Natural variations of TFIIAγ gene and LOB1 promoter contribute to citrus canker disease resistance in Atalantia buxifolia

Citrus canker caused by Xanthomonas citri subsp. citri (Xcc) is one of the most devastating diseases in citrus industry worldwide. Most citrus cultivars such as sweet orange are susceptible to canker disease. Here, we utilized wild citrus to identify canker-resistant germplasms, and found that Atalantia buxifolia, a primitive (distant-wild) citrus, exhibited remarkable resistance to canker disease. Although the susceptibility gene LATERAL ORGAN BOUNDARIES 1 (LOB1) could also be induced in Atalantia after canker infection, the induction extent was far lower than that in sweet orange. In addition, three of amino acids encoded by transcription factor TFIIAγ in Atalantia (AbTFIIAγ) exhibited difference from those in sweet orange (CsTFIIAγ) which could stabilize the interaction between effector PthA4 and effector binding element (EBE) of LOB1 promoter. The mutation of AbTFIIAγ did not change its interaction with transcription factor binding motifs (TFBs). However, the AbTFIIAγ could hardly support the LOB1 expression induced by the PthA4. In addition, the activity of AbLOB1 promoter was significantly lower than that of CsLOB1 under the induction by PthA4. Our results demonstrate that natural variations of AbTFIIAγ and effector binding element (EBE) in the AbLOB1 promoter are crucial for the canker disease resistance of Atalantia. The natural mutations of AbTFIIAγ gene and AbLOB1 promoter in Atalantia provide candidate targets for improving the resistance to citrus canker disease.


Introduction
Citrus canker is one of the most devastating bacterial diseases in citrus industry worldwide. It causes severe necrosis symptoms on the leaves and fruits, accelerating the dropping of citrus fruit and leaves [1]. This disease causes considerable yield losses, increases in bactericide cost, ecosystem risks, and even negative impacts on socio-economy [2]. One of economic and environment-friendly approaches is to improve the resistance of the host plants. The pathogenic bacteria of Xanthomonas citri strains harbor different host range. For example, XccA W and XccA � strains have a narrow host range including Mexican lime, whereas XccA can cause disease in most commercial citrus varieties [3][4][5].
Since almost all citrus cultivars are susceptible to canker disease [6], there have been extensive studies of its pathogenesis. Previous studies have shown that Xanthomonas bacteria contain the type III secretion system (T3SS), and that different types of Xanthomonas strains have different numbers of type III secretion (T3S) effectors. Transcription activator-like effectors (TALEs) belong to the AvrBs3/PthA family of T3SS effectors, and they are vital for canker bacteria to form pustule on citrus [5,7]. A typical TALE processes an N-terminal translocation signal, a central repeat domain consisting of 34 amino acids, 3 nuclear localization signals, transcription factor binding motifs (TFBs), and C-terminal amino acid activation domain [8,9]. PthA4 of Xcc can activate LATERAL ORGAN BOUNDARIES 1 (LOB1) gene expression [10], and the expression of susceptibility genes can be suppressed either by variation of the TFIIAγ or by mutation of the effector binding element (EBE) [11]. LOB1 is a transcription factor belonging to the LATERAL ORGAN BOUNDARIES (LOB) gene family, which not only controls the expansion and growth of plant cells, but also promotes bacterial growth and pustule formation in citrus [12,13].
Transcription factor IIA (TFIIA) is vital for the transcriptional regulation in eukaryotes. In humans, TFIIA contains three subunits, including α, β and γ subunits, among which α and β subunits are encoded by the same gene, while in yeast, TFIIA only contains the TOA1 and TOA2 subunits with TOA2 homologous to human TFIIAγ subunit [14,15]. Several studies have illustrated that TFIIA is required for RNA polymerase II-dependent transcription, and it can stabilize the TATA box-binding protein (TBP)-TFIID complex in the TATA box region of the promoters [16][17][18]. In plants, TFIIAγ is expressed in most tissues, especially in the young and active tissues [19]. In addition, TFIIAγ is associated with the disease resistance of rice [20]. In rice, it has been reported that TFBs are found to be vital for the infection of Xanthomonas bacteria, that TFBs can interact with the host basal transcription factor IIA gamma subunit (OsTFIIAγ5) to promote the expression of susceptibility genes, and that silencing OsTFIIAγ5 results in the increased resistance to Xanthomonas oryzae pv. oryzae (Xoo) and Xanthomonas oryzae pv. oryzicola (Xoc) [20]. However, its allele xa5, which carries a V to E mutation at the 39 th amino acid position, could not interact with the TFBs of Xoo and Xoc [21,22]. The mutation at the 39 th amino acid could lead to the interaction of xa5 with an acidic activation domain (AAD) of avirulence protein Avrxa5, thus impeding host cell transcription, eventually resulting in subsequent cell death as well as the resistance reaction [23,24]. In sweet orange, TALE TFBs could also interact with basal transcription factor (CsTFIIAγ) to promote Xcc infection [20].
In rice, SWEET genes belong to the sucrose transporter family, and are required for the susceptibility to rice blight. Natural mutations in the EBEs of SWEET genes have been reported in rice blight resistant varieties [11,25]. Editing the EBE regions of TALE-induced SWEET genes impedes the expression of corresponding susceptibility genes [26]. To the best of our knowledge, the polymorphism of the EBEs in the susceptibility gene promoter has not been reported in citrus canker resistant varieties so far.
Citrus has a broad spectrum of resources ranging from primitive, wild, and cultivated varieties. Currently, little is known about the resistance or susceptibility of primitive or wild citrus to canker disease. Atalantia buxifolia (Chinese box orange), as a primitive citrus, shows tolerance to diverse abiotic and biotic stresses and is sometimes used as rootstock for the grafting of commercial citrus [27,28]. It becomes possible to identify resistant genes to citrus canker disease with the availability of the genomes of Atalantia and other wild germplasms [29,30]. In this study, we found that Atalantia is resistant to citrus canker. The susceptibility gene LOB1 was induced in Atalantia after inoculation with Xcc, but its induction degree was much lower in Atalantia than in sweet orange. In contrast to CsTFIIAγ of sweet orange, AbTFIIAγ of Atalantia could hardly support the expression of the CsLOB1 gene induced by PthA4, and the activity of the AbLOB1 promoter was significantly lower than that of CsLOB1 induced by PthA4. Our results indicate that the natural mutations of AbTFIIAγ gene and AbLOB1 promoter are vital for the canker resistance of Atalantia.

Resistance of Atalantia to citrus canker
Great research efforts have been made to evaluate the canker disease resistance of various commercial citrus cultivars and the relatives, and almost all cultivars have been found to be susceptible to the disease [2,7]. To explore the canker resistant germplasms, we expanded the research scope to investigate wild citrus in tribe Citrinae belonging to the subfamily Aurantioideae. Ten citrus varieties were chosen for canker disease evaluation. The disease lesion area was determined at 12 d after the inoculation with Xcc. Based on the results, the citrus varieties were classified into three categories: susceptible (lesion area = 2-4 mm 2 ), tolerant (lesion area = 1-2 mm 2 ), and resistant (lesion area = 0-1 mm 2 ) (S1 Fig). Three wild citrus varieties including wild mandarin, wild pummelo, and citron showed different degrees of susceptibility to citrus canker. Wild mandarin and citron showed tolerance to citrus canker in the early stages, but exhibited small lesions at 12 d after inoculation. The wild pummelo of purple pummelo were susceptible to citrus canker. However, remarkable resistance was observed in Atalantia buxifolia, a distant wild relative of citrus (Fig 1).
A low bacterial titer of Xcc was used to further evaluate the canker disease development in Atalantia. Sweet orange, a variety known to be susceptible to canker disease, was used as the control. Canker development was assessed at 7 d and 12 d after Xcc inoculation (Fig 2). At 7 d, canker lesion was not observed on the leaves of Atalantia, but obvious canker symptoms appeared on the leaves of sweet orange (Fig 2A). Bacterial growth evaluation results showed that the population of Xcc decreased at 7 and 12 d in Atalantia, compared with that in sweet orange, indicating the inhibition of bacterial growth (Fig 2B).

Differentially expressed genes of Atalantia in response to canker infection
To reveal the molecular basis for the resistance of Atalantia to Xcc, samples were collected from leaves inoculated with Xcc (treatment) and leaves inoculated with sterile water (control) at different time points (hour 6, 24 and 48). A total of approximately 772 million paired-end reads (32 million reads for each library on average) were obtained by Illumina sequencing Atalantia buxifolia resistance to citrus canker. The phylogenetic tree was constructed by using the maximum likelihood tree method and the substitution model GTRGAMMA in the RAxML software. Murraya koenigii was used as the outgroup. Fully expanded leaves were treated with Xcc (10 8 CFU/mL) to evaluate citrus canker resistance. The symptoms were observed at 7 and 12 d after inoculation. Red indicates canker susceptible citrus (Wild pummelo: purple pummelo; Cultivated pummelo: guanxi pummelo; Cultivated technology (S1 Table). Gene ontology (GO) analysis results indicated that the up-regulated genes in Atalantia were enriched in pathways such as defense response and biotic stimulus response, while those in sweet orange were enriched in polysaccharide metabolic and catabolic pathways at 48 h after the inoculation (Fig 3A). The cross-comparison Venn diagram of differentially expressed genes (DEGs) showed that eight DEGs were overlapped between Atalantia and sweet orange, one of which was citrus canker susceptibility gene LOB1 (S2 Table) [10]. However, the transcriptome data showed that the relative expression level of AbLOB1 was much lower than that of CsLOB1. Quantitative real-time PCR data confirmed that the expression level of CsLOB1 was three folds as high as that of AbLOB1 (Fig 3B). To confirm expression of the DEGs (S3 Table), quantitative RT-PCR was conducted for 10 candidate genes chosen from the transcriptional profile. These unigenes such as pathogenesis-related 1 (PR1), HopW1-1-interacting 2 (WIN2), dirigent-like protein 22, and pathogenesis-related 4 (PR4) were up-regulated in Atalantia from 6 h to 48 h after Xcc inoculation, while these genes were down-regulated in sweet orange. Gene RPS5 (Resistant to pseudomonas syringae 5) and quinone oxidoreductase gene were only significantly induced in Atalantia at 6 h, 24 h, 48 h after Xcc inoculation. Other genes such as repressor GA3 (RGA3), cytochrome P450 (CYP76C4) were up-regulated in Atalantia and down-regulated in sweet orange at 48 h after Xcc inoculation (Figs 3C and S2). Correlations between the ten genes expression and RNA-seq data were shown in S2C Fig

Genetic variations of TFIIAγ in resistant and susceptible citrus and their interaction with TAL effectors
Previous studies have shown that TFIIAγ could stabilize TAL effectors in the TATA box region and induce LOB1 expression and susceptibility [20]. We further investigated the and CsTFIIAγ was exposed on the surface of a β-sheet, and that the side chain of leucine (L81) in CsTFIIAγ was longer than that of valine (V81) in AbTFIIAγ.

PLOS GENETICS
proteins to further verify their interaction. Pull-down assay results indicated that His-tagged TFBi or TFBii interacted with the GST-tagged AbTFIIAγ and CsTFIIAγ proteins, but not with GST alone (Fig 4E and 4F).

Enhancement of resistance to Xcc by silencing of TFIIAγ in sweet orange
A previous report has revealed that transient interference of CsTFIIAγ in sweet orange enhanced its resistance to Xcc [20]. Here, we suppressed the CsTFIIAγ gene expression in sweet orange leaves by RNA interference (RNAi) for the functional complementation of AbTFIIAγ because of the unavailability of the gene transformation system for Atalantia. The results showed that the reduction of CsTFIIAγ gene expression resulted in the decrease in the disease lesion area and the inhibition of the bacterial growth and the CsLOB1 expression, compared with the control (Fig 5).

Complementation assay of AbTFIIAγ and CsTFIIAγ
AbTFIIAγ or CsTFIIAγ was transformed into a vector containing the promoter CaMV 35S and terminator NOS, respectively. Subsequently, the resultant two vectors were respectively  (Fig 6A and 6B). In order to further clarify the function of AbTFIIAγ, we performed the complementary assay in Nicotiana benthamiana. First, N. benthamiana TFIIAγ (NbTFIIAγ) was silenced, and the N. benthamiana phytoene dehydrogenase gene was used as the positive control to confirm the effectiveness of the virus-induced gene silencing (VIGS). Obvious albino phenotype was observed at 15 d ( Fig  6C). CsLOB1 promoter fused with the β-glucuronidase (GUS) reporter gene vector and 35S promoter-driven pthA4 vector were transformed into NbTFIIAγ-silenced tobacco to detect the function of AbTFIIAγ and CsTFIIAγ. We first confirmed that gene AbTFIIAγ and CsTFIIAγ were expressed in NbTFIIAγ-silenced tobacco (S5 Fig), then we checked the promoter activity.

PLOS GENETICS
The results showed that the complementary CsTFIIAγ restored the reduced GUS activity of CsLOB1 promoter in NbTFIIAγ-silenced plants, while the complementary AbTFIIAγ hardly restored the reduced activity of CsLOB1 promoter which was similar to that of complementary empty vector (Fig 6D and 6E).

Significant lower promoter activity of AbLOB1 than that of CsLOB1 mediated by PthA4
Previous research has shown that the PthA4 of Xcc306 can bind to the promoter of LOB1 to increase its expression [10]. We further compared AbLOB1 and CsLOB1 promoters and coding sequences, and found two single nucleotide polymorphisms (SNPs) in their EBE regions of promoters (S6A Fig). Amino acid alignment revealed that LOB1 was highly conserved (S6B Fig). To further verify the activities of the two promoters, AbLOB1 and CsLOB1 promoters were fused to pKGWFS7 vector containing the β-glucuronidase (GUS) reporter gene [10]. No significant difference in GUS activity was observed between AbLOB1 or CsLOB1 co-infiltrated with empty vector PBI121, but the GUS activity of AbLOB1 was significantly lower than that of CsLOB1 when these two promoters were co-infiltrated with vector 35S:pthA4 (Fig 7A and 7B). We further compared the activities of these two promoters in sweet orange leaves by transient expression mediated by Xcc [10]. The results showed that GUS activity of AbLOB1 was also significantly lower than that of CsLOB1 when these two promoters were co-infiltrated with the Xcc, whereas no GUS activity of two promoters was observed upon the co-infiltration with the mutant strain Xcc306ΔpthA4 (Fig 7C and 7D).

Discussion
It has been reported that cultivated citrus varieties are more susceptible to canker disease than wild citrus, and that wild citrus varieties have a broad spectrum of disease resistance, whereas cultivated citrus varieties have lost certain resistance to different degrees during domestication [2,6]. For example, Meiwa kumquat obtain a durable resistance to Xcc by upregulating a host susceptibility gene to elicit immune responses [31]. Tracing back to wild germplams is an alternative strategy for identifying gene resources for breeding purpose. Chinese box orange (Atalantia buxifolia) is widely spread in Southern China, Philippines, and Japan [32,33]. It is a distant wild relative of Citrus, and it is occasionally used as rootstock due to its tolerance to diverse biotic and abiotic stresses [28]. In this study, we demonstrated that Atalantia, as a wild variety, was resistant to citrus canker.
LOB1 is a susceptibility gene whose expression is crucial for the formation of pustule in different citrus varieties [10,12]. We found that the expression of LOB1 was remarkably lower in Atalantia than in sweet orange. Previous studies have indicated that TFIIAγ can stabilize and increase the expression of the LOB1 gene [20]. Considering this, we examined the genetic variations of TFIIAγ in resistant and susceptible varieties, and found that natural mutations in Atalantia, AbTFIIAγ could hardly support TALE-mediated CsLOB1 gene expression (Fig 6). Homology modeling of AbTFIIAγ and CsTFIIAγ proteins and their mutant proteins revealed that the 81 st residues of AbTFIIAγ and CsTFIIAγ were exposed on the surface of a β-sheet, and that the side chain of leucine (L81) was longer than that of valine (V81). We speculated that leucine (L81) in sweet orange might be more conducive to the stabilization of the protein complex (TBP)-TFIID in the TATA box region of LOB1 promoter due to its longer alkyl side chain than valine (V81) in Atalantia, which may partly explain the difference expression of LOB1 in sweet orange and Atalantia. Based on the above results, it could be concluded that Atalantia possessed an unique allele AbTFIIAγ, which contributed to the canker resistance in Atalantia.
The mutation of EBE on the AbLOB1 promoter also contributed to the disease resistance in Atalantia. We found two substitutions at the 7 th (C to T) and 13 th (T to C) position in the EBE region of promoter AbLOB1 (S6A Fig). A previous study has shown that a single base insertion in the EBE region could offset PthA4-mediated CsLOB1 expression in citrus, and that the substitution at the 9 th (C to T) position could compromise PthA4-induced CsLOB1 expression [10]. Consistently, a substitution at the 10 th position in the EBE region appeared to compromise AvrXa7-induced OsSWEET14 expression in a study of rice blight [25]. Our results revealed that the natural mutation of EBE on the AbLOB1 promoter also compromised PthA4-induced LOB1 expression (Fig 7). To our knowledge, the expression of LOB1 is crucial for the formation of pustule. A comparison of LOB1 gene expression 48 h after inoculation with Xcc or Xcc306ΔpthA4 in Atalantia and sweet orange revealed that the expression of AbLOB1 inoculated with Xcc was similar to that of CsLOB1 inoculated with Xcc306ΔpthA4 ( S7 Fig). It is known that the Xcc306ΔpthA4 strain is not pathogenic in citrus, and that low expression of LOB1 can reduce the formation of pustule [10]. On the other hand, the inability of Xcc to grow on the leaf of Atalantia (Fig 2B) and the up-regulation of the disease defense-related genes (Figs 3C and S2) suggested that an active response occurred in Atalantia after Xcc infection.
Our data demonstrated that both cis-and trans-regulatory elements of AbLOB1 contributed to the canker resistance of Atalantia. The mutations might provide some useful target sites for improving the resistance to citrus canker, a devastating and stubborn disease which is mostly controlled by chemicals at present [34,35]. The current control approaches are costly due to the use of bactericide, and environmentally-and ecologically-unfriendly [36,37]. Breeding canker-resistant cultivars is a promising strategy for solving the above problems. Recently, genome editing technology has been widely applied to breeding disease-resistant cultivars due to its high efficiency and accuracy. In rice, SWEET genes are the members of sucrose transporter gene family, and are required for the susceptibility to rice blight. Gene editing in the EBE regions of SWEET11, SWEET13, and SWEET14 promoters could confer rice with broadspectrum resistance to bacterial blight [38]. In citrus, editing the susceptibility gene CsLOB1 and its promoter could enhance citrus canker resistance. However, most of the edited citrus might still be infected with canker disease to different degrees [39,40]. Our data indicated the CsTFIIAγ could regulate the expression of gene CsLOB1. It is worthwhile to evaluate the phenotype and agronomic performances of citrus plants whose TFIIAγ gene and EBEs of LOB1 are edited. Homology recombination [41,42] and single base editing [43] are promising approaches to simultaneously modifying TFIIAγ and EBEs of LOB1 in susceptible citrus.

Materials and methods
Plant materials and pathogen. All the citrus varieties used in this study were taken from the National Citrus Breeding Center of Huazhong Agricultural University. All the transgenetic and control plants were grown in a greenhouse at 25-30˚C. The X. citri strain 3213 (hereafter referred to as Xcc) and the mutant strain Xcc306ΔpthA4 were grown on nutrient agar medium at 28˚C as previously reported [44].
Assay of pathogenicity. Fully expanded leaves were inoculated with Xcc (10 6 and 10 8 CFU/ml) and Xcc306ΔpthA4 (10 8 CFU/ml) with an inoculating needle (0.5 mm in diameter). Each inoculation site consisted of six pricks according to previous reports [45] with minor modifications. Bacterial suspension was dropped into each inoculation site. The disease lesion area was measured (36 punctures on average) with ImageJ 2.0. To examine the bacterial growth in citrus plants, leaf disk with 0.5 cm diameter in inoculated area was punched at 0, 1, 7, and 12 d after inoculation. DNA was extracted from 100 mg fresh weight of inoculated leaf disks, and 100 ng of total nucleic acid per inoculated sample was used as the template for quantitative polymerase chain reaction (qPCR). pthA of Xcc was used to calculate the bacterial population using the following formula [46,47]. Copy Number ðXcc; pthAÞ ¼ 10 ð38:3À ctÞ=3:56 : Construction of phylogenetic tree of Citrinae. SNPs contained in the conserved singlecopy genes in citrinae genomes were used for the construction of the phylogenetic tree of 10 varieties, namely, Murraya exotica, Atalantia, Citron, Wild mandarin (mangshan mandarin), Cultivated mandarin (Ponkan), Trifoliate orange, Lemon (Eureka lemon), Wild pummelo (purple pummelo), Cultivated pummelo (guanxi pummelo), Sweet orange. The maximum likelihood tree was constructed by using the substitution model GTRGAMMA in the RAxML software with Murraya koenigii as the outgroup. A total of 1,000 rapid bootstrap inferences were performed. The bootstrap value greater than 60 was labelled at each node in the tree.
Gene expression analysis. Total RNA was extracted using the HiPure HP Plant RNA Mini Kit (Magen, Guangzhou, China) according to the manufacturer's protocol. RNA samples were reverse transcribed into cDNA using the Maxima H Minus First-Strand cDNA Synthesis Kit (Thermo Scientific, Shanghai, China). The qRT-PCR was performed with SYBR Green PCR Master Mix (Applied Biosystems, American), and amplification was performed on ABI 7900 Fast Real Time System (PE; Applied Biosystems). The elongation factor (EF1α) was used as the endogenous gene of citrus, while Ubiquitin (UBQ) was selected as the endogenous gene of tobacco. The used primers were listed in S4 Table. The relative gene expression was calculated using 2 −ΔΔCt method.
Transcriptome data analysis. Total RNA was extracted from sterile water-or Xcc (10 8 CFU/ml)-inoculated Atalantia and sweet orang leaves at 6 h, 24 and 48 h after inoculation for RNA sequencing. The RNA-seq reads were mapped to the reference genome of sweet orange by HISAT2 [48]. The mapping results were transformed and sorted by samtools [49]. Gene expression values were normalized as Fragments Per Kilobase per Million (FPKM) by Cufflinks package [50]. The genes with P < 0.01 and an absolute value (fold change) log2 ratio � 1 were defined as differentially expressed genes (DEGs). DEGs from the RNA seq data were analyzed and presented in S3 Table. Gene ontology term (GO) enrichment analysis was performed using Agrigo (https://www.Agrigo.com/) with FDR < 0.05. Our RNA-seq data were submitted to NCBI with genbank accession numbers of PRJNA612768 and PRJNA612769.
Molecular cloning and sequence analysis of TFIIAγ and LOB1. The TFIIAγ gene sequences were cloned from the cDNA of the ten citrus varieties (Murraya exotica, Atalantia, Citron, mangshan mandarin, Ponkan, Trifoliate orange, Eureka lemon, purple pummelo, guanxi pummelo, Sweet orange). Gene AbLOB1 and CsLOB1 and their promoter sequences were amplified from the cDNA and DNA of Atalantia and sweet orange. The primers used for amplification were listed in S4 Table. The gene ID of AbTFIIAγ was sb14580, and that of CsTFIIAγ gene was Cs3g16970 in the citrus genome database (http://citrus.hzau.edu.cn/cgibin/orange/blast). Sequence alignment of TFIIAγ and LOB1 was conducted by ClustalW2 and GENEDOC software.
Homology modeling of TFIIAγ. The structures of AbTFIIAγ and CsTFIIAγ were homology modeled using SWISS-MODEL online service with default parameters (https:// swissmodel.expasy.org/). The crystal structure of transcription initiation factor IIA from human HsTFIIA (PDB ID: 5M4S) was used as the template. AbTFIIAγ and CsTFIIAγ exhibited 53% and 49% sequence identity with the HsTFIIA template, respectively. The structures of AbTFIIAγ and CsTFIIAγ were generated by PyMOL.
Luciferase complementation assay. The full-length coding sequence (CDS) of TFIIAγ without stop codons was cloned into vector JW-like-771-nLuc, and sequence TFBi/TFBii were cloned into vector JW-like-772-cLuc. The primers were listed in S4 Table. All the vectors were transformed into Agrobacterium tumefacien strain GV3101. Then, the Agrobacterium strain carrying the two constructed reporter vectors (JW-like-771-nLuc and JW-like-772-cLuc at a ratio of 1:1) was infiltrated into tobacco leaves at OD 600 nm = 0.8. The images of luciferase signal were taken at 2 d via a charge coupled device camera (LB985 NightSHADE) from the Key Laboratory of Horticultural Plant Biology, Ministry of Education.
Pull-down assay. The full-length TFIIAγ and TFBs were fused into GST-tagged PGEX-6p and HIS-tagged PET-32a, respectively. The proteins with GST-tag or His-tag were expressed in E.coli BL21 strain in vitro and purified with a GST purification kit (Sangon Biotech, Shanghai, China) or Ni-NTA purification kit (Sangon Biotech, Shanghai, China). Both types of proteins were purified following the manufacturer's protocol. The GST-tagged proteins were incubated with Mag-Beads GST fusion protein purification kit (Sangon Biotech, Shanghai, China) for two hours, and washed four times. After one-hour incubation of His-tagged protein, the Mag-Beads were eluted and target protein was separated. The eluted proteins were tested with anti-GST (Smart-lifesciences, Changzhou, China) or anti-His (Smart-lifesciences, Changzhou, China) by using western blotting.
CsTFIIAγ silencing assay. CsTFIIAγ gene sequence (174 bp from the ATG start codon) was cloned from sweet orange cDNA and fused into vector pk7GWIWG2D (provided by professor Chunying Kang of Key Laboratory of Horticultural Plant Biology). The self-complementary RNAi vector pk7GWIWG2D had the selection tag eGFP controlled by 35S promoter. The vector CsTFIIAγ-pk7GWIWG2D was transformed into Agrobacterium tumefaciens strain EHA105. The resultant Agrobacterium was further transformed into sweet orange epicotyl explants, as previously reported [51,52].
Vector construction. NbTFIIAγ (174 bp from ATG start codon) and NbPDS (369 bp of the coding sequence) were amplified from the Nicotiana benthamiana genome and fused into the tobacco pTRV2 vector. The complete CDS of AbTFIIAγ and CsTFIIAγ was amplified and fused into the overexpression vector PK7WG2D. Promoter CsLOB1 and AbLOB1 were amplified (296 bp upstream from LOB1 coding sequence) and fused into uidA (β-glucuronidase (GUS) reporter gene vector pKGWFS7. The pthA4 was amplified from X. citri strain 3213 genome and transferred into the PBI121 vector. Primer information was presented in S4 Table. All the constructs were transferred into GV3101 and suspended in the solution containing 10 mM MgCl 2 , 10 mM Mes (pH 5.6) and 100 μM acetosyringone.
Virus-induced gene silencing (VIGS) and AbTFIIAγ functional analysis. To investigate the putative function of AbTFIIAγ, VIGS assay was performed according to previous reports [53]. Phytoene desaturase (PDS) gene was used as the positive control. The mixed Agrobacterium GV3101 strains containing pTRV1and pTRV2 or pTRV1 and NbTFIIAγ-pTRV vectors were infiltrated into three-week-old tobacco, respectively. The inoculated tobacco was then transferred to a culture room and incubated at 22˚C in the dark for two days, and then exposed to the cycle of 16-hour light and 8-hour darkness for one week. Subsequently, the plants were cultured at 25˚C in the cycle of 16-hour light and 8-hour darkness for one week. When an obvious albino phenotype was observed, Agrobacterium GV3101 strains containing the 35S: pthA4 and pCsLOB1:GUS mixed with 35S:CsTFIIAγ or 35S:AbTFIIAγ, or empty vector were co-infiltrated into NbTFIIAγ-silenced tobacco. Samples were collected 2 days after co-infiltration for gene expression and GUS activity analysis.
For a further analysis of AbTFIIAγ gene function, we complemented AbTFIIAγ into CsTFIIAγ-silenced citrus line (RNAi-1). In brief, the overexpression vector 35S:AbTFIIAγ, 35S:CsTFIIAγ, and empty vector PK7WG2D were separately transferred into CsTFIIAγsilenced sweet orang leaves. Five hours later, Xcc was infiltrated at the same area at an OD 600nm = 0.3, as previously described [10]. Gene expression was analyzed 4 days after Xcc inoculation.
GUS activity assay. Firstly, GUS activity assay was performed in tobacco, vector 35S: pthA4 and empty vector mixed with pAbLOB1:GUS or pCsLOB1:GUS were co-injected into tobacco leaves, respectively. The treated leaves were collected for GUS staining and GUS activity assay at day 2 after co-injection. We further analyzed the GUS activity in sweet orang leaves mediated by Xcc. Vector pAbLOB1:GUS or pCsLOB1:GUS was injected into sweet orange leaves, as previously reported [10]. Samples were collected at day 4 after vector injection. GUS staining assay was performed with GUS staining kit (MREDA, Shanghai, China) according to the manufacturer's protocol with minor modifications. GUS activity assay was performed with the GUS activity assay kit (FCNCS, Nanjing, China) according to the manufacturer's protocol.