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American Society of Plant Biologists The Protein Encoded by Oncogene 6b from Agrobacterium tumefaciens Interacts with a Nuclear Protein of Tobacco
a Division of Biological Science, Graduate School of Science, Nagoya University, Furo-cho, Chikusa-ku, Nagoya 464-8602, Japan 2 To whom correspondence should be addressed. E-mail yas{at}bio.nagoya-u.ac.jp; fax 81-52-789-2966
The 6b gene in the T-DNA from Agrobacterium has oncogenic activity in plant cells, inducing tumor formation, the phytohormone-independent division of cells, and alterations in leaf morphology. The product of the 6b gene appears to promote some aspects of the proliferation of plant cells, but the molecular mechanism of its action remains unknown. We report here that the 6b protein associates with a nuclear protein in tobacco that we have designated NtSIP1 (for Nicotiana tabacum 6b–interacting protein 1). NtSIP1 appears to be a transcription factor because its predicted amino acid sequence includes two regions that resemble a nuclear localization signal and a putative DNA binding motif, which is similar in terms of amino acid sequence to the triple helix motif of rice transcription factor GT-2. Expression in tobacco cells of a fusion protein composed of the DNA binding domain of the yeast GAL4 protein and the 6b protein activated the transcription of a reporter gene that was under the control of a chimeric promoter that included the GAL4 upstream activating sequence and the 35S minimal promoter of Cauliflower mosaic virus. Furthermore, nuclear localization of green fluorescent protein–fused 6b protein was enhanced by NtSIP1. A cluster of acidic residues in the 6b protein appeared to be essential for nuclear localization and for transactivation as well as for the hormone-independent growth of tobacco cells. Thus, it seems possible that the 6b protein might function in the proliferation of plant cells, at least in part, through an association with NtSIP1.
Agrobacterium cells that harbor a Ti plasmid induce the formation of crown gall tumors on dicotyledonous plants. Upon infection of a plant by Agrobacterium, a specific region of the Ti plasmid, known as T-DNA, is transferred to the plant cell and integrated into the chromosomal DNA in the nucleus. Plant cells that have been transformed with T-DNA can proliferate autonomously to generate a tumor, which is a consequence, for the most part, of the expression of genes that are responsible for the biosynthesis of auxin; and cytokinin (iaaM [tms1] or iaaH [tms2] for auxin; ipt [tmr] for cytokinin) in the T-DNA (Weiler and Spanier, 1981  ; Akiyoshi et al., 1984).
In addition to these genes, gene 6b, which is localized at the tml locus (Garfinkel et al., 1981
Various hypotheses have been proposed to explain the effects of the 6b protein on cell proliferation and organ development. It has been suggested that the 6b gene might function in the activation and/or inactivation of cytokinin and auxin (Hooykaas et al., 1988
Some clues to the mode of action of the 6b protein might be found in its amino acid sequence. However, there are no obvious motifs in 6b that are suggestive of a particular cellular function, even though there is a cluster of acidic amino acid residues near the C terminus (Levesque et al., 1988
Investigations in animals of oncogenicity that is caused by pathogenic factors such as the Rb and E1A proteins have contributed to our understanding of the mechanisms of cell proliferation and differentiation in animal systems (Nevins, 1991 In designing the present study, we postulated that the 6b protein might affect some process in the induction of cell division via interactions with a plant protein. We screened a tobacco cDNA library in an effort to identify candidate 6b-interacting proteins. We isolated several cDNA clones and characterized a cDNA that encoded a putative transcription factor, designated NtSIP1 (for Nicotiana tabacum 6b–interacting protein 1). We then demonstrated that NtSIP1 was localized in the nuclei of tobacco cells and enhanced the nuclear localization of 6b. Furthermore, we found that 6b activated transcription in tobacco cells. We propose that NtSIP1 might be responsible for some of the phenotypic effects of the 6b gene.
Acidic Region of the 6b Protein Is Required for Callus Formation and Shoot Regeneration on Hormone-Free Medium We first examined whether the acidic region of the 6b protein is required for cell growth on phytohormone-free medium. In all of the experiments described in this article, with the exception of the experiment described in the next section, we used the 6b gene from pTiAKE10 for our analysis because the formation of calli in response to the 6b gene from pTiAKE10 on hormone-free medium was more efficient than that in response to the 6b genes from other Ti plasmids (Spanier et al., 1989 ; Wabiko and Minemura, 1996). Hereafter, for simplicity's sake, we refer to the 6b gene from pTiAKE10 simply as 6b. We constructed a His and T7 epitope–tagged 6b gene and a similar 6b A gene, in which the entire acidic region (residues 164 to 184) had been deleted (His-T7-6b and His-T7-6bA, respectively) (Table 1, Figure 1A)
. These constructs were linked to the 35S promoter of Cauliflower mosaic virus (P35S) in the binary vector pBI121. Each fusion gene was introduced into cells of leaf discs of tobacco. Shoot-bearing calli were generated on phytohormone-free medium from leaf discs that had been transformed with the His-T7-6b gene within 3 weeks (Figure 1Ba). In contrast, no calli were generated on phytohormone-free medium from His-T7-6bA–transformed leaf discs and from discs transformed with the vector pBI121 (Figures 1Bb and 1Bc). As shown in Figure 1Bd, the amount of His-T7-6bA protein synthesized in tobacco cells was similar to that of the His-T7-6b protein. We also examined a mutation in the region adjacent to the acidic region for its effect on hormone-independent growth. The mutation resulted in the same phenotype as His-T7-6b (data not shown). These results indicated that the C-terminal acidic region of 6b was necessary for the induction of shoot-bearing calli on phytohormone-free medium.
Isolation of cDNAs for 6b-Interacting Proteins by Screening with the Yeast Two-Hybrid System To isolate tobacco cDNAs for 6b-interacting proteins, we screened a cDNA library prepared from tobacco Bright Yellow 2 (BY-2) cells using the yeast two-hybrid system. We first examined the potential background transcriptional activity of 6b proteins in yeast cells. The DNA fragment encoding the DNA binding domain of LexA was fused with 6b genes from two types of Ti plasmid, pTiAKE10 and pTiB6S3trac, and the transcriptional activity of the product of each of the fusion genes was measured. The transcriptional activity of the product of the 6b gene derived from pTiB6S3trac [6b(B6)] was lower than that of the product of the 6b gene from pTiAKE10, even though 6b(B6) had some background activity (data not shown). To reduce the background still further, we introduced deletions in the region that encoded the acidic region of 6b and decided to use, as "bait," the 6b C(B6) DNA construct, in which the DNA sequence corresponding to the C-terminal peptide from the middle of the acidic region to the C terminus had been deleted (residues 173 to 208) (Figure 1A). LexA-fused 6bC(B6) had low transcriptional activity in yeast and thus was suitable for screening with the two-hybrid system.
Using the truncated construct, we screened
Using the two-hybrid system, we next examined whether the acidic region of 6b was required for the interaction with NtSIP1. Because the LexA-fused 6b gene exhibited strong transcriptional activity in yeast cells, we fused the cDNA for NtSIP1 to the LexA sequence (LexA:cNtSIP1) to generate a bait construct and fused the 6b gene or the 6b
cNtSIP1 Encodes a Nuclear Protein with a Triple Helix Motif A computer-assisted homology search revealed that there are several homologs (F14P22.220, MOP10_9, F9F8.9, and F11B9.6) of the NtSIP1 gene in the genome of Arabidopsis (Figure 3A). The amino acid sequence of NtSIP1 was 43% identical to that of the predicted product of F14P22.220, 36% identical to that of MOP10_9, 34% identical to that of F9F8.9, and 27% identical to that of F11B9.6. A phylogenetic tree analysis indicated that NtSIP1 was related closely to F14P22.220 of Arabidopsis. The amino acid sequences of NtSIP1 and F14P22.220 aligned throughout the length of the proteins with several small gaps. Amino acid sequences corresponding to a triple helix motif and nuclear localization signals are conserved in all of these deduced sequences (Figure 3A).
We fused the cDNA for a modified form of green fluorescent protein (sGFP) (Chiu et al., 1996 DNA gel blot analysis with genomic DNA from tobacco yielded a single band of DNA when the entire cNtSIP1 was used as a probe, suggesting that NtSIP1 is a single-copy gene (data not shown). We also examined the sites and levels of accumulation of NtSIP1 transcripts in normal tobacco plants. We found that NtSIP1 transcripts accumulated in roots, stems, mature leaves, and shoot apices, which included the shoot apical meristem, and levels of transcripts were significantly higher in shoot apices than in other organs (data not shown).
NtSIP1 Interacts with 6b in Vitro
NtSIP1 Enhances the Nuclear Localization of the 6b Protein in Tobacco Cells
The nuclear localization of sGFP-6b was not defined as clearly in suspension-cultured BY-2 cells (Figure 5Ba) as it was in mesophyll cells, perhaps because the level of expression of NtSIP1 in BY-2 cells was lower than that in mesophyll cells (Figure 5Ad). To examine this possibility, we cotransfected BY-2 cells transiently with P35S-linked sGFP:6b and P35S-linked cNtSIP1. As shown in Figures 5Ba and 5Bb, the relative intensity of fluorescence from sGFP-6b in nuclei was higher after cotransfection with P35S-linked cNtSIP1 (Figure 5Bb) than after cotransfection with the empty vector DNA (pBI221; Figure 5Ba). When BY-2 cells were cotransfected with P35S-linked sGFP:6b
To quantify the relative intensities of fluorescence in nuclei, we chose nine cells at random in each experiment with a particular combination of genes. We measured the fluorescence per unit area of the nucleus and of a cytoplasmic region within each cell and calculated average values for each experiment. The average value from the nuclei was divided by that from the cytoplasmic region to provide a relative value in each case (Figure 5C). The relative value for cells that expressed sGFP:6b and cNtSIP1 (Figure 5C, bar b) was higher than that for cells that expressed sGFP:6b alone (Figure 5C, bar a), sGFP:6b These results indicated that NtSIP1 enhanced the nuclear localization of sGFP-6b in BY-2 cells and that the acidic region of 6b was necessary for the enhancement of the nuclear localization of sGFP-6b.
A Fusion Protein Composed of the DNA Binding Domain of Yeast GAL4 and 6b Activates Transcription in Tobacco Cells
6b . Protein Affects the Transcription of Plant Genes The present study showed that the 6b protein encoded by the T-DNA of Agrobacterium can associate with the nuclear protein NtSIP1 of tobacco (Figures 2, 4, and 5) and that 6b was itself localized in the nuclei of plant cells (Figure 5). It seems likely that the NtSIP1 protein is a transcription factor because it includes two NLS-like sequences and a sequence that is similar to that of the triple helix motif of rice transcription factor GT-2 (Figure 3), a protein that binds to the GT box in the phyA promoter (Dehesh et al., 1992 ). In addition, the GALDBD-6b protein induced the expression of a reporter gene that was driven by a GAL4 UAS-fused promoter in BY-2 cells (Figure 6). The 6b protein included a cluster of acidic amino acid residues near its C terminus, and this cluster was necessary for the interaction of 6b with NtSIP1, for transactivation of the reporter gene by 6b, and for generation of shoot-bearing calli by 6b in the absence of exogenous plant hormones (Figure 1). Our observations suggest that the 6b protein in plant cells might affect the transcription of certain plant genes directly, which might induce at least some of the phenotypic abnormalities that are known to be associated with the expression of 6b, as described in the Introduction. Genes controlled by NtSIP1 might be candidates for such genes. Thus, the present study provides a new paradigm for the action of a gene that is introduced into plant cells upon infection by a pathogenic bacterium. Full understanding of the roles and actions of NtSIP1 requires further experimentation. The present results do not exclude possible roles for 6b in the cytoplasm, because we did detect 6b in the cytoplasm of plant cells as well as in the nuclei.
Experiments with GAL4 fusion proteins demonstrated that a protein encoded by the avirulence (avr) gene avrXa10 of Xanthomonas oryzae can activate transcription in plant cells and that the acidic region of AvrXa10 is required for both transcriptional activation and avirulence activity (Zhu et al., 1998
Role of the Interactions of 6b with Plant Proteins Such as NtSIP1 in Phenotypic Expression Regardless of the actual mechanism of the nuclear localization of 6b, the existence of NtSIP1, a nuclear protein that interacts with 6b, suggests that the efficiency of the nuclear localization of 6b might depend on cellular levels of all 6b-interacting proteins, including NtSIP1, and such levels also might depend on the specific type of cell or tissue. In this regard, it is noteworthy that sGFP-6b accumulated much more efficiently in the nuclei of mesophyll cells than in the nuclei of BY-2 cells. This might have been caused by differences in the total amounts of 6b-interacting proteins between the two types of cells. As described in Results, we isolated a second 6b-interacting protein, designated NtSIP2, which remains to be characterized in detail. We also found recently that a tobacco transcription factor with an obvious DNA binding motif interacted with 6b (data not shown). It seems likely that there are several 6b-interacting proteins in plants and that the phenotypes generated by the expression of 6b might depend on the types of 6b-interacting protein.
6b . Protein Might Function as a Transcriptional Coactivator/Mediator or as a Repressor The functions of NtSIP1 might be affected by 6b, but functional interactions between these proteins remain to be examined. The functions of NtSIP1 in plant growth and development under normal conditions also need to be clarified. The accumulation of NtSIP1 transcripts in the shoot apex is consistent with a role in plant growth. In addition, it will be of interest to determine whether there might be a relationship between the functions of this protein and the actions of phytohormones. "Reverse genetics," using transgenic tobacco plants that express sense and antisense cDNAs, as well as dominant inhibitory cDNAs, might be helpful in approaching these problems. We also have been studying Arabidopsis and have found that transgenic Arabidopsis plants that carried the 6b gene exhibited various developmental abnormalities, including leaf curling, serration, and dwarfism (our unpublished data). A computer-assisted homology search revealed that there were several homologs of genes for NtSIP1 in the Arabidopsis genome. Among them, the predicted amino acid sequence from F14P22.220 exhibited the strongest similarity to that of NtSIP1 (Figure 3). The functions of this hypothetical protein remain to be determined, and mutational analysis of this and similar genes might provide further clues to the functions of NtSIP1.
Plant Materials Tobacco (Nicotiana tabacum cv SR1), used as the host for transformation, was grown on Murashige and Skoog (1962) medium prepared with 1% agar in light (3000 to 5000 lux) for 16 hr/day and in darkness for 8 hr/day at 26°C. Suspension cultures of the Bright Yellow 2 cell line of tobacco (BY-2 cells) were maintained as described previously (Banno et al., 1993).
Transformation
Construction of Plasmids
For screening by the yeast two-hybrid system, DNA with a deletion from codon 173 to codon 208 of the 6b(B6) gene was generated by polymerase chain reaction and designated 6b
Yeast Two-Hybrid Screening
Interactions between 6b and NtSIP1 in Yeast
Preparation of Protoplasts and Assays of Transcriptional Activation
For assays of transcriptional activation, cells were incubated for 24 hr in darkness at 26°C and then subjected to enzymatic assays as described in the instructions from the manufacturer of the assay system (Dual-Luciferase Reporter Assay System; Promega, Madison, WI). The assay of firefly luciferase activity was initiated by adding 20 µL of a solution of extracted protein to 100 µL of Luciferase Assay Reagent II. Quenching of the luminescence of firefly luciferase and concomitant activation of Renilla luciferase for normalization were accomplished by adding Stop and Glo reagent in Dual-Luciferase Reporter Assay System to the sample tube immediately after quantitation of the activity of the firefly luciferase. Luciferase activities were measured with a photomultiplier as described elsewhere (Kondo et al., 1993
Subcellular Localization of sGFP-Fused 6b and sGFP-Fused NtSIP1
Expression and Purification of Recombinant Proteins and Immunochemical Analysis
Accession Numbers
The authors thank Dr. Chiyoko Machida for helpful discussions. This work was supported in part by a grant for the Research for the Future Program from the Japan Society for the Promotion of Science (No. JSPS-RFTF 97L00601) and by a Grant-in-Aid for Scientific Research on Priority Areas (No. 10182101) from the Ministry of Education, Science, Culture, and Sports of Japan. T.F. and Y.U. were supported by the Japan Society for the Promotion of Science.
Article, publication date, and citation information can be found at www.plantcell.org/cgi/doi/10.1105/tpc.010360.
1 Current address: National Institute for Basic Biology, 38 Nishigounaka, Myo-daiji-cho, Okazaki 444-8585, Japan. Received August 16, 2001; accepted October 25, 2001.
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Abstract
INTRODUCTION
4 x 106 independent yeast transformants and isolated 10 positive clones, which we divided into two groups after comparing the patterns of digestion by restriction enzymes of the inserts in the cDNA clones. The product of one of the cDNAs was designated NtSIP1, the cDNA was designated cNtSIP1, and the corresponding tobacco gene was designated NtSIP1. 
-helices with short intervening loops (
-mercaptoethanol and concentrated with an Ultrafree-4 centrifugal filter unit (Nihon Millipore). His-T7-NRK1 (NRK1 is a member of the tobacco family of mitogen-activated protein kinases) was produced in E. coli and purified similarly (a gift from T. Soyano, Nagoya University, Japan). Two kinds of recombinant protein (0.5 µg each) were mixed in 100 µL of binding buffer (100 mM NaCl, 50 mM Tris-HCl, pH 7.5, 1 mM EDTA, 0.5% [w/v] Triton X-100, 5 mM 
