JP2001299118A - C3 plant body capable of expressing photosynthetic enzyme of c4 plant - Google Patents

Abstract

PROBLEM TO BE SOLVED: To provide a C3 plant with a raised photosynthetic activity. SOLUTION: This C3 plant is obtained by transducing a DNA containing an expression regulatory region of an enzyme gene constituting a photosynthetic pathway of a C4 plant and a structural gene of the enzyme constituting the photosynthetic pathway into a C3 plant cell. The resultant C3 plant is capable of highly expressing the enzyme.

Description

DETAILED DESCRIPTION OF THE INVENTION

[0001]

TECHNICAL FIELD [0001] The present invention relates to a C3 plant having a gene for an enzyme constituting the C4 photosynthetic pathway (hereinafter referred to as C4 photosynthetic gene) and highly expressing this C4 photosynthetic gene.

[0002]

2. Description of the Related Art Plants are classified into C3 plants, C4 plants and succulent photosynthesis (CAM) plants according to the type of the initial fixation product of carbon dioxide in the photosynthetic carbonic acid fixation pathway.
90% or more of the plants on the earth belong to C3 plants, and include, for example, agriculturally useful plants such as rice and wheat. The photosynthetic pathway of this C3 plant is also called the Calvin pathway, and the enzyme involved in CO ₂ fixation in this pathway is ribulose-1,5-diphosphate carboxylase. This enzyme has a low affinity for CO ₂ and, conversely, a high affinity for oxygen, so that the efficiency of the CO ₂ fixation reaction and, consequently, the photosynthesis reaction is low.

[0003] On the other hand, C4 plants have evolved to overcome this inefficient CO ₂ fixation reaction, have a mechanism for concentrating CO ₂ , and have high photosynthetic ability. The enzyme involved in CO ₂ fixation in the photosynthetic pathway of this C4 plant is phosphoenolpyruvate carboxylase. This enzyme is not inhibited by oxygen and has a high ability to immobilize CO ₂ .

[0004] CAM plants have a photosynthetic system adapted to a dry environment, and this photosynthetic system is considered to be a kind of advanced form of C3 photosynthesis.

[0005] By imparting the photosynthetic function of C4 plants to C3 plants, it is expected that the photosynthetic ability and substance producing ability of agriculturally useful C3 plants (eg, rice) will be greatly improved. Therefore, several attempts have been made to introduce the C4 photosynthesis gene into C3 plants. For example, a promoter highly expressed in leaf tissue of a C3 plant (for example, a chlorophyll a / b binding protein gene promoter or a cauliflower mosaic virus (CaMV) 35S promoter) is added to a photosynthetic gene of a C4 plant (phosphoenolpyruvate carboxylase (PEPC) gene). ) To create a recombinant DNA, C
Although it has been reported to be introduced into three plants, tobacco, PEPC activity in C3 plants only increased 2-3 times, at best (Kogami et al., Transgenic Research 3: 287).
-296 (1994)). On the other hand, a fusion gene of the β-glucuronidase (GUS) gene of Escherichia coli and the 5 ′ flanking region (promoter region) of the PEPC gene was introduced into a C3 plant, tobacco, in order to examine the action of the C4 photosynthesis gene promoter. Thus, an example of expressing the GUS gene at a high level has been reported (Matsuoka et al., Plant Physiol. 111: 949-957 (199).
6)). However, the maize PEPC genomic gene having the C4 photosynthetic gene expression regulatory region (promoter active region) was introduced into tobacco, but its PEPC activity was only a few.
There are reports that they only increased by a factor of two (Hudspeth
Et al., Plant Physiol. 98: 458-464 (1992)). Therefore, there has not been reported any case in which the gene of an enzyme involved in photosynthesis is actually highly expressed, and a technology for enhancing the photosynthetic ability of C3 plants by highly expressing the photosynthetic genes of C4 plants in C3 plants is expected. I have.

[0006]

The object of the present invention is to solve the above-mentioned problems, and an object of the present invention is to highly express the photosynthetic gene of a C4 plant in a C3 plant.

[0007]

As described above, an example in which an attempt was made to introduce a genomic gene (PEPC) constituting the photosynthetic pathway of C4 plant maize (Poaceae) into C3 plant Tobacco (Solanaceae) However, the expression efficiency was low. However, the present inventors have developed C4 plants that are evolutionarily phylogenetically related to C3 plants.
By simultaneously introducing the expression control region of the enzyme that constitutes the photosynthetic pathway of the plant and the structural gene of the enzyme that constitutes the C4 photosynthetic pathway into the C3 plant, the expression efficiency of the enzyme that constitutes the photosynthetic pathway of the C4 plant is greatly improved. Thus, the present invention has been completed.

[0008] The present invention relates to a C3 plant, a C3 plant tissue, or a C3 plant seed that expresses a gene of a C4 plant closely related to evolutionary phylogeny, wherein the gene of an enzyme constituting the photosynthetic pathway of the C4 plant is provided. And a DNA containing a structural gene of an enzyme that constitutes the photosynthetic pathway of the C4 plant.
The present invention relates to a C3 plant, a C3 plant tissue, or a C3 plant seed which highly expresses an enzyme constituting a plant photosynthetic pathway.

In a preferred embodiment, the C4 plant is a monocotyledonous plant, and the C3 plant, C3 plant tissue, or C3 plant seed is a monocotyledonous plant, plant tissue, or plant seed.

In a preferred embodiment, the C4
The plant is a dicotyledonous plant, the C3 plant, C3 plant tissue,
Alternatively, the C3 plant seed is a dicotyledonous plant, plant tissue, or plant seed.

[0011] In a further preferred embodiment, the C4
The genomic gene of the C4 plant is a DNA containing the expression regulatory region of the gene of the enzyme that constitutes the photosynthetic pathway of the plant and the structural gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant.

In a more preferred embodiment, the genomic gene of the C4 plant is a genomic gene of a Poaceae plant, and the C3 plant is a Poaceae plant, a Poaceae plant tissue, or a Poaceae seed.

In a most preferred embodiment, the genomic gene of the C4 plant is a corn phosphoenolpyruvate carboxylase genomic gene,
C3 gramineous plant is rice.

Further, the present invention relates to a method for producing a C3 plant, a C3 plant tissue, or a C3 plant seed which highly expresses an enzyme constituting a photosynthetic pathway of a C4 plant which is closely related to evolutionary phylogeny, DNA containing an expression regulatory region of a gene of an enzyme constituting the photosynthetic pathway of a C4 plant closely related to evolutionary phylogeny and a structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant
Transforming the cells of a C3 plant with
Regenerating a C3 plant cell into a C3 plant tissue or a C3 plant; and, in the case of a C3 plant seed, further comprising: obtaining a seed from the C3 plant.

[0015] In a preferred embodiment, the C4 plant is a monocotyledonous plant, and the C3 plant, C3 plant tissue, or C3 plant seed is a monocotyledonous plant, plant tissue, or plant seed.

In a preferred embodiment, the C4
The plant is a dicotyledonous plant, the C3 plant, C3 plant tissue,
Alternatively, the C3 plant seed is a dicotyledonous plant, plant tissue, or plant seed.

In a further preferred embodiment, the C4
The genomic gene of the C4 plant is a DNA containing the expression regulatory region of the gene of the enzyme that constitutes the photosynthetic pathway of the plant and the structural gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant.

In a more preferred embodiment, the genomic gene of the C4 plant is a genomic gene of a Poaceae plant, and the C3 plant is a Poaceae plant, a Poaceae tissue, or a Poaceae seed.

In a most preferred embodiment, the genomic gene of the C4 plant is a corn phosphoenolpyruvate carboxylase genomic gene,
C3 gramineous plant is rice.

[0020]

DESCRIPTION OF THE PREFERRED EMBODIMENTS The present invention will be described below in detail.

(Definition) In the specification of the present application, the phrase "evolutionally phylogenetically related" means that they are closely related taxonomically, for example, that they belong to the same family.

As used herein, the term "plant" includes a plant, a plant cell, a plant tissue, and a seed.

When referring to a C3 plant, CO3 is involved in the C3 photosynthetic pathway.
_2. A plant that fixes ₂ and includes monocotyledonous plants such as rice, wheat and barley, and dicotyledonous plants such as soybean, potato and sweet potato.

C4 plants are plants that fix CO _{2 in the} C4 photosynthetic pathway, and include monocotyledonous plants such as corn, sugarcane and sorghum, and dicotyledonous plants such as Flaveleria and Amaranthus.

"Enzymes constituting the C4 photosynthetic pathway" refer to enzymes involved in photosynthesis of C4 plants, and include carbonic anhydrase (CA),
Phosphoenolpyruvate carboxylase (PEPC), pyruvate orthophosphate dikinase (PPDK), malate dehydrogenase (MDH), malic enzyme, alanine-
Oxaloacetate aminotransferase, phosphoenolpyruvate carboxykinase (PEPCK) and the like. Expression control regions and structural genes of these enzyme genes can be used in the present invention.

As used herein, “highly expressed” refers to C3
When the gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant is introduced into the plant, the specific activity (activity per unit protein mass) of the enzyme in the crude extract of the green leaf of the C3 plant after the introduction is changed by the C3 before the introduction.
It means that the specific activity of the enzyme in the plant is at least 10 times or more. Preferably it is 40 times or more, more preferably 75 times or more, and most preferably 100 times or more.

As used herein, the term “expression control region” refers to a region having a sequence that regulates the expression of a structural gene. The expression control region includes, but is not limited to, for example, a transcription control sequence, a post-transcription control sequence, and / or a transcription termination sequence. "Transcriptional regulatory sequences" include sequences such as promoters, repressors, activators, enhancers, and the like. "Post-transcriptional regulatory sequences" refer to primary transcripts whose post-transcriptional processing (eg, poly A addition,
Cap sequences, splicing, etc.). "Transcription termination sequence" includes a sequence involved in termination of transcription, such as a terminator. These expression control regions can be separately arranged upstream or downstream of the structural gene depending on their characteristics. The intron also corresponds to the expression control region.

As used herein, “DNA containing the expression control region of the enzyme gene constituting the photosynthetic pathway of the C4 plant and the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant” refers to the expression regulatory region and the structure of the enzyme. Recombination with gene D
It means an NA sequence, a genomic gene sequence containing an expression control region and a structural gene of an enzyme, or an expression vector containing this recombinant DNA sequence or genomic gene sequence. This DN
A also includes chemically synthesized DNA.

When referring to a structural gene, a DNA encoding an enzyme protein part (which may contain introns)
And cDNA from mRNA.

The expression vector incorporates "a DNA containing an expression control region of an enzyme gene constituting a photosynthetic pathway of a C4 plant and a structural gene of an enzyme constituting a photosynthetic pathway of a C4 plant", and operates in a host cell. Refers to nucleic acid sequences that are ligated in an obtainable manner. The expression vector may contain expression control sequences (eg, various control elements such as promoter, enhancer, terminator, etc.) other than the C4 plant expression control region to be introduced. This expression control sequence can also be used to control the expression of C4 plants.

(Isolation of Expression Regulatory Regions and Structural Genes of Enzymes Constituting Photosynthetic Pathway of C4 Plant) In the present invention, C4 plants and C3 plants which are closely related in evolutionary phylogeny are used.
Preferably, they are plants belonging to the same family. More preferably, when the gene of C4 monocotyledon is used, it is transformed into C3 monocotyledon, or when the gene of C4 dicotyledon is used, it is transformed into C3 dicotyledon.

The structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant can be isolated by a well-known method. MRNA, which is a transcription product of the structural gene of this enzyme, is isolated, and cDNA is prepared therefrom. Using this cDNA, genomic DNA can be screened to obtain the expression regulatory region of this enzyme. A genomic gene fragment of about 8 Kb including maize PEPC has already been isolated (Eur. J. Biochem. 181: 593-598, 198).
9) This genomic gene fragment can be used as it is because it contains expression regulatory regions called upstream and downstream of PEPC structural gene and intron.

Another gene constituting the C4 photosynthetic pathway, PPDK
Genomic genes (corn) have also been isolated (Matsuoka et al., J. Biol. Chem. 265: 16772-16777 (199).
0)), which can be used in the present invention. The expression regulatory regions of this PPDK genomic gene are similar to PEPC, and these expression regulatory regions can be used in the present invention. Furthermore, NADP-
A genomic gene for malic enzyme has also been isolated (Rotherm
el et al., J. Biol. Chem. 264: 19587-19592, 1989). The expression control region and structural gene of this genomic gene can also be used in the present invention.

Using the expression regulatory regions of the genes (eg, PEPC, PPDK, malic enzyme) constituting the C4 photosynthetic pathway, carbonic anhydrase (CA), phosphoenolpyruvate carboxylase (PEPC), pyruvate Orthophosphate dikinase (PPDK), malate dehydrogenase (M
DH), malic enzyme, alanine-oxaloacetate aminotransferase, structural genes of phosphoenolpyruvate carboxykinase (PEPCK), and the like.

The structural gene of malate dehydrogenase or alanine-oxaloacetate aminotransferase can be obtained by a method known to those skilled in the art: these enzymes are isolated and purified, and a partial amino acid sequence is determined. By making and hybridizing a probe based on the amino acid sequence: Expression control regions of these enzymes can also be used in the present invention. If the genomic gene encoding the obtained enzyme contains an expression control region and a structural gene, this genomic gene can be used as it is. The expression control region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant can be determined by comparing the sequence of the expression region of another plant gene.

A recombinant gene having an expression control region of an enzyme constituting the photosynthetic pathway of a C4 plant and a structural gene can be prepared by a method well known to those skilled in the art. This recombinant gene is
It may have multiple expression control regions and / or structural genes.

The genomic gene of the enzyme constituting the photosynthetic pathway of the obtained C4 plant, or the recombinant DNA obtained above
The sequence can be used for transformation of C3 plants, either as such or in the form of an expression vector connected to a vector. In addition, a plurality of recombinant DNA sequences or genomic genes may be incorporated, or two or more kinds may be incorporated.

(Construction of Expression Vector) It is well known to those skilled in the art that the vector for preparing the expression vector can be selected according to the purpose of expression and the host cell.
The starting vector may suitably have a promoter, an enhancer, a T-DNA region and a drug resistance gene.

The vector used to construct the expression vector of the present invention does not necessarily require a promoter for expressing the C4 plant gene. This is because the expression regulatory region (promoter) of the C4 plant, which is closely related to the evolutionary phylogeny, is considered to function also in the expression regulatory system of the C3 plant. However, it may be preferable that the expression vector used in the present invention has an expression control region. Examples of the promoter in this case include a promoter whose expression is induced by a certain stress such as a tobacco infection-specific protein PR1a, a CaMV 35S promoter, a nopaline synthase (NO
The promoter of S) and the like can be mentioned, but not limited thereto.

An enhancer can be used for high expression. As the enhancer, an enhancer region containing a sequence upstream of the CaMV 35S promoter is preferable. A plurality of enhancers may be used.

A terminator can also be used. Examples of the terminator include, but are not limited to, a CaMV35S terminator, a nopaline synthase terminator (TNOS), and a tobacco PR1a gene terminator.

As the drug resistance gene, it is desirable that a transformed plant can be easily selected. Neomycin phosphotransferase 2 (NPT2) gene, hygromycin phosphotransferase (HPT) gene and the like can be suitably used. The promoter for expressing the drug resistance gene includes, but is not limited to, the above-mentioned plant gene promoter. Preferably, it is highly expressed constitutively
The CaMV35S promoter can be used. The NPT2 gene is useful for detecting a transformed strain and a transformed cell.
The HPT gene is expressed when the gene is integrated into the nuclear genome of the plant, and the plant becomes hygromycin-resistant, confirming that the gene has been introduced into the nuclear genome.

As a starting vector for constructing an expression vector used in the present invention, a pBI-based vector, a pUC-based vector, or a pTRA-based vector can be suitably used. A pBI binary vector can be suitably used. This vector is a gene of a region (T-region) that can be introduced into a plant,
NPT2 gene (which confers kanamycin resistance) expressed under the control of a plant promoter is included as a marker gene. A pBI vector can introduce a target gene into a plant via Agrobacterium. For example, pB
I121, pBI101, pBI101.2, pBI101.3 and the like. Preferably, pBI101 and a vector derived therefrom can be used.

As pUC-type vectors, for example, pUC1
8, pUC19, pUC9 and the like.

The binding of the expression controlling region of the enzyme constituting the photosynthetic pathway of the C4 plant to the vector and the DNA containing the structural gene can be prepared by a method well known to those skilled in the art. For example, when using a pBI vector, the multicloning site is cut with an appropriate enzyme, the target DNA is inserted, Escherichia coli is transformed, a transformant is selected, and the expression vector is recovered.

(Introduction of Recombinant DNA Sequence or Expression Vector into C3 Plant Cell) The C3 plant to be transformed includes, but is not limited to, rice, wheat, barley, soybean, potato and the like. Plant cells from these plants can be prepared by methods well known to those skilled in the art.

The introduction of the recombinant DNA sequence or the expression vector into the prepared plant cells includes a method involving Agrobacterium and a method involving direct introduction into cells. Agrobacterium-mediated methods include, for example, the method of Nagel et al.
crobiol. Lett., 67, 325 (1990)). In this method, first, for example, an expression vector is transformed into Agrobacterium by electroporation, and then the transformed Agrobacterium is transformed into Plant Molecu
lar Biology Manual (SB Gelvin et al., Academic
Press Publishers). Methods for directly introducing an expression vector into cells include an electroporation method and a gene gun method.

(Regeneration of Recombinant Plant Cells into Plants or Plant Tissues) C3 plant cells into which a recombinant gene or an expression vector has been introduced are first selected by drug resistance such as kanamycin resistance, and then selected by a conventional method. , Plant tissues and plants can be regenerated to obtain seeds. To confirm the expression of the enzyme constituting the photosynthetic pathway of the C4 plant in the transformed C3 plant, a method well known to those skilled in the art can be used. For example,
From a plant tissue of a gramineous plant, a leaf of the plant, according to a conventional method, DN
A is extracted, Southern hybridization using a partial sequence of the introduced C4 photosynthesis gene as a probe,
Alternatively, proteins can be extracted and assayed for activity, or activity stained to confirm transformation and expression.

(Measurement of Photosynthetic Ability) The photosynthetic activity (CO ₂ compensation point) of the transformed plant is determined, for example, by Hudspeth et al., Plant Phy.
98: 458-464 (1992), using an ADC infrared gas analyzer. Briefly, fresh leaves are placed in a Plexiglass chamber.
r), while irradiating with 1000 μmol / m ² / s photosynthetic photon flow density, keep the temperature at 30 ° C, stir the air in the chamber, measure the CO ₂ concentration continuously, Measure the concentration at which the CO ₂ concentration is constant.

[0050]

EXAMPLES Hereinafter, the present invention will be specifically described by exemplifying a maize PEPC genomic gene as DNA having an expression control region and a structural gene of an enzyme constituting a photosynthetic pathway of a C4 plant, and rice as a C3 plant. Although described, it goes without saying that the present invention is not limited to this embodiment. In addition,
Restriction enzymes, plasmids and the like used in this example can be obtained from Takara Shuzo Co., Ltd., Toyobo Co., Ltd. or the like.

(Example 1: Isolation of maize PEPC genomic gene) The maize PEPC genomic gene was obtained from the literature (Eu
r. J. Biochem. 181: 593-598, 1989). Maize (Zea mays L. cv. Golden Cross
(Bantam) in balm curite, 30 ° C, 4
The cells were cultured under dark and light conditions (20 Klx) for one day. Mat
Genomic DNA was isolated from yellowed leaves according to the method of Suoka et al., Plant Physiol. 85: 942-946 (1985). This genomic DNA was cut with XbaI and fractionated by 10-40% sucrose density gradient centrifugation. The obtained XbaI fragment was incorporated into a phage λong C (Stratagene) having an XbaI arm, packaged in vitro, and produced by Matsuoka et al., Plant Cell Physio.
l. 30: 47-486 (1989) Sequence 5'-GTCCACGAGAAGATCC
Plaque hybridization was performed using AGGG-3 'as a probe (a cDNA clone (pPEP3055) isolated using this probe could also be used as a probe). Positive clones were isolated and their nucleotide sequences were determined using the dideoxy method. An XbaI-XbaI fragment of about 8 Kb containing the full-length PEPC structural gene was obtained. FIG. 1 shows a restriction enzyme map of the obtained DNA fragment containing PEPC, and FIG.
4 to FIG.

As a result of analyzing the sequence of the XbaI-XbaI fragment of about 8 Kb, it was found to have an expression regulatory region as shown in Table 1 below.

[0053]

[Table 1]

Example 2 Construction of Expression Vector The binary vector pIG121-Hm (FIG. 5) was converted to pBI101 (Jefferson).
EMBO J. 6: 3901-3907 (1987), pIG221 (Ohta et al., Pla
nt Cell Physiol. 31: 805-813 (1990), and pLAN101MH
Constructed using YG (a gift from Dr. Ko Shimamoto). This vector contains the NPT2 gene controlled by the NOS promoter and terminator, a multiple cloning site, the β-GUS gene from E. coli, and the HPT gene under the control of 35S CaMV and having TNOS.

The vector pIG121-Hm was first used for HindIII-S
The fragment was cut with stI and the large fragment was recovered. About 8 Kb of the corn PEP obtained above was added to the cut vector.
The XbaI-XbaI fragment of the C gene was ligated and introduced into E. coli JM109. Kanamycin resistant strains were collected and analyzed by restriction enzyme analysis.
Expression vector PEPC with PEPC gene introduced in the right direction
genome / pBIH2 was obtained (FIG. 6).

Example 3 Expression Vector PEPCgenome / pBI
Introduction of H2 into rice) (Transformation of Agrobacterium tumefaciens) Agrobacteri
um tumefaciens EHA101 (obtained from Dr. Nester, University of Washington) was cultured at 28 ° C. in a medium containing 50 μg / ml kanamycin and 100 μg / ml hygromycin, and Nagel et al.
According to the method of ibiol. Lett., 67, 325 (1990)), a cell culture solution was prepared, the expression vector PEPCgenome / pBIH2 was introduced into the above bacteria by electroporation, and a hygromycin-resistant strain was selected.

(Transformation of rice cells and regeneration of rice individuals)
Agroba transformed with expression vector PEPCgenome / pBIH2
cterium was obtained and AB agar medium (Chilton et al., Proc. Natl.
d. Sci. USA. 71: 3672-3676 (1974)), and colonies were formed with AAM medium (Hiei et al., Plant J. 6: 271-282 (1992)).
4)) and co-cultured with rice (Oryza sativa) callus for 3 days. Thereafter, the above bacteria were removed with a medium containing 50 μg / ml of hygromycin, subcultured with a hygromycin selective medium every two weeks, and transformed rice cells were selected.
As a result of redifferentiation by a conventional method, 38 independent transformed rice individuals were obtained.

Example 4 Detection of PEPC Gene Expression in Transformed Rice The expression levels of the obtained 38 transformed rice individuals, non-transformed rice, and maize PEPC were examined as follows. PEPC activity is determined by Edwards et al., Aus
t. J. Plant Physiol. 15: 385-395 (1988). PEPC enzymes are available from Hudspeth et al., Plant Physiol.
98: 458-464 (1992). Briefly, about 0.5 g of green leaves were collected, snap frozen in liquid nitrogen and ground into a fine powder. A 10-fold amount of extraction buffer was added and further triturated. 50 mM extraction buffer
Hepes-KOH pH 8.0, 10 mM MgCl ₂ , 1 mM EDTA, 10 mM DTT,
Consisted of 10% (w / v) insoluble PVP, 12.5% (v / v) glycerol, 10 μM leupeptin, and 1 mM PMSF. The crude extract was filtered with Miracloth (Calbiochem, La Jolla, CA). The filtrate was centrifuged at 4 ° C., 15,000 rpm for 5 minutes, and the supernatant was desalted with Sephadex G-25 previously equilibrated with an extraction buffer without PVP. The eluates were pooled, and the enzyme activity and protein content were measured.

FIG. 7 shows the results. In FIG. 7, WT is
Wild represents, ie, untransformed rice, and Corn represents corn. PEPC of crude extract of green leaves of untransformed rice
The relative activity was expressed as relative to 1. Maize had about 40 times the activity of rice. Transformed rice
Four out of 38 strains showed higher PEPC activity than corn. By the transformation, a strain having about 115 times the activity was obtained (having about 3 times the activity of corn). It is surprising that simply introducing the genomic gene of a C4 plant into a C3 gramineous plant expresses PEPC activity beyond that expressed in C4 plants.

(Example 5: Improvement of photosynthesis in transformed rice) The non-transformed rice obtained in Example 4, the transformed rice having about 7 times and 75 times the PEPC activity of the non-transformed rice were used. Was used to measure the photosynthetic rate. Table 2 shows the results
Shown in

[0061]

[Table 2]

The transformed rice having about 75 times the PEPC activity of the non-transformed rice shows that the compensation point was reduced by about 10% and the photosynthetic activity was greatly increased.

[0063]

EFFECT OF THE INVENTION By introducing into a C3 plant an expression regulatory region of an enzyme gene constituting the C4 biosynthetic pathway and a structural gene of an enzyme constituting the C4 photosynthetic pathway in a C4 plant which is closely related to evolutionary phylogeny, The photosynthetic activity of C3 plants is greatly increased.

[0064]

[Sequence list]

[0065]

[SEQ ID NO: 1] Sequence length: 20 Sequence type: Nucleic acid Topology: Linear Sequence type: Probe Sequence: GTCCA CGAGA AGATC CAGGG 20

[Brief description of the drawings]

FIG. 1 is a diagram showing a restriction map of a DNA fragment containing a PEPC gene. Bold lines indicate exons.

FIG. 2 is a diagram showing a base sequence of an approximately 8 Kb DNA fragment containing a PEPC gene.

FIG. 3 is a continuation of FIG. 2;

FIG. 4 is a continuation of FIG.

FIG. 5 is a diagram showing a binary vector pIG121-Hm.

FIG. 6 shows the structure of the expression vector PEPCgenome / pBIH2.

FIG. 7 shows the PEPC activity of transformed rice.

 ──────────────────────────────────────────────────続 き Continued on the front page (72) Inventor Seiichi Toki 2-1-2 Kannondai, Tsukuba, Ibaraki Pref. Ministry of Agriculture, Forestry and Fisheries Agricultural and Biological Resources Institute (72) Inventor Maurice Sun-Ben. Kuh United States of America Pullman Washington State University Washington

Claims (36)

[Claims] 1. A C3 plant that expresses a gene of a C4 plant closely related to the evolutionary phylogeny, wherein the expression control region of a gene of an enzyme constituting a photosynthetic pathway of the C4 plant and the C4 plant
A C3 plant having DNA containing a structural gene of an enzyme constituting a photosynthetic pathway of a plant, wherein the structural gene of the enzyme constituting a photosynthetic pathway of the C4 plant is expressed more than is expressed in the C4 plant. 2. The C3 plant according to claim 1, wherein the C4 plant is a monocotyledonous plant and the C3 plant is a monocotyledonous plant. 3. The C3 plant according to claim 1, wherein the C4 plant is a dicotyledonous plant, and the C3 plant is a dicotyledonous plant. 4. A DNA comprising the expression control region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant and the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant is C4.
The C3 plant according to any one of claims 1 to 3, which is a plant genomic gene. 5. The C3 plant according to claim 4 , wherein the genomic gene of the C4 plant is a genomic gene of a grass plant, and the C3 plant is a C3 grass plant. 6. The C3 plant according to claim 5, wherein the genomic gene of the C4 plant is a genomic gene of phosphoenolpyruvate carboxylase of maize, and the C3 gramineous plant is rice. 7. A method for producing a C3 plant that highly expresses an enzyme constituting the photosynthetic pathway of a C4 plant that is closely related to evolutionary phylogeny, comprising the steps of: DNA containing a structural gene for an enzyme that constitutes the photosynthetic pathway of the plant and the structural gene for the enzyme that constitutes the photosynthetic pathway of the C4 plant,
Transforming the cells of three plants; and regenerating the transformed C3 plant cells into C3 plants, wherein the C3 plants are enzymes constituting the photosynthetic pathway of the C4 plants. The method according to claim 1, wherein the structural gene is expressed more than in the C4 plant. 8. The method according to claim 7, wherein the C4 plant is a monocotyledonous plant, and the C3 plant is a monocotyledonous plant. 9. The method according to claim 7, wherein the C4 plant is a dicotyledon, and the C3 plant is a dicotyledonous plant. 10. The DNA comprising the expression control region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant and the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant is C-type.
The method for producing a C3 plant according to any one of claims 7 to 9, which is a genomic gene of four plants. 11. The method for producing a C3 plant according to claim 10 , wherein the genomic gene of the C4 plant is a genomic gene of a grass plant, and the C3 plant is a C3 grass plant. 12. The genomic gene of the C4 plant is a genomic gene of corn phosphoenolpyruvate carboxylase, and the C3 gramineous plant is rice.
A method for producing a C3 plant according to claim 11. 13. A C3 plant tissue which expresses a gene of a C4 plant closely related to the evolutionary phylogeny, wherein the expression control region of a gene of an enzyme constituting a photosynthetic pathway of the C4 plant and a photosynthetic pathway of the C4 plant A C3 plant tissue, comprising a DNA containing a structural gene of an enzyme that constitutes the above, and expressing the structural gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant more than is expressed in the C4 plant. 14. The C3 plant tissue according to claim 13, wherein the C4 plant is a monocotyledonous plant and the C3 plant tissue is a monocotyledonous plant. 15. The C3 plant tissue according to claim 13, wherein the C4 plant is a dicotyledonous plant and the C3 plant tissue is a dicotyledonous plant. 16. The DNA containing the expression control region of the gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant and the DNA containing the structural gene of the enzyme that constitutes the photosynthetic pathway of the C4 plant is C-type.
The C3 plant tissue according to any one of claims 13 to 15, which is a genomic gene of four plants. Genomic gene of claim 17, wherein the C4 plant is a genomic gene of the rice plant, wherein the C3 plant is a C3 grasses C3 plant tissue according to claim 1 6. 18. The genomic gene of the C4 plant is a genomic gene of phosphoenolpyruvate carboxylase of maize, and the C3 gramineous plant is rice.
A C3 plant tissue according to claim 17. 19. A method for producing a C3 plant tissue which highly expresses an enzyme constituting the photosynthetic pathway of a C4 plant which is closely related to an evolutionary phylogeny, comprising the steps of: DNA containing a structural gene for an enzyme that constitutes the photosynthetic pathway of the plant and the structural gene for the enzyme that constitutes the photosynthetic pathway of the C4 plant,
Transforming the cells of three plants; and regenerating the transformed C3 plant cells into C3 plant tissue, wherein the C3 plant tissue is an enzyme constituting the photosynthetic pathway of the C4 plant The method according to claim 1, wherein the structural gene is expressed more than in the C4 plant. 20. The method for producing a C3 plant tissue according to claim 19, wherein the C4 plant is a monocotyledonous plant, and the C3 plant tissue is a monocotyledonous plant tissue. 21. The method for producing a C3 plant tissue according to claim 19, wherein the C4 plant is a dicotyledonous plant, and the C3 plant tissue is a dicotyledonous plant tissue. 22. A DNA comprising the expression regulatory region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant and the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant is C-type.
The method for producing a C3 plant tissue according to any one of claims 19 to 21, which is a genomic gene of four plants. Genomic gene of claim 23, wherein the C4 plant is a genomic gene of the rice plant, wherein the C3 plant is a C3 poaceous plant, how to create a C3 plant tissue according to claim 2 2. 24. The C4 plant genomic gene is a maize phosphoenolpyruvate carboxylase genomic gene, and the C3 gramineous plant is rice.
A method for preparing a C3 plant tissue according to claim 23. 25. A C3 plant seed which expresses a gene of a C4 plant closely related to the evolutionary phylogeny, wherein the expression control region of a gene of an enzyme constituting the photosynthetic pathway of the C4 plant and the photosynthetic pathway of the C4 plant A C3 plant seed, which comprises a DNA containing a structural gene of an enzyme constituting the C4 plant, and expresses the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant more than is expressed in the C4 plant. 26. The C4 plant is a monocotyledon, and the C3 plant seed is a monocotyledon seed.
The C3 plant seed according to item 1. 27. The C4 plant is a dicotyledon, and the C3 plant seed is a dicotyledon seed.
The C3 plant seed according to item 1. 28. A DNA comprising the expression control region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant and the DNA containing the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant,
28. The C3 plant seed according to any one of claims 25 to 27, which is a genomic gene of four plants. 29. The genomic gene of the C4 plant is a genomic gene of a Poaceae plant, and the C3 plant seed is C3
It is a seed grasses, C3 plant seed according to claim 2 8. 30. The genomic gene of the C4 plant is a genomic gene of phosphoenolpyruvate carboxylase of maize, and the C3 gramineous plant is rice.
A C3 plant seed according to claim 29. 31. A method for producing a C3 plant seed which highly expresses an enzyme constituting a photosynthetic pathway of a C4 plant which is closely related to an evolutionary phylogeny, comprising the steps of: DNA containing a structural gene for an enzyme that constitutes the photosynthetic pathway of the plant and the structural gene for the enzyme that constitutes the photosynthetic pathway of the C4 plant,
Transforming cells of three plants; the transformed C
Regenerating the three plant cells into a C3 plant; and
Obtaining a seed from three plants, wherein the C3 plant seed expresses a structural gene of an enzyme constituting the photosynthetic pathway of the C4 plant more than is expressed in the C4 plant. . 32. The C4 plant is a monocotyledon, and the C3 plant seed is a monocotyledon seed.
The method for producing a C3 plant seed according to the above. 33. The C4 plant is a dicot, and the C3 plant seed is a dicot seed.
The method for producing a C3 plant according to the above. 34. A DNA containing the expression control region of the gene of the enzyme constituting the photosynthetic pathway of the C4 plant and the structural gene of the enzyme constituting the photosynthetic pathway of the C4 plant,
34. The method for producing a C3 plant seed according to any one of claims 31 to 33, which is a genomic gene of four plants. Genomic gene of claim 35 wherein said C4 plant is a genomic gene of the rice plant, wherein the C3 plant is a C3 poaceous plant, how to create a C3 plant seed according to claim 3 4. 36. The genomic gene of the C4 plant is a corn phosphoenolpyruvate carboxylase genomic gene, and the C3 gramineous plant is rice.
A method for producing a C3 plant seed according to claim 35.