neoformans. PLoS Biol 2006;4:e410. doi: 10.1371/journal.pbio.0040410 17121456

53. Jung WH, Saikia S, Hu G, Wang J, Fung CK, D’Souza C, et al. HapX Positively and Negatively Regulates the Transcriptional Response to Iron Deprivation in Cryptococcus neoformans. PLoS Pathog 2010;6:e1001209. doi: 10.1371/journal.ppat.1001209 21124817

54. Li H, Mapolelo DT, Dingra NN, Keller G, Riggs-Gelasco PJ, Winge DR, et al. Histidine 103 in Fra2 Is an Iron-Sulfur Cluster Ligand in the [2Fe-2S] Fra2-Grx3 Complex and Is Required for in Vivo Iron Signaling in Yeast. J Biol Chem 2011;286:867–76. doi: 10.1074/jbc.M110.184176 20978135

55. Jacques J-F, Mercier A, Brault A, Mourer T, Labbé S. Fra2 Is a Co-Regulator of Fep1 Inhibition in Response to Iron Starvation. PLoS One 2014;9:e98959. doi: 10.1371/journal.pone.0098959 24897379

56. Li H, Outten CE. Monothiol CGFS glutaredoxins and BolA-like proteins: [2Fe-2S] binding partners in iron homeostasis. Biochemistry 2012;51:4377–89. doi: 10.1021/bi300393z 22583368

57. Kim H-J, Lee K-L, Kim K-D, Roe J-H. The iron uptake repressor Fep1 in the fission yeast binds Fe-S cluster through conserved cysteines. Biochem Biophys Res Commun 2016;478:187–92. doi: 10.1016/j.bbrc.2016.07.070 27444384

58. Schrettl M, Bignell E, Kragl C, Joechl C, Rogers T, Arst HN, et al. Siderophore biosynthesis but not reductive iron assimilation is essential for Aspergillus fumigatus virulence. J Exp Med 2004;200:1213–9. doi: 10.1084/jem.20041242 15504822

59. Schrettl M, Bignell E, Kragl C, Sabiha Y, Loss O, Eisendle M, et al. Distinct Roles for Intra- and Extracellular Siderophores during Aspergillus fumigatus Infection. PLoS Pathog 2007;3:e128. doi: 10.1371/journal.ppat.0030128 17845073

60. Yasmin S, Alcazar-Fuoli L, Gründlinger M, Puempel T, Cairns T, Blatzer M, et al. Mevalonate governs interdependency of ergosterol and siderophore biosyntheses in the fungal pathogen Aspergillus fumigatus. Proc Natl Acad Sci U S A 2012;109:E497–504. doi: 10.1073/pnas.1106399108 22106303

61. McDonagh A, Fedorova ND, Crabtree J, Yu Y, Kim S, Chen D, et al. Sub-Telomere Directed Gene Expression during Initiation of Invasive Aspergillosis. PLoS Pathog 2008;4:e1000154. doi: 10.1371/journal.ppat.1000154 18787699

62. Petzer V, Wermke M, Tymoszuk P, Wolf D, Seifert M, Ovaçin R, et al. Enhanced labile plasma iron in hematopoietic stem cell transplanted patients promotes Aspergillus outgrowth. Blood Adv 2019;3:1695–700. doi: 10.1182/bloodadvances.2019000043 31167821

63. Pontecorvo G, Roper JA, Hemmons LM, Macdonald KD, Bufton AWJ. The genetics of Aspergillus nidulans. Adv Genet 1953;5:141–238. 13040135

64. Bayram O, Krappmann S, Ni M, Bok JW, Helmstaedt K, Valerius O, et al. VelB/VeA/LaeA complex coordinates light signal with fungal development and secondary metabolism. Science 2008;320:1504–6. doi: 10.1126/science.1155888 18556559

65. Mattern IE, Punt PJ, Van den Hondel CAMJJ. A vector for Aspergillus transformation conferring phleomycin resistance. Fungal Genet Rep 1988;35:25. doi: 10.4148/1941-4765.1533

66. Langfelder K, Jahn B, Gehringer H, Schmidt A, Wanner G, Brakhage AA. Identification of a polyketide synthase gene (pksP) of Aspergillus fumigatus involved in conidial pigment biosynthesis and virulence. Med Microbiol Immunol 1998;187:79–89. 9832321

67. Krappmann S, Jung N, Medic B, Busch S, Prade RA, Braus GH. The Aspergillus nidulans F-box protein GrrA links SCF activity to meiosis. Mol Microbiol 2006;61:76–88. doi: 10.1111/j.1365-2958.2006.05215.x 16824096

68. Nødvig CS, Nielsen JB, Kogle ME, Mortensen UH. A CRISPR-Cas9 system for genetic engineering of filamentous fungi. PLoS One 2015;10:1–18. doi: 10.1371/journal.pone.0133085 26177455

69. Gsaller F, Eisendle M, Lechner BE, Schrettl M, Lindner H, Müller D, et al. The interplay between vacuolar and siderophore-mediated iron storage in Aspergillus fumigatus. Metallomics 2012;4:1262–70. doi: 10.1039/c2mt20179h 23151814

70. Punt PJ, Oliver RP, Dingemanse MA, Pouwels PH, van den Hondel CA. Transformation of Aspergillus based on the hygromycin B resistance marker from Escherichia coli. Gene 1987;56:117–24. doi.org/10.1016/0378-1119(87)90164-8 2824287

71. Gressler M, Zaehle C, Scherlach K, Hertweck C, Brock M. Multifactorial Induction of an Orphan PKS-NRPS Gene Cluster in Aspergillus terreus. Chem Biol 2011;18:198–209. doi: 10.1016/j.chembiol.2010.12.011 21236704

72. Hervás-Aguilar A, Peñalva MA. Endocytic Machinery Protein SlaB Is Dispensable for Polarity Establishment but Necessary for Polarity Maintenance in Hyphal Tip Cells of Aspergillus nidulans. Eukaryot Cell 2010;9:1504–18. doi: 10.1128/EC.00119-10 20693304

73. Harlow E, Lane DP. Antibodies: A Laboratory Manual. Cold Spring Harbor Laboratory Press; 1988.

74. López-Berges MS, Pinar M, Abenza JF, Arst HN, Peñalva MA. The Aspergillus nidulans syntaxin PepAPep12 is regulated by two Sec1/Munc-18 proteins to mediate fusion events at early endosomes, late endosomes and vacuoles. Mol Microbiol 2016;99:199–216. doi: 10.1111/mmi.13226 26395371

75. Liu H-L, Osmani AH, Ukil L, Son S, Markossian S, Shen K-F, et al. Single-step affinity purification for fungal proteomics. Eukaryot Cell 2010;9:831–3. doi: 10.1128/EC.00032-10 20363899

76. Diebold M-L, Fribourg S, Koch M, Metzger T, Romier C. Deciphering correct strategies for multiprotein complex assembly by co-expression: application to complexes as large as the histone octamer. J Struct Biol 2011;175:178–88. doi: 10.1016/j.jsb.2011.02.001 21320604

Štítky
Genetika Reprodukční medicína

Článek vyšel v časopise

PLOS Genetics


2019 Číslo 9
Nejčtenější tento týden
Nejčtenější v tomto čísle
Kurzy

Zvyšte si kvalifikaci online z pohodlí domova

Důležitost adherence při depresivním onemocnění
nový kurz
Autoři: MUDr. Eliška Bartečková, Ph.D.

Koncepce osteologické péče pro gynekology a praktické lékaře
Autoři: MUDr. František Šenk

Sekvenční léčba schizofrenie
Autoři: MUDr. Jana Hořínková, Ph.D.

Hypertenze a hypercholesterolémie – synergický efekt léčby
Autoři: prof. MUDr. Hana Rosolová, DrSc.

Multidisciplinární zkušenosti u pacientů s diabetem
Autoři: Prof. MUDr. Martin Haluzík, DrSc., prof. MUDr. Vojtěch Melenovský, CSc., prof. MUDr. Vladimír Tesař, DrSc.

Všechny kurzy
Přihlášení
Zapomenuté heslo

Zadejte e-mailovou adresu, se kterou jste vytvářel(a) účet, budou Vám na ni zaslány informace k nastavení nového hesla.

Přihlášení

Nemáte účet?  Registrujte se

#ADS_BOTTOM_SCRIPTS#