This application is the U.S. National Phase under 35 U.S.C. §371 of International Application PCT/JP2009/069977, filed Nov. 26, 2009, which was published in a non-English language, which claims priority to JP Patent Application No. 2008-304006, filed Nov. 28, 2008.
The present invention relates to a transformed soybean plant which accumulates an Alzheimer's disease vaccine in its seeds, and use thereof.
Alzheimer's disease is a neurodegenerative disease caused by accumulation of a causative substance such as β-amyloid in brain, causing damage to nerve cells. Although the number of patients suffering from Alzheimer's disease is expected to increase upon the advent of an aging society, prophylactic agents and therapeutic agents for the disease are hardly available, and development of new prophylactic agents, therapeutic agents, vaccines and the like has been demanded. Vaccines against Alzheimer's disease have been developed using β-amyloid, which is a causative substance of the disease, as an antigen, but development of the vaccines was difficult because of problems such as side effects. Therefore, development of a vaccine using a β-amyloid antigenic determinant (epitope) which does not cause side effects, and establishment of mass production techniques for the vaccine are required.
Soybean is an exalbuminous seed, which does not have albumen and accumulates its nutrition in the germ corresponding to the cotyledon. About 40% of the whole volume of a seed, which corresponds to the germ, is occupied by storage proteins. Therefore, soybean has characteristics as a storage tissue different from those of other crops such as rice and maize that accumulate starch in albumen as a major reserve substance, so that it is a crop suitable for being made to produce and accumulate an exogenous protein. The major seed storage proteins in soybean are 11S globulin (glycinin) and 7S globulin (β-conglycinin). The spatial structures of these seed storage proteins and the mechanisms of their accumulation in the cell have been elucidated, and it is known that the genes encoding them have portions called variable regions. It is thought that the spatial structures of the proteins can be maintained even after insertion of an exogenous gene into the variable regions and that the properties of the storage proteins are not affected by such insertion.
In general, a β-amyloid antigenic determinant is a protein (peptide) having a relatively low molecular weight composed of several amino acids, and it has been difficult to make the peptide highly accumulated in seeds of a transformed soybean for the purpose of mass production of the peptide by introducing a gene encoding the peptide to the soybean, since the peptide was degraded by enzymes such as proteases in the cells.
On the other hand, as transformed crops that accumulate biologically active peptides and vaccines in their seeds, a transformed soybean that accumulates a hypotensive peptide (Patent Document 1), a transformed rice that accumulates a vaccine against allergy to cedar pollen (Patent Document 2), a potato that produces β-amyloid (Non-patent Document 1) and a tomato that produces β-amyloid (Non-patent Document 2) are known.
However, a transformed soybean that highly accumulates an Alzheimer's disease vaccine composed of a β-amyloid antigenic determinant (epitope), and mass production techniques for the vaccine using the soybean have not been known so far.
Common bean is a plant belonging to Leguminosae, to which soybean also belongs, and the content of protein in a seed of common bean is 20%. It is known that arcelin, which is one of the major seed storage proteins in common bean, can be divided into plural types, that is, arcelin 1 to 7, and that the homologies among the nucleotide sequences of the part encoding their structural proteins are high. The structures of the arcelin proteins in common bean have been less analyzed compared to those in soybean, and only the spatial structures of arcelin 1 and 5 have been revealed.
Further, it is known that prolamin, which is one of the major seed storage proteins in rice, is an indigestible protein which can be divided into several types (e.g., 10K, 13K and 16K) having different molecular weights. The spatial structure of prolamin has not been revealed.
Patent Document 1: JP 2006-238821 A
Patent Document 2: JP 2004-321079 A
Non-patent Document 1: Federation of European Biochemical Societies (2005) vol. 579, pp. 6737-6744.
Non-patent Document 2: Biotechnology Letters (2008) vol. 30, pp. 1839-1845.
The present invention aims to provide a transformed soybean plant which can be made to produce and accumulate an Alzheimer's disease vaccine in its seeds. Further, the present invention aims to provide a method for producing an Alzheimer's disease vaccine using the transformed soybean.
The present inventors intensively studied to solve the above problems.
As a result, the present inventors succeeded in preparation of a transformed soybean plant having a gene encoding a modified seed storage protein introduced therein, which gene has been obtained by inserting a gene encoding an Alzheimer's disease vaccine to a variable region(s) of a gene encoding a wild-type seed storage protein, and also succeeded in production and accumulation of the Alzheimer's disease vaccine in seeds of the transformed soybean plant.
Further, the present inventors discovered that a transformed soybean plant produced by introducing the gene encoding a modified seed storage protein to soybean in which an endogenous seed storage protein(s) is/are deficient can efficiently produce and accumulate the Alzheimer's disease vaccine in its seeds.
That is, the present invention provides:
Since the transformed soybean plant of the present invention can highly accumulate an Alzheimer's disease vaccine in its seeds, the Alzheimer's disease vaccine can be efficiently produced using the transformed soybean plant.
The present invention will now be described in detail.
1. Gene Encoding Wild-Type Seed Storage Protein
Examples of the wild-type seed storage protein in the present invention include the respective subunits constituting soybean 11S globulin, the respective subunits constituting soybean 7S globulin, arcelin in common bean, prolamin in rice, globulin in rice, and further, seed storage proteins in other crops. Preferred examples of the wild-type seed storage protein include the A1aB1b subunit of 11S globulin and the α subunit and β subunit of 7S globulin in soybean, among which the A1aB1b subunit of 11S globulin in soybean is more preferred.
Further, examples of the wild-type seed storage protein in the present invention include proteins containing the amino acid sequences shown in SEQ ID NO:2, SEQ ID NO:37 and SEQ ID NO:45, and proteins containing amino acid sequences having identities of not less than 80%, preferably not less than 90%, more preferably not less than 95% to these amino acid sequences.
Here, the identity (%) between amino acid sequences means the maximum identity (%) between the amino acid sequences which is obtained by aligning the two amino acid sequences to be compared while introducing, as required, gaps thereto (alignment). The alignment for the purpose of determining the identity between amino acid sequences can be carried out using various methods which are well-known to those skilled in the art. For example, publicly available computer software such as BLAST, BLAST-2, ALIGN and Megalign (DNASTAR) software and commercially available software such as Gene Works 2.5.1 software (Teijin System Technology, Inc.) and GENETIX-WIN (Software Development Co., Ltd) may be used.
Examples of the gene encoding a wild-type seed storage protein in the present invention include genes encoding the respective subunits constituting soybean 11S globulin, genes encoding the respective subunits constituting soybean 7S globulin, a gene encoding arcelin in common bean, a gene encoding prolamin in rice, a gene encoding globulin in rice, and further, genes encoding seed storage proteins in other crops. Preferred examples of the gene include a gene encoding the A1aB1b subunit of 11S globulin and genes encoding the α subunit and β subunit of 7S globulin in soybean, among which a gene encoding the A1aB1b subunit of 11S globulin in soybean is more preferred.
Further, examples of the gene encoding a wild-type seed storage protein in the present invention include genes containing the nucleotide sequences shown in SEQ ID NO:1, SEQ ID NO:36 and SEQ ID NO:44, and genes containing nucleotide sequences having identities of not less than 80%, preferably not less than 90%, more preferably not less than 95% to these nucleotide sequences.
Here, the identity (%) between nucleotide sequences means the maximum identity (%) between the nucleotide sequences which is obtained by aligning the two nucleotide sequences to be compared while introducing, as required, gaps thereto (alignment). The alignment for the purpose of determining the identity between nucleotide sequences can be carried out using various methods which are well-known to those skilled in the art. For example, publicly available computer software such as BLAST, BLAST-2, ALIGN and Megalign (DNASTAR) software and commercially available software such as Gene Works 2.5.1 software (Teijin System Technology, Inc.) and GENETIX-WIN (Software Development Co., Ltd) may be used.
2. Gene Encoding Modified Seed Storage Protein
The gene encoding a modified seed storage protein in the present invention means a gene produced by inserting a gene encoding an Alzheimer's disease vaccine to a variable region(s) of a gene encoding a wild-type seed storage protein such that frameshift does not occur.
Here, “inserting a gene encoding an Alzheimer's disease vaccine such that frameshift does not occur” means that the gene encoding an Alzheimer's disease vaccine has been inserted to a variable region(s) of a gene encoding a wild-type seed storage protein such that the amino acid sequence of the modified seed storage protein excluding the amino acid sequence of the Alzheimer's disease vaccine is identical to the amino acid sequence of the corresponding wild-type seed storage protein.
Further, “inserting a gene encoding an Alzheimer's disease vaccine” means that the gene encoding an Alzheimer's disease vaccine has been inserted without causing deletion of a nucleotide sequence encoding the variable region(s), as well as that all or a part of the nucleotide sequence encoding the variable region(s) was substituted with the gene encoding an Alzheimer's disease vaccine.
In the present invention, a variable region of a gene encoding a wild-type seed storage protein means a region which allows, even when an exogenous gene has been inserted thereto such that frameshift does not occur, the protein expressed from the resulting gene to maintain a stable spatial structure equivalent to that of the wild-type seed storage protein, thereby allowing maintenance of the properties of the wild-type seed storage protein.
For example, when the gene encoding a wild-type seed storage protein is the gene encoding the A1aB1b subunit of soybean 11S globulin containing the amino acid sequence of SEQ ID NO:2, five portions including the region encoding amino acid positions 20-28 (variable region I), the region encoding amino acid positions 111-128 (variable region II), the region encoding amino acid positions 198-216 (variable region III), the region encoding amino acid positions 268-315 (variable region IV) and the region encoding amino acid positions 490-495 (variable region V) in SEQ ID NO:2 are known as variable regions (
Further, when the gene encoding a wild-type seed storage protein is a gene containing a nucleotide sequence encoding an amino acid sequence which has a certain identity to the amino acid sequence shown in SEQ ID NO:2, that is, the amino acid sequence shown in SEQ ID NO:2 except that one or more amino acids are substituted, inserted, added and/or deleted, the variable regions are the region encoding the amino acid sequence corresponding to amino acid positions 20-28, the region encoding the amino acid sequence corresponding to amino acid positions 111-128, the region encoding the amino acid sequence corresponding to amino acid positions 198-216, the region encoding the amino acid sequence corresponding to amino acid positions 268-315 and the region encoding the amino acid sequence corresponding to amino acid positions 490-495.
Here, when two amino acid sequences to be compared are aligned with each other to attain the maximum identity (%) between the amino acid sequences while introducing gaps as required, the “amino acid sequence corresponding to” a particular amino acid sequence means a partial amino acid sequence that corresponds to the other particular partial amino acid sequence. Such an amino acid sequence can be easily specified by those skilled in the art.
When plural variable regions exist in the gene encoding a wild-type seed storage protein, the gene encoding a modified seed storage protein can be prepared by inserting a gene encoding an Alzheimer's disease vaccine to one or more of the variable regions.
For example, when a gene encoding the A1aB1b subunit of soybean 11S globulin containing the amino acid sequence of SEQ ID NO:2 is used as the gene encoding a wild-type seed storage protein, any one of the variable regions II, III, IV and V may be selected as the variable region to which the gene encoding an Alzheimer's disease vaccine is to be inserted, and the gene encoding an Alzheimer's disease vaccine is more preferably inserted to the variable region III. Further, as the variable regions to which the gene encoding an Alzheimer's disease vaccine is to be inserted, two or more regions among the variable regions II, III, IV and V may be selected, and, for example, insertion into the three regions II, III and IV at the same time, insertion into the four regions II, III, IV and V at the same time, and the like can be carried out. Here, introduction of the gene encoding an Alzheimer's disease vaccine needs to be carried out such that frameshift does not occur in the nucleotide sequence encoding the wild-type seed storage protein.
Further, when a gene encoding common bean arcelin 5 containing the amino acid sequence shown in SEQ ID NO:37 is used as the gene encoding a wild-type seed storage protein, since the variable region(s) of the gene is/are not known, it is necessary to compare its DNA sequence with that of the A1aB1b subunit to confirm disordered regions, and to compare its amino acid sequence and spatial structure with those of other similar storage proteins to confirm the differences in the gaps of the sequence and the structural differences, thereby assuming the variable region(s). It is preferred to insert the gene encoding an Alzheimer's disease vaccine into the region encoding amino acid positions 149-150 (variable region A) and/or the region encoding amino acid positions 250-251 (variable region B) in SEQ ID NO:37, which regions can be specified by such assumption.
Further, when the gene encoding the wild-type seed storage protein contains a nucleotide sequence encoding an amino acid which has a certain identity to the amino acid sequence shown in SEQ ID NO:37, that is, the amino acid sequence shown in SEQ ID NO:37 except that one or more amino acids are substituted, inserted, added and/or deleted, the gene encoding an Alzheimer's disease vaccine is preferably inserted into the region encoding the amino acid sequence corresponding to amino acid positions 149-150, the region encoding the amino acid sequence corresponding to amino acid positions 250-251 in SEQ ID NO:37.
Further, when a gene encoding rice prolamin containing the amino acid sequence shown in SEQ ID NO:45 is used as the gene encoding a wild-type seed storage protein, since the spatial structure and the variable region(s) of the gene are not known, it is necessary to compare its amino acid sequence with those of other similar storage proteins to confirm the gap structure, thereby assuming the variable region(s). It is preferred to insert the gene encoding an Alzheimer's disease vaccine into the region encoding amino acid positions 110-111 (variable region a) in SEQ ID NO:45, which region can be specified by such assumption.
Further, when the gene encoding the wild-type seed storage protein contains a nucleotide sequence encoding an amino acid which has a certain identity to the amino acid sequence shown in SEQ ID NO:45, that is, the amino acid sequence shown in SEQ ID NO:45 except that one or more amino acids are substituted, inserted, added and/or deleted, the gene encoding an Alzheimer's disease vaccine is preferably inserted into the region encoding the amino acid sequence corresponding to amino acid positions 110-111 in SEQ ID NO:45.
3.Gene Encoding Alzheimer's Disease Vaccine
The gene encoding an Alzheimer's disease vaccine in the present invention is not restricted as long as it is a DNA encoding a protein or a peptide having a function as a vaccine against Alzheimer's disease, and is preferably a DNA encoding a β-amyloid antigenic determinant composed of a peptide of about 5 to 25 amino acids constituting a part of β-amyloid. Examples of the DNA include DNAs encoding the amino acid sequence of SEQ ID NO:3.
Since a nucleotide sequence encoding β-amyloid is known (GenBank accession No. AB113349), it is possible to isolate a DNA encoding β-amyloid or a β-amyloid antigenic determinant from a cDNA library, by a screening operation based on this nucleotide sequence information. A DNA encoding a β-amyloid antigenic determinant can be prepared also by chemical synthesis.
Further, in the present invention, the Alzheimer's disease vaccine can also be inserted to a variable region(s) of a gene encoding a seed storage protein in such a manner that plural genes encoding the vaccine are tandemly linked to each other, thereby allowing expression of the vaccine. For example, the gene encoding a β-amyloid antigenic determinant may be inserted, such that frameshift does not occur, to a variable region(s) in such a manner that an integer number of 1 to 20, preferably an integer number of 1 to 5, more preferably an integer number of 1 to 3, especially preferably 2 copies of the gene are linked to each other.
Further, when the gene encoding an Alzheimer's disease vaccine is inserted into the gene encoding a wild-type seed storage protein, a nucleotide sequence(s) which encode(s) a sequence recognized by a protease may also be added to the 5′-end and/or the 3′-end of the gene encoding an Alzheimer's disease vaccine. By this, the Alzheimer's disease vaccine can be cleaved out with the protease from the modified seed storage protein produced in seeds. Examples of such a protease include thermolysin.
4. Vector for Gene Transfer
The vector for gene transfer of the present invention may have a structure wherein a promoter that induces soybean seed-specific expression is linked to the upstream of the gene. Further, a terminator may also be linked to the downstream of the gene.
Examples of the promoter that induces soybean seed-specific expression include the soybean 11S globulin promoter and the common bean arcelin promoter, and examples of the terminator include the soybean 11S globulin terminator, the common bean arcelin 2 terminator, the 35S terminator and the NOS terminator of cauliflower mosaic virus.
Examples of the soybean 11S globulin promoter include the promoter of the soybean 11S globulin A1aB1b subunit having the sequence shown in SEQ ID NO:18, and the soybean 11S globulin promoter may be one having an identity of not less than 95% to this sequence as long as it has a seed-specific promoter activity. Examples of the soybean 11S globulin terminator include the terminator of the soybean 11S globulin A1aB1b subunit having the sequence shown in SEQ ID NO:21, and the soybean 11S globulin terminator may be one having an identity of not less than 95% to this sequence as long as it has a seed-specific terminator activity.
Examples of the common bean arcelin promoter include the promoter of common bean arcelin 2 having the sequence of nucleotide positions 1399-3860 in SEQ ID NO:56, and the common bean arcelin promoter may be one having an identity of not less than 95% to this sequence as long as it has a seed-specific promoter activity. Examples of the common bean arcelin terminator include the common bean arcelin 2 terminator having the sequence shown in SEQ ID NO:59, and the common bean arcelin terminator may be one having an identity of not less than 95% to this sequence as long as it has a seed-specific terminator activity.
To the vector of the present invention, a selection marker gene for selecting recombinants, and a reporter gene for confirming expression of the introduced gene may be inserted. Examples of the selection marker gene include the hygromycin resistance gene, the phosphinothricin resistance gene or the like, and examples of the reporter gene include the β-glucuronidase (GUS) gene, chloramphenicol acetyltransferase (CAT) gene, luciferase (LUC) gene and GFP gene or the like.
The vector of the present invention may be obtained also by inserting a DNA fragment, which contains a promoter for induction of seed-specific expression, a gene encoding a modified storage protein linked to the downstream of the promoter, and a terminator linked to the further downstream, to a vector comprising the above-described selection marker gene and/or reporter gene.
5. Soybean Plant which can be Transformed
Examples of the soybean which can be transformed in the present invention include varieties which are generally used for food, for feed or for producing oil. The soybean to be transformed is preferably partially or totally deficient for the endogenous seed storage proteins, and examples of the soybean include those which are partially or totally deficient for soybean 11S globulin and/or soybean 7S globulin. Here, “partially deficient” means cases where the expression level is lower than in the wild type, as well as cases where only a part of the subunits are completely deficient, and cases where the expression levels of only a part of the subunits are lower than those in the wild type. Particular examples of the soybean include the mutant line EnB1, which is deficient for soybean 11S globulin, the mutant line QY2, which is deficient for soybean 7S globulin, and the mutant line QF2, which is deficient for both 11S globulin and 7S globulin. Further examples of the soybean include progeny lines derived by hybridization between such defective lines and common varieties (e.g., Jack or the like).
Confirmation of the fact that the soybean is partially or totally deficient for endogenous soybean 11S globulin and/or soybean 7S globulin can be carried out by electrophoresis of the storage proteins prepared from seeds.
6. Preparation of Transformed Soybean Plant
Examples of the material which may be used for preparation of the transformed soybean plant include plant tissues such as roots, stems, leaves, seeds, embryos, ovules, ovaries, shoot apices, anther and pollens, and sections thereof; and plant cultured cells such as undifferentiated calluses, adventive embryos and protoplasts or the like.
The introduction of the gene encoding a modified seed storage protein to the above material may be carried out by various methods which have already been reported and established, and it is preferred to introduce the above-mentioned vector for gene transfer using the Agrobacterium method, PEG method, electroporation method, particle gun method, whisker ultrasonic method or the like.
Using the resistance effect given by the selection marker gene as an index, cells of the transformed soybean plant can be selected from the material to which the gene encoding a modified seed storage protein has been introduced. From the selected cells, a transformed soybean plant body can be obtained through the step of regenerating a plant body, which step has been reported for each plant species.
By cultivating the thus obtained transformed soybean plant body to allow seed ripening, seeds of the transformed soybean of the present invention can be obtained, and the Alzheimer's disease vaccine of interest can be obtained in the transformed seeds.
Whether or not the gene encoding the Alzheimer's disease vaccine has been introduced into the plant body can be confirmed by the PCR method, Southern hybridization method, Northern hybridization method, Western blotting method or the like. For example, by extracting protein from seeds of the transformed soybean plant body and carrying out Western blotting by immunostaining using a primary antibody specific to the Alzheimer's disease vaccine and a secondary antibody labeled with horseradish peroxidase (HRP) or the like, it is possible to confirm appropriate introduction of the gene encoding the Alzheimer's disease vaccine, accumulation of the Alzheimer's disease vaccine in the seeds, and the amount of the vaccine accumulated.
The performance of the Alzheimer's disease vaccine contained in the modified seed storage protein accumulated in the seeds of the transformed soybean plant can be evaluated by, for example, using a disease-model mouse that develops Alzheimer's disease. More particularly, the modified seed storage protein containing the Alzheimer's disease vaccine, or the Alzheimer's disease vaccine cleaved out from the modified seed storage protein with a protease followed by purification, is administered to the above model mouse by subcutaneous injection or oral administration. The performance of the Alzheimer's disease vaccine can be evaluated by investigating production of antibodies against the Alzheimer's disease vaccine, the amount of β-amyloid, brain tissue, and/or behavior disorder in the mouse. The modified seed storage protein containing the Alzheimer's disease vaccine, or the Alzheimer's disease vaccine cleaved out from the modified seed storage protein with a protease followed by purification, may be administered as a mixture with an adjuvant.
The Alzheimer's disease vaccine can be produced in a large amount by cultivating and then collecting seeds of the transformed soybean that accumulates a modified seed storage protein containing the vaccine, in the outdoor field, or closed facilities for cultivation where the environment is artificially controlled.
The seeds wherein the modified seed storage protein containing the Alzheimer's disease vaccine is accumulated can be used for prophylaxis and/or therapy of Alzheimer's disease, as a composition containing the Alzheimer's disease vaccine. For example, the seeds processed by pulverization or the like may be made into the form of a tablet, granule, powder, capsule, beverage or the like.
Further, the above composition may contain the modified seed storage protein accumulated in the seeds, which protein has been extracted and purified. For example, after a ground product of the seeds subjected to defatting and heat treatment, the modified seed storage protein containing the Alzheimer's disease vaccine of interest may be purified by an apparatus such as liquid chromatography. Further, the above-described composition may contain the Alzheimer's disease vaccine which has been prepared by treating the modified seed storage protein with a protease and purifying the resulting product, thereby partially or totally removing the part of the wild-type seed storage protein from the modified seed storage protein.
The present invention will now be described more concretely by way of Examples, but the present invention is not restricted to these Examples.
The procedures of the experimental methods carried out in the Examples below are those according to “Molecular Cloning” 2nd Ed. (J. Sambrook et al., Cold Spring Harbor Laboratory press, published in 1989) unless otherwise specified.
Construction of Expression Plasmids for Modified Soybean 11S Globulin A1aB1b
Expression plasmids for expression of genes encoding modified A1aB1b containing the peptide having the amino acid sequence shown in SEQ ID NO:3 (hereinafter abbreviated as Aβ4-10), which is known as a β-amyloid antigenic determinant, in soybean seeds were constructed. The procedure for the construction is shown in
An oligonucleotide having three copies of a nucleotide sequence encoding Aβ4-10 which are tandemly linked to each other (the sense strand, SEQ ID NO:4) and the oligonucleotide having its complementary sequence (the antisense strand, SEQ ID NO:5) were synthesized using the custom DNA synthesis service by FASMAC Co., Ltd. (the sense strand and the antisense strand are hereinafter referred to as 410F and 410R, respectively). Unless otherwise specified, the hereinafter-mentioned oligonucleotides were those synthesized using the custom DNA synthesis service by the above manufacturer. In the presence of ATP at a final concentration of 1 mM, 100 pmol each of 410F and 410R was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.), and the reaction solutions after the reaction were mixed together, followed by heating the resulting mixture at 94° C. for 10 minutes and then allowing the mixture to cool gradually to 37° C. for 1 hour, thereby carrying out annealing. By this process, a double-stranded DNA fragment encoding a peptide wherein three copies of Aβ4-10 are tandemly linked to each other ((Aβ4-10)×3) was obtained.
Using, as a template, the plasmid pBSK-A1aB1b (obtained from Kyoto University) wherein cDNA of the known A1aB1b gene (GenBank accession No. AB113349) is cloned at the SmaI site of pBluescript II SK(−) (manufactured by Stratagene), PCR was carried out to amplify a fragment containing the vector portion such that the 5′-end and the 3′-end of the fragment are positioned at a specific variable region of the gene encoding A1aB1b. The obtained DNA fragment was ligated with the double-stranded DNA fragment encoding (Aβ4-10)×3, to prepare the gene encoding a modified A1aB1b. The method is more concretely described below.
A total of five primer sets, that is, the primer set (PS-1) composed of the primer pair of SEQ ID NOs:6 and 7 for insertion into the variable region II, the primer set (PS-2) composed of the primer pair of SEQ ID NOs:8 and 9 for insertion into the variable region III, the primer set (PS-3) composed of the primer pair of SEQ ID NOs:10 and 11 and the primer set (PS-4) composed of the primer pair of SEQ ID NOs:12 and 13 for insertion into the variable region IV, and the primer set (PS-5) composed of the primer pair of SEQ ID NOs:14 and 15 for insertion into the variable region V, of the gene encoding A1aB1b having the sequence shown in SEQ ID NO:1 were prepared. The primers were synthesized such that nucleotide substitutions for introducing amino acid substitutions in the immediate downstream of the insertion regions were introduced in order to allow cleaving out of (Aβ4-10)×3 from the modified A1aB1b proteins using a protease thermolysin.
The regions in the nucleotide sequence shown in SEQ ID NO:1, into which the DNA encoding (Aβ4-10)×3 was inserted using the respective primer sets are hereinafter referred to as the PS-1 region, PS-2 region, PS-3 region, PS-4 region and PS-5 region, respectively.
PCR was performed using 10 ng of pBSK-A1aB1b as a template and 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 5 minutes of extension at 68° C. The reaction solution contained 200 μM dNTP mixture, 1.5 mM MgSO4 solution, each of the above primers at a concentration of 1 μM, and KOD-Plus-Ver.2 buffer containing 1 unit of KOD-Plus-(manufactured by Toyobo Co. Ltd.). The hereinafter-mentioned PCRs were carried out using the same composition except for the primers, unless otherwise specified.
Using DNA Ligation Kit (manufactured by TAKARA BIO), 50 fmol of each of the thus obtained DNA fragments and 150 fmol of the double-stranded DNA fragment encoding the above-described (Aβ4-10)×3 were subjected to ligation reaction at 16° C. for 40 minutes. The reaction product was used for transformation of E. coli DH5α competent cells (manufactured by TAKARA BIO) to obtain plural transformed E. coli cells. From the obtained E. coli cells, plasmid DNAs were extracted and purified, followed by analyzing their nucleotide sequences using the DNA sequencing service by FASMAC Co., Ltd. In the case where PS-1 was used, the result of the nucleotide sequence analysis of 12 clones of the transformed E. coli showed that one clone had one molecule of the double-stranded DNA fragment encoding (Aβ4-10)×3 in a state where the fragment was correctly inserted in the forward direction. Further, 24 clones, 54 clones, 30 clones and 12 clones were analyzed in the cases where PS-2, PS-3, PS-4 and PS-5 were used, respectively, and one each clone having one molecule of the double-stranded DNA fragment encoding (Aβ4-10)×3 in a state where the fragment was correctly inserted in the forward direction was obtained. The probability with which a modified A1aB1b gene wherein the fragment was correctly inserted can be obtained varied among the insertion sites, and insertion of the fragment was especially difficult in the case where PS-3 was used.
All of the thus prepared genes encoding modified A1aB1b were subjected to confirmation of their nucleotide sequences. Unless otherwise specified, the hereinafter-mentioned determination of nucleotide sequences was carried out using the DNA sequencing service by FASMAC Co., Ltd.
Subsequently, in order to prepare the modified A1aB1b genes wherein DNAs encoding (Aβ4-10)×3 are inserted in plural variable regions, PCR was carried out using the above-prepared genes encoding modified A1aB1b as templates and the primer sets that were the same as described above. Ligation reaction of the obtained DNA fragment and the double-stranded DNA fragment encoding the above-described (Aβ4-10)×3 peptide was repeated, to prepare the genes encoding modified A1aB1b. By this process, plasmids containing the genes encoding modified A1aB1b, in which DNAs encoding (Aβ4-10)×3 are inserted in plural variable regions of the A1aB1b gene, were prepared. The particular insertion regions, and the names of the genes encoding modified A1aB1b corresponding thereto are shown in Table 1.
To allow soybean seed-specific expression of the genes encoding modified A1aB1b prepared as described above, the promoter region and the terminator region of the wild-type A1aB1b gene were isolated.
Using, as a probe, the promoter region of the known partial genome sequence of the A1aB1b gene (GenBank accession No. X15121) containing a partial promoter sequence of the A1aB1b gene of 639 bp, a Misuzudaizu TAC library (www.kazusa.or.jp/ja/plant/PG2HP Transformation competent bacterial artificial chromosome) kept in National Agricultural Research Center for Hokkaido Region, National Agriculture and Food Research Organization was screened. As a result of analysis of the nucleotide sequence of the obtained clone, it was revealed that the promoter region located 2202 bp upstream of the translation initiation site of the A1aB1b gene was contained in the clone. Based on the obtained nucleotide sequence, a primer set composed of the oligonucleotide pair of SEQ ID NOs:16 and 17 was prepared, which primer set was then used for carrying out PCR in order to isolate the promoter region.
The above PCR was performed using the genomic DNA of Misuzudaizu as a template and 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 2 minutes 30 seconds of extension at 68° C. By this process, a promoter fragment of the A1aB1b gene having a length of 2202 bp (Gy1P) (SEQ ID NO:18) was obtained.
Subsequently, in order to isolate the terminator region of the A1aB1b gene, a primer set composed of SEQ ID NOs:19 and 20 was prepared based on the known partial genomic sequence of the wild-type A1aB1b gene (GenBank accession No.X53404), which primer set was then used for carrying out PCR.
The above PCR was performed using the genomic DNA of Misuzudaizu as a template and 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 1 minute of extension at 68° C. By this process, a terminator fragment of the wild-type A1aB1b gene having a length of 1052 bp (Gy1T) (SEQ ID NO:21) was obtained.
To allow seed-specific expression of the genes encoding modified A1aB1b, each of the genes encoding modified A1aB1b, and Gy1P and Gy1T, which were obtained as described above, were ligated with the known pUHG vector (Y. Kita, K. Nishizawa, M Takahashi, M. Kitayama, M. Ishimoto. (2007) Genetic improvement of somatic embryogenesis and regeneration in soybean and transformation of the improved breeding lines. Plant Cell Reports 26:439-447) (
In order to obtain DNA fragments encoding 5 types of modified A1aB1b among those described above, PCR was carried out using the above-described A1aB1bM2 (SEQ ID NO:22), A1aB1bM3 (SEQ ID NO:24), A1aB1bM4-1 (SEQ ID NO:26), A1aB1bM1 (SEQ ID NO:28) and A1aB1bM5 (SEQ ID NO:30) as templates, and the primer set composed of the oligonucleotide pair of SEQ ID NOs:32 and 33.
The above PCR was performed using 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 2 minutes of extension at 68° C. By this process, a DNA fragment of each modified A1aB1b gene was obtained.
The DNA fragment of the modified A1aB1b gene, the promoter DNA fragment and the terminator DNA fragment were subjected to phosphorylation reaction, and then ligated into pUHG vector which had been preliminarily digested with SmaI and dephosphorylated with CIAP (manufactured by TAKARA BIO INC.). By analyzing the nucleotide sequences of the obtained clones, clones in which the Gy1P promoter, the gene encoding modified A1aB1b and the Gy1T terminator are correctly linked in this order were selected.
By this process, the following five types of plant transformation vectors (pUHG A1aB1bM1, pUHGA1aB1bM2, pUHGA1aB1bM3, pUHGA1aB1bM4-1 and pUHGA1aB1bM5) that express the genes encoding modified A1aB1b in a seed-specific manner were constructed.
Construction of Expression Plasmid for Modified Common Bean Arcelin
Expression plasmids for expression, in soybean seeds, of genes encoding modified arcelin in which two copies of Aβ4-10 tandemly linked to each other (hereinafter abbreviated as (Aβ4-10)×2) are inserted were constructed.
Since the variable region(s) of the gene encoding the known common bean arcelin 5-1 (GenBank accession No. Z50202) (SEQ ID NO:36) has/have not been revealed, assumption of the variable region(s) was carried out. Based on assumption of the variable region(s) by comparison of the DNA sequence with that of A1aB1b, it was revealed that the disorder region is restricted to the C terminus. Therefore, it was thought that the peptide sequence may be inserted into the C terminus. In order to further specify the variable region, the DNA sequence of the gene was compared with that of phytohemagglutinin, which belongs to 2S albumin as arcelin does, and it was revealed that the loop structure of 8 to 10 residues found in phytohemagglutinin is absent in the downstream of the lysine (amino acid position 149 in SEQ ID NO:37), which is the corresponding portion in Arc5-1. Therefore, the nucleotide sequence region in SEQ ID NO:36 that encodes this portion (amino acid positions 149-150) was assumed to be the variable region A. Subsequently, arcelin 1 was compared with one of the storage proteins of common bean, phaseolin. As a result, a gap of 7 residues was found in the downstream of asparagine corresponding to amino acid position 250 of SEQ ID NO:37. Therefore, the nucleotide sequence region encoding this portion (amino acid positions 250-251) was assumed to be the variable region B.
In order to incorporate the DNA encoding (Aβ4-10)×2 into the assumed variable regions of the gene encoding Arc5-1, the oligonucleotide encoding (Aβ4-10)×2 (420F, SEQ ID NO:34) and the oligonucleotide complementary thereto (420R, SEQ ID NO:35) were synthesized.
In the presence of ATP at a final concentration of 1 mM, 100 pmol each of 420F and 420R was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.), and the reaction solutions after the reaction were mixed together, followed by heating the resulting mixture at 94° C. for 10 minutes and then allowing the mixture to cool gradually to 37° C. for 1 hour, thereby carrying out annealing. By this process, a double-stranded DNA fragment encoding (Aβ4-10)×2 was obtained.
Using, as a template, the plasmid pBSK-Arc5-1 (kept in National Agricultural Research Center for Hokkaido Region, National Agriculture and Food Research Organization) obtained by inserting cDNA encoding Arc5-1 into the SmaI site of pBluescript II SK(−) (manufactured by Stratagene), PCR was carried out to obtain a DNA fragment containing the vector portion, such that the amino acid portion of a particular variable region of the gene encoding Arc5-1 is positioned at the ends. This DNA fragment was ligated with the double-stranded DNA fragment encoding (Aβ4-10)×2 synthesized as described above, to prepare a plasmid containing the gene encoding modified Arc5-1.
The method is more concretely described below.
A total of two primer sets, that is, the primer set (PS-A) composed of the primer pair of SEQ ID NOs:38 and 39 for insertion into the variable region A, and the primer set (PS-B) composed of the primer pair of SEQ ID NOs:40 and 41 for insertion into the variable region B, in the gene encoding Arc5-1 were prepared. The primers were synthesized such that nucleotide substitutions for introducing amino acid substitutions in the immediate upstream and downstream of the insertion regions were introduced in order to allow cleaving out of Aβ4-10 from the modified Arc5-1 proteins using a protease thermolysin.
The regions in the nucleotide sequence of SEQ ID NO:36, into which the DNA encoding (Aβ4-10)×2 was inserted using the respective primer sets are hereinafter referred to as the PS-A region and PS-B region, respectively.
PCR was carried out using 10 ng of pBSK-Arc5-1 as a template. This PCR was performed using 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 4 minutes of extension at 68° C. The thus obtained DNA fragment and the double-stranded DNA fragment encoding the above-described (Aβ4-10)×2 were subjected to ligation reaction.
By this process, 2 types of plasmids containing a gene encoding modified Arc5-1, wherein the DNA encoding (Aβ4-10)×2 is inserted in a variable region of the gene encoding Arc5-1, were prepared. The particular insertion regions of the DNAs encoding (Aβ4-10)×2, and the names of the genes encoding modified Arc5-1 corresponding thereto are shown in Table 2.
In order to allow soybean seed-specific expression of modified Arc5-1, each of the above obtained Arc5M1 and Arc5M2, and Gy1P and Gy1T derived from the A1aB1b gene in the above Example 1, were ligated with the pUHG vector to construct an expression plasmid. In order to obtain DNA fragments encoding modified Arc5-1, PCR was carried out using the above-described Arc5M1 and Arc5M2 as templates, and the primer set composed of the oligonucleotide pair of SEQ ID NOs:42 and 43.
The above PCR was performed using 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 1 minute of extension at 68° C. By this process, a DNA fragment of each modified Arc5-1 gene was obtained.
The DNA fragment of the modified Arc5-1 gene, Gy1P and Gy1T were subjected to phosphorylation reaction, and then ligated into the pUHG vector which had been preliminarily digested with SmaI and dephosphorylated.
By this process, plant transformation vectors pUHG Arc5M1 and pUHG Arc5M2 that express the modified Arc5-1 genes in a seed-specific manner were constructed.
Construction of Expression Plasmid for Modified Rice Prolamin
An expression plasmid for expression, in soybean seeds, of a gene encoding modified prolamin in which DNA encoding (Aβ4-10)×2 is inserted was constructed.
Since the variable region(s) of the gene encoding the known rice prolamin 10K, RP10 (GenBank accession No. E09782) (SEQ ID NO:44), has/have not been revealed, assumption of the variable region(s) was carried out. The amino acid sequence of RP10 was compared with that of zein delta, which is one of the major storage proteins in maize. As a result, a gap of 11 residues was found in the downstream of lysine corresponding to amino acid position 110 of SEQ ID NO:45. Therefore, the nucleotide sequence region encoding this portion (amino acid positions 110-111) was assumed to be the variable region a.
Subsequently, using, as a template, the plasmid pBSK-RP10 (kept in National Agricultural Research Center for Hokkaido Region, National Agriculture and Food Research Organization) obtained by cloning the cDNA encoding the rice prolamin 10K, RP10, into the SmaI site of pBluescript II SK(−) (manufactured by Stratagene), PCR was carried out to obtain a DNA fragment containing the vector portion, such that the amino acid portion of the particular variable region a of the gene encoding RP10 is positioned at the ends. This DNA fragment was ligated with the double-stranded DNA fragment encoding (Aβ4-10)×2 synthesized in Example 2, to prepare a plasmid containing a gene encoding modified RP10.
The method is more concretely described below.
A primer set composed of the primer pair of SEQ ID NOs:46 and 47 for insertion into the variable region a in the gene encoding RP10 was prepared. The primers were synthesized such that nucleotide substitutions for introducing amino acid substitutions in the immediate upstream and downstream of the insertion region were introduced in order to allow cleaving out of the Aβ4-10 peptide from the modified RP10 protein using a protease thermolysin.
PCR was carried out using 10 ng of pBSK-RP10 as a template. This PCR was performed using 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 4 minutes of extension at 68° C. The obtained DNA fragments and the double-stranded DNA fragment encoding the above-described (A(β4−10)×2 were subjected to ligation reaction.
By this process, a plasmid (RP10M1) containing a gene encoding modified RP10, wherein the DNA encoding (Aβ4-10)×2 is inserted in the variable region of the gene encoding RP10, was prepared.
In order to allow seed-specific expression of the gene encoding modified RP10, the gene encoding modified RP10, and Gy1P and Gy1T obtained in the above Example 1 were ligated with the pUHG vector to construct an expression plasmid. In order to obtain a DNA fragment encoding modified RP10, PCR was carried out using the above-described RP10M1 as a template, and the primer set composed of SEQ ID NOs:48 and 49.
The above PCR was performed using 50 μL /reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 25 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 57° C. and 1 minute of extension at 68° C. By this process, a DNA fragment encoding modified RP10 was obtained.
The DNA fragment encoding modified RP10, and the promoter DNA fragment and the terminator DNA fragment were subjected to phosphorylation reaction, and then ligated into the pUHG vector which had been preliminarily digested with SmaI and dephosphorylated.
By this process, a plant transformation vector pUHG RP10M1 that expresses the gene encoding modified RP10 in a seed-specific manner was constructed.
Construction of Expression Plasmids for Respective Modified Types Using Arcelin 2 Promoter
Expression plasmids for expressing, in soybean seeds, the genes encoding modified A1aB1b prepared in Example 1 with a common bean-derived arcelin 2 promoter were constructed.
(1) Isolation of Common Bean-Derived Arcelin 2 Promoter
From 1 g of fresh leaves of the wild species of common bean (line number: G12866), 50 μg of genomic DNA was extracted using DNeasy Plant Maxi kit (manufactured by QIAGEN).
After digesting 280 ng of the genomic DNA with the restriction enzyme SauIIIAI, dGTP was added to the resulting digestion product, followed by carrying out single-nucleotide extension reaction (the first extension reaction) using klenow enzyme (manufactured by Promega KK). Thereafter, the reaction product was ligated with the RWA-1 adapter included in RightWalk Kit™ using Ligation high (manufactured by Toyobo Co., Ltd.), and the resulting ligation product was used as a template for PCR to isolate the DNA in the upstream region of the arcelin 2 gene.
Subsequently, based on the nucleotide sequence of cDNA of the known common bean arcelin 2 gene (GenBank accession No. M28470), oligonucleotides having the nucleotide sequences shown in SEQ ID NOs: 50 and 51 (which were designated the primer SP1 and the primer SP2, respectively) were prepared using the custom synthesis service by FASMAC Co., Ltd.
Thereafter, PCR was carried out using, as a template, 2.8 ng of the above-constructed genomic DNA to which the adapter was ligated, the primer WP-1 included in RightWalk Kit™ and the primer SP1. The above PCR was performed using 50 μL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 35 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 65° C. and 5 minutes of extension at 68° C. The reaction solution contained 200 μM dNTP mixture, 1.5 mM MgSO4 solution, each of the above primers at a concentration of 1 μM, and KOD-Plus-Ver.2 buffer containing 1 unit of KOD-Plus-(manufactured by Toyobo Co. Ltd.).
Thereafter, the reaction solution was 100-fold diluted, and the second PCR was carried out using 1 μL of the resulting dilution as a template, the primer WP-2 included in RightWalk Kit™ and the primer SP2. The composition of the solution and the temperature conditions in the second PCR were the same as those in the first PCR except for the template and the primers.
The amplified DNA fragment was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.) in the presence of ATP at a final concentration of 1 mM, and then ligated with pBluescriptII SK(−) (manufactured by Stratagene) that had been preliminarily treated with SmaI.
This reaction product was designated Arc2P(i), and its nucleotide sequence was determined using the DNA sequencing service by FASMAC Co., Ltd. As a result, it was confirmed that the product contains a novel region having a length of 844 bp in the upstream of the initiation codon of the arcelin 2 gene.
Thereafter, in order to isolate the region located further upstream, new primers were prepared to carry out the second elongation reaction.
After digesting 280 ng of the genomic DNA with the restriction enzyme BglII, dGTP was added to the resulting digestion product, followed by carrying out single-nucleotide extension reaction using klenow enzyme (manufactured by Promega KK). Thereafter, the reaction product was ligated with the RWA-1 adapter included in RightWalk Kit™, and the resulting ligation product was used as a template for PCR to isolate the promoter.
Subsequently, based on the nucleotide sequence of cDNA of the known common bean arcelin 2 gene (GenBank accession No. M28470), an oligonucleotide having the nucleotide sequence shown in SEQ ID NO:52 (which was designated the primer secondSP1) was prepared, and, based on the nucleotide sequence located in a region of 844 bp upstream of the initiation codon, which was obtained in the first extension reaction, an oligonucleotide having the nucleotide sequence shown in SEQ ID NO:53 (which was designated the primer secondSP2) was prepared.
Thereafter, PCR was carried out using, as a template, 2.8 ng of the above-constructed genomic DNA to which the adapter was ligated, the primer WP-1 included in RightWalk Kit™ and the primer secondSP1. The composition of the solution and the temperature conditions in the PCR were the same as those in the above-described first extension reaction except for the template and the primers.
Thereafter, the above PCR solution was 100-fold diluted, and the second PCR was carried out using 1 μL of the resulting dilution as a template, the primer WP-2 included in RightWalk Kit™ and the primer secondSP2. The composition of the solution and the temperature conditions in the second PCR were the same as those in the first PCR except for the template and the primers.
The amplified DNA fragment was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.) in the presence of ATP at a final concentration of 1 mM, and then ligated with pBluescriptII SK(−) (manufactured by Stratagene) that had been preliminarily treated with SmaI.
This reaction product was designated Arc2P(ii), and its nucleotide sequence was determined. Thereafter, in order to isolate the region located further upstream, new primers were prepared to carry out the third elongation reaction.
After digesting 280 ng of the genomic DNA with the restriction enzyme XbaI, dCTP was added to the resulting digestion product, followed by carrying out single-nucleotide extension reaction using klenow enzyme (manufactured by Promega KK). Thereafter, the reaction product was ligated with the RWA-2 adapter included in RightWalk Kit™, and the resulting ligation product was used as a template for PCR to isolate the promoter.
Subsequently, based on the nucleotide sequence of 197 bp obtained in the second extension reaction, oligonucleotides having the nucleotide sequences shown in SEQ ID NOs: 54 and 55 (which were designated the primer thirdSP1 and the primer thirdSP2, respectively) were prepared.
Thereafter, PCR was carried out using, as a template, 2.8 ng of the above-constructed genomic DNA to which the adapter was ligated, the primer WP-1 included in RightWalk Kit™ and the primer thirdSP1. The composition of the solution and the temperature conditions in the PCR were the same as those in the above-described first extension reaction except for the template and the primers.
Thereafter, the above PCR solution was 100-fold diluted, and the second PCR was carried out using 1 μL of the resulting dilution as a template, the primer WP-2 included in RightWalk Kit™ and the primer thirdSP2. The composition of the solution and the temperature conditions in the second PCR were the same as those in the first PCR except for the template and the primers.
The amplified DNA fragment was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.) in the presence of ATP at a final concentration of 1 mM, and then ligated with pBluescriptII SK(−) (manufactured by Stratagene) that had been preliminarily treated with SmaI.
This reaction product was designated Arc2P(iii), and its nucleotide sequence was determined. As a result it was confirmed that the product contains a novel region having a length of 2819 bp in the upstream of Arc2P(ii) (3860 bp in total). Thus, by the three times of extension reaction, DNA(Arc2P) having a length of 3860 bp which contains the 5′-untranslated region in the upstream of the initiation codon of the arcelin 2 gene, wherein the novel promoter sequence is included, was obtained (SEQ ID NO:56, in which the promoter region corresponds to nucleotide positions 1399-3860).
(2) Isolation of Common Bean-Derived Arcelin 2 Terminator
After digesting 280 ng of the genomic DNA extracted in the above (1) with the restriction enzyme NheI, dCTP was added to the resulting digestion product, followed by carrying out single-nucleotide extension reaction using klenow enzyme (manufactured by Promega KK). Thereafter, the reaction product was ligated with the RWA-2 adapter included in RightWalk Kit™ using Ligation high (manufactured by Toyobo Co., Ltd.), and the resulting ligation product was used as a template for PCR to isolate the terminator gene.
Subsequently, based on the nucleotide sequence of cDNA of the known common bean arcelin 2 gene (GenBank accession No. M28470), oligonucleotides having the nucleotide sequences shown in SEQ ID NOs:57 and 58 (which were designated the primer SP3 and the primer SP4, respectively) were prepared.
Thereafter, PCR was carried out using, as a template, 2.8 ng of the above-constructed genomic DNA to which the adapter was ligated, the primer WP-1 included in RightWalk Kit™ and the primer SP3. The above PCR was performed using 50 gL/reaction of a reaction solution, by carrying out 1 cycle of 2 minutes of denaturation at 94° C. and then 35 cycles of 30 seconds of denaturation at 94° C., 30 seconds of annealing at 65° C. and 5 minutes of extension at 68° C. The reaction solution contained 200 μM dNTP mixture, 1.5 mM MgSO4 solution, each of the above primers at a concentration of 1 μM, and KOD-Plus-Ver.2 buffer containing 1 unit of KOD-Plus-(manufactured by Toyobo Co. Ltd.).
Thereafter, the reaction solution was 100-fold diluted, and the second PCR was carried out using 1 μL of the resulting dilution as a template, the primer WP-2 included in RightWalk Kit™ and the primer SP4. The composition of the solution and the temperature conditions in the second PCR were the same as those in the first PCR except for the template and the primers.
The amplified DNA fragment was subjected to phosphorylation reaction with T4 Polynucleotide Kinase (manufactured by TAKARA BIO INC.) in the presence of ATP at a final concentration of 1 mM, and then ligated with pBluescriptII SK(−) (manufactured by Stratagene) that had been preliminarily treated with SmaI.
This reaction product was designated Arc2T, and its nucleotide sequence was determined. As a result, it was confirmed that the product contains a novel region having a length of 795 bp in the downstream of the stop codon of the arcelin 2 gene wherein the 3′-untranslated region is included (SEQ ID NO:59).
(3) Construction of Various Modified Expression Plasmids
In order to express the genes encoding modified A1aB1b in seeds, the genes encoding various modified A1aB1b obtained in Example 1, and Arc2P and Arc2T were ligated with the known pUHG vector (mentioned above,
The DNA fragment of each modified A1aB1b gene, the promoter DNA fragment and the terminator DNA fragment were subjected to phosphorylation reaction, and then ligated with the pUHG vector that had been preliminarily digested with SmaI and dephosphorylated with CIAP (manufactured by TAKARA BIO INC.). By analyzing the nucleotide sequences of the obtained clones, clones in which the Arc2P promoter, the gene encoding modified A1aB1b and the Arc2T promoter are correctly linked in this order were selected.
By this process, the following three types of plant transformation vectors (pUHGA2PA1aB1bM1, pUHGA2PA1aB1bM3 and pUHGA2PA1aB1bM5) that express the genes encoding modified A1aB1b under the control of the arcelin 2 promoter in a seed-specific manner were constructed.
In the same manner, a plant transformation vector pUHGA2PRP10M1 that expresses the gene encoding the above-mentioned RP10M1 in a seed-specific manner was constructed.
Introduction of Gene Encoding Modified Seed Storage Protein to Soybean
By the known method (K. Nishizawa, Y. Kita, M. Kitayama, M. Ishimoto. (2006) A red fluorescent protein, DsRed2, as a visual reporter for transient expression and stable transformation in soybean. Plant Cell Reports 25:1355-1361), 30 adventitious embryonic masses (with diameters of not more than 3 mm) were induced from immature seeds of the soybean variety Jack and a mutant line deficient for 11S globulin and 7S globulin that are major seed storage proteins (kept in National Agricultural Research Center for Hokkaido Region, National Agriculture and Food Research Organization) (Y. Kita, K. Nishizawa, M Takahashi, M. Kitayama, M. Ishimoto. (2007) Genetic improvement of somatic embryogenesis and regeneration in soybean and transformation of the improved breeding lines. Plant Cell Reports 26:439-447), and these adventitious embryonic masses were placed in 1.5 ml tubes, followed by carrying out the gene transfer operation by the whisker ultrasonic method (JP 3312867 B).
In a 1.5 ml tube, 5 mg of whiskers made of potassium titanate LS20 (manufactured by Titan Kogyo, Ltd.) were placed, and the tube was left to stand for 1 hour, followed by removing and completely distilling ethanol to obtain sterile whiskers. Into the tube containing the whiskers, 1 ml of sterile water was added, and the resulting mixture was stirred well. The mixture of whiskers and sterile water was subjected to centrifugation, and water as the supernatant was discarded. In such a manner, the whiskers were washed. This washing operation for the whiskers was repeated 3 times. Thereafter, 0.5 ml of the known MS liquid medium was added to the tube to obtain a whisker suspension.
To the tube containing the whisker suspension obtained as described above, the above-described 30 adventitious embryonic masses (with diameters of not more than 3 mm) were added, and the resulting mixture was stirred, followed by centrifuging the mixture at 1000 rpm for 10 seconds to precipitate the adventitious embryonic masses and the whiskers. The supernatant was discarded to obtain a mixture of the adventitious embryonic masses and the whiskers.
Into the tube containing the above mixture, 20 μl (20 μg) each of the expression vectors for the modified seed storage proteins prepared in Examples 1 to 4 was added, and the resulting mixture was sufficiently mixed by shaking to obtain a uniform mixture.
Subsequently, this tube containing the uniform mixture was subjected to centrifugation at 18000×g for 5 minutes. The mixture after the centrifugation was mixed by shaking again. This operation was repeated 3 times.
The thus obtained tube containing the adventitious embryonic masses, the whiskers and the vector was placed in the bath of an ultrasonic generator such that the tube was sufficiently soaked therein. An ultrasonic wave with a frequency of 40 kHz was radiated to the tube at an intensity of 0.25 W/cm2 for 1 minute. Thereafter, this mixture was left to stand for 10 minutes at 4° C. The mixture processed with ultrasonication in such a manner was washed with the above-described MS liquid medium.
The processed adventitious embryonic masses were cultured in the known liquid medium for growing adventitious embryos for 1 week by rotary shaking culture (100 rpm), and then cultured in a fresh liquid medium for growing adventitious embryos containing hygromycin B (15 mg/l) (Roche Diagnostics, Mannheim, Germany) for 1 week. Further, the adventitious embryonic masses were cultured in a liquid medium for growing adventitious embryos containing 30 mg/l hygromycin B for 4 weeks (while exchanging the medium every week), and then subjected to selection culture in a liquid medium for growing adventitious embryos containing 45 mg/l hygromycin B for 1 week. The gene transfer was carried out for 12 microtubes per vector.
Hygromycin-resistant adventitious embryonic masses were transferred to a liquid medium for maturation of adventitious embryos, and the culture was continued with shaking (100 rpm) for 4 weeks to allow maturation of the adventitious embryos. The mature adventitious embryos were dried by being left to stand in a sterile Petri dish for 3 to 5 days, and then transferred to the known solid medium for germination. After carrying out germination culture for 7 to 10 days, the embryos were transferred to the known rooting medium, thereby allowing the germinated seedlings to grow. After the growth of roots and buds, the plants were transferred to a pot containing soil, and high humidity was maintained until acclimation.
Preparation of Transformed Soybean Plant to which Modified Seed Storage Protein Gene was Introduced
By such a process, 6 individuals of transformed soybean plants produced by introducing A1aB1bM1, 6 individuals of transformants produced by introducing A1aB1bM2, 5 individuals of transformants produced by introducing A1aB1bM3, 5 individuals of transformants produced by introducing A1aB1bM4-1, and 9 individuals of transformants produced by introducing A1aB1bM5, to the Jack variety were prepared. Further, 3 individuals of transformed soybean plants to which Arc5M1 was introduced, 3 individuals of transformants to which Arc5M2 was introduced, and 2 individuals of transformed soybean plants to which RP10M1 was introduced were prepared.
Further, 12 individuals of transformed soybean plants produced by introducing A1aB1bM1, and 6 individuals of transformed soybean plants produced by introducing RP10M1, to the above-described mutant line deficient for 11S globulin and 7S globulin (hereinafter referred to as the seed storage protein-deficient variety) were prepared.
Further, 5 individuals of transformed soybean plants produced by introducing A1aB1bM3 to the seed storage protein-deficient variety were prepared.
Further, 8 individuals of transformants produced by introducing A2PA1aB1bM 1, 33 individuals of transformants produced by introducing A2PA1aB1bM3, 32 individuals of transformants produced by introducing A2PA1aB1bM5, and 9 individuals of transformants produced by introducing A2PRP10M1, to the seed storage protein-deficient variety were prepared.
These plant bodies of transformed soybean were acclimatized to ambient humidity, and the cultivation was continued under the conditions of 10000 1× and illumination for 16 hours per day, after which seeds were harvested from all the individuals. By such a process, seeds of the transformed soybean plants of the T1 generation were obtained.
Evaluation of Amount of Aβ4-10 Accumulated in Seeds of Transformed Soybean
Total protein was extracted from the seeds of the transformed soybeans obtained in the above Example 6, and the accumulated amount of Aβ4-10 was evaluated by Western blotting using an antibody specific to Aβ4-10. For lines having large accumulated amounts, quantitative analysis was carried out.
1) Amount of Accumulation of Aβ4-10 Expressed as Modified A1aB1b
20 μg of total protein extracted from seeds of each transformed soybean was separated by SDS-PAGE, and allowed to react with an antibody specific to Aβ4-10, followed by detection using ECL Advance Western Blotting Detection Kit (manufactured by GE Healthcare Bio-Science KK). A chemiluminescence image was captured by LAS4000miniPR (manufactured by FUJIFILM Corporation), and quantitative analysis was carried out using MultiGage, which is an analysis software included in the apparatus. As a standard sample for quantification, a His-Tag-linked recombinant protein A1aB1bM1 prepared by the E. coli expression system was used.
As a result, the signal band corresponding to Aβ4-10 was confirmed for each line of the transformed soybean seeds obtained in the above Example 6, so that accumulation of Aβ4-10 was confirmed. Among the lines, the transformed soybean seeds prepared by introducing A1aB1bM1, A1aB1bM3 and A1aB1bM5 to the Jack variety (lines No. 10-2, No. a-2 and No. 6-6) and the transformed soybean seeds prepared by introducing A1aB1bM1 to the seed storage protein-deficient variety (line No. 16-2), in which Aβ4-10 was highly accumulated, were subjected to measurement of the amounts of accumulation of Aβ4-10. The results are shown in Table 3.
Further, comparison of the accumulated amounts of the modified seed storage protein in the transformed soybeans prepared by introducing A1aB1bM1 (the gene in which three copies of Aβ4-10 are inserted) to the Jack variety and to the seed storage protein-deficient variety was carried out by Western blot analysis. The results are shown in
Further, the accumulated amount of the modified seed storage protein in the transformed soybeans prepared by introducing A1aB1bM3 (the gene in which a single copy of Aβ4-10 is inserted) to the seed storage protein-deficient variety was measured by Western blot analysis. The results are shown in Table 4.
2) Amount of Accumulation of Aβ4-10 Expressed as Modified Arcelin
20 μg of total protein extracted from seeds of each transformed soybean was separated by SDS-PAGE, and allowed to react with an antibody specific to Aβ4-10, followed by Western blot detection of Aβ4-10 using ECL Advance Western Blotting Detection Kit (manufactured by GE Healthcare Bio-Science KK). As a result, the signal bands corresponding to the Aβ4-10 peptide was confirmed for the transformed soybean seeds to which Arc5M1 was introduced (line 2-1) and the transformed soybean seeds to which Arc5M2 was introduced (line 2-2), so that accumulation of Aβ4-10 was confirmed (
3) Amount of Accumulation of Aβ4-10 Expressed as Modified Prolamin
20 μg of total protein extracted from seeds of the RP10M1-transformed soybean (lines 1-1 and 4-2) was separated by SDS-PAGE, and allowed to react with an antibody against Aβ4-10, followed by Western blot detection using ECL Advance Western Blotting Detection Kit (manufactured by GE Healthcare Bio-Science KK). As a result, the signal bands corresponding to the Aβ4-10 peptide was confirmed for the transformed soybean seeds of the respective lines to which PR10M1 was introduced, so that accumulation of the Aβ4-10 peptide was confirmed (
Similarly, the signal bands corresponding to the Aβ4-10 peptide was confirmed for the seeds of the RP10M1-transformed soybean, so that accumulation of Aβ4-10 was confirmed. The accumulated amount in this case was about 380 μg/g seed for the No. 1-1 line.
4) Amount of Accumulation of Aβ4-10 Expressed as Modified A1aB1b by Arcelin 2 Promoter
20 μg of total protein extracted from seeds of each transformed soybean was separated by SDS-PAGE, and subjected to the detection in the same manner as in 1) in Example 7.
As a result, the signal bands corresponding to Aβ4-10 was confirmed for the respective lines of transformed soybean seeds obtained in the above Example 6, so that accumulation of Aβ4-10 was confirmed (
Further, it was confirmed that the amount of accumulation of Aβ4-10 in the transformed soybean seeds prepared by introduction of the gene into the seed storage protein-deficient variety, which amount of accumulation was assumed based on the intensity of the signal band, for A2PA1aB1bM1 (line 4-6) was almost equivalent to that for A1aB1bM1 (line 7-1), and that these amounts of accumulation were clearly larger than those for A1aB1bM1 (line 8-1) prepared by introduction of the gene into the Jack variety (
Assay of Effect of Modified Seed Storage Protein
A1aB1bM1 prepared in the above Example 1 was expressed in E. coli by the known method, to produce the protein.
In order to obtain the recombinant protein encoded by A1aB1bM1, the E. coli expression plasmid pETA1aB1bM1 was prepared by ligating A1aB1bM1 with the pET21-d vector (manufactured by Novagen).
The above-described pETA1aB1bM1 was introduced to E. coli AD494 (manufactured by Novagen) by a conventional method, and the recombinant E. coli was cultured in 50 ml of the known TB medium (supplemented with kanamycin at a final concentration of 15 mg/l and carbenicillin at a final concentration of 50 mg/l) at 37° C. for 18 hours, followed by adding 10 ml of the culture to 1000 ml of the known LB medium (supplemented with kanamycin at a final concentration of 15 mg/l, carbenicillin at a final concentration of 50 mg/l and sodium chloride at a final concentration of 500 mM) as a production medium and carrying out culture at 37° C. for 2 hours. Thereafter, IPTG was added to a final concentration of 1 mM, and the recombinant E. coli was then cultured at 20° C. for 48 hours. The cells of E. coli after the culture were collected by centrifugation at 8000 rpm for 15 minutes. From the bacterial cells after the collection, the fraction of soluble protein was extracted using BugBuster Protein Extraction Reagent (manufactured by Novagen). From the obtained fraction of soluble protein, the recombinant protein encoded by A1aB1bM1 (A1aB1bM1 protein) was purified using Ni-NTA His-Bind Resins (manufactured by Novagen).
In physiological saline, 50 μg of A1aB1bM1 having the β-amyloid antigenic determinant (Aβ4-10) was dissolved, and the resulting solution was administered to Alzheimer's disease model mice (TgCRND8) of 4-weeks old five times at intervals of 1 week by subcutaneous injection (3 individuals/group). A control group was prepared by expressing the unmodified gene encoding the wild-type A1aB1b in E. coli in the same manner as described above, and administering the obtained wild-type A1aB1b to the mice. Nine weeks after the administration, blood was collected from the mice, and production of antibodies against Aβ4-10 was confirmed by the known sandwich method by ELISA. The antibody titer was evidently higher in the group to which the A1aB1bM1 protein was administered compared to the group to which the A1aB1b protein was administered, so that the vaccine effect of the recombinant protein encoded by A1aB1bM1 was confirmed.
Thermal Stability of Modified Seed Storage Protein in Soybean Seeds
The transformed soybean seeds obtained in the above Example 6 were subjected to various heat treatments to test the thermal stability of the modified seed storage protein in the seeds.
1) Roasted Group of Transformed Soybean Seeds
The A1aB1bM3-transformed soybean seeds were pulverized, and 10 mg of the pulverized product was processed in an autoclave sterilization equipment at 100° C. for 10 minutes, followed by extracting total protein by the method described in the above Example 7 and evaluating the amount of accumulation of Aβ4-10 in the seeds by Western blotting using an antibody specific to Aβ4-10.
2) Water-Boiled Group of Transformed Soybean Seeds
The A1aB1bM3-transformed soybean seeds were pulverized, and 30 μl of distilled water was added to 10 mg of the pulverized product, and the resultant was processed in an autoclave sterilization equipment at 100° C. for 10 minutes, followed by extracting total protein by the method described in the above Example 7 and evaluating the amount of accumulation of Aβ4-10 in the seeds by Western blotting using an antibody specific to Aβ4-10.
3) Group in which Extract from Transformed Soybean Seeds was Heat-Treated
The A1aB1bM3-transformed soybean seeds were pulverized, and total protein was extracted by the method described in the above Example 7, followed by processing the total protein in an autoclave sterilization equipment at 100° C. for 10 minutes. Thereafter, the amount of accumulation of Aβ4-10 in the seeds was evaluated by Western blotting using an antibody specific to Aβ4-10.
As a result, the signal bands corresponding to Aβ4-10 was confirmed in the roasted group and the water-boiled group. It was confirmed that the amounts were equivalent to that in the heat-untreated group, and hence that the modified seed storage protein in the seeds is heat-stable (
Form of (β-Amyloid Antigenic Determinant
The peptide having the amino acid sequence of Aβ-10 (P1), the peptide having the amino acid sequence wherein two copies of P1 are tandemly linked (P2), and the peptide having the amino acid sequence wherein three copies of P1 are tandemly linked (P3) were synthesized using a custom peptide synthesis service.
Subsequently, KLH-P1, KLH-P2 and KLH-P3, wherein a carrier protein key-limpet-hemocyanin (KLH, Mw. 1000000) is linked to the N-termini of the peptides P1, P2 and P3, respectively, through cysteine (Cys) as a cross-linker, were prepared.
In physiological saline, 50 μg each of these KLH-P1, KLH-P2 and KLH-P3 was dissolved, and the resulting solution was administered to mice (BALBc) of 4-weeks old five times at intervals of 1 week by subcutaneous injection (3 individuals/group). Nine weeks after the administration, blood was collected from the mice to collect antiserum. The obtained antiserum was affinity-purified to prepare purified antibodies against KLH-P1, KLH-P2 and KLH-P3.
Commercially available synthetic Arβ42 in amounts of 400 and 1000 picomoles was subjected to electrophoresis by SDS-PAGE, and the above-described purified antibodies against KLH-P1, KLH-P2 and KLH-P3 were allowed to react with the Aβ42, followed by detection using ECL Advance Western Blotting Detection Kit (manufactured by GE Healthcare Bio-Science KK). The chemiluminescence image was captured by LAS4000miniPR (manufactured by FUJIFILM Corporation), and the signal intensities were compared to assume the binding capacities of the antibodies to Aβ42. As a result, it was shown that the signal intensity for KLH-P2 was evidently stronger than the signal intensities for KLH-P1 and KLH-P3, and hence that a specific antibody having a high antibody titer against Aβ can be obtained by tandemly linking two copies of the peptide having the amino acid sequence of Aβ4-10 (
Industrial Applicability
Since, by the present invention, it is possible to produce and accumulate an Alzheimer's disease vaccine in soybean seeds as a fusion protein with a seed storage protein such as soybean 11S globulin or 7S globulin, common bean arcelin, or rice prolamin, a large amount of the Alzheimer's disease vaccine can be produced and supplied for prophylaxis and therapy of Alzheimer's disease.
Number | Date | Country | Kind |
---|---|---|---|
2008-304006 | Nov 2008 | JP | national |
Filing Document | Filing Date | Country | Kind | 371c Date |
---|---|---|---|---|
PCT/JP2009/069977 | 11/26/2009 | WO | 00 | 5/20/2011 |
Publishing Document | Publishing Date | Country | Kind |
---|---|---|---|
WO2010/061899 | 6/3/2010 | WO | A |
Number | Name | Date | Kind |
---|---|---|---|
6576820 | Takaiwa et al. | Jun 2003 | B1 |
20030232758 | St. George-Hyslop et al. | Dec 2003 | A1 |
20070136896 | Takaiwa et al. | Jun 2007 | A1 |
20070192905 | Piller et al. | Aug 2007 | A1 |
20070280953 | Rosenberg et al. | Dec 2007 | A1 |
Number | Date | Country |
---|---|---|
WO 2006093277 | Sep 2006 | WO |
Entry |
---|
Takagi et al (PNAS, 102(48), pp. 17525-17530, 2005). |
Youm et al (Biotechnol Lett., 30, pp. 1839-1845, 2008). |
Takaiwa et al (AAY80994, published Jun. 5, 2000). |
GenBank AB353075 (published 2007). |
Oono, et al. “Analysis of ER Stress in Developing Rice endosperm Accumulating β-amyloid Peptide,” Plant Biotechnology Journal, vol. 8, No. 6, pp. 691-718, Mar. 15, 2010. |
Extended European Search Report dated May 12, 2029, issued to the corresponding European patent application No. 09829144.6. |
Adachi, et al. “Crystal Structure of Soybean Proglycinin A1aB1b Homotrimer,” Journal of Molecular Biology, vol. 305, pp. 291-305, 2001. |
Hasagawa, et al. “2-6 Technological Development of Soybean that Produces Highly Functional Substance,” Preprints of Biotechnology Symposium, Nov. 6, 2008, 28th, pp. 87-88. |
Manea, et al. “Polypeptide Conjugates Comprising a β-Amyloid Plaque-Specific Epitope as New Vaccine Structures Against Alzheimer's Disease,” Biopolymers, vol. 76, pp. 503-511, 2004. |
Takagi, et al. “A Rice-based Edible Vaccine Expressing Multiple T Cell Epitopes Induces Oral Tolerance for Inhibition of Th2-mediated IgE Responses,” Proceedings of the National Academy of Sciences USA, vol. 102, No. 48, pp. 17525-17530, 2005. |
Terakawa, et al. 3-6 Technological Development of Soybean that Produces Highly Functional Substance, Preprints of Biotechnology Symposium, Nov. 6, 2007, pp. 103-104. |
Utsumi, et al. “Synthesis, Processing and Accumulation of Modified Glycinins of Soybean in the Seeds, Leaves and Stems of Transgenic Tobacco,” Plant Science, vol. 92, pp. 191-202, 1993. |
Utsumi, “X-ray Crystallography for Molecular Designing of Soybean Protein Having Enhanced/Given Functionality,” The 3rd Result Report, pp. 69-70, 1995. |
Youm, et al. “Transgenic Potato Expressing Aβ Reduce Aβ Burden in Alzheimer's Disease Mouse Model,” FEBS Letters, vol. 579, pp. 6737-6744, 2005. |
Youm, et al. “Transgenic Tomatoes Expressing Human Beta-amyloid for Use as a Vaccine Against Alzheimer's Disease,” Biotechnology Letters, vol. 30, pp. 1839-1845, 2008. |
International Search Report issued to international application No. PCT/JP2009/069977 dated Feb. 9, 2010. |
Office Action issued in continuation-in-part application, U.S. Appl. No. 13/290,960, mailed on Apr. 25, 2014. |
Kokjohn et al., “Amyloid precursor protein transgenic mouse models and Alzheimer's disease: Understanding the paradigms, limitations, and contributions”, Alzheimer's and Dementia, vol. 5, pp. 340-347 (2009). |
Office Action issued in corresponding Japanese Patent Application No. 2009-269231, mailed on May 7, 2014, with partial English translation. |
Prak et al., “Design of genetically modified soybean proglycinin A1aB1b with multiple copies of bioactive peptide sequences,” Peptides, vol. 27(6), pp. 1179-1186 (2006). |
Number | Date | Country | |
---|---|---|---|
20110243975 A1 | Oct 2011 | US |