The rice blast fungus Magnaporthe oryzae differentiates specialized cells called appressoria that are required for fungal penetration into host leaves. In this study, we identified the novel basic leucine zipper (bZIP) transcription factor BIP1 (B-ZIP Involved in Pathogenesis-1) that is essential for pathogenicity. BIP1 is required for the infection of plant leaves, even if they are wounded, but not for appressorium-mediated penetration of artificial cellophane membranes. This phenotype suggests that BIP1 is not implicated in the differentiation of the penetration peg but is necessary for the initial establishment of the fungus within plant cells. BIP1 expression was restricted to the appressorium by both transcriptional and post-transcriptional control. Genome-wide transcriptome analysis showed that 40 genes were down regulated in a BIP1 deletion mutant. Most of these genes were specifically expressed in the appressorium. They encode proteins with pathogenesis-related functions such as enzymes involved in secondary metabolism including those encoded by the ACE1 gene cluster, small secreted proteins such as SLP2, BAS3, BAS4, and AVR-Pi9 effectors, as well as plant cuticle and cell wall degrading enzymes. Interestingly, this BIP1 network is different from other known infection-related regulatory networks, highlighting the complexity of gene expression control during plant-fungal interactions. Promoters of BIP1-regulated genes shared a GCN4/bZIP-binding DNA motif (TGACTC) binding in vitro to BIP1. Mutation of this motif in the promoter of MGG_08381.7 from the ACE1 gene cluster abolished its appressorium-specific expression, showing that BIP1 behaves as a transcriptional activator. In summary, our findings demonstrate that BIP1 is critical for the expression of early invasion-related genes in appressoria. These genes are likely needed for biotrophic invasion of the first infected host cell, but not for the penetration process itself. Through these mechanisms, the blast fungus strategically anticipates the host plant environment and responses during appressorium-mediated penetration.
Author summary: The identification of gene regulatory networks controlling pathogenicity is a major research goal for understanding plant infection and for developing new strategies for disease control. Rice is the staple food for half the world's population, but its cultivation is threatened by the rice blast fungus Magnaporthe oryzae that causes severe yield losses. This fungus can breach intact plant leaves using specialized cells called appressoria. Here, we have identified in a pathogenicity mutant screen using random insertional mutagenesis, the novel M. oryzae bZIP transcription factor BIP1 that is essential for the infection. BIP1 is not implicated in the development of appressoria or the subsequent penetration of host leaves, but is necessary for the initial establishment of the fungus within plant cells. BIP1 orchestrates the expression of a unique set of early invasion-related genes within appressoria, encoding secreted effectors, enzymes, secondary metabolism-related enzymes, and signaling membrane receptors. Our experimental data suggest that BIP1 controls their expression by interacting directly with a TGACTC motif present in their promoters. Remarkably distinct from other known pathogenicity networks, the BIP1 regulatory network underscores the intricate control of fungal gene expression during infection. BIP1 seems to prepare M. oryzae for early biotrophic growth during appressorium-mediated penetration.
The fungus Magnaporthe oryzae (syn. Pyricularia oryzae) is pathogenic on a wide range of cereals, including wheat, barley, and rice, and is one of the most damaging fungal plant pathogens [[
Regulatory networks specific to each stage of the infection process have been revealed in plant pathogenic fungi [[
In this study, we report the identification of a novel M. oryzae transcription factor involved in pathogenicity, BIP1 (bZIP TF Involved in Pathogenesis-1), whose expression is restricted to the appressorium. BIP1 deletion mutants were non-pathogenic on rice and barley, and differentiated melanized appressoria unable to penetrate into host leaves but penetrated into artificial cellophane membranes. A genome-wide transcriptional analysis revealed a unique set of genes controlled by BIP1, which defined a novel appressorium-specific regulatory network.
An insertional mutagenesis screen was performed in M. oryzae isolate P1.2 using restriction enzyme-mediated insertion (REMI, [[
Graph: (A) Detached barley leaves were inoculated with droplets of conidial suspensions (3.105 conidia/mL) from M. oryzae wild-type isolate P1.2, insertion mutant M763, a Δbip1 deletion mutant and Δbip1 complemented with a wild-type copy of BIP1 (Δbip1:BIP1). Pictures were taken 6 days after inoculation (dai). (B) Four-week-old rice plants were spray-inoculated with conidial suspensions from isolates P1.2, M763 Δbip1 or Δbip1:BIP1 (5.104 conidia/mL) and pictures were taken 7 dai.
Graph: The BIP1 gene is composed of three introns (black lines) and four exons with a 5'-UTR of 234 bp, a 3'-UTR of 1217 bp (both gray boxes) and a CDS of 798 bp (black arrows). 5'-RACE identified transcription starts at positions –53 bp and– 234 bp from the ATG (grey arrows). In the M763 insertion mutant, plasmid pAN7.1 (white triangle) was inserted in the third BIP1 intron, downstream of the exon encoding the bZIP domain. Restriction sites used for cloning are displayed. The BIP1 protein (266 aa) has a bZIP domain located near the N-terminal end (white box).
Graph: (A) Detached barley leaves were inoculated with conidial suspensions of isolates P1.2 (wild-type, WT) or Δbip1 and peeled 24 and 72 hai for observation under a microscope (x400). Melanized appressoria developed normally in WT and Δbip1. Bulbous infection hyphae were visible at 24 hai in WT, but were absent in Δbip1, even at 72 hai. Size bar = 10 μm. (B) Observation of hyphal penetration in barley cells at 48 hai using confocal microscopy (63X) and fungal staining with WGA-Alexa488 after tissue fixation. No infection hyphae were observed in epidermal cells of barley leaves infected by Δbip1 mutant, whereas Δbip1:BIP1 and P1.2-infected barley leaves showed numerous invasive infection hyphae resulting from successful penetrations of barley epidermal cells. Fluorescence of WGA-Alexa488-stained fungal cells was excited with 488 nm light and is shown in green. Fluorescence of calcofluor-stained plant cells was excited with 380 nm light and is shown in blue. Lower panel: 3D reconstruction from Z-stack. Size bar = 10 μm. (C) Observation of appressorium-mediated penetration in rice sheath cells of strains P1.2 and Δbip1 at 48 hai using confocal microscopy (63X). No infection hyphae were observed in epidermal cells of rice sheaths infected with Δbip1 mutant whereas epidermal cells of rice sheaths infected with P1.2 were filled with infection hyphae resulting from penetration events. Fungal cells were stained with the WGA-Alexa488 after tissue fixation. Fluorescence of WGA-Alexa488-stained fungal cells was excited with 488 nm light and is shown in green and combined with a bright-field image of the leave. Individual bright-field and fluorescence images are shown in S6 Fig. Size bar = 10μm. Ap: appressorium, Gt: germ tube, Co: conidium, IH: invasive hyphae.
Graph: Conidia of wild-type (P1.2), Δbip1 mutant and Δbip1 complemented strains were deposited on cellophane membrane, and appressoria (black arrows) and pseudo-infection hyphae growing into the membrane (white arrows) were visualized by differential interference contrast microscopy at 48 hai and 72 hai. Bar = 10μm.
MGG_08118 encodes a protein of 266 amino acids with one putative nuclear localization signal and a basic leucine zipper (bZIP) domain similar to those of the Saccharomyces cerevisiae bZIP TFs GCN4 and YAP1 (S8A Fig). The protein domain search tools CD (https://
Graph: Phylogenetic tree of bZIP domains of TFs from M. oryzae and five selected Pezizomycotina species (MGG: Magnaporthe oryzae, NCU: Neurospora crassa; ANID: Aspergillus nidulans, BC1G: Botrytis cinerea, SNOG: Parastagonospora nodorum, Fusarium graminearum). In red, the clade of BIP1 and its orthologs. bZIP TFs were identified using the Interpro motif IPR004827 and the Superfamily motif SSF57959. In addition, BIP1 and its closest homologs, bZIP TF MGG_08587, as well as their orthologs identified by blastp searches and the Panther motif PTHR11462 were added to this dataset. bZIP domain sequences were extracted from the protein sequences and aligned with ClustaL omega (S1 data). The phylogenetic tree was constructed using the maximum likelihood method with RxML.
Quantitative RT-PCR (qRT-PCR) showed that BIP1 was expressed at the same high levels in conidia and appressoria differentiated on Teflon and displayed only a low level of expression in mycelium from axenic culture (Fig 6A). In infected barley leaves, BIP1 was detected as early as 8 hours after inoculation (hai) and reached its maximal level of expression at 17 hai, which coincides with appressorium maturation and precedes host leaf penetration (Fig 6B). To further investigate BIP1 expression, a Δbip1 mutant was transformed with a transcriptional fusion vector carrying three copies of eGFP under the control of the BIP1 promoter and its 5' and 3'UTR sequences. The fungal transformants were analyzed by fluorescence microscopy at different stages of the infection of barley leaves. GFP fluorescence was detected specifically in mature appressoria with a maximal level of expression between 15 and 48 hai, but not in conidia, mycelium, nor infection hyphae (Fig 6C). The absence of GFP fluorescence in conidia despite the detection of BIP1 mRNA by qRT-PCR, suggested a post-transcriptional control of BIP1 expression. Such control could involve BIP1 5'UTR and 3'UTR sequences present in the transformation construct. To monitor the expression of the BIP1 protein and its subcellular localization, a translational fusion vector carrying a BIP1-3xeGFP fusion under the control of the BIP1 promoter and its 5' and 3'UTRs, was introduced in the Δbip1 mutant. Confocal laser scanning microscopy detected GFP fluorescence specifically in the nucleus of mature appressoria but not in conidia, nor germinating hyphae and young appressoria (Fig 6D). These experiments showed that BIP1 is an appressorium-specific TF with a nuclear localization, expressed after the migration of the nucleus into the appressorium.
Graph: (A) BIP1 expression in different M. oryzae tissues. BIP1 expression was monitored using qRT-PCR with RNA extracted from conidia (Co), mycelium (Myc), and 24h old appressoria (App) differentiated on Teflon of the P1.2 wild-type strain. (B) BIP1 expression during infection of barley leaves. Quantification of BIP1 expression by real-time RT-PCR using RNA from infected barley leaves collected at different time points after droplet inoculation with wild-type conidial suspensions. Data were normalized relative to the constitutively expressed gene ILV5. Each data point is the average of three biological replicates. Standard deviation is indicated by error bars. (C) BIP1 expression in appressoria during infection. Δbip1 transformants expressing a pBIP1:3xeGFP transcriptional fusion construct were inoculated on barley leaves. Mature appressoria were analysed at 20 hai using transmitted white light (left) or fluorescence microscopy with eGFP filters (right). (D) Localization of BIP1 in nuclei from appressoria. Conidia from a Δbip1 transformant expressing a pBIP1:BIP1-3xeGFP translational fusion were deposited on a hydrophobic Teflon membrane and appressoria developed 24hai, were stained with DAPI and calcofluor and observed using transmitted light (left), eGFP fluorescence microscopy (middle) and blue fluorescence microscopy (DAPI and calcofluor, right). Scale 10 μm.
To identify genes regulated by BIP1, a genome-wide differential expression analysis of WT and Δbip1 mutant appressoria differentiated on Teflon membranes was performed using a M. oryzae oligonucleotide microarray. This differential expression analysis identified 42 genes down-regulated in Δbip1 appressoria, but no up-regulated genes (Table 1). These BIP1-regulated genes were classified into seven classes according to the cellular functions of their corresponding protein (Table 1). The largest class gathered 12 genes coding for proteins involved in secondary metabolism (SM) (Table 1). Among them, nine were located within the ACE1 gene cluster (Table 1), a 57 kb genomic region that contains 15 SM genes including the avirulence gene ACE1 coding for an hybrid polyketide synthase/non-ribosomal peptide synthetase (PKS-NRPS) [[
Graph
Table 1 Genes down-regulated in Δbip1 appressoria differentiated on Teflon. The expression ratios are log2 transformed. * Comparison of appressoria and in vitro grown mycelium. RNA seq comparing appressoria and germinating conidia from Osés-Ruiz et al., 2021 [[
Gene Class Function Gene name Gene cluster Reference μarray qPCR1 Ap qPCR2 WT Ap/ My RNAseq WT* Ap/ Gc EMSA MGG_02420 Metabolism Sugar 1,4 lactone oxidase -1.6 nid MGG_02530 Metabolism Quinate permease -1.9 nid MGG_02559 Metabolism Molybdenum cofactor sulphurase -1.6 2.4 MGG_03263 Metabolism Betaine aldehyde dehydrogenase [ -1.5 2.8 MGG_04240 Metabolism FAD oxidoreductase -1.5 4.4 MGG_04738 Metabolism Short-chain dehydrogenase -1.6 5.1 MGG_09681 Metabolism Gluconolactonase -2.4 4.3 MGG_08236 Secondary Metabolism Polyketide synthase -2.2 6.3 MGG_08377 Secondary Metabolism O-Methyltransferase [ -2.1 6.6 MGG_08378 Secondary Metabolism Cytochrome P450 [ -2.8 6.6 MGG_08379 Secondary Metabolism Cytochrome P450 [ -2.4 7.3 MGG_08380 Secondary Metabolism Enoyl reductase [ -3.8 -10.0 13.3 7.4 Yes MGG_08381 Secondary Metabolism Diels-alderase [ -4.1 -11.3 11.1 9.4 Yes MGG_08386 Secondary Metabolism Zn finger transcription factor [ -1.8 -5 10.8 6.6 No MGG_08387 Secondary Metabolism Cytochrome P450 [ -1.8 7.1 MGG_08391 Secondary Metabolism Enoyl reductase [ -2.7 7.3 MGG_11096 Secondary Metabolism Thioesterase -1.2 4.6 MGG_13405 Secondary Metabolism Terpene synthase -1.3 9.7 MGG_15928 Secondary Metabolism Cytochrome P450 [ -1.6 -3.0 11.6 10.2 MGG_02201 Secreted Enzyme Peptidase A1 -4.1 -9.0 11.6 8.5 Yes MGG_03771 Secreted Enzyme Feruloyl esterase [ -2.1 8.2 MGG_05855 Secreted Enzyme α/β Hydrolase -1.6 4.1 MGG_08480 Secreted Enzyme α/β Hydrolase -2.6 4.5 MGG_11966 Secreted Enzyme Cutinase -1.6 7.8 MGG_17153 Secreted Enzyme Chitinase -1.6 2.3 MGG_00751 Secreted Protein small secreted protein -1.1 1.4 MGG_03468 Secreted Protein Lysm domain protein [ -2.8 5.1 MGG_03504 Secreted Protein small secreted protein -1.6 1.9 MGG_05638 Secreted Protein small secreted protein -2 8.8 MGG_06666 Secreted Protein small secreted protein -2.3 2.2 MGG_07934 Secreted Protein small secreted protein -1.8 8.0 MGG_08428 Secreted Protein small secreted protein -2.8 7.0 MGG_09693 Secreted Protein Biotrophy assoc.protein 2 [ -2.2 2.7 MGG_11610 Secreted Protein Biotrophy assoc.protein 3 [ -3.1 nid MGG_12655 Secreted Protein small secreted protein [ -3.2 6.8 MGG_17425 Secreted Protein small secreted protein -2.3 3.6 MGG_02160 Signaling GPCR PTH11 family, CFEM -1.2 -1.1 3.4 2.2 MGG_03526 Signaling N6 Adenine DNA methylase -1.7 3.2 MGG_03584 Signaling GPCR PTH11 family, CFEM -3.3 -1.7 0.5 6.4 Yes MGG_06535 Signaling GPCR PTH11 family -2.9 -3.9 7.2 3.8 Yes MGG_10544 Signaling GPCR cAMP Glucose receptor-like -1.7 7 MGG_00545 Unknown Unknown -2.7 3.7
qRT-PCR experiments were performed with eight BIP1-regulated genes from three functional categories using RNAs from Δbip1 and wild-type appressoria differentiated on Teflon. All eight genes were down-regulated by at least 2-fold in Δbip1 appressoria, seven more than 10- fold (Table 1, qPCR1, Δbip1/wt). Seven of the eight candidate genes were strongly up-regulated in WT appressoria as compared to WT mycelium (Table 1, qPCR2, Ap/My). This result was confirmed by independent, published appressorium RNAseq data [[
Taken together, our results show that BIP1 coordinates the expression of a specific set of 40 infection-related genes during appressorium-mediated penetration.
Analysis of promoter sequences 1 kb upstream from the start codon, showed an enrichment of a conserved TGACTC sequence similar to the GCN4-like binding motif in the promoters of the 40 genes down-regulated in Δbip1 appressoria. Indeed, using MEME, the motif was found in 36% of the BIP1-regulated genes and only 12% of the 12.593 promoters of M. oryzae (FIMO analysis, p-value 10
To analyze whether BIP1 may regulate its target genes by direct binding to these GCN4-like binding motifs, in vitro electrophoretic mobility shift assays (EMSA) were performed using recombinant BIP1 protein and radiolabeled 50-bp oligonucleotides centered on the TGACTC sequences of the promoters from six randomly chosen BIP1-regulated genes (S3 Table). BIP1 bound to an oligonucleotide covering the two motifs of the bidirectional promoter shared by MGG_08380 (RAP2) and MGG_08381 (ORF3) from the ACE1 gene cluster (Fig 7A). This binding was reduced by an excess of non-labeled probes and was strongly reduced or abolished by mutations of, respectively, the first or both core motifs (Figs 7A and 8A). BIP1 also bound to probes centered on the single GCN4-like binding motif of the promoter from MGG_02201 (peptidase) (Fig 7A). In addition, BIP1 bound to the oligonucleotides covering the GCN4-like motifs of the promoters from the PTH11-like genes MGG_03584, and MGG_06535 (Fig 7A). In all cases, BIP1 binding was reduced by competition with unlabeled probes. Only the oligonucleotides corresponding to the four TGACTC motifs of MGG_08386 coding the BC2 TF from the ACE1 gene cluster did not bind BIP1 (S3 Table). Taken together, among the five promoters tested with EMSA, four (MGG_02201; MGG_03584; MGG_06535; MGG_08380/ MGG_08381) have at least one GCN4-like motif binding to BIP1. The alignment of sequences from oligonucleotides binding to BIP1 in vitro highlighted the motif CATGACTCG as a possible extension of the BIP1 binding site sequence (Fig 7B).
Graph: (A) Radioactively labeled oligonucleotide probes centered on the TGACTC motifs of promoters from MGG_08381/MGG08380 (ORF3/RAP2), MGG_02201 (Peptidase), MGG_03584 (PTH11-like), MGG_06535 (PTH11-like) genes were incubated in the presence of binding buffer (FP, free probe), BIP1 rabbit reticulocyte lysate (BIP1), BIP1 lysate with unlabeled probe (1:2 or 1:10 molar ratios) or rabbit reticulocyte lysate lacking the BIP1 expression construct (Lysate) before non-denaturing PAGE. For MGG_08381/MGG08380 (ORF3/RAP2), oligo probes carrying a mutation in the first or both GCN4 motif were tested in addition to the wild-type oligonucleotide. The mutant oligonucleotide probes pORF3-mut1 and pORF3-mut2 are shown with mutated bases in blue. (B) The oligonucleotides bound by BIP1 in EMSA were aligned on the TGACTC core sequence and submitted to WebLogo to define the BIP1-binding consensus motif.
To test the functional role of the TGACTCG binding site found in the promoters of BIP1-regulated genes, we selected MGG_08381 from the ACE1 gene cluster specifically expressed in appressoria [[
Graph: (A) Binding of BIP1 to an ORF3 promoter fragment relies on the presence of GCN4 motifs. Labeled oligonucleotide probes containing either the two GCN4-like TGACTC motifs of MGG_08381 (ORF3) (left) or a probe mutated for these motifs and the connecting 6 nucleotides (right) were incubated in the presence of binding buffer (FP, free probe), BIP1 rabbit reticulocyte lysate (BIP1), BIP1 lysate with unlabeled probe (1:2 or 1:10 molar ratios), or rabbit reticulocyte lysate lacking the BIP1 expression construct (Lysate) before non-denaturing PAGE. (B) Transgenic M. oryzae isolates carrying the GFP reporter gene under the control of the wild-type ORF3 promoter or a mutant promoter lacking the two BIP1 binding motifs were inoculated on barley leaves and mature appressoria were analyzed 20 hai by fluorescence microscopy for transmitted white light (top) and green fluorescence (bottom). Scale bars = 10 μm.
In this study, we have identified BIP1 (MGG_08118) a novel bZIP TF of M. oryzae involved in fungal pathogenicity. BIP1 and its closest paralog (MGG_08587) have not been detected in previous genome-wide surveys of bZIP TFs in the rice blast fungus [[
BIP1 deletion mutants (Δbip1) were non-pathogenic on rice and barley leaves (Fig 1). Although they differentiated melanized appressoria with normal turgor, they were unable to penetrate into intact or wounded host leaves (Figs 3, S2 and S7). This phenotype is different from mutants impaired in appressorium maturation, turgor generation or appressoria adhesion, which cannot penetrate intact leaves, but still infect wounded leaves, such as Δbuf1, deficient for melanin biosynthesis, ΔcpkA, defective for cAMP signaling and Δsps1 defective for spermine synthase [[
M. oryzae mutants unable to infect wounded plant as Δbip1, were affected in genes essential for penetration peg formation like PLS1, NOX2, MPS1 or MST12 [[
In most other M. oryzae mutants with defects in early invasive infectious growth, primary infection hyphae (PIH) are formed in the first infected cell before being arrested [[
Fifteen other bZIP TFs with defective mutant phenotypes, have been described in M. oryzae (S4 Table). Seven of these bZIP TF mutants display phenotypes associated with either stress response, development (mostly sporulation) or specific growth conditions, but not pathogenicity on plants (S4 Table). Some of them control basic cellular processes, like MobZIP12, which encodes an ortholog of A. nidulans MeaB, a regulator of nitrogen assimilation [[
Genome-wide analysis of the appressorium transcriptome identified 40 genes down-regulated in the Δbip1 mutant in comparison to wild-type. Most of these BIP1-regulated genes (93%) were over-expressed in mature wild-type appressoria as observed for BIP1 (Table 1). Promoters of these BIP1-regulated genes shared a TGACTC GCN4/bZIP-like binding motif that bound in vitro to BIP1. Mutations of this motif in the promoter of MGG_08381.5 (ORF3 from the ACE1 cluster) abolished in vitro BIP1 binding and its appressorium-specific expression (Fig 8). Together, these results suggest that in mature appressoria BIP1 activates the expression of a unique set of genes by binding to a TGACTC motif present in their promoters. The specificity of this regulatory network likely results from the fact that BIP1 expression is restricted to the appressorium.
BIP1-regulated genes encoded proteins with very different cellular functions, i.e. small secreted proteins, enzymes involved in secondary metabolism, cell wall degradative enzymes, or GPCRs. However, a shared feature of these proteins is their putative involvement in the infection process. Cuticle and plant cell wall degrading enzymes from the BIP1 network included a cutinase, a peptidase and a feruloyl esterase. The cutinase, MGG_11966, already described as specifically expressed during penetration [[
Only few appressorium-specific regulatory networks have been characterized in M. oryzae. The best defined are the appressorium-specific gene networks controlled by TFs MST12 and HOX7 activated by the PMK1 MAP kinase signaling pathway [[
The bZIP TF MoAP1 (MobZIP21 in S4 Table) is required for infection and other cellular processes such as resistance to oxidative stress and development [[
The Zinc-Finger TF MoEITF1 and the bZIP TF MoEITF2 (MobZIP20 in S4 Table) are specifically required for infection [[
For the previously mentioned transcription factor WOR1, whose mutant, like Δbip1, is unable to invade the first infected cell, only selected genes were analyzed for altered expression in mutant appressoria. The effector BAS2, which was downregulated in Δbip1, was overexpressed in Δwor1. On the reverse, the effectors BAS1, BAS4, AVR-Pita, Pwl2 and MC69, whose expression were not altered in Δbip1, were down-regulated in the WOR1 mutant. Therefore, we assume that the regulatory networks of BIP1 and WOR1 are distinct.
The discovery of BIP1, which has been missed in previous studies on M. oryzae bZIP TFs, sheds new light on the control of fungal gene expression during plant infection. BIP1 is required for the expression of a unique set of genes essential for early invasive infectious growth. This novel appressorium-specific regulatory network opens new perspectives for understanding the control of fungal gene expression during early stages of infection. We show that BIP1 controls the expression of its target genes by binding to a GCN4 bZIP motif present in their promoter and thereby activating their transcription. The specificity of BIP1 seems determined by its expression confined to mature appressoria by transcriptional and post-transcriptional control mechanisms. Additional regulatory networks specific to the appressorium have been characterized in M. oryzae (e.g. MST12, MoEITF1, MoEITF2: [[
M. oryzae isolate P1.2 used in this study was provided by the Centre de Coopération Internationale en Recherche Agronomique pour le Développement (CIRAD). Isolates, media composition, maintenance, and transformation of the fungus and sexual crosses have been previously described [[
Insertional mutagenesis was performed by the transformation of protoplasts according to the Restriction Enzyme-Mediated Integration (REMI) procedure [[
Southern blot analyses of the M763 mutant and co-segregation analyzes in progenies of a cross between M763 and a wild type strain (M4) showed that it contained a single linearized pAN7.1 plasmid insertion. A 0.4 kb NdeI-SspI genomic restriction fragment flanking one of the junctions between the inserted plasmid and the genomic DNA (Fig 2) was recovered by plasmid rescue and used to screen a M. oryzae genomic cosmid library. A 6 kb XhoI-BglII restriction fragment hybridizing to this probe was identified and subcloned for complementation analysis (Fig 2). Pathogenicity was restored in 90% of the transformants of M763 with this restriction fragment, demonstrating that the M763 phenotype is due to the mutation of a gene present within this fragment. A M. oryzae cDNA library was screened with the 0.4 kb NdeI-SspI probe, yielding four cDNAs of 2 kb with the same open reading frame as
Screening of the REMI hygromycin-resistant transformants for the loss of pathogenicity was carried out as previously described [[
Preparation of M. oryzae genomic DNA was performed as previously described [[
For plasmid rescue [[
Transcription initiation sites of BIP1 were determined by scanning the sequence of 5' RACE products obtained using the GeneRacer kit (Invitrogen), and RNA from conidia or appressoria of M. oryzae isolate P1.2 as templates. Reverse transcription was performed with gene-specific RACE1 primer (exon 3 of BIP1 gene, S5 Table). Reverse primer RACE2 (exon 2 of BIP1) and the RNA primer provided with the kit were used for the PCR amplification of the cDNA. 5' RACE products were cloned into pCR-4Blunt-TOPO.
The upstream (LB-BIP1; 1.2 kb) and downstream (RB-BIP1; 1.36 kb) regions flanking BIP1 were obtained by PCR amplification using P1.2 genomic DNA as a template, Pfu turbo polymerase (Stratagene, La Jolla, CA) and the couples of primers KO1/KO2-SfiIa and KO3-SfiIb/KO4, respectively (S1 Fig and S5 Table). Primers KO2-SfiIa and KO3-SfiIb bear an asymmetric SfiIa or SfiIb restriction site. The resulting amplification products were digested with SfiI (2h, 50°C). In parallel, the 1.4 kb hygromycin resistance cassette (hph) driven by the TrpC promoter from Aspergillus nidulans was obtained by digestion of plasmid pFV8 (gift from Dr. F. Villalba, Bayer CropScience) with SfiI. The three asymmetric restriction fragments were ligated using T4 DNA ligase to assemble the 3.7 kb pRBIP1 deletion cassette, which was cloned into pCR-4Blunt-TOPO (Invitrogen, Carlsbad, CA). The deletion cassette was amplified by PCR using KO5 and KO6 primers and Pfu turbo polymerase. Transformations of P1.2 protoplasts were performed using 3 μg of deletion cassette.
For the transcriptional fusion of the BIP1 promoter (1345 bp) with 3xeGFP, a restriction fragment containing the BIP1 promoter (946 bp) and BIP1 ORF was purified after digestion of pCM763 with EcoRI and introduced into plasmid pUC19 (accession number: L09137), to give pUC19-pBIP1-BIP1ORF. BIP1 ORF was removed from pUC19-pBIP1-BIP1ORF by digestion with NcoI and NaeI. It was replaced by a restriction fragment containing 3xeGFP, obtained by digestion of plasmid pUMA647 [[
Observations were carried out using detached barley leaves (cultivar Plaisant) infected with droplets of conidial suspensions. eGFP fluorescence was monitored 20–24 hai with a Zeiss epifluorescence microscope equipped with a 488/DM510-550 filter. Nuclei were stained using 4,6-diamidino-2-phenylindole (DAPI, 32 670, Fluka) at 0.8 μg.mL
Microarray assays were performed using the Agilent M. oryzae oligonucleotide microarray (version 1) platform. 2 μg of total RNA were used to generate fluorescently labeled aRNA probes with the MessageAmp aRNA Amplification kit (Ambion->Agilent) and Cy3 or Cy5 mono-reactive dye (Amersham) as directed in the Ambion protocol. All RNA was quantified using a NanoDrop ND-1000 spectrophotometer (NanoDrop Technologies) and assayed qualitatively using an Agilent 2100 BioAnalyzer both before and after amplification. Hybridizations were performed as described by Agilent. For each of the three biological replicates, two technical repeats consisting of two slides each were performed. To account for variation due to differences between the two dyes, the labeling dyes for each strain-specific probe were swapped on one slide of each of the technical pairs. Hybridized slides were scanned using an Affymetrix 428 scanner and the resulting images were analyzed using GenePix 4.0 (Axon). Raw expression data were imported into GeneSpring 7.3 (Agilent) and subjected to Lowess normalization, using 20% of the data to fit the Lowess curve at each point in the plot of log intensity versus log ratio. Expression ratio cutoffs of 2.0 and 0.6 were applied to select up-regulated and down-regulated genes, respectively. The raw data generated by the Axon Genepix software was also analyzed using the GeneData Expressionist Refiner and Analyst software package. Data from the 3 biological replicates were imported into GeneData Expressionist Refiner and submitted to a Bayesian background subtraction with a background standard deviation set to 1 and a decay rate of 1000. This method allows the subtraction of background while avoiding a negative signal. Background subtracted data underwent a LOWESS normalization using 10% of the data to fit the smoothing curve. Normalized data was imported into GeneData Expressionist Analyst. For each chip the control and signal channels were kept separate, generating 24 independent data points for each gene (12 wild-type and 12 mutant). An additional median normalization was applied to the whole data set to account for variation between slides. N-way ANOVA was used to determine the effect caused by the mutation on gene expression. A p-value was calculated for each gene, representing the significance that a gene's expression is affected by the mutation. Setting this p-value at 10
bZIP transcription factors were identified in six ascomycetes genomes (Magnaporthe oryzae, Neurospora crassa, Fusarium graminearum, Botrytis cinerea, Aspergillus nidulans, Phaeosphaeria nodorum) from Ensembl fungi by detecting the presence of proteins with a bZIP domain using the following database motifs (cd14688, IPR004827, SSF57959, PTHR11462). Amino acid sequences encoding all bZIP domains in these six species of ascomycetes were aligned using Clustal Omega (S1 Data). This alignment was visualized using Jalview and was used for building the phylogenetic tree. Phylogenetic analysis was carried out using NGPhylogeny by Maximum likelihood-based inference of phylogenetic trees with Smart Model Selection. The branches were measured using Shimodaira–Hasegawa like Approximate likelihood-ratio test (SH-like aLRT). The tree was mid-point rooted and visualized using the Interactive Tree of Life (iTol) tool. Analyses of promoter sequences for potential conserved cis-regulatory elements were carried out using the Weeder algorithm v 1.3 [[
RNA was extracted from detached leaves of barley cultivar Plaisant or rice cultivar Sariceltik inoculated with droplets of conidia of either isolate P1.2 or Δbip1 mutant 24 hai and 17 hai, respectively. Three independent replicate samples were harvested for each treatment and RNAs were extracted separately. Genomic DNA was removed using DNA-free (Ambion). Five μg of total RNA were reverse transcribed using the ThermoScript RT-PCR system (Invitrogen) according to the manufacturer's instructions. The resulting cDNAs were diluted 10 times for analysis. Real-time PCR was carried out with the LightCycler Faststart DNA Master SYBR Green I kit (Roche Diagnostics) using a Light Cycler 1.2 (Roche Diagnostics). Primers used for qPCR are listed in S5 Table. Constitutively expressed EF1-alpha and ILV5 genes were used for normalization as previously described [[
Recombinant BIP1 protein was generated in vitro using the TnT Quick Coupled Transcription/Translation system (Promega) according to the manufacturer's protocol. The T7 expression construct was amplified from p763c1 using the primers BIP1-RL5, and BIP1-RL-Strep2, gel purified and used directly in the in vitro transcription/translation reaction. Double-stranded oligonucleotide probes were constructed by denaturing (95°C, 10 min) and annealing (room temperature, 30 min) complementary single-stranded oligonucleotides in equimolar amounts to give a final concentration of 6 pmol/μL. Probes (3 pmol) (S3 Table) were labeled using T4 polynucleotide kinase (NEB) and γ
MGG_08381.7 terminator (1589bp) was amplified with primers TERMMGG_08381.7NotI+ and TERMMGG_08381.7EcoRI- using Pfu Turbo polymerase (S5 Table). The PCR product, digested by NotI and EcoRI, was introduced into plasmid pCB1635, which carries a glufosinate resistance marker [[
S1 Fig
Gene replacement of BIP1.
A. M. oryzae BIP1 locus regions used to construct the gene replacement vector. 1.2 kb and 1.36 kb genomic regions (respectively Left Border and Right Border grey boxes) flanking the BIP1 ORF were amplified using P1.2 genomic DNA and primers shown as arrows (S5 Table). The four exons of BIP1 are shown as black boxes separated by introns. B. Structure of the BIP1 locus in the Δbip1 mutants. Hatched boxes correspond to the hygromycin resistance cassette. Grey boxes represent the Left and Right Border sequences flanking the BIP1 ORF used to construct the gene replacement vector. C. Analysis of the transformants by Southern blot. Genomic DNA was digested with HindIII and probed with the 1.36 kb RB fragment (top) and 0.85 kb hph cassette (bottom). Lanes 1, 2, and 3, Δbip1 transformants; lane 4, Wild type (P1.2).(PDF)
S2 Fig
Appressorium differentiation and collapsing rates of strains P1.2, Δbip1 and Δbip1:BIP1 for different PEG8000 concentrations.
A. Differentiation of appressoria was observed at 16 hai on Teflon membrane. Error bars represent standard deviations. B. Collapsing of appressoria formed on Teflon membrane was assessed 24 hai with PEG8000 at 4%, 10% and 25%. Tree independent experiments with each three different replicate samples were performed. No significant differences in collapsing rates were observed between the three strains (Anova: F = 0.50, P = 0.74, Df = 4).(PDF)
S3 Fig
Conidiation rates of strains P1.2, Δbip1 and Δbip1:BIP1.
Conidiation rates (conidia.mL
S4 Fig
Mycelial growth of strains P1.2, Δbip1 and Δbip1:BIP1.
A. Five-day-old rice medium cultures of P1.2, Δbip1 and Δbip1:BIP1. B. Mycelial growth diameters (cm) of 5, 7 and 9-day-old rice medium cultures. No significant difference was observed between Δbip1 and wild-type P1.2 (t-Test day 5, p = 1) or between Δbip1 and Δbip1:BIP1 complemented strain (t-Test day5, p = 1). B shows results from three independent experiments each performed with three different replicate samples. Error bars are standard deviations.(PDF)
S5 Fig
Stress sensitivity of P1.2 (WT), Δbip1, Δbip1:BIP1 strains.
P1.2, Δbip1, Δbip1:BIP1 strains were cultured on CM medium without or with stress agent (cell wall integrity stressors: 0.003 or 0.005% SDS (A,B), 200 or 400 μg.mL
S6 Fig
Observation of appressorium-mediated penetration in rice sheath cells of strains P1.2 and Δbip1 at 48 hai using confocal microscopy (63X).
No infection hyphae were observed in epidermal cells of rice sheaths infected with Δbip1 mutant whereas epidermal cells of rice sheaths infected with P1.2 were filled with infection hyphae resulting from penetration events. Fluorescence of WGA-Alexa488-stained fungal cells was excited with 488 nm light and is shown in green. Ap: appressorium, Co: conidium, IH: invasive hyphae, size bar = 10μm.(PDF)
S7 Fig
Pathogenicity assays on barley leaves for strains P1.2, Δbip1 and Δbip1:BIP1.
Droplets of conidial suspensions (5.10
S8 Fig
bZIP domain of BIP1.
A. Alignment of bZIP domains from BIP1, BIP1 orthologues from N. crassa (NcBIP1, NCU03847), F. graminearum (FgBIP1, FGRAMPH1_01G06311), B. cinerea (BcBIP1, Bcin09g05210), A. nidulans (AnBIP1, ANIA_00825) and P. nodorum (SNOG_11592). S. cerevisiae Gcn4 (ScGCN4, YEL009C) and S. cerevisiae Yap1 (ScYAP1, YML007W) TFs were added for comparison. bZIP domains were extracted from protein sequences and aligned using Clustal omega. 100% identical amino acids are highlighted in black. 90–80% similar amino acids are highlighted in dark grey. 70–60% similar amino acids are highlighted in light grey. NLS: nuclear localization signal predicted using Hidden Markov Model for nuclear localization signal prediction. B. Functional domains identified in BIP1 protein using CDD database (bZIP-YAP, CD14688 domain) and previous analysis using YAP1 fungal TFs (A).
(PDF)
S9 Fig
Phylogenetic analysis of M. oryzae feruloyl esterase MGG_03771.
Minimal Evolution tree of selected fungal sequences encoding feruloyl esterases or tannases. A. niger FaeA and two orthologous sequences were used as an outgroup. The scale bar shows a distance equivalent to 0.5 amino acid substitutions per site. Bootstrap values (1000 bootstraps) are presented at the nodes. Biochemically characterized proteins are in bold.(PDF)
S1 Table
ACE1 cluster expression in Δbip1 during barley infection 24 hai.
(PDF)
S2 Table
Expression of 15 BIP1-regulated genes during initial stages of rice infection (16hpi).
(PDF)
S3 Table
Summary of BIP1 binding to target promoter used for EMSA.
(PDF)
S4 Table
Summary of bZIP transcription factors in M.
oryzae.(PDF)
S5 Table
Primers used in this study.
(PDF)
S1 Data
Alignment of bZIP domain sequences used to generate Fig 4 (Fasta format).
(FASTA)
Thomma Bart P.H.J. Section Editor Wilson Richard A Academic Editor
24 Apr 2023
Dear Lecturer Lambou,
Thank you very much for submitting your manuscript "The bZIP transcription factor BIP1 of the rice blast fungus is essential for infection and regulates a specific set of appressorium genes" for consideration at PLOS Pathogens. As with all papers reviewed by the journal, your manuscript was reviewed by members of the editorial board and by several independent reviewers. In light of the reviews (below this email), we would like to invite the resubmission of a significantly-revised version that takes into account the reviewers' comments.
This work focused on characterizing a new bZIP transcription factor, BIP1, found to be required for appressorial function and the expression of a subset of genes including those encoding effectors, cell wall modifying enzymes or enzymes required for secondary metabolism that might (or in some cases have been shown previously) contribute to virulence. In the absence of BIP1, the mutant forms appressoria, but no invasive hyphae are detected, suggesting penetration is impaired. The work is interesting and might shed new light on the genetic regulation of infection.
The reviewers suggest how the paper might be improved, but generally hit on one of two major flaws of the paper that I am also concerned about, namely that it is not shown what the physiological basis for infection impairment is and, I might also add, it is not shown what underlying gene expression changes in Δbip1 directly result in the loss of appressorium penetration and/ or IH development. Thus, the work currently lacks critical details about Bip1 function that need to be resolved.
With regards to appressorial physiology, it must be determined if loss of infection is due to impaired turgor or other maturation defects as suggested by Reviewers 1 and 3 or whether, as Reviewer 2 indicates, penetration pegs are formed and capable of penetrating host rice cells. I might also add that the authors should check whether Δbip1 appressoria are defective in mucilage for adhesion. A recent study of a mutant, Δsps1, which is also Δbip1-like but was not included in the list on line 517, showed it produced a peg but was reduced for adhesion, which impaired turgor, as determined using cellophane assays and turgor measurements (Rocha et al. 2020; DOI: 10.1038/s41564-020-0786-x). Thus, the authors should similarly assess Δbip1 appressoria on cellophane, as well as measure their turgor, in order to determine if they form pegs or have altered mucilage production that would affect adhesion and turgor. Alternatively, Δbip1 might form normal appressoria and pegs which penetrate host cells but fail to elaborate IH. This would be harder to assess, but not impossible by using, for example, SEM to show peg penetration takes place. I agree with Reviewer 2 that rice experiments are essential throughout. Other cellular markers of appressorium formation, as suggested by Reviewer 3, might also be informative here. Editorially, therefore, we request that turgor and penetration peg formation data be added to the paper.
With regards to my second point, I am also concerned that it is not known which Bip1-controlled genes are required for appressoria penetration and/ or IH elaboration. Knocking out in WT some downstream candidate genes to show they result in a similar Δbip1-phenotype, or constitutively expressing one or two candidates in Δbip1, might be useful here.
Other good points are raised by the reviewers, such as whether conidiation is affected in Δbip1, and these should all be addressed.
We cannot make any decision about publication until we have seen the revised manuscript and your response to the reviewers' comments. Your revised manuscript is also likely to be sent to reviewers for further evaluation.
When you are ready to resubmit, please upload the following:
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Important additional instructions are given below your reviewer comments.
Please prepare and submit your revised manuscript within 60 days. If you anticipate any delay, please let us know the expected resubmission date by replying to this email. Please note that revised manuscripts received after the 60-day due date may require evaluation and peer review similar to newly submitted manuscripts.
Thank you again for your submission. We hope that our editorial process has been constructive so far, and we welcome your feedback at any time. Please don't hesitate to contact us if you have any questions or comments.
Sincerely,
Richard A Wilson
Academic Editor
PLOS Pathogens
Bart Thomma
Section Editor
PLOS Pathogens
Kasturi Haldar
Editor-in-Chief
PLOS Pathogens
Michael Malim
Editor-in-Chief
PLOS Pathogens
***
This work focused on characterizing a new bZIP transcription factor, BIP1, found to be required for appressorial function and the expression of a subset of genes including those encoding effectors, cell wall modifying enzymes or enzymes required for secondary metabolism that might (or in some cases have been shown previously) contribute to virulence. In the absence of BIP1, the mutant forms appressoria, but no invasive hyphae are detected, suggesting penetration is impaired. The work is interesting and might shed light on
The reviewers suggest how the paper might be improved, but generally hit on one of two major flaws of the paper that I am also concerned about, namely that it is not shown what the physiological basis for infection impairment is and, I might also add, it is not shown what underlying gene expression changes in Δbip1 directly result in the loss of appressorium penetration and/ or IH development. Thus, the work currently lacks critical details about Bip1 function that need to be resolved.
With regards to appressorial physiology, it must be determined if loss of infection is due to impaired turgor or other maturation defects as suggested by Reviewers 1 and 3 and determine, as Reviewer 2 indicates, whether or not penetration pegs are formed and capable of penetrating host rice cells. I might also add that the authors should check whether Δbip1 appressoria are defective in mucilage for adhesion. A recent study of a mutant, Δsps1, which is also Δbip1-like but was not included in the list on line 517, showed it produced a peg but was reduced for adhesion, which impaired turgor, as determined using cellophane assays and turgor measurements (Rocha et al. 2020; DOI: 10.1038/s41564-020-0786-x). Thus, the authors here should similarly assess Δbip1 appressoria on cellophane, as well as measure their turgor, in order to determine if they form pegs or have altered mucilage production that would affect adhesion and turgor. Alternatively, Δbip1 might form normal appressoria and pegs which penetrate host cells but fail to elaborate IH. This would be much harder to assess, but not impossible by using, for example, SEM to show peg penetration takes place. I agree with Reviewer 2 that rice experiments are essential throughout. Other cellular markers of appressorium formation, as suggested by Reviewer 3, might also be informative here. Editorially, therefore, we request that turgor and penetration peg formation data be added to the paper.
With regards to my second point, I am also concerned that it is not known which Bip1-controlled genes are required for appressoria penetration and/ or IH elaboration. Knocking out in WT some downstream candidate genes to show they result in a similar Bip1-phenotype or constitutively expressing one or two candidates in Δbip1 might be useful here.
Other good points are made by the reviewers, such as whether conidiation is affected in bip1, and these should all be addressed.
Reviewer's Responses to Questions
Please use this section to discuss strengths/weaknesses of study, novelty/significance, general execution and scholarship.
Reviewer #1: This manuscript describes the identification and characterization of a bZIP transcription factor BIP1 of the rice blast fungus essential for infection and regulation of appressorium genes. All experiments were straight forward and all data were logically interpreted. However, there are a few things to be clarified to improve the quality of this manuscript.
Reviewer #2: This manuscript details the identification of a transcription factor involved in the regulation of appressorium penetration in Magnaporthe oryzae. The authors report on a novel gene involved in the regulation of appressorium-mediated penetration. This data provides insight into a network of genes that are involved in M. oryzae penetration and how this is crucial for pathogenicity. These findings may provide avenues for the generation of disease mitigation strategies.
This manuscript is very well written. The authors provide a good overview of appressoria structure and of transcription factor networks in M. oryzae. However, this manuscript would benefit from the addition of experiments that would further confirm the findings of the authors.
Reviewer #3: This is a very well-written and interesting manuscript that provides important new insight into the role of a previously overlooked basic leucine zipper (bZIP) transcription factor BIP1, in orchestrating appressorium-mediated plant infection by the blast fungus, Magnaporthe oryzae. While transcriptional control of �bip1 insertion/deletion mutants are able to form melanized appressoria, but these are non-functional and cannot penetrate leaves. The authors demonstrate that BIP1 controls the expression of 40 pathogenicity-related genes, all of which share a GCN4/bZIP-binding DNA motif. These genes include known secreted effectors and enzymes involved in secondary metabolism, among others. The authors convincingly demonstrate that Bip1 binds to these sequences in an in vitro assay. The authors go on to show that mutation of this DNA motif abolished expression of a secondary metabolism gene cluster. Overall, the data are of a high-quality and support the conclusions made by the authors.
Without looking at additional subcellular makers it's not possible to conclude that appressoria from bip1 mutants are fully mature. As the authors note in Line 517, using light microscopy alone, bip1 mutants look identical to nox2 and mst12 knockout mutants. However, careful cell biological analysis using various fluorescent subcellular markers reveals differences in the terminal phenotypes. It's probably beyond the scope of this manuscript, but it would be interesting to try and further resolve the nature of the terminal phenotype.
Figure 5. I'm curious as to whether the use of 3xeGFP was necessary due to low or undetectable fluorescence with single copy eGFP, or whether this was simply chosen by default?
Further, was nuclear localization of Bip1-3xeGFP present in all/most nuceli, or was there heterogeneity within the population? It might be nice to have some quantitation, but this is not absolutely necessary. It might also be compelling to perform time-lapse imaging to resolve precisely when Bip1-3xeGFP becomes localized to the appressorium nucleus. How long after mitotic division and nuclear migration is it before fluorescence is detectable in the nucleus? Again, not essential, but if it can be done easily, it might add some value.
Figure 6 and 7. I'm curious as to how many times the DNA-binding assays were performed? If multiple replicates already exist, it might be nice to quantify these.
A very minor point: Lines 360 and 408 mention "randomly" selecting genes/promotors to study further, but I couldn't see any mention in the methods of how this process was randomized. Did the authors just select their favourites or was this truly randomized, and if so how?
***
Please use this section to detail the key new experiments or modifications of existing experiments that should be absolutely required to validate study conclusions.
Generally, there should be no more than 3 such required experiments or major modifications for a "Major Revision" recommendation. If more than 3 experiments are necessary to validate the study conclusions, then you are encouraged to recommend "Reject".
Reviewer #1: 1. Deletion of BIP gene still formed well melanized appressoria, but did not penetrate, even wounded leaves. Instead of just saying defective, authors may check the turgor of appressoria formed by deletion mutant using plasmolysis/cytolysis. Further it would be better authors present all phenotypes of the mutant measured in this study including stress responses to speculate more on defective in invasive growth.
- 2. Expression of BIP1 gene. There is difference between on the Teflon (conidia and appressoria) and barley leaves. What is the explanation, plant (e.g. how about on the onion?) or host effect? RNAseq was done the samples from Teflon. However, it is not clear what type of RNA sample used for oligonucleotide microarray. Authors identified 42 down regulated genes from bip1 deletion mutant and binding motif TGACTCG. These 42 were from microarray data. How about RNAseq data? Since authors already has RNAseq data of bip1 deletion mutant during appressorium formation, more comprehensive genome-wide identification/analysis would be available.
- 3. Identification of BIP1 binding motif. It would be better if authors could provide genome-wide presence of this motif, not limited to 42 genes!
Reviewer #2: Comments:
Many experiments conducted in this manuscript are performed in barley. All experiments should be conducted using rice plants to fully validate the results obtained using barley. This is especially important when conducting gene expression profile and microscopy analyses.
Lines 150-151: Referencing Figure 1 and Figure 3 does not support the claims by the authors. Results from infection on wounded leaves must be shown in the manuscript and should be performed using rice.
In line 223, the authors mention BIP1 has a nuclear localization signal. However, this is not represented as mentioned in Supplementary Figure 2. It would be ideal if the authors included a schematic representation of the sequence of BIP1, highlighting the NLS and other domains within the gene.
In addition to the previous point, the authors can generate truncations of the BIP1 protein, with or without the NLS, to show the functionality of the NLS in BIP1. This would strongly support the findings from the authors in Figure 5D that indeed BIP1 localizes to the nucleus of the appressoria via its operational NLS.
In the materials and methods on line 784, the authors state that they use onion epidermis for experiments. However, there are no figures depicting the results of using onion for microscopy work. The authors should include the results from these experiments that are listed in this section.
While the authors state that there is no additional phenotype seen in this BIP1 mutant, the authors need to include morphological characterization in axenic conditions, conidiation data, and appressorium formation assays using the BIP1 mutant and WT strain.
This manuscript would benefit from conducting cell wall integrity and oxidative stress tests on the BIP1 mutant strain compared to the WT to see if there are additional defects with the mutant strain. Even if these findings show negative data, the authors can include these results in the supplementary section to depict the full profile of this fungal mutant strain.
How can the authors guarantee that the strain is not penetrating rather than not proliferating inside the cell? Figure 1A shows small lesions when infecting barley with the BIP1 mutant. If this mutant is highly involved in penetration peg formation, the authors should present penetration rate statistics on rice between the WT and BIP1 mutant strain to show the overall percentage of infection.
Additional experiments need to be conducted to show that the penetration peg is defective in the BIP1 mutant. Microscopy work using rice and the BIP1 mutant strain at varying time points of infection would allow readers to see defects in penetration peg formation and invasive hyphae growth.
How is the BIP1 localization in the conidia versus the mycelia in the 3xGFP strain? This data would complement the gene expression profile presented in Figure 5A.
Authors should consider statistics analysis for the pathogenicity assays and appressoria formation.
Reviewer #3: n/a
***
Please use this section for editorial suggestions as well as relatively minor modifications of existing data that would enhance clarity.
Reviewer #1: 1. Promotor mutation of MGG08381. Are there any phenotypes including appressorium formation and invasive growth?
2. In Figure 5, what are the units of expression levels (A and B)? Sp should be Conidia?
Reviewer #2: (No Response)
Reviewer #3: (No Response)
***
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Reviewer #1: No
Reviewer #2: No
Reviewer #3: No
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21 Aug 2023
Attachment
Submitted filename: 2023_08_16_BIP1_Response to editor and reviewers-Final.docx
Thomma Bart P.H.J. Section Editor Wilson Richard A Academic Editor
11 Sep 2023
Dear Lecturer Lambou,
Thank you very much for submitting your manuscript "The bZIP transcription factor BIP1 of the rice blast fungus is essential for infection and regulates a specific set of appressorium genes" for consideration at PLOS Pathogens. As with all papers reviewed by the journal, your manuscript was reviewed by members of the editorial board and by several independent reviewers. In light of the reviews (below this email), we would like to invite the resubmission of a significantly-revised version that takes into account the reviewers' comments.
Because penetration of bip1 appressoria were not assayed in the revised version of the paper as requested, it is not possible to conclude that this mutant is defective in appressorial penetration, thus the conclusions of the work are unsafe. Cellophane assays of peg formation are standard means of addressing this. In the absence of determining whether or not bip1 appressoria form penetration pegs, an alternative explanation is that this mutant does form pegs that penetrate leaf surfaces, but Bip1 is then required for elaborating primary hyphae from the peg, or for elaborating invasive hyphae from primary hyphae. Considering pegs and primary hyphae cannot be observed in planta by confocal microscopy, the role of Bip1 in infection-related development is currently ambiguous. To reach the high bar for publication in PLoS Pathogens, bip1 penetration peg formation must be assayed.
We cannot make any decision about publication until we have seen the revised manuscript and your response to the reviewers' comments. Your revised manuscript is also likely to be sent to reviewers for further evaluation.
When you are ready to resubmit, please upload the following:
[
[
Important additional instructions are given below your reviewer comments.
Please prepare and submit your revised manuscript within 60 days. If you anticipate any delay, please let us know the expected resubmission date by replying to this email. Please note that revised manuscripts received after the 60-day due date may require evaluation and peer review similar to newly submitted manuscripts.
Thank you again for your submission. We hope that our editorial process has been constructive so far, and we welcome your feedback at any time. Please don't hesitate to contact us if you have any questions or comments.
Sincerely,
Richard A Wilson
Academic Editor
PLOS Pathogens
Bart Thomma
Section Editor
PLOS Pathogens
Kasturi Haldar
Editor-in-Chief
PLOS Pathogens
Michael Malim
Editor-in-Chief
PLOS Pathogens
***
Reviewer's Responses to Questions
Please use this section to discuss strengths/weaknesses of study, novelty/significance, general execution and scholarship.
Reviewer #2: This manuscript details the identification of a transcription factor involved in the regulation of appressorium penetration in Magnaporthe oryzae. The authors report on a novel gene involved in the regulation of appressorium-mediated penetration. This data provides insight into a network of genes that are involved in M. oryzae penetration and how this is crucial for pathogenicity. These findings may provide avenues for the generation of disease mitigation strategies.
The authors have included many of the comments as suggested by the Reviewers. Specifically, the experiments conducted have been done in rice plants to agree with the stated findings. Some additional pieces of information and experiments are needed, however, for clarity and validation of results.
Reviewer #3: I appreciate the authors' inclusion of new data from a cytorrhysis assay, which helps to further resolve the phenotype of the Bip1 mutant in demonstrating that turgor production is comparable with the wild type, which strengthens the manuscript. However, without further cell biological investigation of appressorium subcellular architecture, using existing fluorescently-tagged fusion constructs, I would still err on the side of caution when referring to the extent of appressorium "maturation" in Bip1 mutants. I don't think that the ability to generate turgor pressure alone, confirms that the appressoria are necessarily fully matured in other respects (e.g cytoskeleton remodelling), although they might well be. Given that the authors outline the importance of the septin and actin cytoskeleton in their intro Line 90 "ROS production by NADPH oxidases as well as septin GTPase-dependent actin organization of the cytoskeleton are required for the cell re-polarization at the pore and the formation of the penetration peg" it would have been nice to examine these elements directly, given the nature of the Bip1 mutant phenotype.
***
Please use this section to detail the key new experiments or modifications of existing experiments that should be absolutely required to validate study conclusions.
Generally, there should be no more than 3 such required experiments or major modifications for a "Major Revision" recommendation. If more than 3 experiments are necessary to validate the study conclusions, then you are encouraged to recommend "Reject".
Reviewer #2: Line 153-154: This statement needs to be proven on the cellophane membrane in order to conclude that penetration is not happening due to an impairment in penetration peg formation. Since the authors were unable to determine if a penetration peg was developed or not, it is not appropriate to state that the Bip1 mutant 'presumably did not produce a penetration peg' given that it may be produced, but be defective in generating invasive hyphae.
It seems that a small amount of lesions are seen when infecting barley with the Bip1 mutant strain. How can the authors justify the small lesions seen in the mutant if no penetration peg was present? Authors need to be cautious about saying that the penetration peg was arrested in the mutant.
Reviewer #3: n/a
***
Please use this section for editorial suggestions as well as relatively minor modifications of existing data that would enhance clarity.
Reviewer #2: It would be ideal to perform a time course of infection for a prolonged time using the Bip1 mutant to see if there is a delay in infection, both in visual disease symptoms and microscopy. If nothing is seen, the manuscript should at least reflect this finding.
Plant growth and infection conditions should be specified in the materials and methods.
Reviewer #3: n/a
***
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Reviewer #2: No
Reviewer #3: No
Figure Files:
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Reproducibility:
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29 Nov 2023
Attachment
Submitted filename: reponse_editeur_final.docx
Thomma Bart P.H.J. Section Editor Wilson Richard A Academic Editor
14 Dec 2023
Dear Lecturer Lambou,
Thank you very much for submitting your manuscript "The bZIP transcription factor BIP1 of the rice blast fungus is essential for infection and regulates a specific set of appressorium genes" for consideration at PLOS Pathogens. We are likely to accept this manuscript for publication, providing that you modify the manuscript according to my recommendations, specifically:
The inclusion of the cellophane penetration assay has strengthened the conclusions of the paper, but I have three further comments raised by the new version of the paper:
Please prepare and submit your revised manuscript within 30 days. If you anticipate any delay, please let us know the expected resubmission date by replying to this email.
When you are ready to resubmit, please upload the following:
[
Please note while forming your response, if your article is accepted, you may have the opportunity to make the peer review history publicly available. The record will include editor decision letters (with reviews) and your responses to reviewer comments. If eligible, we will contact you to opt in or out
[
Important additional instructions are given below your reviewer comments.
Thank you again for your submission to our journal. We hope that our editorial process has been constructive so far, and we welcome your feedback at any time. Please don't hesitate to contact us if you have any questions or comments.
Sincerely,
Richard A Wilson
Academic Editor
PLOS Pathogens
Bart Thomma
Section Editor
PLOS Pathogens
Kasturi Haldar
Editor-in-Chief
PLOS Pathogens
Michael Malim
Editor-in-Chief
PLOS Pathogens
***
Reviewer Comments (if any, and for reference):
Figure Files:
While revising your submission, please upload your figure files to the Preflight Analysis and Conversion Engine (PACE) digital diagnostic tool, https://pacev2.apexcovantage.com. PACE helps ensure that figures meet PLOS requirements. To use PACE, you must first register as a user. Then, login and navigate to the UPLOAD tab, where you will find detailed instructions on how to use the tool. If you encounter any issues or have any questions when using PACE, please email us at figures@plos.org.
Data Requirements:
Please note that, as a condition of publication, PLOS' data policy requires that you make available all data used to draw the conclusions outlined in your manuscript. Data must be deposited in an appropriate repository, included within the body of the manuscript, or uploaded as supporting information. This includes all numerical values that were used to generate graphs, histograms etc.. For an example see here:
Reproducibility:
To enhance the reproducibility of your results, we recommend that you deposit your laboratory protocols in protocols.io, where a protocol can be assigned its own identifier (DOI) such that it can be cited independently in the future. Additionally, PLOS ONE offers an option to publish peer-reviewed clinical study protocols. Read more information on sharing protocols at https://plos.org/protocols?utm_medium=editorial-email&utm_source=authorletters&utm_campaign=protocols
References:
Please review your reference list to ensure that it is complete and correct. If you have cited papers that have been retracted, please include the rationale for doing so in the manuscript text, or remove these references and replace them with relevant current references. Any changes to the reference list should be mentioned in the rebuttal letter that accompanies your revised manuscript. If you need to cite a retracted article, indicate the article's retracted status in the References list and also include a citation and full reference for the retraction notice.
27 Dec 2023
Attachment
Submitted filename: 2023_12_26_reponse_editeur.docx
Thomma Bart P.H.J. Section Editor Wilson Richard A Academic Editor
4 Jan 2024
Dear Lecturer Lambou,
We are pleased to inform you that your manuscript 'The bZIP transcription factor BIP1 of the rice blast fungus is essential for infection and regulates a specific set of appressorium genes' has been provisionally accepted for publication in PLOS Pathogens.
Before your manuscript can be formally accepted you will need to complete some formatting changes, which you will receive in a follow up email. A member of our team will be in touch with a set of requests.
In addition, the inclusion of the rice leaf sheath images to fig 3 is good, but it is not immediately obvious that these are from fixed samples. Thus, the images may look atypical to some readers expecting live-cell imaging (for example, the rice cell walls are not visible even in the bright field image, and I assume this is due to the fixation process?). My recommendation is that it is noted in the figure legend that the samples are fixed (ie. "..and fungal staining with WGA-Alexa488 after fixation")
Please note that your manuscript will not be scheduled for publication until you have made the required changes, so a swift response is appreciated.
IMPORTANT: The editorial review process is now complete. PLOS will only permit corrections to spelling, formatting or significant scientific errors from this point onwards. Requests for major changes, or any which affect the scientific understanding of your work, will cause delays to the publication date of your manuscript.
Should you, your institution's press office or the journal office choose to press release your paper, you will automatically be opted out of early publication. We ask that you notify us now if you or your institution is planning to press release the article. All press must be co-ordinated with PLOS.
Thank you again for supporting Open Access publishing; we are looking forward to publishing your work in PLOS Pathogens.
Best regards,
Richard A Wilson
Academic Editor
PLOS Pathogens
Bart Thomma
Section Editor
PLOS Pathogens
Kasturi Haldar
Editor-in-Chief
PLOS Pathogens
Michael Malim
Editor-in-Chief
PLOS Pathogens
***
Reviewer Comments (if any, and for reference):
Thomma Bart P.H.J. Section Editor Wilson Richard A Academic Editor
17 Jan 2024
Dear Lecturer Lambou,
We are delighted to inform you that your manuscript, "The bZIP transcription factor BIP1 of the rice blast fungus is essential for infection and regulates a specific set of appressorium genes," has been formally accepted for publication in PLOS Pathogens.
We have now passed your article onto the PLOS Production Department who will complete the rest of the pre-publication process. All authors will receive a confirmation email upon publication.
The corresponding author will soon be receiving a typeset proof for review, to ensure errors have not been introduced during production. Please review the PDF proof of your manuscript carefully, as this is the last chance to correct any scientific or type-setting errors. Please note that major changes, or those which affect the scientific understanding of the work, will likely cause delays to the publication date of your manuscript. Note: Proofs for Front Matter articles (Pearls, Reviews, Opinions, etc...) are generated on a different schedule and may not be made available as quickly.
Soon after your final files are uploaded, the early version of your manuscript, if you opted to have an early version of your article, will be published online. The date of the early version will be your article's publication date. The final article will be published to the same URL, and all versions of the paper will be accessible to readers.
Thank you again for supporting open-access publishing; we are looking forward to publishing your work in PLOS Pathogens.
Best regards,
Michael Malim
Editor-in-Chief
PLOS Pathogens
By Karine Lambou; Andrew Tag; Alexandre Lassagne; Jérôme Collemare; Pierre-Henri Clergeot; Crystel Barbisan; Philippe Perret; Didier Tharreau; Joelle Millazo; Elia Chartier; Ronald P. De Vries; Judith Hirsch; Jean-Benoit Morel; Roland Beffa; Thomas Kroj; Terry Thomas and Marc-Henri Lebrun
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