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. 2017 Mar 20;8:370. doi: 10.3389/fpls.2017.00370

Transcriptomes of Ralstonia solanacearum during Root Colonization of Solanum commersonii

Marina Puigvert 1,2, Rodrigo Guarischi-Sousa 3, Paola Zuluaga 1,2, Núria S Coll 2, Alberto P Macho 4, João C Setubal 3,*, Marc Valls 1,2,*
PMCID: PMC5357869  PMID: 28373879

Abstract

Bacterial wilt of potatoes—also called brown rot—is a devastating disease caused by the vascular pathogen Ralstonia solanacearum that leads to significant yield loss. As in other plant-pathogen interactions, the first contacts established between the bacterium and the plant largely condition the disease outcome. Here, we studied the transcriptome of R. solanacearum UY031 early after infection in two accessions of the wild potato Solanum commersonii showing contrasting resistance to bacterial wilt. Total RNAs obtained from asymptomatic infected roots were deep sequenced and for 4,609 out of the 4,778 annotated genes in strain UY031 were recovered. Only 2 genes were differentially-expressed between the resistant and the susceptible plant accessions, suggesting that the bacterial component plays a minor role in the establishment of disease. On the contrary, 422 genes were differentially expressed (DE) in planta compared to growth on a synthetic rich medium. Only 73 of these genes had been previously identified as DE in a transcriptome of R. solanacearum extracted from infected tomato xylem vessels. Virulence determinants such as the Type Three Secretion System (T3SS) and its effector proteins, motility structures, and reactive oxygen species (ROS) detoxifying enzymes were induced during infection of S. commersonii. On the contrary, metabolic activities were mostly repressed during early root colonization, with the notable exception of nitrogen metabolism, sulfate reduction and phosphate uptake. Several of the R. solanacearum genes identified as significantly up-regulated during infection had not been previously described as virulence factors. This is the first report describing the R. solanacearum transcriptome directly obtained from infected tissue and also the first to analyze bacterial gene expression in the roots, where plant infection takes place. We also demonstrate that the bacterial transcriptome in planta can be studied when pathogen numbers are low by sequencing transcripts from infected tissue avoiding prokaryotic RNA enrichment.

Keywords: Ralstonia solanacearum, bacterial wilt, Solanum commersonii, RNA sequencing, transcriptomics, disease resistance, potato brown rot

Introduction

Changes in pathogen gene expression control the switch from a commensal to a parasitic relationship with the host, which may subvert the host metabolism or development to the pathogen's benefit (Stes et al., 2011). However, there is still limited information concerning how this is controlled. Understanding how these trophic relationships initiate and persist in the host requires deciphering the functional adaptations at the transcriptomic level. Pioneer studies of the expression profiles of bacterial animal pathogens in infected tissues showed that the genes induced more strongly contributed to bacterial virulence and/or survival in the host (reviewed in La et al., 2008).

Ralstonia solanacearum is the causal agent of the destructive bacterial wilt disease in tropical and subtropical crops, including tomato, tobacco, banana, peanut, and eggplant (Hayward, 1991; Peeters et al., 2013). The disease in potato is also called brown rot and is endemic in the Andean region, where potato is a staple food, causing an important impact on food production and the economy (Priou, 2004; Coll and Valls, 2013). Disease control of bacterial wilt is very challenging, because of the bacterium aggressiveness, its persistence in the field and the lack of resistant commercial varieties in any of its hosts. Potato breeding programs have used wild species related to Solanum tuberosum, such as Solanum commersonii, as sources of resistance against bacterial wilt (Kim-Lee et al., 2005; Siri et al., 2009).

As in most Gram-negative animal and plant pathogens, the major pathogenicity determinant in R. solanacearum is the type three secretion system (T3SS) (Boucher et al., 1987). This system injects bacterial proteins called effectors directly into the eukaryotic host cells to manipulate the host defenses and establish disease (Buttner, 2016; Popa et al., 2016a). Amongst other factors that contribute to R. solanacearum virulence are motility—either caused by flagella or type IV pili- and the reactive oxygen species (ROS)- detoxifying enzymes (Meng, 2013).

In vitro studies using microarrays allowed the study of R. solanacearum virulence gene expression and the discovery of novel regulatory networks (Occhialini et al., 2005; Valls et al., 2006). However, the first studies on gene expression in planta using quantitative reporters indicated that R. solanacearum virulence genes showed unexpected expression patterns (Monteiro et al., 2012). Contrary to what was believed based on in vitro studies, it was demonstrated that the genes encoding the T3SS genes and its associated effectors were transcribed in planta at late stages of infection (Monteiro et al., 2012). These findings were later confirmed in transcriptomic studies with R. solanacearum extracted from infected tomato and banana plants (Jacobs et al., 2012; Ailloud et al., 2016). However, these studies in planta could only be performed from heavily colonized plants, as limited pathogen biomass has hindered until recently the investigation of gene expression at the early stages of the interaction, when plants are still asymptomatic.

In a previous work, we demonstrated that rRNA-depleted RNAs obtained from infected roots could be used to determine the transcriptomic responses of S. commersonnii plants resistant or susceptible to bacterial wilt through RNA sequencing (Zuluaga et al., 2015). Here, we have used these sequences to extract R. solanacearum UY031 transcripts in silico and have compared them to the bacterial transcriptomes obtained in synthetic media to investigate the pathogen RNAs expressed during early infection. Our results reveal differential expression of a number of known and putative transcriptional regulators and virulence factors during early plant colonization, providing insight into their role in infection.

Materials and methods

Bacterial strains, plant accessions, and growth conditions

The R. solanacearum isolate UY031, phylotype IIB, sequevar 1, originally isolated from potato (Siri et al., 2011), carrying the LUX-operon under the psbA promoter (Monteiro et al., 2012) was used for all experiments. Bacteria were routinely grown in rich B medium as described (Monteiro et al., 2012).

S. commersonnii accessions F97 (susceptible to bacterial wilt) and F118 (moderately resistant) obtained from a segregating population were used in this work and propagated in vitro as described (Zuluaga et al., 2015).

Sample preparation

As a control condition, bacteria were grown for 2 days on rich solid medium without tetrazolium chloride or antibiotics at the appropriate dilution to obtain separate colonies. Bacteria were recovered from plates and mixed with 5% of an ice-cold transcription stop solution [5% (vol/vol) water-saturated phenol in ethanol]. Cells were centrifuged at 4°C for 2 min at maximum speed and the bacterial pellet was immediately frozen in liquid nitrogen.

For plant RNA samples, S. commersonii F97 and F118 roots were inoculated as described in Zuluaga et al. (2015). Briefly, plant roots from 2-week old plants grown in soil were injured with a 1 ml pipette tip and inoculated by soil drenching with a bacterial solution at 107 colony forming units (cfu)/ml. Control plants were mock-inoculated with water. After inoculation, plants were kept in a growth chamber at 28°C in long-day conditions. Luminescence quantification was used to select plants with comparable infection levels in the susceptible and the resistant accessions, corresponding to approximately 105 colony forming units per g of tissue (Cruz et al., 2014).

RNA extraction, sequencing, and library preparation

Total RNA from bacterial cultures was extracted using the SV Total RNA Isolation System kit (Promega) following the manufacturer's instructions for Gram-negative Bacteria. Infected plant RNA extractions were carried out as described (Cruz et al., 2014). RNA concentration and quality was measured using the Agilent 2100 Bioanalyzer. For rRNA depletion, 2.5 μg of RNA were treated with the Ribo-zero(™) magnetic kit for bacteria (Epicenter). Three biological replicates per condition were subjected to sequencing on an Illumina-Solexa Genome Analyzer II apparatus in the Shanghai PSC Genomics facility using multiplexing and kits specially adapted to obtain 100 bp paired-end reads in stranded libraries. Raw sequencing data is available in the Sequence Read Archive under the accession code SRP096020.

Read mapping, quantification, and differential gene expression analysis

FASTQC was used to evaluate the quality of the RNA-seq raw data. R. solanacearum reads were identified from total infected root sequences using Bowtie2 (version 2.2.6; Langmead and Salzberg, 2012) as described in the results section. The completely sequenced genome of strain UY031 (Guarischi-Sousa et al., 2016) was used as reference. For identification of R. solanacearum reads, the Burrows-Wheeler Alignment (BWA) tool was initially used. However, a high number of reads from mock-inoculated control samples mapped to the bacterial genome (Table 1). Visual evaluation of these mapped reads using the Integrative Genomics Viewer (IGV) tool (Robinson et al., 2011; Thorvaldsdottir et al., 2013) showed that most contained mismatches to the R. solanacearum genome sequence, indicating that they likely belonged to contaminating bacteria. BWA was thus assayed with more stringent parameters (-B 20-O 30-E 5-U 85), to increase penalties for mismatches, gap openings, gap extension, and unpaired read pairs, resulting in a reduction of only half of the reads mapping to the genome. Finally, Bowtie2 was assayed, once more using stringent parameters to penalize mismatches and gaps (–mp 30–rdg 25,15–rfg 25,15). In this case, mapped reads levels in mock-inoculated plants could be considered background compared to the high read numbers from inoculated samples, thus, Bowtie2 was finally used in all samples analyzed, including RNA-seq reads coming from in vitro grown bacteria (Table 1). Alignments were summarized by genes on counting tables using HTSeq-count (version 0.6.1 p1; Anders et al., 2015) and NCBI's reference annotation (genome features were extracted from NCBI's RefSeq sequences NZ_CP012687.1 and NZ_CP012688.1); alignments with quality lower than 10 were discarded. Differential expression (DE) analysis was carried out with the DESeq2 (version 1.12.3; Love et al., 2014) package in R (version 3.3.2). Benjamini–Hochberg procedure was used for multiple testing corrections. Genes with log2(fold-change) > 0.5 and q < 0.01 were considered as differentially expressed. We used these thresholds to select for relevant and robust differentially expressed genes. Final annotation of the genome was defined based on the NCBI gene locus and the gene name and description of the reference R. solanacearum GMI1000 genome annotation (Supplementary Table 1).

Table 1.

Number and percentage of aligned reads to the R. solanacearum UY031 genome from mock-inoculated (Control) and inoculated Solanum commersonii accessions.

BWAa BWA_stringentb Bowtie2_stringent
Conditionc Replica Total reads Reads % Reads % Reads %
Resistant mock-inoculated 1 83867508 110859 0.1 66083 0.1 601 0.0
2 88913944 42040 0.0 25296 0.0 771 0.0
Resistant infected 1 71855042 348369 0.5 330968 0.5 290036 0.4
2 96470501 943974 1.0 924297 1.0 879112 0.9
3 23473454 249285 1.1 234153 1.0 183728 0.8
Susceptible mock-inoculated 1 100234418 70173 0.1 40797 0.0 300 0.0
2 27594608 15060 0.1 8889 0.0 137 0.0
Susceptible infected 1 75368620 249382 0.3 232550 0.3 211561 0.3
2 93023963 2103356 2.3 2010284 2.2 1867585 2.0
3 24695183 518872 2.1 484873 2.0 410525 1.7
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a

Burrows-Wheeler Alignment.

b

Burrows-Wheeler Alignment using stringent parameters as described in methods.

c

Samples from Zuluaga, Solé, Lu, BMC Genomics, 2015.

Homology analysis

get_homologs (version 2.0; Contreras-Moreira and Vinuesa, 2013) was used for searching R. solanacearum UY031 homologous genes on R. solanacearum GMI1000, R. solanacearum IPO1609 and R. solanacearum UW551 strains as well as in Pseudomonas syringae pv. syringae B728a; NCBI RefSeq sequences GCF_001299555.1, GCF_000009125.1, GCF_001050995.1, GCF_000167955.1, and GCF_000012245.1, respectively. Default algorithm of bidirectional best-hits was used on homologous genes search.

Functional categories

R. solanacearum UY031's genes were functionally categorized using two different strategies. Firstly, functional categories from Pseudomonas syringae pv. syringae B728a as defined by Yu et al. (2013), were translated to R. solanacearum UY031 based on homology information between the two strains. Although the P. syringae-derived categories should be more specific and accurate for another bacterial plant pathogen, almost 70% of the R. solanacearum UY031 genes could not be classified using this method. Therefore, a second strategy based on Clusters of Orthologous Groups (COG) categories was applied. Genome features were extracted from NCBI's RefSeq annotation and cdd2cog.pl script (version 0.1; Leimbach, 2016) was used to assign COG IDs and functional categories to the differentially expressed genes (Supplementary Table 1).

Results

Obtaining R. solanacearum sequences from infected root tissues

cDNA libraries from rRNA-depleted RNAs isolated from S. commersonii roots inoculated with R. solanacearum were sequenced using Illumina technology as previously reported (Zuluaga et al., 2015). To generate the transcriptomic profile of the bacteria growing inside root tissues, R. solanacearum UY031 sequences were obtained following the pipeline detailed in Figure 1. First, reads from mock-inoculated plants were used as a control to determine the best alignment tool to map against the R. solanacearum UY031 reference genome (Guarischi-Sousa et al., 2016; see material and methods). The Bowtie2 alignment tool with stringent parameters was used, as it retained a number of R. solanacearum reads in mock-inoculated plants that could be considered background levels compared to the high read numbers from inoculated samples (Table 1). All samples were analyzed with Bowtie2, including RNA-seq reads coming from in vitro grown bacteria. We determined that around 1% of the total sequenced reads from plant tissues corresponded to R. solanacearum and these were retained for further analyses. S. commersonnii sequences accounted on average for 63.15% of the total reads sequenced and the remaining reads corresponded mostly to contamination by other bacterial endophytes. The retrieved bacterial sequences were quantified and differentially expressed (DE) genes comparing the different conditions were determined. Total RNAs from infected S. commersonii enabled transcript quantification for over 96% of R. solanacearum UY031 predicted genes (4,609 out of the 4,778; Guarischi-Sousa et al., 2016).

Figure 1.

Figure 1

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Workflow of the transcriptomic analysis. RNAseq was carried out from roots of infected and mock-inoculated Solanum commersonii resistant and susceptible varieties and from bacteria grown in solid rich B medium. Three biological replicates were used for each condition. Total extracted RNAs were treated with Ribo-zero to remove rRNA and sequenced using Illumina technology. Raw reads were aligned against the R. solanacearum UY031 genome using different alignment tools and mapping was visually evaluated with the IGV Browser. Mapped reads were quantified using count tables and differential expression (DE) analysis was carried out.

Similar R. solanacearum genes are differentially expressed upon infection of resistant and susceptible S. commersonii plants

In order to compare the R. solanacearum gene expression patterns during infection of resistant and susceptible wild potato plants, we analyzed separately the bacterial reads obtained from infected S. commersonii accessions F118 and F97, respectively. Surprisingly, only two out of the 4,609 genes for which expression was detected showed differential expression between the two genotypes. The differentially-expressed (DE) genes, RSUY_RS08455, and RSUY_RS16950, were both up-regulated in bacteria grown inside the resistant accession (Table 2). The first gene corresponds to an uncharacterized member of the MarR transcriptional regulator family, while the second encodes a hypothetical protein.

Table 2.

R. solanacearum UY031 genes differentially expressed in resistant vs. susceptible S. commersonii.

UY031 NCBI locusa UY031 Prokka locusb GMI1000 locusc Gene product Log2FC Adjusted p-value
RSUY_RS08455 RSUY_17320 RSc1295 MarR family transcriptional regulator 2.37 0.0004
RSUY_RS16950 RSUY_34650 RSp0403 hypothetical protein 2.53 0.0017
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a

According to R. solanacearum UY031 genome annotation available at GenBank (NCBI).

b

According to R. solanacearum UY031 genome annotation from Guarischi-Sousa et al. (2016).

c

According to the homology Supplementary Table 1.

Since R. solanacearum showed extremely similar (>99.9%) transcriptional behavior during interaction with both S. commersonii accessions, bacterial reads from both accessions were treated as biological replicates in the rest of this study.

R. solanacearum activates stress-related genes and shuts down metabolic activities during early root colonization

The R. solanacearum in planta gene expression dataset was compared to a reference condition consisting of bacteria grown on solid rich B medium. Bacteria grown on solid medium were used as the reference condition instead of liquid cultures. R. solanacearum colonies grown on solid media better mimic the biofilms and microcolonies formed by R. solanacearum during early infection, when most bacteria occupy plant intercellular spaces (Mori et al., 2016). A total of 422 genes were differentially expressed during pre-symptomatic infection (231 up-regulated and 191 down-regulated), compared to growth on rich medium (Supplementary Table 2). These DE genes were classified into the functional categories previously used for gene expression studies in the plant pathogenic bacterium P. syringae (Yu et al., 2013; Supplementary Table 3). The number of successfully classified genes in each category was quantified in differentially induced or repressed groups and in the whole genome as a reference (Figure 2). This analysis revealed four categories highly over-represented in the up-regulated genes and under-represented in down-regulated genes: stress, secretion, chemosensing, and motility and phage and insertion sequences (IS). These categories represent together approximately 20% of the total induced genes in planta. The opposite trend (under-representation in up-regulated and over-representation in down-regulated genes) is observed in the categories including genes for transport and metabolism of amino acids and carbohydrates. In addition, the categories replication and DNA repair, transport, fatty acid metabolism and cofactor metabolism are strongly under-represented amongst the up-regulated genes in planta (Figure 2).

Figure 2.

Figure 2

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Percentage of DE genes classified into Pseudomonas syringae-derived functional categories (Yu et al., 2013). Genes DE between growth in planta vs. rich medium were classified according to the functional categories described for P. syringae (Yu et al., 2013). Categories were grouped by function similarity for better visualization (Supplementary Table 4). As a reference, functional category distribution considering all annotated genes in the UY031 genome is shown.

We used the P. syringae categories because they were created to describe the genes of a bacterial plant pathogen and are thus very informative for this study. However, the same analysis was carried out using the widely used but more general COG categories, and the results confirmed the previously-described tendencies (Supplementary Figure 1). Genes involved in carbohydrate, amino acid, lipid, cofactor, and secondary metabolism were over-represented among those down-regulated in planta. A clear enrichment of replication, cell motility and recombination and repair (where IS elements are included) was observed in the up-regulated genes. Interestingly, a clear asymmetry was seen for unclassified genes in this case, for they represent 40% of the up-regulated but only 7% of the down-regulated genes.

Closer scrutiny of the up-regulated genes in the plant revealed that the category secretion included 11 genes encoding the T3SS and its associated effectors and four chemosensing and motility genes, coding for pilus assembly and flagellum transcriptional activators (Table 3).

Table 3.

R. solanacearum UY031 genes differentially expressed in potato roots vs. solid rich medium.

Function UY031 NCBI locusa UY031 Prokka locusb GMI1000 locusc Log2FC Gene name Gene product
RALSTONIA SOLANACEARUM VIRULENCE GENES
Type III secretion system and effectors RSUY_RS19685 RSUY_40420 RSp0855 7.80 hrpY Type III secretion system protein HrpY
RSUY_RS19795 RSUY_40640 RSp0877 4.66 popA Type III effector protein PopA
RSUY_RS19790 RSUY_40630 RSp0876 4.27 popB Type III effector protein PopB
RSUY_RS20380 RSUY_41860 RSp1024 3.96 awr5_1 Type III effector protein AWR5
RSUY_RS22080 RSUY_45370 RSp0900 3.94 popF1 Type III effector protein PopF1
RSUY_RS16550 RSUY_33840 RSp0304 3.76 ripD Type III effector protein RipD
RSUY_RS19785 RSUY_40620 RSp0875 3.35 popC Type III effector protein PopC
RSUY_RS19735 RSUY_40520 RSp0865 3.08 hrpK Type III secretion system protein HrpK
RSUY_RS19690 RSUY_40430 RSp0856 2.86 hrpX Type III secretion system protein HrpX
RSUY_RS19770 RSUY_40590 RSp0872 2.69 hrcT HrcT family type III secretion system export apparatus protein
RSUY_RS09370 RSUY_19160 2.44 ripV2 Type III effector protein RipV2
RSUY_RS19150 RSUY_39290 RSp0731 −2.61 ripTPS Trehalose-6-phosphate synthase
RSUY_RS21730 RSUY_44630 RSp1374 −2.88 ripS2 Type III effector protein SKWP2
RSUY_RS21610 RSUY_44390 RSp1277 −3.50 ripQ Type III effector protein RipQ
Motility RSUY_RS04635 RSUY_09450 RSc0727 3.14 pilV Type IV pilus modification protein PilV
RSUY_RS22435 RSUY_46110 RSp1412 2.65 flhC Transcriptional activator FlhC
RSUY_RS02415 RSUY_04970 RSc2974 2.62 pilN Tfp pilus assembly protein PilN
RSUY_RS22440 RSUY_46120 RSp1413 2.47 flhD Flagellar transcriptional activator FlhD
RSUY_RS04630 RSUY_09440 RSc0726 2.30 pilW Pilus assembly protein PilW
RSUY_RS02410 RSUY_04960 RSc2975 2.28 pilM Pilus assembly protein PilM
RSUY_RS04330 RSUY_08850 RSc0668 2.20 pilG Two-component system response regulator
RSUY_RS04335 RSUY_08860 RSc0669 1.95 pilH Two-component system response regulator
RSUY_RS11250 RSUY_22930 RSc1986 1.24 fimV Tfp pilus assembly protein FimV
RSUY_RS04590 RSUY_09370 RSc0718 −3.56 pilY Pilus assembly protein PilY
Stress responses RSUY_RS22220 RSUY_45660 RSp1581 3.16 katE Catalase katE
RSUY_RS00425 RSUY_00900 RSc3398 3.10 hmpX flavohemoprotein
RSUY_RS17495 RSUY_35830 RSp0245 2.64 ahpC1 Peroxiredoxin
RSUY_RS17500 RSUY_35840 RSp0246 2.21 ahpF Alkyl hydroperoxide reductase subunit F
RSUY_RS04770 RSUY_09720 RSc0754 1.96 Peroxidase
RSUY_RS04870 RSUY_09930 RSc0775 1.82 katGb Catalase katGb
RSUY_RS01185 RSUY_02450 RSc3254 −3.11 alkyl hydroperoxide reductase
Other virulence factors RSUY_RS18925 RSUY_38830 RSp0676 3.71 metE Methionine synthase II (cobalamin-independent)
RSUY_RS01465 RSUY_03030 RSp0693 3.38 hdfA Dioxygenase
RSUY_RS14015 RSUY_28660 RSc0408 2.22 rpoN1 RNA polymerase sigma-54 factor
RSUY_RS17795 RSUY_36440 RSp1529 1.72 efe 2-oxoglutarate-dependentethylene/succinate-forming enzyme
RSUY_RS04455 RSUY_09100 RSc0693 −2.19 kdtA 3-deoxy-D-manno-octulosonic-acid transferase
Type II Secretion System RSUY_RS01675 RSUY_03470 RSc3109 −2.63 gspJ General secretion pathway protein GspJ
RSUY_RS16275 RSUY_33280 RSp0148 −3.19 gspE General secretion pathway protein GspE
Type VI secretion system RSUY_RS19215 RSUY_39440 RSp0746 2.25 Type VI secretion protein
Cofactor metabolism and transport RSUY_RS04050 RSUY_08280 RSc2633 −2.92 pabB aminodeoxychorismate synthase component I
Quorum sensing RSUY_RS01010 RSUY_02100 RSc3286 −3.24 solI Acyl-homoserine-lactone synthase
RALSTONIA SOLANACEARUM GENES INVOLVED IN PLANT COLONIZATION
Aminoacid metabolism RSUY_RS21930 RSUY_45070 RSp1263 2.019462 nadB2 L-aspartate oxidase
RSUY_RS04790 RSUY_09760 RSc0758 1.900185 Tryptophan 2,3-dioxygenase 1
RSUY_RS01705 RSUY_03530 RSc3103 −1.93219 4-hydroxyphenylpyruvate dioxygenase
RSUY_RS00955 RSUY_01990 RSc3295 −1.97096 gcvP glycine dehydrogenase
RSUY_RS00965 RSUY_02010 RSc3293 −2.1387 gcvT aminomethyltransferase
RSUY_RS08880 RSUY_18160 RSc1381 −2.22786 glutathione ABC transporter permease GsiC
RSUY_RS02965 RSUY_06080 RSc2867 −2.45751 dppD1 peptide ABC transporter substrate-bindingprotein
RSUY_RS19000 RSUY_38980 RSp0691 −2.63642 hmgA homogentisate 1,2-dioxygenase
RSUY_RS08860 RSUY_18120 RSc1377 −2.72373 transcriptional regulator
RSUY_RS00950 RSUY_01980 RSc3296 −2.82715 sdaA2 L-serine ammonia-lyase / L-serine ammonia-lyase
RSUY_RS18995 RSUY_38970 RSp0690 −2.93699 hmgB fumarylacetoacetase
RSUY_RS08895 RSUY_18190 RSc1384 −3.10843 D-aminopeptidase
RSUY_RS08865 RSUY_18130 RSc1378 −3.44342 isoaspartyl peptidase
Carbohydrate metabolism RSUY_RS22935 RSUY_47230 RSp1633 −1.90617 xylF D-xylose ABC transporter substrate-bindingprotein
RSUY_RS22945 RSUY_47250 RSp1635 −2.40016 xylH xylose ABC transporter permease
RSUY_RS21965 RSUY_45140 RSp1270 −2.4781 glycosyl hydrolase
RSUY_RS22940 RSUY_47240 RSp1634 −2.98048 xylG D-xylose ABC transporter ATP-binding protein
RSUY_RS17060 RSUY_34910 RSp0423 −3.65067 aldolase
RSUY_RS22950 RSUY_47260 RSp1636 −4.75552 NAD-dependent dehydratase
Transcriptional and response regulators RSUY_RS08455 RSUY_17320 RSc1295 4.365537 MarR family transcriptional regulator
RSUY_RS22955 RSUY_47270 RSp1637 −1.62836 LacI family transcriptional regulator
RSUY_RS06090 RSUY_12470 RSc2209 −1.75486 LysR family transcriptional regulator
RSUY_RS00225 RSUY_00480 RSc0040 −2.26596 two-component system response regulator
RSUY_RS00910 RSUY_01900 RSc3301 −2.57757 putA trifunctional transcriptional regulator
Siderophore biosynthesis RSUY_RS17055 RSUY_34900 RSp0422 −2.30463 siderophore biosynthesis protein
RSUY_RS03590 RSUY_07350 RSc2729 −2.4997 membrane protein / membrane protein
RSUY_RS17040 RSUY_34870 RSp0419 −2.75083 siderophore biosynthesis protein
RSUY_RS17050 RSUY_34890 RSp0421 −2.94313 siderophore biosynthesis protein
Nitrogen metabolism RSUY_RS14025 RSUY_28680 RSc0406 2.27 ptsN PTS IIA-like nitrogen-regulatory protein PtsN
RSUY_RS17995 RSUY_36860 RSp0980 2.24 narL DNA-binding response regulator
RSUY_RS11470 RSUY_23380 RSc2031 −3.3167 ureE urease accessory protein UreE
Transporters RSUY_RS20760 RSUY_42660 RSp1283 2.005142 porin
RSUY_RS11090 RSUY_22610 RSc1951 −2.22 cation acetate symporter
RSUY_RS22930 RSUY_47220 RSp1632 −2.42488 oprB porin
RSUY_RS05795 RSUY_11880 RSc2274 −2.96894 ragC Cation efflux protein
Organic acid metabolism RSUY_RS19540 RSUY_40110 RSp0826 3.403389 5-dehydro-4-deoxyglucarate dehydratase
RSUY_RS19480 RSUY_39990 RSp0814 2.44631 mqo malate:quinone oxidoreductase
RSUY_RS11960 RSUY_24410 RSc2358 −1.7429 ppc phosphoenolpyruvate carboxylase
Proteases RSUY_RS12475 RSUY_25460 RSc2465 2.359347 clpS ATP-dependent Clp protease adaptor ClpS
RSUY_RS18550 RSUY_38040 RSp0603 2.211049 serine protease
RSUY_RS14120 RSUY_28870 RSc0388 −1.98903 zinc protease
Lipid metabolism RSUY_RS17295 RSUY_35410 2.478807 Acyl-CoA synthetase
RSUY_RS01975 RSUY_04090 RSc3052 −2.40887 glpK glycerol kinase
Energy RSUY_RS08510 RSUY_17430 RSc1305 3.640811 fpr ferredoxin–NADP(+) reductase
RSUY_RS08360 RSUY_17120 RSc1276 3.417949 cytochrome c oxidase, cbb3-type subunit I
Signal transduction RSUY_RS23055 RSUY_47460 RSc0617 1.988909 signal peptidase
RSUY_RS01700 RSUY_03520 RSc3104 1.73953 calcium sensor EFh
Stress related RSUY_RS13090 RSUY_26760 RSc0582 2.610905 avrD-like protein
RSUY_RS21705 RSUY_44580 RSp1306 −2.11404 speE2 spermidine synthetase
Cofactor metabolism and transport RSUY_RS02845 RSUY_05840 RSc2886 −2.57058 adenylate cyclase
Recombination and repair RSUY_RS07890 RSUY_16140 RSc1189 −2.09233 recombinase RecB
Translation RSUY_RS15445 RSUY_31580 RSc0085 −2.70405 cca multifunctional CCA protein
Hypothetical proteins RSUY_RS19605 RSUY_40240 4.758974 hypothetical protein
RSUY_RS17575 RSUY_35990 RSp0261 4.146986 membrane protein
RSUY_RS16950 RSUY_34650 RSp0403 3.74634 hypothetical protein
RSUY_RS22040 RSUY_45290 RSp0982 3.589851 hypothetical protein
RSUY_RS12885 RSUY_26330 RSc0613 3.409348 hypothetical protein
RSUY_RS08290 RSUY_16960 RSc1262 3.394474 hypothetical protein
RSUY_RS06775 RSUY_13900 RSc0971 3.025981 hypothetical protein
RSUY_RS20375 RSUY_41850 3.019263 hypothetical protein
RSUY_RS01105 RSUY_02290 RSc3270 2.806237 hypothetical protein
RSUY_RS15470 RSUY_31630 RSc0080 2.792044 hypothetical protein
RSUY_RS14600 RSUY_29830 RSc0297 2.641501 hypothetical protein
RSUY_RS05760 RSUY_11810 RSc2280 2.552951 hypothetical protein
RSUY_RS10215 RSUY_20850 RSc1622 2.233892 hypothetical protein
RSUY_RS12820 RSUY_26200 2.213444 hypothetical protein
RSUY_RS22015 RSUY_45240 RSp1546 2.185718 hypothetical protein
RSUY_RS01435 RSUY_02950 RSc0616 2.148496 hypothetical protein
RSUY_RS06705 RSUY_13730 RSc0953 2.116755 hypothetical protein
RSUY_RS01875 RSUY_03890 RSc3072 2.098485 hypothetical protein
RSUY_RS04190 RSUY_08560 RSc2555 1.909667 membrane protein
RSUY_RS05940 RSUY_12170 RSc2238 1.775776 hypothetical protein
RSUY_RS04990 RSUY_10170 RSc0799 −1.56204 hypothetical protein
RSUY_RS02135 RSUY_04410 RSc3030 −2.05111 hypothetical protein
RSUY_RS20585 RSUY_42270 −2.22451 membrane protein
RSUY_RS14980 RSUY_30600 RSc0211 −2.4077 membrane protein
RSUY_RS17045 RSUY_34880 RSp0420 −2.58002 membrane protein
RSUY_RS15175 RSUY_31000 RSc0146 −2.83465 hypothetical protein
PUTATIVE VIRULENCE GENES AND PLANT COLONIZATION METABOLIC ACTIVITIES
Transporters RSUY_RS00490 RSUY_01050 RSc3386 3.50 metal ABC transporter substrate-binding protein
RSUY_RS17605 RSUY_36050 RSp0429 3.24 MFS transporter
RSUY_RS20020 RSUY_41100 RSp0931 2.92 ABC transporter
RSUY_RS19045 RSUY_39070 RSp0706 −1.77 metal-dependent hydrolase
RSUY_RS18205 RSUY_37320 RSp0481 −2.03 ABC transporter substrate-binding protein
RSUY_RS18195 RSUY_37300 RSp0479 −2.09 amino acid ABC transporter ATPase
RSUY_RS21220 RSUY_43600 RSp1181 −2.11 transporter
RSUY_RS18895 RSUY_38770 RSp0670 −2.14 acriflavine resistance protein B / transporter protein
RSUY_RS17425 RSUY_35690 RSp0234 −2.37 MFS transporter
RSUY_RS09885 RSUY_20190 RSc1738 −2.40 ABC transporter ATPbinding protein
RSUY_RS21615 RSUY_44400 RSp1278 −2.49 MFS transporter
RSUY_RS21315 RSUY_43800 RSp1200 −2.60 RND transporter
RSUY_RS03020 RSUY_06190 RSc2856 −2.72 MFS transporter
RSUY_RS01560 RSUY_03230 RSc3134 −2.94 MFS transporter
RSUY_RS06940 RSUY_14230 RSc1002 −2.95 membrane protein
RSUY_RS15855 RSUY_32410 −2.98 oprM RND transporter
RSUY_RS20395 RSUY_41890 −2.99 ybtP ABC transporter ATP-binding protein
RSUY_RS15985 RSUY_32660 RSp0078 −3.05 MFS transporter
RSUY_RS18200 RSUY_37310 RSp0480 −3.17 amino acid ABC transporter permease
RSUY_RS19050 RSUY_39080 RSp0707 −3.19 ABC transporter ATP-binding protein
RSUY_RS21055 RSUY_43260 RSp1114 −3.35 RND transporter
RSUY_RS01890 RSUY_03920 RSc3069 −3.50 MFS transporter
RSUY_RS22255 RSUY_45730 RSp1595 −3.73 ABC transporter ATP-binding protein
RSUY_RS04055 RSUY_08290 RSc2632 −3.85 ABC transporter ATP-binding protein
Lipid metabolism RSUY_RS14075 RSUY_28780 RSc0396 3.29 ipk 4-diphosphocytidyl-2C-methyl-D-erythritolkinase
RSUY_RS10705 RSUY_21830 RSc1540 3.14 acyltransferase
RSUY_RS19325 RSUY_39670 2.15 Phosphatidylserine/phosphatidylglycerophosphate/cardiolipin synthase
RSUY_RS09620 RSUY_19650 RSc1772 −2.06 alpha/beta hydrolase
RSUY_RS14790 RSUY_30210 RSc0262 −2.17 glyoxylate/hydroxypyruvate reductase A
RSUY_RS00675 RSUY_01440 RSc3346 −2.24 alpha/beta hydrolase
RSUY_RS13905 RSUY_28430 RSc0427 −2.30 beta-ketoacyl-[acyl-carrier-protein] synthaseII
RSUY_RS09090 RSUY_18590 −2.77 Lysophospholipase
RSUY_RS01035 RSUY_02150 RSc3283 −2.82 glxR 2-hydroxy-3-oxopropionate reductase
RSUY_RS10955 RSUY_22330 RSc1874 −2.82 NUDIX hydrolase
RSUY_RS14265 RSUY_29170 RSc0357 −2.86 gpsA glycerol-3-phosphate dehydrogenase (NAD(P)(+))
RSUY_RS11775 RSUY_23990 RSc2091 −3.04 ABC transporter permease
RSUY_RS15945 RSUY_32580 RSp0036 −3.05 acyl-CoA dehydrogenase
RSUY_RS21855 RSUY_44890 RSp1245 −3.30 esterase
RSUY_RS20415 RSUY_41930 −3.31 Acyl-coenzyme A synthetase
RSUY_RS21590 RSUY_44350 −3.32 Dehydrogenases
RSUY_RS20425 RSUY_41950 −3.60 Polyketide synthase
RSUY_RS14720 RSUY_30070 RSc0275 −3.61 short-chain dehydrogenase
RSUY_RS10105 RSUY_20630 RSc1643 −4.27 ispD 2-C-methyl-D-erythritol 4-phosphatecytidylyltransferase
Other putative virulence factors RSUY_RS16085 RSUY_32860 RSp0112 2.09 carbonic anhydrase
RSUY_RS00735 RSUY_01550 RSp0085 1.66 type IV secretion protein Rhs
RSUY_RS00905 RSUY_01890 RSc3302 −2.04 priA primosomal protein N'
RSUY_RS15535 RSUY_31760 RSc0068 −2.06 smf DNA processing protein DprA
RSUY_RS14955 RSUY_30550 RSc0222 −2.29 rtcR Fis family transcriptional regulator
RSUY_RS17190 RSUY_35180 RSp0181 −3.10 activator of HSP90 ATPase
RSUY_RS14940 RSUY_30520 RSc0226 −3.23 rtcA RNA 3'-terminal phosphate cyclase
Sulfur metabolism and transport RSUY_RS12265 RSUY_25040 RSc2425 3.22 cysI1 Sulfite reductase/sulfite reductase
RSUY_RS07020 RSUY_14390 RSc1019 2.23 nifS Cysteine desulfurase IscS
RSUY_RS12250 RSUY_25010 RSc2422 2.14 cysD Sulfate adenylyltransferase small subunit
RSUY_RS12245 RSUY_25000 RSc2421 1.89 cysN Sulfate adenylyltransferase
RSUY_RS07025 RSUY_14400 RSc1020 1.60 nifU Iron-sulfur cluster scaffold-like protein
RSUY_RS17845 RSUY_36540 RSp1519 −3.36 Membrane protein
Cofactor metabolism and transport RSUY_RS11705 RSUY_23850 RSc2077 1.85 ilvI acetolactate synthase
RSUY_RS18660 RSUY_38270 RSp0615 −2.97 cbiA cobyrinic acid a,c-diamide synthase
RSUY_RS18690 RSUY_38330 RSp0621 −2.97 cbiL precorrin-2 C(20)-methyltransferase
RSUY_RS18680 RSUY_38310 RSp0619 −3.00 cbiG cobalamin biosynthesis protein CbiG
RSUY_RS03905 RSUY_07990 RSc2663 −3.51 ATP:cob(I)alamin adenosyltransferase
Phosphate mobilization RSUY_RS10765 RSUY_21950 RSc1529 2.01 pstS1 phosphate ABC transporter substrate-bindingprotein PstS
RSUY_RS07715 RSUY_15790 RSc1160 1.63 suhB Inositol monophosphatase
RSUY_RS10750 RSUY_21920 RSc1532 1.52 pstB phosphate ABC transporter ATP-binding protein
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a

According to R. solanacearum UY031 genome annotation available at GenBank (NCBI).

b

According to R. solanacearum UY031 genome annotation from Guarischi-Sousa et al. (2016).

c

According to the homology Supplementary Table 1.

Taken together, these results show a major induction of stress-related activities and an inhibition of the central metabolism when the bacterium grows in planta compared to synthetic media.

R. solanacearum virulence genes are differentially expressed in wild potato roots

Among the 422 genes DE during S. commersonii root colonization, 34% (80 induced and 65 repressed genes) had been identified in previous studies analyzing gene expression of R. solanacearum cells recovered from infected plant stems (see references below). Notably, 73 genes were also DE in microarray analyses of R. solanacearum UW551 -a phylotype IIB strain highly similar to UY031- isolated from tomato (Jacobs et al., 2012). Also, 42 genes have been shown to be induced in a temperature-dependent manner when bacteria grew in tomato xylem or rhizosphere (Bocsanczy et al., 2014; Meng et al., 2015). In addition, 31 DE genes (most of them induced in planta) are part of either the HrpB or HrpG regulons, which are known to trigger expression of the T3SS and other virulence genes in response to direct plant cell contact (Valls et al., 2006).

Amongst the R. solanacearum genes induced during plant colonization, 31 encode already reported virulence traits (Table 3). As expected, genes encoding the T3SS (hrpY, hrpX, hrpK, hrcT) and some of its related effectors (ripV2, popC, ripD, popF1, awr5_1, popB, and popA) were induced inside the plant (Boucher et al., 1987; Cunnac et al., 2004). Motility and adherence genes were also up-regulated, including type IV pili (pilG, pilH, pilN, pilM, pilY, pilW, and fimV), as well as the transcriptional activators of the flagellum genes flhC and flhD (Kang et al., 2002; Tans-Kersten et al., 2004). Other induced genes encoding described factors that are key for bacterial virulence included hdfA (Delaspre et al., 2007), efe (Valls et al., 2006), metE (Plener et al., 2012), and rpoN1 (Lundgren et al., 2015; Ray et al., 2015; Table 3). Peroxidases, catalases (katE, katG) and alkyl hydroperoxide reductases (ahpC1, ahpF), which have been described to combat the oxidative stress response during plant infection (Rocha and Smith, 1999; Flores-Cruz and Allen, 2009; Ailloud et al., 2016) were also induced. Similarly, the flavohemoprotein hmpX, involved in NO-detoxification (Dalsing and Allen, 2014), was also induced.

In contrast, only 10 reported virulence determinants were down-regulated, including the type III effectors ripQ, ripS2, and ripTPS, the quorum sensing regulator solI (Flavier et al., 1997) and the Type II secretion system genes gspE, gspJ (Table 3).

R. solanacearum genes for plant colonization are differentially expressed in S. commersonii roots

Thirty-six R. solanacearum genes previously described as related to plant colonization in gene expression studies in other plant species were also induced in potato. Few metabolic genes were induced in planta, being an exception nadB2, involved in the degradation of L-aspartate in the xylem (Brown and Allen, 2004) and the ptsN and narL nitrogen metabolism genes, known to be active during plant colonization (Dalsing and Allen, 2014; Dalsing et al., 2015; Table 3).

Amongst the down-regulated genes, 42 had also been described as specifically down-regulated during plant colonization (Jacobs et al., 2012). Most repressed genes encoded metabolic enzymes and transporters. Examples are the xylose transporters xylF, xylG, and xylH, glycine catabolism genes gcvP, gcvT, and gcvA, the adenilate cyclase coding gene RSUY_RS02845, four siderophore biosynthesis genes and 11 genes involved in amino acid metabolism (Table 3). Also, the stress response gene speE2 and five transcriptional and response regulators were repressed in planta.

Novel putative virulence genes and metabolic traits involved in early stages of wild potato infection by R. solanacearum

Transcriptomic analysis of S. commersoni early root infection revealed highly induced R. solanacearum virulence factors still uncharacterized in this pathogen that may play a role at this stage of the interaction with the host. An example of this is suhB, a global virulence regulator controlling the type III and type VI secretion systems, flagellum biosynthesis, and biofilm formation in the human pathogens Burkholderia cenocepacia and Pseudomonas aeruginosa (Rosales-Reyes et al., 2012; Li et al., 2013). Similarly, a P. aeruginosa orthologue of the in planta induced type IV secretion gene Rhs has been described as a virulence determinant (Kung et al., 2012).

Metabolic traits that might be key at this point of plant infection are the assimilatory sulfate reduction pathway and phosphate mobilization, since cysD, cysN, and cysI (sulfate reduction) and pstB and pstS1 (phosphate mobilization) were induced during S. commersonii root infection. Also, carbonic anhydrase (RSUY_RS16085), which plays a role in disease establishment between potato and Phytophthora infestans (Restrepo et al., 2005), was also found to be up-regulated in the R. solanacearum interaction with wild potato.

The most important category amongst the R. solanacearum genes down-regulated in S. commersonii with so far no assigned functions in plant colonization or virulence was metabolite transporters. Almost half of these corresponded to the ABC-family, including five amino acid transporters. In contrast, the seven major facilitator superfamily (MFS) transporters found in this category are involved with carbohydrate transport. The rest of genes were classified as permeases or RND (Resistance-Nodulation-Division) efflux systems (Table 3). The major metabolic activities identified as repressed in planta for the first time were lipid mobilization and cofactor metabolism, such as the anaerobic cobalamin biosynthesis operon (cbiA, cbiG, and cbiL), and stress-response genes such as rtcA and rtcR, involved in RNA repair (Das and Shuman, 2013).

In sum, our work reflects important gene expression changes between parasitic life and growth in rich medium (see below). This was corroborated by the fact that seven genes annotated as response regulators were also DE, five of them induced (Table 3).

Discussion

Some R. solanacearum virulence and stress-responsive genes are induced irrespective of the plant host

1/3 of the R. solanacearum genes DE during potato infection had been also found DE when the bacterium colonized other plant species and many of these correspond to virulence determinants. For instance, we found that genes encoding the type III secretion system and its associated effectors (popA, popB, popC, popF1, ripD, ripV2, and awr5_1) were induced in potato (Table 3). Except for awr5_1, all these effectors had already been described as up-regulated when the bacterium grew in tomato and in melon (Ailloud et al., 2016), likely indicating that they are part of the minimal gene set required for bacterial virulence. Similarly, the effector ripTPS was down-regulated both in potato (Table 3) and during the interaction with melon (Ailloud et al., 2016). Also sharing similar up-regulation in potato (Table 3) and tomato are the transcriptional activators flhC and flhD (Jacobs et al., 2012), which regulate flagellum-encoding genes (Tans-Kersten et al., 2004) and the nitrogen metabolism genes narL, ptsN, and hmpX (Dalsing and Allen, 2014; Dalsing et al., 2015), implying that they all play a key role during plant infection. Additional genes induced during potato colonization had been described as key for virulence on other plant hosts, including small molecule hdfA (Delaspre et al., 2007), the ethylene forming enzyme efe (Valls et al., 2006), the methionine metabolism gene metE (Plener et al., 2012) and the alternative sigma factor rpoN1 (Lundgren et al., 2015; Ray et al., 2015). These factors may be also considered essential for growth in planta, irrespective of the infected species.

Several transposable elements had been identified in an in vivo screening for genes expressed during R. solanacearum growth in tomato plants (Brown and Allen, 2004), and we found 16 transposases up-regulated in potato (Table 3). This may reflect common stressing conditions in various plant hosts, as stress is known to turn on transcription of transposable elements in various organisms (Capy et al., 2000). Oxidative stress seems also a condition generally encountered by R. solanacearum in plant tissues, as peroxidases, catalases, and peroxiredoxins, required for the bacterium to combat this stress in different plants (Rocha and Smith, 1999; Flores-Cruz and Allen, 2009; Ailloud et al., 2016), were also induced in potato.

Changes in the host environment and/or the disease stage may account for opposing bacterial virulence gene expression in different plants

Some of the R. solanacearum virulence genes DE in potato showed opposite trends in other host plants. ripQ and ripS2, two of the three type III secreted effectors inhibited in potato were, respectively, upregulated and not DE in melon, tomato and banana (Ailloud et al., 2016). Interestingly, these two downregulated effectors, together with the also repressed stress response gene speE2, are located in a genomic region that is deleted in the avirulent R. solanacearum strain UY043 (Siri et al., 2014), which suggests their involvement in bacterial virulence. Similarly, the effector awr5_1, which was described to trigger hypersensitive response (HR) in tobacco and to inhibit the TOR pathway (Sole et al., 2012; Popa et al., 2016b), showed opposite regulation in potato when compared to tomato and melon (Ailloud et al., 2016), suggesting that it may play host-specific roles. Similarly, genes pilG, pilH, pilN, pilM, pilY, and pilW, coding for structural components of the type IV pili involved in twitching motility and adherence (Liu et al., 2001; Kang et al., 2002) were induced in the current work but repressed in other plant species (Jacobs et al., 2012).

In addition, some virulence determinants well-described as induced during growth in planta were repressed or not DE in potato. Remarkably, the exopolysaccharide synthesis and regulation genes (eps) as well as most known cell wall degrading enzymes (pehA, pehB, pehC, egl, and cbhA), which are virulence determinants (Schell, 2000) induced during tomato infection (UW551 strain) infection (Jacobs et al., 2012) were absent from the potato DE dataset.

Differences in the host environment or in the tissue environment and disease stage are the two most plausible reasons for the discrepancies between virulence gene expression data in potato and in other plant hosts. We favor the latter explanation, as our samples were collected from bacteria growing in the root (including apoplastic and xylematic bacteria) at early times after inoculation while all previous transcriptomic work had been performed from bacteria extracted from xylem at later infection stages.

Three independent observations support the existence of stage-specific environmental cues that differentially affect gene expression in this work compared to previous studies. First, genes that are induced at high bacterial densities are absent from the potato DE genes. Examples are the mentioned exopolysaccharide synthesis genes or the quorum sensing regulator solI, repressed in our conditions but slightly induced in bacteria isolated from the tomato shoot xylem (Jacobs et al., 2012). In the low bacterial cell densities in the roots the phcA cell-density regulator was not induced, impeding solI or eps expression (Huang et al., 1995; Flavier et al., 1997). Second, three out of the six type III effectors that are induced in potato were described as secreted at early stages (Lonjon et al., 2016), two of them (popF1 and popA) also proposed to play an important role in the first steps of infection (Kanda et al., 2003). On the contrary, only two out of the 38 described as “late” effectors (ripD and popC) were induced in our root transcriptome. Third, the afore-mentioned transcriptional regulators flhC and flhD responsible for the activation of the flagellum genes were up-regulated in potato root samples (Table 3) and also in the tomato xylem (Jacobs et al., 2012), but only in the latter were the flagellum structural genes induced, suggesting that the potato transcriptome represents an earlier stage where complete activation of this regulon has not yet occurred. These observations imply that our transcriptome represents a snapshot of a precise stage of the genetic programs deployed consecutively during plant colonization.

Finally, we cannot rule out that changes in R. solanacearum DE genes in different studies are due to the use of different strains. Differing transcriptomes of two R. solanacearum strains in the same plant environment have already been reported (Ailloud et al., 2016). However, the fact that previous gene expression studies were performed with strain UW551, which is genetically extremely close to UY031 used here, render this explanation unlikely. Standardization of the plant inoculation and sampling procedures and a systematic analysis of plant-pathogen interactions dissecting gene expression over time in a defined strain-host pathosystem would clarify the nature of the observed discrepancies between transcriptomic studies.

The R. solanacearum metabolic state during potato root colonization

From the transcriptomic information gathered in this work, we can infer for the first time the environmental conditions encountered by R. solanacearum in the root, the site where plant infection takes place.

A first observation is that the bacterium seems to start to run out of O2. An indication of this is the highly induced Cbb3-cco, a high affinity cytochrome c oxidase known to contribute to the growth of R. solanacearum and other bacteria in microaerobic or anoxic environments (Colburn-Clifford and Allen, 2010; Hamada et al., 2014), such as the plant xylem (Pegg, 1985). Upregulation of the low O2 affinity cytochrome ubiquinol oxidase genes cyoA1 and cyoB1 reinforces the notion of a microaerobic rather than an anoxic environment. In agreement with this, nrdB, which is required for growth in aerobiosis (Casado et al., 1991), was up-regulated, and nrdG and nrdD, required in strict anaerobiosis (Garriga et al., 1996; Ailloud et al., 2016) were not induced. Further, the cbiA, cbiL, and cbiG genes, which are involved in anaerobic cobalamin synthesis (Roessner and Scott, 2006), were repressed. Another indication of microaerobic conditions is the induction of genes driving nitrate and sulfate anaerobic respiration. Examples are the cys genes, involved in the assimilatory sulfate reduction pathway (Kredich, 1992), ptsN—a nitrogen-dependent regulatory protein, rpoN1, -the global nitrogen regulator- and narL -the nitrate/nitrite-responsive transcriptional regulator- were all induced in wild potato roots. All these findings suggest that during early root infection R. solanacearum is experiencing the transition from an aerobic environment to the anaerobic conditions established at the onset of disease during xylem colonization (Ailloud et al., 2016).

Another take home message from the root transcriptomes is that few central metabolic pathways seem to be active. It was previously described that a large proportion of the R. solanacearum genes involved in amino acid metabolism and transport was down-regulated during growth in the xylem (Ailloud et al., 2016) and we found that this was also the case during growth in the root tissues at early stages of infection. For instance, the glycine catabolism genes gcvP, gcvT, and gcvA as well as the dipeptide uptake gene dppD1 were repressed in both cases (Table 3; Ailloud et al., 2016). Other R. solanacearum metabolic genes previously known to be repressed in planta also down-regulated here included carbohydrate metabolism genes such as the xylose transporter operon xylFGH and Glucosamine 6-phosphate synthetase, the key enzyme controlling amino sugar biosynthesis (Milewski, 2002; Jacobs et al., 2012). Lipid metabolism was also strikingly repressed during root colonization. Out of the 21 DE genes involved in lipid mobilization, only 2 have been found in previous gene expression studies in R. solanacearum (Table 3; Jacobs et al., 2012). Thus, the downregulation of lipid metabolism could be specific to early infection stages or to wild potato colonization. In this sense, lipid metabolism has been reported to play an important role during plant-host interactions by modulating defense responses in plants and pathogen infection (Casadevall and Pirofski, 2001; Wenk, 2006). Cofactor metabolism was also repressed including the folate synthesis gene pabB (Table 3), already known to be down-regulated in planta (Shinohara et al., 2005), the cobalamin biosynthesis genes and adenilate cyclase. Repression of adenylate cyclase, which is a global metabolic regulator in bacteria (Ullmann and Danchin, 1980), illustrates the magnitude of the metabolic shutdown experienced by R. solanacearum in the roots of S. commersonii.

In contrast with the global metabolic shutdown, aspartate and tryptophan catabolism genes were up-regulated when R. solanacearum grew in the plant roots. The aspartate catabolism gene nadB2 had already been identified as an essential gene for in planta growth in an in vivo screening (Brown and Allen, 2004). Interestingly, aspartate is the second most abundant aminoacid in the tomato apoplast and less so in the xylem (Zuluaga et al., 2013), which is in agreement with the bacterium mostly thriving in the apoplastic root spaces at the early infection times analyzed. Also induced was the Tryptophan 2,3-dioxygenase. Concentrations of this aminoacid are high at lateral root emergence sites (Jaeger et al., 1999), and it was suggested that it is also present in the tomato apoplast (Yu et al., 2013). Induction of tryptophan catabolism would thus be indicative of early plant colonization.

These results likely indicate the existence of a trade-off between the expression of virulence and metabolic genes. This has already been described in a previous study where the quorum-sensing-dependent regulatory protein PhcA regulated a trade-off between production of R. solanacearum exopolysaccharides and bacterial proliferation (Peyraud et al., 2016).

Proposed new virulence determinants important for early root colonization

RSUY_RS08455 and RSUY_RS16950 were found to be upregulated in a resistant S. commersonii accession compared to a susceptible one (Table 2), as well as during root colonization compared to rich medium (Table 3). Although these genes also appeared in the microarray transcriptome of bacteria extracted from infected tomato xylem vessels (Jacobs et al., 2012), they have not been characterized.

Similarly, the gene encoding an avrD-like protein was up-regulated in tomato xylem (Jacobs et al., 2012) and in wild potato (Table 3). AvrD is required in P. syringae for the synthesis of syringolide, small molecules that can elicit a hypersensitive response on resistant plants (Keen et al., 1990; Mucyn et al., 2014). In R. solanacearum the avrD-like protein encoding gene is activated by the master virulence regulator HrpG (Valls et al., 2006). Considering the persistence of these three genes among the up-regulated during plant colonization, we suggest that they encode for potential virulence factors, probably necessary independently of the host or the infection stage.

Three genes found up-regulated in S. commersonii (suhB, rhs and the carbonic anhydrase gene RSUY_RS16085, Table 3) have been involved in bacterial virulence on animals and constitute putative virulence genes in R. solanacearum. Although classified as a phosphate mobilization gene (Table 3), suhB is a super-regulator involved in the proper rRNA folding (Singh et al., 2016). It plays a role in virulence of animal bacterial pathogens, influencing T3SS, T6SS, flagellum and biofilm regulation and probably acts in opposite ways in different bacteria (Rosales-Reyes et al., 2012; Li et al., 2013). Interestingly, SuhB differential expression was also observed in two R. solanacearum strains (Meng et al., 2015). The function of Rhs (Rearrangement Hot Spot) proteins is ill-defined but they are considered to promote recombination (Lin et al., 1984). Interestingly, a member of the Rhs family was described to be induced during infection and associated with increased bacterial numbers and decreased survival in mice during pneumonia caused by P. aeruginosa (Kung et al., 2012). Finally, carbonic anhydrase catalyzes the inter-conversion between carbon dioxide and bicarbonate but is also required for growth of many animal pathogenic microorganisms (Capasso and Supuran, 2015). In addition, a role in disease establishment between potato and Phytophthora infestans was also reported (Restrepo et al., 2005), suggesting the possible implication of CAs during host colonization. These evidences suggest that suhB, rhs, and RSUY_RS16085 encode putative virulence factors shared between gram-negative bacterial pathogens that infect animals and plants.

The assimilatory sulfate reduction pathway (cysD, cysN, and cysI) and the phosphate mobilization (pstB and pstS1) were also induced during root colonization (Table 3). cysD and cysN, encode an ATP sulfurylase that produces APS, which can be in turn reduced to PAPS to ultimately synthesize cysteine by cysI. A study carried out in a closely related plant pathogenic bacterium, Xanthomonas oryzae pv. Oryzae, was demonstrated that mutation of either raxP or raxQ (homologs of cysD and cysN) impaired production of APS and PAPS and were required for the correct activity of the avirulence protein AvrXa21 (Shen et al., 2002). Further, several studies demonstrated that mutations on the pst system, responsible for phosphate uptake, affected virulence in diverse animal pathogenic bacteria (Rao et al., 2004; Lamarche et al., 2005, 2008). Altogether, these studies suggest that both systems might be regulators of bacterial pathogenicity, which could also be conserved in plant pathogens.

Finally, the rtcA and its regulator rtcR are down-regulated in planta (Table 3). The rtc system is involved in the regulation of the RNA repair system for ribosome homeostasis through the activation of rtcR by different agents and genetic lesions which in turn activates the rtcAB genes (Das and Shuman, 2013). The rtc system was also involved in the functioning of chemotaxis and motility in Escherichia coli (Engl et al., 2016), as mutations in either rtcA or rtcB increased motility. Since rtc acts a repressor of motility, its down-regulation in S. commersonii colonization could influence bacterial motility, a key virulence determinant.

Author contributions

MP performed experiments, analyzed data and wrote the manuscript; RG analyzed data; PZ performed experiments; NC designed the research and wrote the manuscript; AM designed experiments and analyzed data; JS designed the research, analyzed data and wrote the manuscript; MV designed the research, performed experiments, analyzed data, and wrote the manuscript.

Funding

This work was funded by projects AGL2013-46898-R, AGL2016-78002-R, and RyC 2014-16158 from the Spanish Ministry of Economy and Competitiveness. We also acknowledge financial support from the “Severo Ochoa Program for Centres of Excellence in R&D” 2016-2019 (SEV-2015-0533) and the CERCA Program of the Catalan Government (Generalitat de Catalunya) and from COST Action SUSTAIN (FA1208) from the European Union. APM is funded by the Chinese Academy of Sciences and the Chinese 1000 Talents Program. MP holds an APIF doctoral fellowship from Universitat de Barcelona and received a travel fellowship allowed by Fundació Montcelimar and Universitat de Barcelona to carry out a short stay in JCS's lab. RGS holds a doctoral fellowship; grant 2012/15197-1, São Paulo Research Foundation (FAPESP) and JCS has a CNPq research fellowship.

Conflict of interest statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Acknowledgments

We thank R. de Pedro for helping in the solid rich medium sample preparation, I. Erill for helping in the transcriptomic data interpretation, S. Genin, and S. Lindow for inspiring discussions, C. Madrid, and C. Balsalobre for advice on transcriptome data interpretation, M. Solé for the potato infection set up and F. Vilaró, M. dalla Rizza, and M.J. Pianzzola for their advice and for providing the S. commersonii genotypes used in this study. We thank the Shanghai PSC Genomics facility for RNA sequencing.

Supplementary material

The Supplementary Material for this article can be found online at: http://journal.frontiersin.org/article/10.3389/fpls.2017.00370/full#supplementary-material

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