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Article

mRNA Turnover Protein 4 Is Vital for Fungal Pathogenicity and Response to Oxidative Stress in Sclerotinia sclerotiorum

by
Chenghuizi Yang
1,2,†,
Lan Tang
2,†,
Lei Qin
1,2,
Weiping Zhong
1,2,
Xianyu Tang
1,2,
Xin Gong
1,2,
Wenqi Xie
2,
Yifu Li
1,2 and
Shitou Xia
1,2,*
1
Hunan Provincial Key Laboratory of Phytohormones and Growth Development, Hunan Agricultural University, Changsha 410128, China
2
College of Bioscience and Biotechnology, Hunan Agricultural University, Changsha 410128, China
*
Author to whom correspondence should be addressed.
These authors contributed equally to this work.
Pathogens 2023, 12(2), 281; https://doi.org/10.3390/pathogens12020281
Submission received: 19 January 2023 / Revised: 2 February 2023 / Accepted: 6 February 2023 / Published: 8 February 2023
(This article belongs to the Special Issue Plant Pathogenic Fungi)
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Abstract

:
Ribosome assembly factors have been extensively studied in yeast, and their abnormalities may affect the assembly process of ribosomes and cause severe damage to cells. However, it is not clear whether mRNA turnover protein 4 (MRT4) functions in the fungal growth and pathogenicity in Sclerotinia sclerotiorum. Here, we identified the nucleus-located gene SsMRT4 using reverse genetics, and found that knockdown of SsMRT4 resulted in retard mycelia growth and complete loss of pathogenicity. Furthermore, mrt4 knockdown mutants showed almost no appressorium formation and oxalic acid production comparing to the wild-type and complementary strains. In addition, the abilities to ROS elimination and resistance to oxidative and osmotic stresses were also seriously compromised in mrt4 mutants. Overall, our study clarified the role of SsMRT4 in S. sclerotiorum, providing new insights into ribosome assembly in regulating pathogenicity and resistance to environmental stresses of fungi.

1. Introduction

A eukaryotic ribosome, which is considered the “factory” for protein synthesis, is composed of one large (60S) and one small (40S) subunit and a variety of ribosomal proteins (r-proteins). The assembly of ribosomes is a highly precise, strictly regulated process that requires energy consumption and involves a series of factors [1,2,3,4]. There are more than 200 types of eukaryotic ribosome assembly factors, including r-proteins, protein complexes and small nucleolar ribonucleoproteins, which can play a role in different stages such as processing, early assembly, nucleolar to nucleocytoplasmic transport, nuclear remodeling, nucleocytoplasmic transport and ribosome maturation [4]. The abnormal function of ribosome assembly factors may affect the maturation, release, transport and final assembly of ribosome subunits, resulting in serious ribosomopathies and severe damage to cells [5]. Many ribosome assembly factors have been identified in yeast, and their defects will lead to a series of cell metabolism and development abnormalities [6,7,8,9]. Moreover, the deletion of BcNop53 significantly inhibited its growth and virulence in Botrytis cinerea [10]. In Magnaporthe oryzae, the ribosome assembly factor MoFap7 is also involved in mycelial growth and virulence production [11].
mRNA turnover protein 4 (MRT4) is considered to be a transacting factor of ribosome assembly and plays an important role in the maturation of pro-60S subunits of eukaryotic ribosomes. In addition, it also participates in intracellular mRNA turnover [12,13,14,15]. MRT4 was first found during the screening of a yeast mRNA turnover protein, and its mutation causes an mRNA decay defect [15]. Later on, MRT4 was also found in ribosome precursor, which was believed to function in ribosome assembly and maturation [16]. At the initial stage of ribosome assembly, MRT4 and Rpl12 form a complex and anchor together on the ribosome stem ring, affecting the assembly of the ribosome stem [17]. As a collateral homolog of r-protein P0, MRT4 successively interacts with the GAR domain of 25S rRNA, and the replacement process mainly occurs in the cytoplasm [13,18]. Pre-rRNA processing factor Nop53 can target MRT4, participating in the regulation of ribosome assembly [10]. In addition, MRT4 plays an important role in cell tolerance in yeast [19]. The loss of AtRDP1 (the homolog of MRT4) could decrease the amount of pollen in Arabidopsis thaliana and inhibit its development, possibly due to ribosome specialization [20]. It was shown that the subcellular localization of human MRT4 is regulated by the C-terminal region under stress [21]. MRT4 was significantly up-regulated within 15 min when screening the possible genes related to the drug resistance of Candida albicans [22], indicating that it may regulate the effectiveness of drugs.
Sclerotinia sclerotiorum (Lib.) de Bary, as a pathogenic fungus with a wide host range, mainly colonizes dicotyledons and can seriously interfere with the growth and development of plants [23,24,25,26]. At present, the main method of controlling S. sclerotiorum is chemical insecticide control, not only pollutes the environment but also has a poor control effect. With the continuous development of technology, an increasing number of biological control methods have been applied in practice [27,28]. Research on the growth and pathogenesis of S. sclerotiorum is conducive to exploring more efficient and environmentally friendly control measures. Most studies of S. sclerotiorum focus on its growth and development, oxalic acid synthesis, and secreted proteins [29,30,31]. Recently, research of mycoviruses (or fungal viruses) has gradually increased [32,33,34]; the open reading frame Ι of SsNSRV-1 influences the growth of mycelia and generation of virulence by regulating host protein synthesis pathways [34]. However, it is not clear whether and how ribosome assembly regulates fungal development and infection in hosts.
In this study, SS1G_11436, which was predicted to be a ribosomal protein, was identified as SsMRT4 in S. sclerotiorum. In order to explore the role of SS1G_11436, the main focus of our study is to clarify the biological effects of SsMRT4 through reverse genetics and provide bases for subsequent research on ribosomal proteins and the comprehensive control of S. sclerotiorum. The results show that the mycelia growth of Ssmrt4 knockdown strains was slow, and more sensitive to stresses. Most importantly, the pathogenicity was completely lost with no appressorium formation and less oxalic acid production in mutant strains, suggesting that SsMRT4 plays a significant role in the formation of appressorium and pathogenicity as well as resistance to oxidative stress in S. sclerotiorum.

2. Materials and Methods

2.1. Fungal Strains and Culture Conditions

A wild-type strain was cultivated on potato dextrose agar (PDA), the knockdown mutants were cultured on PDA with 200 μg/mL hygromycin B (Roche), and the complemented strains were subcultured on PDA with 75 μg/mL G418 Sulfate (Geneticin) (Yeasen). All of them were cultured in an incubator maintained at 20 °C for daily storage.

2.2. Plant Materials and Growth Conditions

Seedlings of A. thaliana or N. benthamiana used in the experiments were cultured in artificial climate chamber at 22 °C with a treatment of 16 h of light exposure and 8 h of darkness; four-week-old plants were used for further tests.

2.3. Identification and Sequence Analysis of SsMRT4

The MRT4 sequences of S. cerevisiae (YKL009W), Fusarium oxysporum Fo47 (EWZ44016.1), Verticillium dahliae (XP_009653586.1, RBQ98059.1, PNH42533.1), B. cinerea B05.10 (BCIN_08g05250), Pyricularia oryzae 70-15 (XP_003713937.1), S. sclerotiorum (SS1G_11436), and Stagonospora sp. SRC1lsM3a (OAK93896.1) were downloaded from the NCBI database. Multiple sequence alignment of the MRT4 protein sequences was carried out by MEGA7.0 software, and then the neighbor-joining (NJ) method was used to construct a phylogenetic tree. Bootstrap was set to 1000. Protein sequence IDs are shown in the phylogenetic tree. The domains contained in the sequence were analyzed by PredictProtein (https://predictprotein.org/ accessed on 16 February 2022).

2.4. Acquisition of Knockdown Mutants and Complementary Strain

The SsMRT4 gene was knocked down from the genome of S. sclerotiorum using the split-marking approach. Primers: ss07gUPF (GACACCTCCCGATTTATTCA)/UR: ss07gUPR (GTGCTCCTTCAATATCATCTTCTCGAGCTTGCGATAGGTAGTG) were designed to amplify nearly 1000 bp of 5′ upstream region of SsMRT4. Primers: ss07g DF (CTTGTTTAGAGGTAATCCTTCTTTTTTCCTGAGTGCTATGCC)/DR: ss07g DR (CGGTTACGCATTTGTTGTT) were designed to amplify the 3′ downstream region of SsMRT4 with nearly 1500 bp. Fragment 1 was composed of the 5′ upstream region of SsMRT4 and 5′ part of hygromycin phosphotransferase cassette, and fragment 2 was composed of the 3′ downstream region of SsMRT4 and 3′ part of hygromycin phosphotransferase cassette. These two fragments were then inserted into the T-vector (pEASY®-Blunt Cloning Kit, TransGen, Beijing, China). The resulting vector, T-MRT4 was used as a template to amplify two split-marker fragments using primers: ss07g UPF(GACACCTCCCGATTTATTCA)/HY-R (AAATTGCCGTCAACCAAGCTC) and YG-F (TTTCAGCTTCGATGTAGGAGG)/ss07g DR(CGGTTACGCATTTGTTGTT). These two fragments were co-transformed into wild-type Sclerotinia protoplasts, which could overlap in the hygromycin resistance gene fragment [35]. Primers ss07g UPF(GTCTACCTCGTCAAGTCTCCA) and ss07g DR (GGACCTATTGAAAGAGTGCG) were used to test whether the SsMRT4 gene was replaced by the hygromycin-resistant gene. Transformants were purified by hyphal tip transfer at least 3 times. An amplified full-length SsMRT4 sequence was used to verify mutant strains.
Since we used a split-marker method to generate mutants, in which the target gene was replaced by a hygromycin-resistant gene on site. The mutant is hygromycin-resistant, which may cause difficulties in the subsequent screening of complementary strains if the antibiotic of a complementary vector is also hygromycin. Thus, to reduce the false-positive rate and improve screening efficiency, we changed the hygromycin resistance of the restorer vector pCH-EF-1 (shared by D. Jiang from Huazhong Agricultural University) to G418 Sulfate (Geneticin), named pCH-EF-neo. For ΔSsMRT4 complementation, the binary vector pCH-EF-neo-MRT4 was constructed using the backbone of pCH-EF-neo. The full-length SsMRT4 gene, including the promoter and coding sequence (CDS), was amplified from WT genomic DNA. Full-length SsMRT4 gene fragment and pCH-EF-neo vector were digested using restriction enzyme XhoI and SacI, then linked by homologous recombinase (ClonExpress® II One Step Cloning Kit, Vazyme, Nanjing, China) to generate the pCH-EF-neo-MRT4 construct. Then, the plasmid was used for SsMRT4 transformation via the polyethylene glycol (PEG)-mediated transformation method [35,36].

2.5. Analysis of Pathogenecity

To determine pathogenicity, small pieces of mycelia were taken from the edge of PDA medium containing wild-type, Ssmrt4-3 and SsMRT4-C strains with 2 mm pieces for A. thaliana and 5 mm pieces for N. benthamiana. Lesion areas were measured 36 h later and counted with Image J. Each experiment was repeated at least three times, and two leaves were used per experiment. The data were analyzed by using SPSS Statistics v.24.0 (IBM, Armonk, NY, USA).

2.6. Compound Appressoria Observation and OA Analysis

A 5 mm mycelia plug of S. sclerotiorum was placed on a glass slide and cultured for 24 h to observe the formation and number of appressoria. Samples were examined and photographed under stereo microscopes (Stemi508, ZEISS, Oberkochen, Germany) and a light microscope (Axio Imager 2, ZEISS, Oberkochen, Germany). After 16 h of inoculation with S. sclerotiorum, onion epidermis was soaked in 0.5% trypan blue solution for 30 min and then decolorized using bleaching solution (ethanol:acetic acid:glycerol = 3:1:1). Samples were examined and photographed under the light microscope (Axio Imager 2, ZEISS).
S. sclerotiorum was inoculated on PDA medium containing 100 μg/mL bromophenol blue to detect whether it secreted oxalic acid.

2.7. RT-qPCR Analysis

To evaluate the SsMRT4 expression levels during mycelia development, wild-type strains were cultured on cellophane over PDA, and hyphae were harvested at 1 and 2 days post inoculation (dpi) (hyphae), 3 and 4 dpi (initial sclerotia), 5~7 dpi (developing sclerotia), and 15 dpi (mature sclerotia). Primers of SsMRT4 and β-tub-ulin used for qPCR were: SsMRT4qF (CCTCCATCATCACCTACTTCC)/SsMRT4 qR: (GGTTCCAAACTAT GTGCCATT) and SsTubqF (ACCTCCATCCAAGAACTC)/SsTubqR (GAACTCCAT CTCGTCCAT). β-tubulin was used as an internal reference. The program setting included holding stage (95 °C, 2 min), cycling stage (95 °C, 20 s; 55 °C, 20 s; 72 °C, 20 s; 40 cycles), and melt curve stage (95 °C, 15 s; 60 °C, 1 min). Quantitative expression assays were performed using SYBR® Green Premix Pro Taq HS qPCR Kit II (Accurate Biology) with StepOneTM Real-time PCR Instrument Thermal Cycling Block. The transcript level of the gene of interest was calculated from the threshold cycle using the 2-ΔΔCT method [37] with three replicates, and data were analyzed using SPSS Statistics v.24.0.

2.8. DAB Staining

Using a sterile punch (5 mm), the mycelia-colonized plugs were punched out from the WT, Ssmrt4-3 and SsMRT4-C1 strains of S. sclerotiorum (5 pieces each) and placed separately in 5 mL centrifugal tube. Next, 2 mL of 1 mg/mL DAB solution was added into each centrifugal tube, and then the samples were incubated for 30 min at 22 °C in the dark, and immediately photographed (Stemi 508, ZEISS).

2.9. Abiotic Stress Response

To test the response of Ssmrt4-3 to cell integrity and different stress, WT, Ssmrt4-3 and SsMRT4-C1 strains were grown on PDA medium with 0.02% SDS, 1 Glucose, 1 M sorbitol, 1 M KCl, 1 M NaCl and H2O2 (2.5, 5 and 7.5 mM), respectively. After 48 h, the diameter and growth inhibition rate of mycelia were measured: Inhibition rate (%) = 100 × (colony diameter of strain on pure PDA—colony diameter of strain with different stress)/(colony diameter of strain on pure PDA).

2.10. Subcellular Localization of SsMRT4

To test the subcellular localization of SsMRT4 in N. benthamiana, an SsMRT4-eGFP fusion gene driven by a 35S promoter was used for subcellular localization observation. The SsMRT4-eGFP constructs were transformed using Agrobacterium GV3101-mediated transformation. The Agrobacterium strains harboring the constructs were used to infiltrate lower epidermal cells of four-week-old N. benthamiana leaves [38]. Leaves were examined 48–72 h after infiltration using a Zeiss LSM710 fluorescence microscope. 4′,6-Diamidino-2-phenylindole (DAPI) was used as a nuclear marker. We applied DAPI staining on leaves for 15 min at room temperature. The excitation and emission wavelengths for DAPI were 385 and 420 nm, respectively; and 470–490nm and 500–540 nm for eGFP, respectively.

3. Results

3.1. Identification of MRT4 in S. sclerotiorum

When SsMRT4 was used as a query sequence to search for homologs in NCBI database, only one candidate gene (SS1G_11436) was identified in S. sclerotiorum (Figure 1A). SS1G_11436 contains a 714-bp ORF with three exons and encodes a protein with a length of 237 amino acids. Phylogenetic tree analysis and sequence alignment showed that SS1G_11436 exhibited a high sequence similarity with B. cinerea MRT4 (BCIN_08g05250) (94.51% identity in amino acid sequence) and S. cerevisiae MRT4 (YKL009W) (42.26% identity in amino acid sequence) (Figure 1B). Similar to BcMRT4 and ScMRT4, SsMRT4 also contains a Ribosomal_L10 domain as predicted (Figure 1C). To clarify the subcellular localization of SsMRT4, a C-terminal eGFP tag was fused to its coding sequence (SsMRT4-eGFP) and transient transformed into the N. Benthamian. As expected, the fused SsMRT4 was located in the nucleus and co-localized with DAPI staining (Figure 1D).

3.2. Knockdown and Complementation of SsMRT4 in S. sclerotiorum

To explore the possible function of SsMRT4, we used a split-marker method to generate mutants (Figure 2A), in which target gene was replaced by hygromycin-resistance gene in site. The homozygous knockout mutant, however, stopped growing within 24 h after inoculation, indicating the lethality of SsMRT4 knockout homozygotes. After continuous purification, we obtained three knockdown strains, Ssmrt4-1, 2, 3, and the expression of SsMRT4 was then detected in these strains. We chose Ssmrt4-3 with the lowest expression of SsMRT4 for the subsequent experiments according to qRT-PCR results (Figure 2B). Then, a genetic complementation test was conducted through agrobacterium-mediated transformation. Subsequently, the expression of SsMRT4 were detected in these Ssmrt4-3 complementary strains, and SsMRT4-C1 with the highest expression was selected for further experiments (Figure 2B).
When the expression patterns of SsMRT4 during different developmental stages were determined though qRT-PCR, the results showed that SsMRT4 was highly expressed during the development of sclerotia stage (Figure 2C). However, we found that the Ssmrt4-3 phenotype was significantly different from wild-type strain in the process of mycelial culture. While wild-type mycelium grew continuously and normally on the surface of PDA, Ssmrt4 knockdown mutants cannot form continuous growth of hyphae on the surface, showing a truncated growth state (Figure 2D). At the same time, the growth rate of hyphae in Ssmrt4 mutants was significantly lower than that of wild-type strains, which were only 0.55 cm/24 hpi (Figure 2E,F). In addition, the number of sclerotia of Ssmrt4-3 was also significantly smaller than that of wild-type strains (Figure 2G,H). On the other hand, the mycelial phenotype and growth rate of the complementary strains were found to be consistent with those of the wild-type strains, indicating that SsMRT4 knockdown is responsible for the mutant phenotype.

3.3. SsMRT4 Is Required for Fungal Pathogenicity of S. sclerotiorum

To examine whether SsMRT4 is related to the pathogenicity of S. sclerotiorum, we inoculated WT, Ssmrt4-3 and SsMRT4-C1 on detached leaves of A. thaliana and N. Benthamian (Figure 3). Under the same infection conditions, leaves inoculated with WT formed obvious necrotic lesions, whereas leaves infected by Ssmrt4-3 did not show any necrosis after 36 h. The same results were observed on undetached leaves in A. thaliana (Figure 3A,C) and N. benthamiana (Figure 3B,D), indicating that SsMRT4 is essential for pathogenicity in S. sclerotiorum.

3.4. SsMRT4 Contributes to Compound Appressorium Formation and Oxalic Acid Production

The formation of compound appressorium is a key factor for the pathogenicity of S. sclerotiorum [39,40]. Compound appressoria formation of WT, Ssmrt4-3 and SsMRT4-C1 was determined on the slide surface after incubation for 16 h. Under the stereo microscopes, compound appressorium could not form at all in Ssmrt4-3 (Figure 4A). After being magnified ten times under the optical microscope, the shape of the compound appressorium can be clearly observed in WT, but no compound appressorium was formed in Ssmrt4-3 (Figure 4B). When the onion epidermis staining with trypan blue was made 16 h after infection, it was found that Ssmrt4-3 could grow a small number of mycelia in onion epidermis, but still could not form normal compound appressorium (Figure 4C).
S. sclerotiorum can secrete oxalic acid to change the pH value during infection, which is more conducive to the process of infection [41]. We inoculated the mycelial plugs on the PDA medium which contained bromophenol blue to detect the oxalic acid secretion of WT, Ssmrt4-3 and SsMRT4-C1. The results show that the PDA inoculated with WT and SsMRT4-C1 turned from blue to yellow, indicating that they could produce oxalic acid normally. However, the color of the medium inoculated with the mutant did not change, suggesting that the knockdown of SsMRT4 means that it is unable to produce acid in S. sclerotiorum (Figure 4D). Thus, SsMRT4 plays a very important role in the formation of the appressorium and the production of oxalic acid.

3.5. SsMRT4 Is Vital for the Oxidative Stress Response

Ribosome assembly factors may play a role in the fungal response to oxidative stress [11]. In order to test this possibility, we inoculated the fungi plugs on PDA containing hydrogen peroxide at different concentrations. With the increase in hydrogen peroxide concentration, the growth of WT and SsMRT4-C1 strains slowed down, but they could still grow on PDA medium containing 7.5 mM H2O2. The Ssmrt4-3 strain, however, could not grow on the medium under oxidative stress (Figure 5A,C). Then, we used 3,3′-diaminobenzidine (DAB) to stain WT, Ssmrt4-3, and SsMRT4-C1. After 30 min, we found that only a few wild-type hyphae were stained light brown, while more places on the surface of the Ssmrt4-3 block were stained dark brown (Figure 5B). It is demonstrated that the H2O2 content in Ssmrt4-3 mycelia was higher than in wild-type mycelia, indicative of a vital role of SsMRT4 under oxidative stress in S. sclerotiorum.

3.6. SsMRT4 Is Essential for the Cellular Integrity of Hyphae under Stresses

To explore the role of SsMRT4 in cell integrity, we inoculated Ssmrt4-3, wild-type and complementary strains on a PDA medium that contained 1 M glucose, 1 M sorbitol, 1 M NaCl, 1 M KCl and 0.02% SDS, respectively. It was found that the growth of S. sclerotiorum was inhibited under both salt ion stress or high osmotic pressure stress. The inhibition caused by salt ion stress was more severe; Ssmrt4-3 could not grow at all (Figure 6). Similarly, the growth of Ssmrt4-3 was completely inhibited on the PDA medium containing 0.02% SDS (Figure 6). Thus, the mutation of SsMRT4 leads to more sensitivity to hyperosmotic stress and cell integrity perturbation in S. sclerotiorum.

4. Discussion

In eukaryotes, the large subunit and small subunit are the two parts necessary for the formation of mature ribosomes in all organisms [2,42]. The ribosome stalk, as the key structure of a large subunit, is necessary for recruitment of translation factors and is crucial for ribosome activity [43,44]. RPP0 (or P0) contains the Ribosomal_L10 domain, a direct homologue of L10 protein in prokaryotes and an important component of ribosome stalk in eukaryotes [45]. The nucleolar protein MRT4 is closely correlated with P0 and contains the Ribosomal_L10 domain. Although SS1G_11436 has only 42.26% amino acid sequence identity with ScMRT4, as the only S. sclerotiorum gene in the phylogenetic tree, it also contains the Ribosomal_L10 domain; therefore, we regard it as SsMRT4. MRT4 is highly conserved in eukaryotes, and exists in the pre-60S ribosome complex rather than the mature 60S subunit. It mainly functions in the nucleolus and nucleoplasm [46]. We transiently expressed SsMRT4 in N. Benthamian, and the eGFP signal shows that SsMRT4 was located in the nucleus, which is consistent with previous results. The deletion of Yvh1 leads to a change in the subcellular localization of MRT4 in yeast [17], whether the same result will occur in S. sclerotiorum requires more experiments to verify. In order to explore the specific role of SsMRT4 in S. sclerotiorum, we replace the SsMRT4 with a hygromycin gene in situ to obtain the mutant strains. Despite the fact that the deletion of MRT4 in yeast does not affect the normal growth of yeast [18], our experimental results show that the complete deletion of SsMRT4 will lead to the premature death of S. sclerotiorum. We speculate that this may be due to differences between species, and the complete deletion of SsMRT4 led to an abnormal ribosome structure that could not normally translate proteins needed for the growth of S. sclerotiorum. Fortunately, three knockdown strains were obtained after continuous purification. Thus, we chose the Ssmrt4-3, whose expression level of SsMRT4 was reduced 50 times compared to the WT in the follow-up study. Although the expression of SsMRT4 has no clear spatiotemporal specificity in the life cycle of S. sclerotiorum, except that it is at the stage of sclerotia development on the seventh day after inoculation on PDA, the growth rate of Ssmrt4-3 is still only a quarter of the wild-type strain. A possible explanation for this might be that SsMRT4 does not need to maintain high expression but is essential for hyphal growth. In addition, we observed that the mutant could hardly form continuous and normal hyphae on the surface of PDA. Corresponding to the high expression of SsMRT4 in the 7dpi and final sclerotia, the number of sclerotia in the Ssmrt4-3 was significantly reduced compared with that of the wild-type strains.
Although the role of MRT4 in fungal infection has not previously been reported, MoFap7, which is also a ribosome assembly factor, has significantly decreased its virulence after being knocked out [11], indicating that ribosome assembly factor may play a role in the formation of fungal virulence. Our results show that after 36 h of infection with Ssmrt4-3, no necrotic lesions appeared on plant surfaces. Then, we extended the infection time and found that the pathogenicity of Ssmrt4-3 is still completely lost after 4 days of inoculation (Figure S1). These studies suggested that SsMRT4 is essential for the pathogenicity of S. sclerotiorum. In order to explore the cause of lost pathogenicity in Ssmrt4-3, we examined the formation of its appressorium and the production of oxalic acid. We found that Ssmrt4-3 could not form appressorium on either glass or onion surface, and no oxalic acid was produced, indicating that the loss of pathogenicity of the mutant is due to its inability to form appressorium and secrete oxalic acid during infection. In the process of resisting the invasion of S. sclerotiorum, host plants will produce a series of immune reactions, including the massive production of ROS [47,48]. As an important part of ROS, H2O2 was added to PDA to simulate this process. It was found that even the lowest concentration of H2O2 made Ssmrt4-3 completely unable to grow. This may be caused by the loss of hydrogen peroxide scavenging ability in the mutant, and led to a high ROS accumulation that inhibited the growth of mycelia. At the same time, the H2O2 content in the Ssmrt4-3 under normal culture conditions was also significantly higher than that in the wild-type strain, which further verified our previous hypothesis.
In conclusion, we identified SsMRT4 and created knockdown mutants of SsMRT4 in S. sclerotiorum. Based on the above results, we established a model (Figure S2) to reveal the function of SsMRT4 in S. sclerotiorum. Firstly, SsMRT4 influences the accumulation of pre-60S subunits as a ribosomal transacting factor, thereby affecting the assembly of immature ribosomes in the nucleus. The damage of ribosome assembly further affects the synthesis of proteins in S. sclerotiorum. The disruption of protein synthesis directly affects the hyphal growth and integrity of ROS clearance pathway in S. sclerotiorum. Secondly, both endogenously produced and exogenously accumulated ROS cannot be eliminated in time, which further affects the growth and development of S. sclerotiorum. Finally, the failure to form mature proteins seriously interferes with the formation of appressorium and secretion of oxalic acid, resulting in the complete loss of pathogenicity of the mutant.

Supplementary Materials

The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/pathogens12020281/s1, Figure S1: Lesion symptoms of WT, Ssmrt4-3 and SsMRT4-C1 on undetached leaves of A. thaliana at 48hpi and 96hpi; Figure S2: A model that reveals the function of SsMRT4 in S. sclerotiorum. SsMRT4 influences the accumulation of the pre-60S subunit as a ribosomal transacting factor, thereby affecting the assembly of immature ribosomes in nucleus. The failure to form mature proteins seriously interferes with the formation of appressorium and secretion of oxalic acid, resulting in complete loss of pathogenicity of the mutant. Furthermore, both endogenously produced and exogenously accumulated ROS cannot be eliminated in time, which further affects the growth and development of S. sclerotiorum.

Author Contributions

C.Y., L.T. and S.X. designed the experiments, C.Y. and L.T. performed most of the described experiments. C.Y., Y.L. and L.Q. performed the screening. X.T., L.Q. and W.Z. conducted the infection experiments. W.Z., X.G. and W.X. analyzed the ROS data. C.Y., L.T. and S.X. wrote the manuscript. All authors reviewed the manuscript. All authors have read and agreed to the published version of the manuscript.

Funding

National Natural Science Foundation of China (grant 31971836) and Provincial (National) Innovation and Entrepreneurship Training Program (grant S202110537018).

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

Not applicable.

Acknowledgments

We cordially thank Xin Li (University of British Columbia) for the critical suggestions regarding the experiments, Daohong Jiang (Huazhong Agricultural University) for sharing pCH-EF-1 plasmid, and Jeffrey Rollins (University of Florida) for sharing WT S. sclerotiorum strain 1980. We would like to thank the National Natural Science Foundation of China (grant 31971836) and Provincial (National) Innovation and Entrepreneurship Training Program (grant S202110537018) for funds awarded to S.X.

Conflicts of Interest

The authors declare no conflict of interest.

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Figure 1. Identification and subcellular localization of SsMRT4. (A) Phylogenetic tree of SsMRT4 was constructed based on amino acid sequences from different fungi. Data were downloaded from EnsemblFungi (http://fungi.ensembl.org/index.html, accessed on 28 December 2022). (B) Alignment of amino acid sequences of B. cinerea MRT4 (BCIN_08g05250), S. cerevisiae MRT4 (YKL009W) and SsMRT4 (SS1G_11436). The predicted domain sequence is highlighted in red box. (C) Protein domain structure analysis. Domain architectures were identified using Pfam database (https://pfam.xfam.org/, accessed on 28 December 2022) (D) SsMRT4 protein subcellular localization in N. Benthamian. Merge: merged by eGFP and DAPI.
Figure 1. Identification and subcellular localization of SsMRT4. (A) Phylogenetic tree of SsMRT4 was constructed based on amino acid sequences from different fungi. Data were downloaded from EnsemblFungi (http://fungi.ensembl.org/index.html, accessed on 28 December 2022). (B) Alignment of amino acid sequences of B. cinerea MRT4 (BCIN_08g05250), S. cerevisiae MRT4 (YKL009W) and SsMRT4 (SS1G_11436). The predicted domain sequence is highlighted in red box. (C) Protein domain structure analysis. Domain architectures were identified using Pfam database (https://pfam.xfam.org/, accessed on 28 December 2022) (D) SsMRT4 protein subcellular localization in N. Benthamian. Merge: merged by eGFP and DAPI.
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Figure 2. Phenotype of SsMRT4 knockdown and complementary strains. (A) Technical process of split marker method. Fragment 1 consists of the upstream part of the gene of interest and the first half of the hygromycin resistance (HY) gene, while fragment 2 consists of the latter half of hygromycin and the downstream part of the gene of interest. These two fragments replaced the gene of interest by homologous recombination with the hygromycin resistance gene. (B) Relative expression level of SsMRT4. β-tubulin was used as an internal reference. Relative expression of SsMRT4 at 1 dpi was set as control. WT, wild-type strain; Ssmrt4-1/2/3, knockdown strains; SsMRT4-C1/C2, complementation strains. (C) Relative expression levels of SsMRT4 during different developmental stages of sclerotia. Error bars represent SD. (D) Hyphae morphology of WT, Ssmrt4-3 and SsMRT4-C1 on PDA. Bar = 1 mm. (E) Semidiameter of mycelial growth at 40 h. The white dotted line is the edge of mycelial growth. (F) Growth rate of WT, Ssmrt4-3 and SsMRT4-C1. (G,H) Sclerotial number per plate of WT, Ssmrt4-3 and SsMRT4-C1. Experiments were conducted three times with similar results. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01). WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
Figure 2. Phenotype of SsMRT4 knockdown and complementary strains. (A) Technical process of split marker method. Fragment 1 consists of the upstream part of the gene of interest and the first half of the hygromycin resistance (HY) gene, while fragment 2 consists of the latter half of hygromycin and the downstream part of the gene of interest. These two fragments replaced the gene of interest by homologous recombination with the hygromycin resistance gene. (B) Relative expression level of SsMRT4. β-tubulin was used as an internal reference. Relative expression of SsMRT4 at 1 dpi was set as control. WT, wild-type strain; Ssmrt4-1/2/3, knockdown strains; SsMRT4-C1/C2, complementation strains. (C) Relative expression levels of SsMRT4 during different developmental stages of sclerotia. Error bars represent SD. (D) Hyphae morphology of WT, Ssmrt4-3 and SsMRT4-C1 on PDA. Bar = 1 mm. (E) Semidiameter of mycelial growth at 40 h. The white dotted line is the edge of mycelial growth. (F) Growth rate of WT, Ssmrt4-3 and SsMRT4-C1. (G,H) Sclerotial number per plate of WT, Ssmrt4-3 and SsMRT4-C1. Experiments were conducted three times with similar results. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01). WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
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Figure 3. SsMRT4 is required for S. sclerotiorum pathogenicity. (A,C) Inoculated lesions of WT, Ssmrt4-3 and SsMRT4-C1 of detached and undetached leaves of A. thaliana and N. benthamiana. Data were recorded at 36 hpi. Bar = 10 mm. (B,D) Lesion areas of WT, Ssmrt4-3 and SsMRT4-C1 on leaves of A. thaliana and N. benthamiana. Image J was used to analyze lesion areas. Experiments were conducted three times with similar results. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01). WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
Figure 3. SsMRT4 is required for S. sclerotiorum pathogenicity. (A,C) Inoculated lesions of WT, Ssmrt4-3 and SsMRT4-C1 of detached and undetached leaves of A. thaliana and N. benthamiana. Data were recorded at 36 hpi. Bar = 10 mm. (B,D) Lesion areas of WT, Ssmrt4-3 and SsMRT4-C1 on leaves of A. thaliana and N. benthamiana. Image J was used to analyze lesion areas. Experiments were conducted three times with similar results. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01). WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
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Figure 4. SsMRT4 affects appressorium formation and oxalate secretion. (A) WT, Ssmrt4-3, and SsMRT4-C1 were placed on glass slides and cultured for 24 h to observe formation and number of appressoria under the stereo microscopes. (B) Compound appressorium observation of WT, Ssmrt4-3 and SsMRT4-C1 under the optical microscope. Red arrows: compound appressorium. (C) Penetration assay of WT, Ssmrt4-3, and SsMRT4-C1 on onion epidermis cells. Invasion mycelial were stained by trypan blue. Red arrows: compound appressorium. (D) Mycelium of WT, Ssmrt4-3 and SsMRT4-C1 grown on PDA medium containing bromophenol blue. Experiments were conducted three times with similar results. WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
Figure 4. SsMRT4 affects appressorium formation and oxalate secretion. (A) WT, Ssmrt4-3, and SsMRT4-C1 were placed on glass slides and cultured for 24 h to observe formation and number of appressoria under the stereo microscopes. (B) Compound appressorium observation of WT, Ssmrt4-3 and SsMRT4-C1 under the optical microscope. Red arrows: compound appressorium. (C) Penetration assay of WT, Ssmrt4-3, and SsMRT4-C1 on onion epidermis cells. Invasion mycelial were stained by trypan blue. Red arrows: compound appressorium. (D) Mycelium of WT, Ssmrt4-3 and SsMRT4-C1 grown on PDA medium containing bromophenol blue. Experiments were conducted three times with similar results. WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
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Figure 5. SsMRT4 affects ROS elimination. (A) Colonial morphology and mycelial growth of WT, Ssmrt4-3 and SsMRT4-C1 under different concentrations of H2O2. (B) DAB staining of WT, Ssmrt4-3 and SsMRT4-C1. (C) Hyphae growth of WT, Ssmrt4-3 and SsMRT4-C1. Experiments were conducted three times with similar results. WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01).
Figure 5. SsMRT4 affects ROS elimination. (A) Colonial morphology and mycelial growth of WT, Ssmrt4-3 and SsMRT4-C1 under different concentrations of H2O2. (B) DAB staining of WT, Ssmrt4-3 and SsMRT4-C1. (C) Hyphae growth of WT, Ssmrt4-3 and SsMRT4-C1. Experiments were conducted three times with similar results. WT, wild-type; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain. Error bars represent SD. Statistical significance was analyzed using Student’s t-test between wild-type and knockdown mutants or complementation strains (** p < 0.01).
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Figure 6. SsMRT4 is essential for cellular integrity of hyphae. (A) Sensitivity of Ssmrt4-3 to hyperosmotic stress and cell integrity perturbation agents. Ssmrt4-3 mutant was inoculated on PDA plates amended with 1 M sorbitol, 1 M glucose, 0.02% sodium dodecyl sulphate (SDS), 1 M NaCl and 1 M KCl, respectively. The inhibition of hyphal growth was then calculated at 48 hpi. (B) Growth inhibition rate of Ssmrt4-3. Error bars represent SD. Statistical significance was analyzed using a Student’s t test between wild-type strains and each mutant (** p < 0.01). WT, wild-type strain; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
Figure 6. SsMRT4 is essential for cellular integrity of hyphae. (A) Sensitivity of Ssmrt4-3 to hyperosmotic stress and cell integrity perturbation agents. Ssmrt4-3 mutant was inoculated on PDA plates amended with 1 M sorbitol, 1 M glucose, 0.02% sodium dodecyl sulphate (SDS), 1 M NaCl and 1 M KCl, respectively. The inhibition of hyphal growth was then calculated at 48 hpi. (B) Growth inhibition rate of Ssmrt4-3. Error bars represent SD. Statistical significance was analyzed using a Student’s t test between wild-type strains and each mutant (** p < 0.01). WT, wild-type strain; Ssmrt4-3, knockdown strain; SsMRT4-C1, complementation strain.
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Yang, C.; Tang, L.; Qin, L.; Zhong, W.; Tang, X.; Gong, X.; Xie, W.; Li, Y.; Xia, S. mRNA Turnover Protein 4 Is Vital for Fungal Pathogenicity and Response to Oxidative Stress in Sclerotinia sclerotiorum. Pathogens 2023, 12, 281. https://doi.org/10.3390/pathogens12020281

AMA Style

Yang C, Tang L, Qin L, Zhong W, Tang X, Gong X, Xie W, Li Y, Xia S. mRNA Turnover Protein 4 Is Vital for Fungal Pathogenicity and Response to Oxidative Stress in Sclerotinia sclerotiorum. Pathogens. 2023; 12(2):281. https://doi.org/10.3390/pathogens12020281

Chicago/Turabian Style

Yang, Chenghuizi, Lan Tang, Lei Qin, Weiping Zhong, Xianyu Tang, Xin Gong, Wenqi Xie, Yifu Li, and Shitou Xia. 2023. "mRNA Turnover Protein 4 Is Vital for Fungal Pathogenicity and Response to Oxidative Stress in Sclerotinia sclerotiorum" Pathogens 12, no. 2: 281. https://doi.org/10.3390/pathogens12020281

APA Style

Yang, C., Tang, L., Qin, L., Zhong, W., Tang, X., Gong, X., Xie, W., Li, Y., & Xia, S. (2023). mRNA Turnover Protein 4 Is Vital for Fungal Pathogenicity and Response to Oxidative Stress in Sclerotinia sclerotiorum. Pathogens, 12(2), 281. https://doi.org/10.3390/pathogens12020281

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