Abstract
Agrobacterium-mediated plant transformation (AMT) is the basis of modern-day plant biotechnology. One major drawback of this technology is the recalcitrance of many plant species/varieties to Agrobacterium infection, most likely caused by elicitation of plant defense responses. Here, we develop a strategy to increase AMT by engineering Agrobacterium tumefaciens to express a type III secretion system (T3SS) from Pseudomonas syringae and individually deliver the P. syringae effectors AvrPto, AvrPtoB, or HopAO1 to suppress host defense responses. Using the engineered Agrobacterium, we demonstrate increase in AMT of wheat, alfalfa and switchgrass by ~250%–400%. We also show that engineered A. tumefaciens expressing a T3SS can deliver a plant protein, histone H2A-1, to enhance AMT. This strategy is of great significance to both basic research and agricultural biotechnology for transient and stable transformation of recalcitrant plant species/varieties and to deliver proteins into plant cells in a non-transgenic manner.
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Introduction
The soil-borne phytopathogen Agrobacterium tumefaciens causes crown gall tumors on various dicotyledonous plants by transferring a piece of its DNA (transfer DNA; T-DNA) and virulence proteins into host cells through the type IV secretion system (T4SS)1. The ability to transfer T-DNA from Agrobacterium to plants has been widely adopted to generate transgenic plants expressing genes of interest for research purposes or for commercial applications2,3. However, the generation of transgenic plants has several drawbacks, including the low transformation efficiency of some plant species/varieties. Plant defense responses against Agrobacterium significantly contribute to recalcitrance4.
Active plant defense against microbial infection relies on innate immune responses triggered by several layers of microbial recognition. The first layer involves the perception of conserved microbial molecules called pathogen-associated molecular patterns (PAMPs) by pattern recognition receptors (PRRs) leading to PAMP-triggered immunity (PTI) that often is sufficient to prevent pathogen growth5. Perception of one of the most abundant A. tumefaciens proteins, the PAMP elongation factor thermo unstable (EF-TU)6, by the Arabidopsis PRR EF-TU receptor (EFR) activates a set of signaling events and defense responses that reduces Agrobacterium-mediated plant transformation (AMT)7. Arabidopsis efr mutants are more susceptible to AMT7. Therefore, reducing or dampening plant basal immunity is not only essential for a successful pathogen to cause disease, but also will aid in AMT.
In contrast to A. tumefaciens which has a T4SS, many Gram-negative plant pathogenic bacteria have a type III secretion system (T3SS) to deliver bacterial proteins directly into their eukaryotic hosts. Many such delivered proteins, known as type III effectors (T3Es), have virulence functions that interfere with host cellular processes to block PTI, thus allowing bacteria to thrive in their hosts and cause disease8. T3SSs are macromolecular machines consisting of protein complexes that assemble a needle-like structure that spans the bacterial inner and outer membranes and traverses the plant cell wall and cell membrane9. The synthesis of effector proteins is co-regulated with proteins encoding the type III secretion apparatus1. Effector proteins contain an export signal at their N-termini with the characteristic composition of amphipathic and polar amino acids10,11. Although the effector protein content varies among pathogens, the genes encoding the type III secretion apparatus are broadly conserved and functional when heterologously expressed. For example, the T3SS from Pseudomonas syringae pv. syringae 61 (Pss61) and Erwinia chrysanthemi expressed in P. fluorescens and Escherichia coli, respectively, allowed these non-pathogenic bacteria to deliver bacterial proteins into plants12,13.
Many T3Es, including AvrPto from P. syringae pv. tomato, can suppress plant basal defense9,14. The interaction between AvrPto and kinase domains of the PRRs Flagellin sensitive2 (FLS2) and EFR leads to the suppression of PTI15. When AvrPto is expressed under the control of an inducible promoter, Arabidopsis becomes more susceptible to transient AMT16. Transient expression of AvrPto by co-infiltration also improves transient transgene expression in Brassica sp.17. Earlier, we showed that Arabidopsis and Nicotiana benthamiana plants compromised for plant defense were more susceptible to AMT18. Recently, the increased transient transformation was achieved in Arabidopsis NahG expressing plants in which the defense signaling hormone salicylic acid is reduced19. Even though these results demonstrate that AMT can be increased by decreasing plant defense responses, practically this strategy cannot be used in the field because of the need for the generation of transgenic plants. An alternative approach to increase plant transformation is by altering the expression of host factors (other than genes involved in plant defense responses) that play a role in plant transformation and regeneration. Several plant proteins, including histones, have been identified to play a role in AMT20,21,22,23,24,25. However, altering the expression of host factors needs a transgenic approach that is time-consuming and creates additional hurdles for deregulation.
Here, we report a strategy based on engineering A. tumefaciens with a T3SS to deliver proteins that suppress plant defense and/or increase transformation. P. syringae pv. tomato T3Es such as AvrPto, AvrPtoB, or HopAO1, when co-delivered along with T-DNA through engineered A. tumefaciens during the transformation process, increase transformation efficiency in Arabidopsis, N. benthamiana, wheat, alfalfa, and switchgrass. Delivery of the plant protein histone H2A-1 also increases transformation efficiency.
Results
T3SS from Pseudomonas syringae pv. syringae 61 is functional in A. tumefaciens
T3SS encoding genes cloned from Pss6126, contained in the plasmid pLN18, are functional in P. fluorescens27 and E. coli12. Here, we tested whether the expression of the Pss61 T3SS in A. tumefaciens is functional to secrete and translocate T3Es. We introduced pLN18, containing the T3SS genes, and a plasmid that can express the effector protein AvrPto tagged with the fluorescent reporter PhiLOV into A. tumefaciens (Fig. 1a). To monitor hrp-dependent effector secretion into the medium, the A. tumefaciens strain expressing T3SS and AvrPto-PhiLOV along with appropriate control strains were cultured in hrp-derepressing medium28. Both cell pellet and supernatant fractions were used for immunoblot analysis. AvrPto-PhiLOV could be found in both the cell pellet and the supernatant fractions for A. tumefaciens containing pLN18 and expressing AvrPto-PhiLOV (Fig. 1b). An A. tumefaciens strain expressing AvrPto-PhiLOV without pLN18 showed the presence of AvrPto-PhiLOV only in the cell pellet and not in the supernatant fraction (Fig. 1b). These results demonstrate that an A. tumefaciens strain expressing a T3SS is able to express a T3E and secrete it from A. tumefaciens into the culture medium.
To demonstrate that the T3E secreted from the engineered A. tumefaciens strain can be delivered into plant cells, we used a previously established split GFP system29,30 by infiltrating N. benthamiana leaves with A. tumefaciens that contain a GFP1-10 gene within the T-DNA of a binary vector (Fig. 1c), followed by infiltration of the same leaves with A. tumefaciens containing pLN18 and expressing AvrPto-GFP11 (Fig. 1c). Live-cell imaging showed green fluorescence signals inside the plant epidermal cells resulting from the assembly of full-length GFP from the interaction of GFP11 and GFP1-10, indicating delivery of AvrPto-GFP11 into plant cells (Fig. 1d). As expected, green fluorescence was not observed in leaves infiltrated with Agrobacterium strains lacking either the T3SS or the tagged effector protein gene (Fig. 1d). FM4-64 staining of the leaves showed plasma membrane localization of AvrPto-GFP, similar to previous reports29 (Supplementary Fig. 1a). Using the same split GFP system, we also showed delivery of other T3Es, including AvrPtoB or AvrB (Supplementary Fig. 1b). To validate our results further, we used another approach to directly deliver AvrPto-PhiLOV from A. tumefaciens containing pLN18 into plant cells (Supplementary Fig. 1c). In addition to demonstrating that the T3SS is functional in A. tumefaciens to secrete T3E in culture and translocate them to plant cells, assembly of a full-length GFP by independent translocation through T4SS and T3SS highlights that both T3SS and T4SS can operate in A. tumefaciens with T3SS translocating proteins and T4SS translocating both proteins and T-DNA.
T3Es delivered by a T3SS in A. tumefaciens improves transformation
The T3E AvrPto suppresses plant innate immunity31 that hinders AMT32. Inducible expression of AvrPto in transgenic Arabidopsis increases transient transformation efficiency16. To determine if AvrPto delivered through a T3SS can increase transient transformation, we transferred pLN18 (containing T3SS genes) and a plasmid that expresses AvrPto under its native promoter into the disarmed A. tumefaciens strain EHA105 containing a binary vector with a β-glucuronidase (GUS)-intron gene within the T-DNA (Supplementary Fig. 2a). This engineered A. tumefaciens strain, along with appropriate controls, was infiltrated into the leaves of Arabidopsis plants. GUS expression significantly increased when A. tumefaciens expresses a T3SS and AvrPto (Fig. 2a and b). To determine if T3SS delivery of AvrPto can also increase stable transformation, we introduced pLN18 and a plasmid expressing AvrPto into the tumorigenic strain A. tumefaciens A208 (Supplementary Fig. 2b). This engineered A. tumefaciens strain A208 was used for Arabidopsis root transformation assay33. Root segments inoculated with the A. tumefaciens strain carrying pLN18 and expressing AvrPto developed significantly more tumors compared to controls (Fig. 2c and d). T-DNA encoded iaaM, iaaH, and ipt genes of tumorigenic strains cause overproduction of phytohormones such as auxin and cytokinin in plants that lead to tumor formation34 and may affect plant defense responses35. Therefore, we tested stable transformation efficiency in Arabidopsis roots using non-tumorigenic strain EHA105 carrying binary vector pCAS120 that gives phosphinothricin (PPT) resistant calli because of a chimeric nos-bar gene expression in plants. Consistent with the tumor results, engineered A. tumefaciens strain carrying pLN18 and expressing AvrPto developed significantly more PPT-resistant calli compared to controls (Fig. 2e and Supplementary Fig. 3a). In addition, we also tested if our engineered A. tumefaciens strain can also enhance the floral dip transformation that is commonly used in Arabidopsis. We used a low concentration of A. tumefaciens (A600 = 0.1) to see subtle differences between the A. tumefaciens strains used. Surprisingly, delivery of AvrPto through T3SS increased the floral dip transformation efficiency by two-fold (Supplementary Fig. 3b).
Similar experiments were performed in a different plant species, N. benthamiana, using the disarmed strain A. tumefaciens GV2260 for transient expression and the tumorigenic strain A. tumefaciens A348 for stable leaf disk transformation22. These results were similar to those using Arabidopsis wherein expression of a T3SS and AvrPto in A. tumefaciens significantly increased both transient and stable transformation (Fig. 3a–d).
Like AvrPto, several other T3Es have the ability to suppress plant basal defense to establish/aid the growth of pathogens and cause disease14. To further examine the effect of other T3Es on AMT, we selected two T3Es from P. syringae pv. tomato: AvrPtoB and HopAO1. Similar to AvrPto, both AvrPtoB and HopAO1 significantly increased the percentage of root segments forming tumors and the weight of leaf disk tumors (Fig. 4 and Supplementary Fig. 4). As a negative control, another set of Arabidopsis root tumor assays was carried out using a HopAI1 construct. Since HopAI1 is targeting the PTI pathway by inhibiting MAPKs downstream of PAMP receptors36, we hypothesized that expression HopAI1 would not increase the susceptibility of the host to A. tumefaciens infection. As expected, we did not see any increase in transformation efficiency in the negative control (Supplementary Fig. 5a). These results suggest that T3Es when delivered through T3SS of engineered A. tumefaciens can enhance both transient and stable transformation in N. benthamiana and Arabidopsis.
Delivery of plant defense suppressing T3Es improves the transformation of crop plants
Both Arabidopsis and N. benthamiana are highly susceptible to stable AMT, and therefore the increase in transformation efficiency we observed by co-delivery of T3Es was only incremental for these species. Despite continuous efforts by many groups, efficient and reproducible Agrobacterium-mediated wheat transformation remains challenging37,38. Most reports of AMT of wheat have focused on the model spring wheat genotypes Fielder and Bobwhite39. We chose to determine if AMT of the wheat cultivar Fielder could be improved by co-delivery of T3Es. Immature embryos of wheat were infected with engineered A. tumefaciens strain AGL1 (pANIC6B) harboring pLN18 and a plasmid expressing T3E. The number of immature embryos that produced transgenic calli and subsequently regenerated shoots were counted. Transgenic plants derived from these regenerated shoots were tested for the activity and presence of reporter genes by GUS histochemical staining and PCR analysis of the GUSPlus and hph genes (Supplementary Fig. 6). A. tumefaciens strains individually delivering AvrPto, AvrPtoB, or HopAO1 through engineered T3SS greatly increased the percentage of individual transgenic plants obtained (Fig. 5a and Supplementary Fig. 7). The A. tumefaciens strain expressing AvrPto produced the best results, with a transformation efficiency ~400% that of the control strain lacking the T3SS components. These results indicate that A. tumefaciens with an engineered T3SS that delivers T3Es can increase the transformation efficiency of a recalcitrant crop species. Wheat transformation assay was also carried out using A. tumefaciens strains expressing HopAI1. Delivery of HopAI1 through T3SS did not have any effect on wheat transformation similar to the results obtained for Arabidopsis root assay (Supplementary Fig. 5b).
To determine if the engineered A. tumefaciens strains can also be used to improve the transformation efficiency of other commercial crop plants, we used our engineered strain that can deliver AvrPto through T3SS on alfalfa line R2336 and switchgrass line NFCX01. We observed 260% increase in transformation efficiency in alfalfa and 400% increase in transformation efficiency in switchgrass (Fig. 5b and c). These results indicate that engineered A. tumefaciens delivering AvrPto can be used to enhance AMT in many commercially important crop plants.
Virulence gene expression is not altered in the engineered A. tumefaciens strains expressing T3SS
As shown above, A. tumefaciens strains expressing T3SS and T3Es effectively increased AMT efficiency. The expression of T3Es in A. tumefaciens may increase virulence gene (vir) expression and thus increase transformation efficiency. To test this, we measured the expression of several vir genes in engineered A. tumefaciens A208 strains using reverse transcription-quantitative PCR (RT-qPCR). No major differences were observed in virA, virB2, virD2, and virE3 gene induction, after acetosyringone treatment, among A. tumefaciens strains with or without the T3SS + T3E (Supplementary Fig. 8). These results, along with those reported in Fig. 2, indicate that the increase in transformation by A. tumefaciens strains expressing T3SS and T3Es is not due to increased expression of vir genes and is most likely due to the delivery of T3Es into plant cells.
AvrPto delivered through engineered A. tumefaciens T3SS reduces the expression of plant defense genes
Based on the role of AvrPto in suppressing plant defense15, and our results showing the delivery of AvrPto along with T-DNA into plants increases AMT (Figs. 2 and 3), we speculated that the increase in AMT efficiency was due to the suppression of plant defense responses. To show that AvrPto delivered through engineered A. tumefaciens T3SS can suppress plant defense responses, we infected Arabidopsis roots with tumorigenic A. tumefaciens A208 expressing a T3SS and AvrPto, or with negative controls, and measured the expression of well-known PTI marker genes including FLG22-induced receptor-like kinase 1 (FRK1), and NDR1/HIN1-like 10 (NHL10). Irrespective of the A. tumefaciens strain used, both the tested defense-related genes were induced in response to A. tumefaciens infection at 2 h after infection when compared to a mock-infected control (Fig. 6). However, 16 h after A. tumefaciens infection, transcripts of defense-related genes were significantly reduced in root samples infected with A. tumefaciens expressing the T3SS and AvrPto compared to control strains (Fig. 6). These results indicate that AvrPto, when delivered through an engineered T3SS of A. tumefaciens, can suppress the plant defense response, thus contributing to increased AMT efficiency.
Delivery of a plant protein from an engineered A. tumefaciens strain expressing a T3SS enhances stable transformation
AMT is a complex process involving functions of both bacterial virulence proteins and plant proteins40. Histone H2A-1 (encoded by the gene HTA1) is involved in T-DNA integration24, and overexpression of HTA1 and truncated HTA1 (tHTA1; coding only the first 39 amino acids) in plants increases transformation efficiency24,41,42. To verify if plant proteins that enhance AMT can also be delivered through an engineered T3SS of A. tumefaciens, we chose HTA1 and tHTA1. Two different promoters, along with N-terminal sequences containing a type III signal from the T3Es AvrRpm1 and AvrRps4, designated as AvrRpm1N and AvrRps4N, respectively, were selected to drive the expression of HTA1 and tHTA1 and export from A. tumefaciens. Using the engineered A. tumefaciens strains, we conducted Arabidopsis root and N. benthamiana leaf disk tumor assays. Both HTA1 and tHTA1 expressing A. tumefaciens strains enhanced the stable transformation efficiency of Arabidopsis and N. benthamiana (Fig. 7a–c and Supplementary Fig. 9a). Transformation assays in crop plants using engineered strains expressing HTA1 also showed increased transformation efficiency in wheat, alfalfa, and switchgrass (Fig. 7d–f, Supplementary Fig. 9b and c). These results indicate that engineered A. tumefaciens expressing a T3SS can also be used to deliver plant proteins to enhance AMT.
Discussion
A. tumefaciens is a plant pathogen that causes crown gall disease in many plant species and has been widely used in the field of plant biotechnology and functional genomic studies, including the recently developed genome-editing technologies3,43. The application of AMT is limited to particular plant species/varieties due to low transformation efficiency, mainly caused by the induction of plant defense responses7,44,45,46. In the present work, we expressed the Pss61 T3SS in A. tumefaciens to deliver T3Es or a plant protein to Arabidopsis, N. benthamiana, and wheat to enhance AMT. We also showed that the increased transformation by T3E AvrPto is associated with an attenuated plant defense response. Many plant pathogenic bacteria contain T3SSs that act as an essential virulence determinant to deliver T3Es that remodel normal plant cellular functions, compromising the plants’ immune responses and promoting bacterial multiplication47. We used the T3SS of P. syringae species because it is well characterized48,49.
The T3SS has some limitations in the size and structure of proteins that it can deliver to the host cell. For example, the fusion of T3Es with a large fluorescent protein-like GFP interferes with effector secretion and translocation because of the inability of the type III ATPase to unfold the tightly packed GFP domain50. Therefore, we explored the possibility of using a small 13 KDa fluorescent reporter PhiLOV51, and successfully demonstrated its use in visualizing effector expression, secretion, and translocation to plant cells (Fig. 1 and Supplementary Fig. 1). Previously, PhiLOV has been used to tag T3Es of animal pathogens to monitor effector secretion and translocation52 and to visualize translocation and localization of A. tumefaciens virulence proteins53. In another study, a split GFP system was used to monitor the secretion of T3Es of P. syringae and R. solanacearum29,30. Recently, a T3SS gene cluster from Xanthomonas euvesicatoria, which is known to secrete large effectors54 was shown to secrete effectors into the plants55. However, heterologous expression of a Xanthomonas T3SS has not yet been reported55.
A previous attempt by Tsuda et al.16 to express T3Es other than AvrPto in planta to increase the transient transformation of Arabidopsis was not successful, likely because these effectors are not targeting the PTI pathway at the PAMP receptor level. We therefore selected the P. syringae T3Es AvrPtoB and HopAO1, which are involved in the early immune signaling of PTI. These proteins target PRRs and disrupt their functions14,56. In our study, both AvrPtoB and HopAO1, when co-delivered with T-DNA, increased the stable transformation of Arabidopsis, N. benthamiana, and wheat (Figs. 4 and 5a).
Research in several laboratories had previously suggested that AMT of wheat was not reproducible across laboratories37,38. Previously, an ~5% transformation efficiency was reported38. Recently, up to 25% AMT frequency of “Fielder” was achieved by manipulating various parameters, including the stage of the donor material and pretreatment by centrifugation38. However, using the conventional transformation method, we could only achieve ~15% stable transformation efficiency (Fig. 5a). With our strategy of co-delivering T3Es along with the T-DNA, we could achieve up to 63% transformation efficiency by delivering AvrPto through a T3SS (Fig. 5a). High transformation efficiency is critical for gene-editing technology, especially in agronomically important plants like wheat. The limitation of this strategy is that it cannot be used in plant varieties that are recalcitrant to regeneration.
To understand whether increased AMT observed in our study is due to higher bacterial virulence or suppression of plant immunity, we investigated the expression of Agrobacterium vir genes and plant defense genes after Agrobacterium infection. Constitutive expression of A. tumefaciens virA can increase tumor formation on Arabidopsis57. Increased transformation efficiencies were also achieved by additional copies of heterologous virB and virG genes when compatible Ti plasmids were used58,59. In the present study, the expression of vir genes in the Agrobacterium strain expressing T3SS and AvrPto did not show major differences from control strains. Agrobacterium infection induces the expression of various plant defense genes, including PR genes and those encoding chitinases and defensins7,32,60. FRK1, a commonly used molecular marker gene to study T3E-mediated suppression of plant defense61,62, is activated by PAMPs and not by other stress-related signals62. Many studies designed to optimize media composition for AMT rely on the expression of FRK1 and NHL10 to monitor plant defense responses63,64,65. We showed that the expression of FRK1, and NHL10 is reduced by an engineered Agrobacterium strain that delivers AvrPto through a T3SS, thus increasing AMT (Fig. 6).
One way to increase the efficiency of AMT is by suppressing the plant defense response as described above or by altering the expression of plant genes that play a role in AMT25. To determine if the engineered Agrobacterium with a T3SS can deliver plant proteins into plants cells, we used A. tumefaciens codon-optimized sequences of HTA1 and tHTA1. The expression of functional proteins in heterologous hosts is often enhanced by codon optimization66,67. Delivery of either HTA1 or tHTA1 through the T3SS increased AMT (Fig. 7).
Transformation and regeneration are major bottlenecks in the generation of transgenic plants or genome-edited plants. Our study aimed to improve transformation in the delivery and integration of T-DNA steps. The chimeric protein of plant developmental gene encoding GROWTH-REGULATING FACTOR 4 (GRF4) and its cofactor GRF-INTERACTING FACTOR 1 (GIF1) (GRF4-GIF1) and GRF5 were shown to enhance regeneration and transformation of both monocot and dicot species68,69. Specific morphogenic genes that are known to induce somatic embryogenesis and regeneration are also used to improve transformation efficiency in monocots70,71. Since constitutive expression of these genes has negative phenotypic and reproductive effects, altruistic transformation is used in maize and sorghum which uses the transient expression of Baby boom and Wuschel2 to promote somatic embryogenesis and regeneration in nearby transformed cells72,73. In the future, these proteins can be potentially delivered through Agrobacterium strain expressing T3SS to improve somatic embryogenesis and plant regeneration.
Heterologous protein expression in plants is achieved by stable or transient transformation by delivery of genes of interest harbored in Agrobacterium T-DNA74. AMT has emerged as a vehicle for the application of clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9-mediated genome editing of plants75. Genome-editing reagents are delivered to plants mostly through a stable transformation that requires segregation of Cas9 by Mendelian segregation to achieve transgene-free genome-edited plants (null segregants)43. In addition, off-target mutations may be increased by constitutive Cas9 expression76, which can be significantly reduced by conditional and transient expression of Cas975. Our approach of delivering proteins from Agrobacterium through a T3SS can not only increase AMT but also has the potential to alleviate the above-mentioned problems of CRISPR-mediated genome editing by delivering bacterially expressed Cas9 to plants through a T3SS instead of generating Cas9 expressing transgenic plants. In addition, our technology side-steps the disadvantages of making transgenic plants that overexpress genes that enhance transformation. Recently, direct delivery of proteins using Agrobacterium’s T4SS is getting attention, particularly in the field of DNA-free genome editing. For example, Cas9 translocation to plants through the T4SS by fusion with VirF translocation signal has been shown77. Previously, DNA modifying proteins such as site-specific recombinase Cre78 and homing endonuclease I-SceI79 have been translocated to plants through the T4SS. Our technology would be a good alternative to deliver genome-editing proteins because the T3SS is evolved for fast and efficient translocation of multiple effectors80.
Methods
Bacterial strains and growth conditions
Bacterial strains and plasmids used in this study are shown in Supplementary Data 1. E. coli DH5α was used for molecular cloning and was grown at 37 °C in Luria-Bertani (LB) medium. HB101 was used for maintaining the helper plasmid pRK2013. A. tumefaciens strains were grown at 28 °C on YEP agar plates or in YEP liquid medium, Agrobacterium minimal medium containing sucrose (AB-sucrose)81, hrp-derepressing liquid medium (HDM)28, or mannitol glutamate/lysogeny (MG/L) medium. Acetosyringone (200 µM) added to AB-MES65 (17.2 mM K2HPO4, 8.3 mM NaH2PO4, 18.7 mM NH4Cl, 2 mM KCl, 1.25 mM MgSO4, 100 µM CaCl2, 10 µM FeSO4, 50 mM MES, 2% glucose (w/v), pH 5.5) and ABM-MS65 (½ AB-MES, ¼ MS, 0.25% sucrose (w/v), pH 5.5) medium was also used. Antibiotics used were spectinomycin (25 µg mL−1), carbencillin (10 µg mL−1), rifampicin (10 µg mL−1), kanamycin (50 µg mL−1), gentamycin (25 µg mL−1), and tetracycline (5 µg mL−1).
Bacterial genetic manipulations and plasmid construction
Promoter sequences of AvrPto (116 bp upstream of ATG) followed by coding sequences without a stop codon, from P. syringae pv. tomato strain DC3000, as well as codon-optimized PhiLOV2.1 sequences, were synthesized and cloned into the broad host range vector pBBR1MCS5 at Eco53kI and KpnI sites to generate pBBR1MCS5-AvrPto-PhiLOV. AvrPto containing its native promoter was also synthesized and cloned into the Eco53kI and KpnI site of pBBR1MCS5 to generate pBBR1MCS5-AvrPto. The coding sequences of AvrPtoB and HopAO1, along with their native promoters (from P. syringae pv. tomato strain DC3000), were synthesized and cloned into the Eco53kI and KpnI site of pBBR1MCS5. Promoter sequences from AvrPtoB and HopAO1 are 93 bp and 86 bp, respectively, upstream of ATG. AvrRpm1N consists of 199 bp upstream of ATG and the first 267 bp of the CDS from P. syringae pv. maculicola27,82. AvrRps4N is defined as 129 bp upstream of ATG and the first 411 bp of the CDS from P. syringae pv. pisi83,84. Full-length and truncated HTA1 (coding first 39 amino acids41) sequences codon-optimized for A. tumefaciens driven by promoters and N-terminal sequences of AvrRpm1 as well as AvrRps4 were synthesized and cloned into Eco53kI and KpnI site of pBBR1MCS5. GenScript (Piscataway, NJ) carried out all DNA syntheses reported here. E. coli DH5α competent cells were transformed by a standard heat-shock procedure. Electroporation was used to introduce all the plasmids into A. tumefaciens strains, with the exception of pLN18. Triparental mating85 was used to mobilize pLN18 into A. tumefaciens strains.
Plant materials and growth conditions
For root transformation assays, Arabidopsis thaliana Columbia-0 (Col-0) plants were grown in B5 medium in an environment-controlled growth chamber at 24 °C, 70% humidity, and a 16/8 h light/dark photoperiod with the light intensity of 50–100 µE m−2 s−1. For leaf infiltration assays, Arabidopsis (Col-0) plants were grown in metromix soil in a controlled growth chamber at 22 °C, 75% humidity, and a 8/16 h light/dark photoperiod with the light intensity of 140 µE m−2 s−1 using fluorescent tubes. N. benthamiana plants were grown in soil in a controlled growth room at 24 °C, 75% humidity, and a 16/8 h light/dark photoperiod with the light intensity of 140 µE m−2 s−1 using fluorescent tubes.
Secretion assays and immunoblotting
To monitor the hrp-dependent effector secretion into the medium, A. tumefaciens strain GV2260 expressing different combinations of AvrPto-PhiLOV, and T3SS were grown on YEP agar plates at 28 °C for 2 days. Two colonies were transferred to HDM medium and cultured for 16 h at 28 °C with shaking at 220 rpm. Pellets from bacterial cultures at A600 = 0.25 were taken for cell pellet fraction analysis. Approximately 20 mL of the cultures (normalized based on the A600 of the bacterial cultures to get an equal protein amount) were separated into pellet and supernatant fractions by centrifuging the culture at 3220 × g for 15 min at 21 °C. The top 15 mL of the supernatant solution was carefully removed without disturbing the pellet. The supernatant solution was passed through a 0.45 µm Durapore PVDF Membrane Millipore filter (Catalog No. SE1M003M00, EMD Millipore Corporation, Burlington, MA), and further centrifugation steps were carried out at 4 °C. The supernatant fractions were concentrated by ultrafiltration using Amicon Ultra-15 Centrifugal Filters (Catalog No. UFC901024, Merck Millipore Ltd, Tullgreen, Ireland), and further concentrated to ~30 µL using Amicon Ultra-0.5 Centrifugal Filters (Catalog No. UFC501024, Merck Millipore Ltd, Tullgreen, Ireland) according to the manufacturer’s instructions. Proteins from the pellet as well as supernatant fractions were subjected to electrophoresis through a SDS-PAGE gel, and immunoblot analysis was carried out using PhiLOV-specific antibody (dilution 1:5000).
Confocal microscopy
A. tumefaciens strain GV2260 carrying GFP1−10 in a binary vector and the engineered A. tumefaciens strain GV2260 expressing a T3SS and various effectors tagged with GFP11 were grown on YEP plates containing the appropriate antibiotics for two days at 28 °C. Single colonies were inoculated into YEP liquid medium and incubated for 16 h, cells were resuspended in an induction medium containing 10 mM MES and 200 µM acetosyringone, and incubated at room temperature for 3 h with slow shaking. The A600 of the culture was adjusted to 0.4. Bacterial strains were syringe-infiltrated on the abaxial side of four-week-old N. benthamiana plants. A. tumefaciens strain GV2260 carrying a GFP1−10 gene in a binary vector was infiltrated 24 h prior to infiltration of GV2260 expressing a T3SS, and effectors, as well as negative controls. Forty-eight hours after infiltration, the infiltrated area was used for acquiring confocal micrographs with a Leica SP8 confocal microscope (Leica Microsystems, Wetzlar, Germany) using Leica Application Suite X (LAS X) software version 3.5.5.19976. GFP was excited at 488 nm and emission was gathered between 493 and 550 nm. Chloroplast autofluorescence emission was gathered between 650 and 732 nm. For FM4-64 staining, leaves were infiltrated with 25 µM FM4-64 (Catalog No. T13320, Invitrogen, Carlsbad, CA) for 1 h before microscopy. Excitations were carried out at 488 and 565 nm and emissions were gathered between 493 and 551, and 700 and 750 nm. For experiments using PhiLOV tagged effectors, excitation was carried out at 458 nm and emission was gathered between 474 and 530 nm.
Agrobacterium-mediated transient and stable transformation assays
Arabidopsis transient transformation assays were carried out by the previously described method86. In brief, A. tumefaciens strain EHA105 carrying different plasmids was used to infiltrate five leaves of 5-weeks-old soil-grown Arabidopsis plants. All five infiltrated leaves were harvested four days after infection for assaying GUS activity using qualitative histochemical staining and from three different plants, all five leaves were pooled for measuring GUS activity by quantitative fluorometric assays. The GUS histochemical staining assay was performed as previously described with some modifications using β-glucuronidase substrate X-gluc dissolved in DMSO87. In brief, plant materials were stained with X-gluc staining solution [100 mM sodium phosphate buffer (pH 7.0), 0.5 mM K3Fe(CN)6, 0.5 mM K4Fe(CN)6, 0.5 mM EDTA, 0.1% Triton X-100, and 1 mg mL−1 X-gluc] for one day at 37 °C in the dark. GUS activity was quantified using fluorometric measurements by the conversion of 4-methylumbelliferyl-β-D-glucuronide (4-MUG) (Catalog No. M9130, Sigma–Aldrich, St. Louis, MO) to 4-methylumbelliferone (4-MU)88. Fluorescence measurements of the 4-MU (excitation at 365 nm, emission at 455 nm) were carried out using a Tecan Infinite® 200 Pro multimode plate reader (Tecan, Switzerland) with i-control version 11 software. GUS activity was calculated using 4-MU (Catalog No. M1381, Sigma–Aldrich, St. Louis, MO) standards. The experiments were repeated three times on different days.
Arabidopsis root transformation assays were performed by following the previously described protocol33. In brief, axenic root segments were infected with A. tumefaciens A208 or its derivatives, co-cultivated for 48 h in the dark at room temperature, and transferred to MS-basal medium supplemented with cefotaxime (200 mg L−1) and ticarcillin (100 mg L−1). Four weeks after infection, tumor numbers were recorded.
Arabidopsis stable transformation root callus assays were carried out as previously described20. In brief, axenic root segments were infected with A. tumefaciens EHA105 containing pCAS120 or its derivatives (A600 = 0.001), co-cultivated for 48 h in the dark at room temperature, and transferred to a callus induction medium supplemented with cefotaxime (200 mg L−1), ticarcillin (100 mg L−1), and phosphinothricin (PPT) (10 mg L−1). Four weeks after infection, the number of root segments forming PPT-resistant calli was recorded. Arabidopsis transformation was performed by floral dip method89. Experiments were carried out in two biological replicates. In each experiment, ten plants were inoculated with strain EHA105 harboring different constructs (A600 = 0.1). T0 seeds were germinated on half-strength MS media containing hygromycin (20 mg L−1). Hygromycin-resistant plants were selected and stained for GUS activity as described above.
For N. benthamiana transient transformation assays, engineered A. tumefaciens strain GV2260 carrying different plasmids were prepared and infiltrated as described above for microscopy. Leaf disks were collected after 4 days of infection and GUS activity assays were carried out as described above. N. benthamiana leaf disk tumor assays were carried out as previously described22. In brief, leaves harvested from greenhouse-grown plants were sterilized using 8% bleach for five minutes, then washed four times with sterile distilled water. Leaf disks made using a cork borer (0.9 cm) were infected with A. tumefaciens strain A348 or its derivatives for 15 min followed by co-cultivation on MS-basal medium for 2 days in the dark at room temperature. Leaf disks were transferred onto MS-basal medium supplemented with cefotaxime (200 mg L−1) and ticarcillin (100 mg L−1). Fifteen days after transfer, the fresh weights of leaf disks were measured for the leaf disk tumorigenesis assay.
Wheat transformation
Wheat plants (cv. Fielder) were grown in a greenhouse with a 16/8 h light/dark photoperiod and 20–22 °C day/19–21 °C night. Immature ears were collected ~14 days after anthesis. The ears were sprayed with 70% ethanol. After removing the glume, lemma, and palea, the immature embryos (IEs) were isolated from these immature seeds under a dissecting microscope in a laminar flow hood. The IEs were centrifuged in 2 mL embryo-collection medium using a fixed-angle rotor at 17,000 × g at 4 °C for 10 min. The IEs were removed from the embryo-collection medium and infected in 1 mL inoculum (A600 = 0.5) of A. tumefaciens strain AGL1 carrying different plasmids grown in MG/L medium with 100 µM acetosyringone. The mixture was shaken at 90 rpm at room temperature for 15 min. The infected IEs were transferred onto co-cultivation medium with the scutellum side up. Plates were sealed with microfilm tape and then vacuum infiltrated for 7 min. The plates were incubated at 24 °C in the dark for 2 days. The embryo axis was removed from the IEs before transferring onto the resting medium, then subsequently cultured in the same conditions for 5 days. The IEs were subjected to two rounds of selection by transferring onto a selection medium containing 15 mg L−1 hygromycin for 2 weeks followed by 30 mg L−1 hygromycin for 3 weeks. The proliferating explants were then transferred onto a shoot regeneration medium with 30 mg L−1 hygromycin and cultured at 24 °C under illumination (16/8 h light/dark) until shoots were produced. The regenerated shoots were transferred to a root regeneration medium containing 15 mg L−1 hygromycin under the same growth conditions. Regenerated plants were transferred to soil and sampled for GUS activity staining (as described above) and genomic DNA extraction to test for the presence of transgenes by PCR for hph and GUSPlus genes. All primers used are listed in Supplementary Data 2.
RT-qPCR
To study the expression levels of A. tumefaciens vir genes, engineered A. tumefaciens strain A208 grown in YEP medium overnight at 28 °C was harvested and resuspended in AB-MES65 medium containing 200 µM acetosyringone. After incubation at room temperature with minimal shaking, bacterial cells were harvested at 24 h and stored at −80 °C for RNA extraction. RNA was extracted using a NucleoSpin RNA mini kit (Catalog No. 740955, Macherey-Nagel, Düren, Germany) according to the manufacturer’s instructions, including in-column genomic DNA digestion. Superscript III Reverse Transcriptase (Catalog No. 18080085, Invitrogen) was used for the synthesis of cDNAs using 1.5 µg of RNA and random hexamers (Catalog No. N8080127, Invitrogen). Quantitative PCR (qPCR) reactions were performed using a CFX Real-time PCR system (Applied Biosystems, Foster City, CA) and a KiCqStart SYBR Green qPCR ReadyMix (MilliporeSigma, St Louis, MO). Quantitative PCR data were collected using Bio-Rad CFX Manager Version 2.1.1022.0523 software. A minimum of three technical replicates and three biological replicates per experiment were done. Relative expression values were calculated using the 2−ΔΔCT method using recA as a housekeeping gene control. All primers used are listed in Supplementary Data 2.
For measuring the expression of plant defense genes, Arabidopsis plants were grown vertically on B5 medium for 12 days. Overnight cultures of engineered A. tumefaciens strain A208 grown in YEP medium at 28 °C were harvested, resuspended in ABM-MS medium containing 200 µM acetosyringone65, and incubated at room temperature with minimal shaking for 5 h. The A600 of all A. ` tumefaciens cultures was adjusted to 1.0 and the bacteria were pipetted onto roots as a thin layer90. For mock infection, ABM-MS medium was used instead of A. tumefaciens cultures. Roots were harvested 2 h and 16 h after infection, rinsed with water and frozen in liquid nitrogen for RNA extraction. RNA was extracted using an RNeasy plant mini kit (Catalog No. 74904, Qiagen, Valencia, CA). Samples were digested with TURBO DNase (Catalog No. AM1907, Invitrogen) to remove genomic DNA. Reverse transcription reactions were performed with 1 µg of RNA in a 20 µL reaction using Oligo(dT)12-18 (Catalog No. 18418012, Invitrogen) and SuperScript III Reverse Transcriptase (Invitrogen). qPCR reactions were performed using a CFX Real-time PCR system (Applied Biosystems) using KiCqStart SYBR Green qPCR ReadyMix (Catalog No. KCQS01, MilliporeSigma). A minimum of three technical replicates and three biological replicates per experiment were done. Relative expression values were calculated using the 2−ΔΔCT method using UBQ10 as a housekeeping control. All primers used are listed in Supplementary Data 2.
Alfalfa transformation
Alfalfa transformation was carried out following the previously described method91. Briefly, A. tumefaciens strain EHA105 harboring different constructs were streaked and cultured on AB agar plates containing different antibiotics at 28 °C for 2–3 days. A single colony was then cultured in AB liquid media, containing the same antibiotics, overnight till the A600 was 0.6–0.8. The young leaflets from 4-6-week-old alfalfa line R2336 plants were sterilized with 20% commercial bleach containing a drop of Tween-20 for 10 min and then washed three times with sterilized water. These leaves were then infected with the A. tumefaciens suspension by resuspending the pellets in a liquid infection medium to an A600 of 0.05 or 0.12 after centrifuging the A. tumefaciens liquid culture at 3500 rpm for 20 min. The infected leaves were blot dried and plated on co-cultivation medium and cultured under 24 °C in the dark for 24–30 h. These trifoliate explants were transferred onto selection medium containing 10 mg mL−1 hygromycin and continued growth for a total of 6–8 weeks under the same conditions. During this selection period, the explants were subcultured every 2 weeks until enough resistant calli produced. The resistant calli were then transferred onto a shoot regeneration medium with 5 mg mL−1 hygromycin and cultured at 24 °C day /20 °C night and 16/8 h light/dark photoperiod with 150 μmol m−2 s−1 light. Shoots regenerated after 2–3 months of transfer were counted and checked by PCR and GUS activity staining.
Switchgrass transformation
Switchgrass transformation was carried out according to previously reported protocol92. Briefly, switchgrass NFCX01 calli induced from inflorescence were infected with A. tumefaciens strain AGL1 carrying different plasmids. After co-cultivation in the dark chamber at 24 °C for 3 days, infected calli were transferred onto a selection medium with 50 mg L−1 hygromycin and cultured in the same conditions for 6–8 weeks. Resistant calli were then transferred onto a regeneration medium with 30 mg L−1 hygromycin and cultured in the light chamber 16/8 h light/dark photoperiod, 24 °C day/20 °C night, and 150 μmol m−2 s−1 light. The regenerated shoots were transferred onto a rooting medium with 10 mg L−1 hygromycin till plants grew big enough for screening by methods described for wheat transgenic plants.
Statistical analysis
GraphPad Prism version 8.0.1 was used for making graphs and ANOVA tests. R version 3.5.2 was used for all Tukey’s post-hoc tests.
Reporting summary
Further information on research design is available in the Nature Research Reporting Summary linked to this article.
Data availability
All relevant data supporting the key findings of this study are available within the article and its Supplementary Information files. Source data are provided with this paper.
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Acknowledgements
This work was supported by the National Science Foundation (grant # IOS-1725122 to K.S.M.) and the Noble Research Institute, LLC. We thank James R. Alfano (University of Nebraska-Lincoln) for providing pLN18, John M. Christie (University of Glasgow) for PhiLOV antibody, Gitta Coaker (University of California, Davis) for AvrPto-GFP11, AvrPtoB-GFP11 and GFP1-10, Michael Kovach (Baldwin Wallace University) for pBBR1MCS5, and Stanton Gelvin (Purdue University) for critical reading of the manuscript and providing A. tumefaciens strain EHA105. We also thank communications department at Noble Research Institute for photography, graphic design, and copy-editing.
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K.S.M. conceptualized the hypothesis. V.R., C.M.R., B.V., Q.J., and K.S.M. conceived and designed the experiments, and did data analysis and wrote the manuscript. V.R., C.M.R., B.V., K.D., J.K., S.O., J.Y., L.Y., G.L., and B.D.P conducted the experiments.
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Raman, V., Rojas, C.M., Vasudevan, B. et al. Agrobacterium expressing a type III secretion system delivers Pseudomonas effectors into plant cells to enhance transformation. Nat Commun 13, 2581 (2022). https://doi.org/10.1038/s41467-022-30180-3
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DOI: https://doi.org/10.1038/s41467-022-30180-3
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