Abstract:
The invention provides a promoter that has high expression strength and can be over-expressed in various tissues of plant, said promoter is a promoter for banana polyubiquitin (polyubiquitin) gene MhUBQ1, and has a sequence as SEQ ID No: 3. The invention provides further a gene expression cassette that contains a promoter comprising a DNA sequence as SEQ ID No: 3, and a polynucleotide having a open reading frame (ORF) linked to the 3′ terminal of said promoter, wherein said promoter can activate the transcription of said polynucleotide in a organism containing said gene expression cassette. The invention provides further a gene expression vector that contains a promoter having a DNA sequence as SEQ ID No: 3. Also, the invention provides a process for producing a transgenic plant or part of organ, tissue or cell thereof containing the above-described gene expression cassette.

Description:
BACKGROUND OF THE INVENTION 
     1. Field of the Invention 
     The invention relates to a gene promoter characterized in that it can be over-expressed in various plant tissues, as well as to applications of said promoter. 
     2. Description of the Prior Art 
     Banana ( Musa  spp.) belongs to Musaceae, Monocotyledon, with its fruit being fragrant and delicious, as well as having high nutritional value. The desired banana protein can be used to produce in large quantities vaccines useful for treating diseases in humans or animals, by using the banana as gene transfer material. The banana can be used to directly uptake the vaccine orally, which is not only more convenient and safer than a vaccine injection, but also prevents proteins from losing their function through denaturizing in cooking, since banana fruit can be eaten raw. 
     In order to enable a transgenic plant to produce protein in large amounts, in the construction of a gene transfer construct selection of a proper promoter for activating the target gene that is highly associated with the production of proteins is important. At present, most conventional technologies for plant gene transfer has use cauliflower mosaic virus 35S (CaMV 35S) promoter to induce the over-expression of target genes in dicotyledon or monocotyledon plants. However, the expression of CaMV 35S promoter in a monocotyledon plant is relatively low. In order to improve the activation ability of a promoter, cloning of a promoter with high expression strength originally present in the monocotyledon plant, such as the Act1 promoter for paddy rice actin gene, Ubi1 promoter for corn polyubiquitin gene, and the like, might be carried out. Among these, the expression strength of Ubi1 promoter in a monocotyledon plant system is higher and more stable than that of CaMV 35S promoter, thereby the gene expression can be increased significantly (Christensen et al., 1992; McElroy et al., 1991). 
     Ubiquitin is a small molecular protein extensively present in a eukaryote. Its gene belongs to a polygene family. Based on its gene structure, it can be classified into three major groups: polyubiquitin gene, ubiquitin extension gene and ubiquitin-like gene. Polyubiquitin gene consists of arranging identical mono ubiquitin gene head-to-tail in a manner of tandem repeat in same direction. There are many types of polyubiquitin gene in plants, each with different modulation mechanisms. Further, there are different expression patterns such as constitutive expression, inducible expression, tissue specific expression and the like. Polyubiquitin gene with constitutive expression can be over-expressed in all tissues and organs, such as parsley ubi 4-2 (Kawalleck et al., 1993) and UBQ10 of  Arabidopsis thialana  (Sun et al., 1997) and the like. 
     Another feature of polyubiquitin gene is that there is a first intron connected tightly with ATG at its 5′-untranslation region, where the sequence at the joint of this intron and exon is highly conserved, which is consistent with AG/gt principle at 5′-terminal cleavage and the ag/GT principle at 3′-terminal cleavage, such as genes of rice RUBQ1 and 2, sunflower UbB1 and 2 as well as  Arabidopsis thialana  UBQ3, 10 and 11. The presence or absence of the first intron might influence the activity of a polyubiquitin gene promoter, and its length varies with species (Norris et al., 1993; Plesse et al., 2001). 
     Many researches had shown that ubiquitin gene promoters isolated from a variety of plants exhibited expression activity in gene transfer system stronger than that of CaMV 35S promoter. Accordingly, studies on the activity and tissue-specific expression of ubiquitin gene promoter in order to assess its applications will become a topic worthy of future investigation. 
     In view of the importance of developing promoters with high activating ability for the biotechnical industry, the inventor had thought to improve and innovate, and finally, after studying intensively for many years, successfully developed the promoter with high expression strength and capable of being over-expressed in various tissues of a plant, as well as its application according to the invention. 
     SUMMARY OF THE INVENTION 
     One object of the invention is to provide a promoter characterized in that it exhibits high expression strength and can be over-expressed in various tissues of a plant. 
     Another object of the invention is to provide an application of the promoter that has high expression strength and can be over-expressed in various tissues of a plant, where by taking advantage of the high ability of activating a downstream gene; the promoter can be used for over-expression of a target gene in various tissues of a plant. 
     Yet another object of the invention is to provide a gene expression vector. Said vector comprises a promoter with high expression strength and can be over-expressed in various tissues of a plant, such that, by cloning a target gene into a plant cell through said vector, said target gene can be over-expressed in various tissues of said plant. 
     A promoter with high expression strength and can be over-expressed in various tissues of a plant that can achieve the above-described objectives of the invention is characterized in that sequences of said promoter are obtained from genomic DNA of banana ( Musa  spp.). By using a fragment of  Arabidopsis thialana  polyubiquitin UBQ3 gene (GenBank accession number L05363; SEQ ID No: 1) as a probe, selection of banana genomic library is carried out, and after several purifications, a banana polyubiquitin genomic clone is obtained. By performing restriction map analysis and nucleic acid sequencing, a banana polyubiquitin gene Mh-UBQ1 is obtained, with its coding region sequence having a GenBank accession number as AF502575 (SEQ ID No: 2), and a 3,093 bp regional sequence (SEQ ID No: 3) ahead of the translation start site (gene code ATG) of banana polyubiquitin gene Mh-UBQ1 is also obtained, wherein said 3,093 bp regional sequence is at 5′upstream region of the translation start site (ATG); wherein said 5′upstream region comprises the postulated gene promoter, 5′-end untranslated region (5′UTR), an postulated exon 1 and intron 1; and wherein said 3,093 bp DNA sequence is used as the banana polyubiquitin gene Mh-UBQ1 promoter in the construction of cloning vector. 
     To analyze the ability of said banana polyubiquitin gene Mh-UBQ1 promoter (SEQ ID No: 3) for activating a downstream gene, said promoter sequence is ligated to the 5′ terminal of the gene sequence of a reporter gene, β-glucuronidase (GUS), to act as the promoter of said reporter gene, and then Mh-UBQ1 promoter is constructed into a  Agrobacterium tumefaciens  cloning vector to form a pMhUBQ1p-GUS plasmid; next, by means of  Agrobacterium tumefaciens  transformation, said pMhUBQ1p-GUS plasmid is cloned into model plants,  Arabidopsis thialana  ecotype Columbia and  Nicotiana tabacum  L., respectively; and finally, the activity of said promoter is assayed by GUS histochemical staining. The results show that said banana polyubiquitin gene Mh-UBQ1 promoter (SEQ ID No: 3) driven target gene to over-express in all tissues of a plant. Accordingly, the inventive banana polyubiquitin gene Mh-UBQ1 promoter (SEQ ID No: 3) possesses activating ability of high expression strength, and can be over-expressed in various tissues of a plant. 
     In addition to providing a promoter that has a high expression strength and can be over-expressed in various tissues of a plant, the invention provides further a gene expression cassette. Said gene expression cassette comprises: (1) the inventive promoter sequence (SEQ ID No: 3), and (2) a length of polynucleotide having an open reading frame (ORF), i.e. a target gene; wherein said polynucleotide is ligated to the 3′ terminal of the inventive promoter, and said promoter can initiate the transcription of said polynucleotide in a organism containing said gene expression cassette. In a preferred embodiment, said target gene is a reporter gene β-glucuronidase (GUS). 
     Further, the inventive banana polyubiquitin gene Mh-UBQ 1 promoter (SEQ ID No: 3) can be constructed into a commercial cloning vector which includes, but not limited to: pBI101, pBI121, pBIN19 (ClonTech), pCAMBIA1301, pCAMBIA1305, pGREEN (GenBank Accession No: AJ007829), pGREEN II (GenBank Accession No: EF590266) (www.pGreen.ac.uk), pGreen0029 (John Innes Centre), to form a gene expression vector. Then, a target gene can be inserted said gene expression vector in a manner that, after inserting said target gene to the 3′ terminal of the inventive promoter, a gene expression cassette described above is formed. Furthermore, the inventive promoter together with the target gene ligated at its 3′ terminal can be transferred in a target plant through gene transfer, and hence change further the genomic constitution of the transgenic plant such that the inventive promoter with the target gene can activate effectively the expression of said target gene in the objective transgenic plant and the progeny thereof. 
     Moreover, the invention provides a process for producing a transgenic plant or part of organ, tissue or cell thereof containing the above-described gene expression cassette, said process comprising following steps:
     step 1: providing a cell or tissue of a target plant;   step 2: transferring a gene expression cassette containing the inventive promoter sequence (SEQ ID No: 3) into the cell or tissue of a target plant obtained in step 1 to obtain a transgenic plant cell or transgenic plant tissue; and   step 3: culturing the transgenic plant cell or transgenic plant tissue obtained in step 2 to produce a transgenic plant or part of organ, tissue or cell thereof comprising the gene expression cassette containing the inventive promoter sequence (SEQ ID No: 3).   

     wherein the gene transfer described in said step 2 includes, but not limited to:  Agrobacterium tumefaciens  mediation, recombinant virus transformation, transposon vector transfer, gene gun, electroporation, micro-injection, pollen tube pathway, liposome-mediation, ultrasonic-mediation transfer, silicon carbide fiber-mediated transformation, electrophoresis, laser microbeam mediation, polyethylene glycol (PEG) mediation, calcium phosphate-mediated transformation, DEAE-dextran transformation and the like. 
     These features and advantages of the present invention will be fully understood and appreciated from the following detailed description of the accompanying Drawings. 
    
    
     
       BRIEF DESCRIPTION OF THE DRAWINGS 
       The patent or application file contains at least one drawing executed in color. Copies of this patent or patent application publication with color drawing(s) will be provided by the Office upon request and payment of the necessary fee. 
         FIG. 1A  is the genomic restriction map of the inventive banana polyubiquitin gene MhUBQ1.  FIG. 1B  is a construction strategy scheme for constructing partial GUS fragment (fragment I).  FIG. 1C  is a construction strategy for constructing said banana polyubiquitin gene Mh-UBQ1 promoter (MhUBQ1p fragment).  FIG. 1D  is a construction strategy scheme for constructing cleaved pGKU.  FIG. 1E  is a construction strategy for constructing a plasmid pMhUBQ1p-GUS of the inventive banana polyubiquitin gene MhUBQ1 promoter. 
         FIG. 2  shows the construction strategy for the transformation vector pGKU of  Agrobacterium tumefaciens.    
         FIG. 3  shows the transient expression of GUS by gene gun transformed said expression vector (pMhUBQ1p-GUS); wherein the materials are  Phalaenopsis  petal, suspended banana cell and banana pericarp, respectively, and the transient expression of CaMV 35S promoter expression vector is used as the control group ( FIGS. 3A , B, and C); and wherein the transient expression of MhUBQ1 promoter expression vector is used as the test group ( FIGS. 3D , E, and F). The white bar on each figure is 0.5 cm in length. 
         FIG. 4  shows the expression analysis of reporter gene β-glucuronidase (GUS) in various tissue of the progeny of  Arabidopsis thialana  transformant containing pMhUBQ1p::GUS-NOS gene expression cassette.  FIG. 4A : GUS histochemical staining results of  Arabidopsis thialana  transformant whole plants grown for different number of days.  FIG. 4B : GUS histochemical staining results of  Arabidopsis thialana  transformant flower organ at different developmental stages, where non-transformed flower organs at each stage were used as the control groups.  FIG. 4C : GUS histochemical staining results of siliques of  Arabidopsis thialana  transformant at different maturing stages, where non-transformed siliques at different stages were used as the control groups. All transformants tissues assayed presented blue color. 
         FIG. 5  shows expression analysis results of reporter gene β-glucuronidase (GUS) at various tissue of  Nicotiana tabacum  L. transformant progeny comprising MhUBQ1p::GUS-NOS gene expression cassette.  FIG. 5A : GUS histochemical staining results of  Nicotiana tabacum  L. transformant whole plants grown for different number of days.  FIG. 5B : GUS histochemical staining results of  Nicotiana tabacum  L. transformant flower organs at different developmental stages, where non-transformed flower organs at different stages were used as control groups. All of the transformant tissues assayed presented blue color. 
     
    
    
     DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT 
     Example 1 
     Cloning of Banana Polyubiquitin Gene Mh-UBQ1 Promoter 
     1. Sources of Banana λEMBL3 Genomic Library (Genomic Library) 
     Banana genomic library was genomic DNA that was extracted from leaves of a banana species,  Musa  spp. cv. Hsien Jin Chiao (AAA group) plant, and the genomic library was constructed then by cleavage substitution of DNA fragments using bacteriophage λEMBL3 as the vector. 
     2. Preparation and Labeling of Nucleic Acid Probe 
     Nucleic acid probe was prepared by using a gene fragment of  Arabidopsis thialana  polyubiquitin UBQ3 gene (GeneBank accession number L05363, SEQ ID No: 1) as the template, and employing Prime-A-Gene kit (Promega, USA) in the process described below: total reaction volume was 50 μL, consisting of 1× labeling buffer, pH 6.6 {50 mM Tris-HCL, pH 8.3, 5 mM MgCl 2 , 2 mM DTT, 0.2 M HEPES [N-(2-hydroxyethyl)piperazine-N′-(2-ethanesulfonic acid)], 26A 260  unit/mL random hexadeoxyribonicleotides}, 20 μM each of dATP, dGTP, and dTTP, 500 ng/mL denatured DNA template, 400 μg/mL Bovine serum albumin (BSA), 50 μCi [α- 32 P] dCTP (333 nM), and 5 unit Klenow DNA Polymerase. The reaction was carried out at 37° C. for 2 hours, and then 2 μL of 0.5 M EDTA (pH 8.0) was added to terminate the reaction. Thereafter, 8 μL of tracking staining agent (50% glycerol, 0.25% bromophenol blue) was added. The reaction solution was passed through Sephadex-G50 chromatographic column, and was eluted with TE (pH 7.6) buffer solution; every 160-180 μL aliquot was collected in a tube. Radioactivities of these aliquots were determined in a scintillation counter (Liquid Scintillation Counter, Beckman 1801) and the aliquot with the highest radioactivity was used as the probe. 
     3. Selection of Banana Polyubiquitin Gene Mh-UBQ1 Genomic Library 
     Banana genomic library was selected by plaque hybridization. At first, E. coli strain XL1-Blue MRA (P2) used as the infiltration host of λEMBL3 was cultured in NZY medium (consisting of 5 g NaCl, 2 g MgSO 4 .7H 2 O, 5 g yeast extract per liter). 1.5 million plaque forming units were selected under high stringency. 
     Bacteriophages were transferred on a nitrocellulose membrane, and the membrane thus transferred was treated in a denaturing buffer (0.5 M NaOH, 1.5 M NaCl) for 2 minutes, then in a neutralization buffer [0.5 M Tris base, 1.5 M NaCl, 0.035% HCl (v/v)] for 5 minutes, and finally incubated in 2×SSPE (1×SSPE, consisting of 0.18 M NaCl, 10 mM NaH 2 PO 4 , 1 mM EDTA pH7.4) for 30 seconds. Thereafter, the membrane was treated in a vacuum oven at 80° C. for 2 hours to immobilize bacteriophage DNA and then was incubated in a solution containing 2×SSPE and 0.1% SDS. The mixture was shaken at room temperature for one hour. Then, the nitrocellulose membrane was transferred in a pre-hybridization solution containing 5×SSPE, 5×BFP (1×BFP consisting of 0.02% BSA, 0.02% Ficoll-400000, 0.02% PVP-360000), 0.1% SDS, 50% formamide and 500 μg/mL salmon sperm DNA. A pre-hybridization reaction was carried out at 37° C. for 2 hours. Next, a hybridization reaction was carried out on the membrane with a radio-labeled probe in 5×SSPE, 1×BFP, 0.1% SDS, 50% formamide and 100 μg/mL salmon sperm DNA at 37° C. for 16˜18 hours. Thereafter, the nitrocellulose membrane was treated twice in a wash buffer I (5×SSPE, 0.1% SDS) at room temperature for 15 minutes, then twice in a wash buffer II (1×SSPE, 0.5% SDS) at 37° C. for 15 minutes to remove non-specific probes. After developing by pressing exposure on an X-film (Kodak XAR film) at −80° C., bacteriophages containing target gene DNA could be detected. Said bacteriophages were isolated from the medium, stored in a SM buffer solution containing 0.03% chloroform. After several purifications, a banana polyubiquitin gene Mh-UBQ1 genomic clone λMhUBQ79 was obtained. 
     4. Extraction of λMhUBQ79 Bacteriophage Clone DNA 
     The thus-obtained liquor containing bacteriophages clone λMhUBQ79 was placed on NZY solid medium. The bacteriophage liquor was grooved with a toothpick, and then 3 mL Top agar containing host cells  E. coli  XL1-Blue MRA (P2) was added, and mixture was cultivated on NZY solid medium at 37° C. for 8 hours. On the next day, mono-plaque agar plaque was picked up from the groove with a capillary. The plaque was spread and cultivated again over a NZY solid medium at 37° C. for 7˜11 hours. Then, the medium was placed in a refrigerator at 4° C. Bacteriophages were lysed by adding SM. The lysate was collected in a centrifuge tube, and chloroform was added to 0.03%, and then was centrifuged at 4° C. and 7,000 rpm (Beckman J2-MC, JS-13.1) for 5 minutes. It was stored at 4° C. for use. Thereafter, the target bacteriophage clone mass reproduced above was used to infect host cells at a bacteria ratio of 5:1 as follow: 1 mL SM buffer solution and 5 mL of 2.5 mM CaCl 2  was added, well-mixed, stored at room temperature for 15 minutes and then at 37° C. for 45 minutes. Then, it was poured in 100 mL 2×NZY liquid medium (0.4% MgSO 4 ·7H 2 O, 2% NaCl, 1% bacto-yeast extract, 2% NZ amine, 0.2% casamino acid, 5 mM MgSO 4 , 25 mM Tris-HCl pH7.5), and was cultured at 37° C. and 240 rpm for more than 8 hours. 4.5 mL chloroform was added, and the mixture was treated by shaking at 37° C. and 240 rpm for 15 minutes, and then the mixture was centrifuged at 4° C. and 7,000 rpm for 20 minutes (Beckman J2-MC, JA 10 rotor). To the supernatant, 100 μL DNase I (1 mg/mL) and 100 μL RNaseA (10 mg/mL) were added. The mixture was treated at 37° C. and 80 rpm for 45. 33 mL of 4M NaCl was added thereto, and the mixture was cooled in an ice bath for 1 hour. Then, 33 mL ice-cold 50% polyethylene glycol was added thereto, and was settled at 4° C. overnight. The mixture was centrifuged at 4° C. and 5,000 rpm for 20 minutes (Beckman J2-MC, JA 10 rotor). The supernatant was discarded. The pellet was air-dried and then was re-suspended in 500 μL PKB solution (10 mM NaCl, 10 mM Tris-HCl pH 8.0, mM EDTA, 0.1% SDS). Thereafter, proteinase K (final concentration 12.5 μg/mL) was added thereto and reacted at 37° C. for 20 minutes. The mixture was extracted successively with equal volume of phenol, PCI (phenol: chloroform: isoamyl alcohol=25:24:1), CI (chloroform:isoamyl alcohol=24:1) and centrifuged at room temperature and 14,000 rpm for 5 minutes. To the supernatant was added 2-fold volume of −20° C. 100% ethanol, and the mixture was centrifuged at 4° C. and 14,000 rpm for 10 minutes. The supernatant was discarded and the pellet was air-dried. The precipitated DNA washed with 70% ethanol, and 100% ethanol, respectively, then dissolved in TE (pH 7.5) buffer solution, and stored at 4° C. for use. 
     5. Sequencing of DNA 
     DNA sequencing was carried out on an automatic nucleic acid sequencer (ABI sequencer 377) to obtain the sequence of the genomic clone λMhUBQ79 of banana polyubiquitin gene Mh-UBQ1, and was analyzed with PC/Gene software from IntelliGenetics Inc. The result was shown in  FIG. 1A , where genomic clone λMhUBQ79 of banana polyubiquitin gene Mh-UBQ1 contained 5′upstream region ahead of the translation start site (ATG) and a coding region. Said 5′upstream region comprised the postulated gene promoter, 5′ terminal untranslation region (5′UTR), postulated exon 1 and intron 1; wherein the second exon of the coding region is consisted of 5 homogeneous ubiquitin genes aligned head-to-tail repeat in same direction (5 homogeneous ubiquitin genes were designed as 1, 2, 3, 4 and 5, respectively); wherein its translation start site (gene code ATG) was located on the first nucleotide of the exon 2. The inventive banana polyubiquitin gene Mh-UBQ1 promoter was selected from the DNA sequence of about 3,093 bp in the 5′ upstream region (5′ upstream) of the translation start site (ATG), as shown in SEQ ID No: 3. 
     Example 2 
     Construction of Vector Containing Banana Polyubiquitin Gene Mh-UBQ1 Promoter 
     Construction strategy of banana polyubiquitin gene Mh-UBQ1 promoter was shown in  FIG. 1E , where 3,093 bp promoter sequence (SEQ ID No: 3) ahead of translation start site of banana polyubiquitin gene Mh-UBQ1 was constructed into a transformation vector pGKU for  Agrobacterium tumefaciens  to replace the original CaMV 35S promoter (35Sp) in a manner that banana polyubiquitin gene Mh-UBQ1 promoter (SEQ ID No: 3) was ligated to the 5′ terminal of reporter gene β-glucuronidase (GUS) gene sequence so as to act as the promoter of said reporter gene. 
     Step 1: Construction of  Agrobacterium tumefaciens  Transformation Vector pGKU 
     The construction strategy for  Agrobacterium tumefaciens  transformation vector pGKU was shown in  FIG. 2 , where a CaMV 35S promoter (35Sp)-reporter gene (GUS)-terminator (NOS-ter) fragment (CaMV 35s::GUS-NOS) on a commercial vector pRT99GUS was constructed into a commercial  Agrobacterium tumefaciens  transformation vector pGreen0029 (John Innes Centre) so as to obtain an  Agrobacterium tumefaciens  transformation vector pGKU. The construction strategy comprised synthesis of CaMV 35S promoter (35Sp) DNA fragment and reporter gene (GUS)-terminator (NOS-ter) DNA fragment through polymerase chain reaction (PCR), respectively; by means of the design of PCR primer, NcoI restrictive cleavage site was inserted on the 3′ terminal of CaMV 35S promoter (35Sp) DNA fragment and the 5′terminal of reporter gene (GUS)-terminator (NOS-ter) DNA fragment, respectively; and finally, these two PCR-derived fragments were constructed in pGreen0029 to obtain  Agrobacterium tumefaciens  transformation vector pGKU. 
     Step 1.1: Obtaining of CaMV 35S Promoter (35Sp) Fragment on a Commercial Vector pRT99GUS 
     By using DNA of a commercial vector pRT99GUS as a template, amplification of DNA sequence of CaMV 35S promoter (35Sp) fragment was carried out through PCR, where PCR used primers with following sequences: 
     
       
         
               
               
               
             
               
               
             
               
               
               
             
               
               
             
               
               
               
             
           
               
                   
                 forward primer S5 (containing HindIII 
                   
               
               
                   
                 restriction site): 
               
             
          
           
               
                 (SEQ ID No: 4) 
                   
               
             
          
           
               
                   
                 5′-tgcatgcatgc   aagctt   g-3′ 
                   
               
               
                   
                                     HindIII 
               
               
                   
                   
               
               
                   
                 reverse primer S3 (containing NcoI restriction 
               
               
                   
                 site): 
               
             
          
           
               
                 (SEQ ID No: 5) 
                   
               
             
          
           
               
                   
                 5′-ata   ccatgg   cccggggatcctctagagtcgaggtcct-3′ 
                   
               
               
                   
                           NcoI 
               
             
          
         
       
     
     The total reaction volume of PCR was 50 μl (comprising: 1 μl genomic DNA, 10 μl 5× Phusion HF buffer solution, 1 μl 10 mM dNTP, 1 μl 20 μM forward primer, 1 μl 20 μM reverse primer, 35.5 μl sterile water, 0.5 μl Phusion DNA polymerase). PCR reaction conditions were: after reaction at 98° C. for 30 seconds, performing total 35 cycles of: reactions at 98° C. for 10 seconds, 60° C. 30 seconds, and 72° C. 60 seconds, and finally, reaction at 72° C. for 10 minutes as elongation. A PCR product of 544 bp in length was synthesized. The PCR product was cleaved with HindIII and NcoI restrictive enzymes to recover a DNA fragment of 470 bp in length (fragment S) which was stored at 4° C. for use. 
     Step 1.2: Obtaining Reporter Gene (GUS)-Terminator (NOS-Ter) Fragment on a Commercial Vector pRT99GUS 
     Similarly, DNA sequence of a commercial vector pRT99GUS was used as a template, and an amplification of DNA sequence of reporter gene (GUS)-terminator (NOS-ter) fragment was carried out by polymerase chain reaction (PCR). Primers used in PCR had following sequences: 
     
       
         
               
               
             
               
               
             
               
               
             
               
               
             
               
               
             
           
               
                 forward primer G5 (containing NcoI restriction 
                   
               
               
                 site): 
               
             
          
           
               
                 (SEQ ID No: 6) 
                   
               
             
          
           
               
                 5′-ata   ccatgg   tacgtcctgtag-3′ 
                   
               
               
                            NcoI 
               
               
                   
               
               
                 reverse primer G3 (containing HindIII restriction 
               
               
                 site): 
               
             
          
           
               
                 (SEQ ID No: 7) 
                   
               
             
          
           
               
                 5′-acggccagtgcc   aagctt   gcat-3′ 
                   
               
               
                                      HindIII 
               
             
          
         
       
     
     Total reaction volume of PCR was 50 μl (comprising: 1 μl genomic DNA, 10 μl of 5× Phusion HF buffer solution, 1 μl of 10 mM dNTP, 1 μl of 20 μM forward primer, 1 μl of 20 μM reverse primer, 35.5 μl sterile water, 0.5 μl Phusion DNA polymerase). PCR reaction conditions were: after reaction at 98° C. for 30 seconds, performing total 35 cycles of reactions at 98° C. for 10 seconds, 60° C. 30 seconds, and 72° C. 60 seconds, and finally, reaction at 72° C. for 10 minutes as elongation. A PCR product of 2,108 bp in length was synthesized. PCR product was cleaved with HindIII and NcoI restriction enzymes, and a DNA fragment (fragment G) of 2,093 bp in length was recovered and stored at 4° C. for use. 
     Step 1.3: DNA Ligation 
     A commercial vector pGreen0029 was cleaved with HindIII restriction enzyme, a DNA fragment (fragment P) of 4,632 bp in length was recovered, and DNA ligations were carried out with fragment S and fragment G obtained separately from the above steps 1.1 and 1.2 to obtain  Agrobacterium tumefaciens  transformation vector pGKU. As shown in  FIG. 2 , in addition to the feature of pGreen, said  Agrobacterium tumefaciens  transformation vector pGKU possessed CaMV 35S promoter (35Sp)-reporter gene (GUS)-terminator (NOS-ter) DNA fragment of a commercial vector pRT99GUS, as well as it had a NcoI restriction site at the 3′terminal of the CaMV 35S promoter (35Sp). Accordingly,  Agrobacterium tumefaciens  transformation vector pGKU could utilize the multiple cloning site comprising SmaI restriction site in pGreen0029, and NcoI restriction site to replace CaMV 35S promoter (35Sp) with other promoter sequence so as to initiate reporter gene GUS. 
     Step 2: Obtaining of Partial Sequence of GUS Fragment 
     For maintaining the self-splicing function (i.e., following ag/GT principle) of intron 1 in banana polyubiquitin gene thus constructed in order to assure the high activating ability of the promoter, NcoI restriction site of  Agrobacterium tumefaciens  transformation vector pGKU was not used but in stead, each insert fragment was prepared through PCR, as shown in  FIG. 1B . By using  Agrobacterium tumefaciens  transformation vector pGKU as the template, a partial GUS fragment from GUS translation start site (ATG) to SnaBI restrictive site was synthesized at first by amplification through PCR. Primers used in PCR had following sequences: 
     
       
         
               
               
             
               
               
             
               
               
             
               
               
             
               
               
             
           
               
                 forward primer G5-1: 
                   
               
             
          
           
               
                 (SEQ ID No: 8) 
                   
               
             
          
           
               
                 5′-atggtacgtcctgtagaaacc-3′ 
                   
               
               
                   
               
               
                 reverse primer G3-1 (containing SnaBI restriction 
               
               
                 site): 
               
             
          
           
               
                 (SEQ ID No: 9) 
                   
               
             
          
           
               
                 5′-tga   tacgta   cacttttcccggc-3′ 
                   
               
               
                           SnaBI 
               
             
          
         
       
     
     Total reaction volume of PCR was 50 μl (comprising: 1 μl genomic DNA, 10 μl 5× Phusion HF buffer solution, 1 μl of 10 mM dNTP, 1 μl of 20 μM forward primer, 1 μl of 20 μM reverse primer, 35.5 μl sterile water, 0.5 μl Phusion DNA polymerase). PCR reaction conditions were: after reaction at 98° C. for 30 seconds, performing total 35 cycles of reactions at 98° C. for 10 seconds, 60° C. 30 seconds, and 72° C. 60 seconds, and finally, reaction at 72° C. for 10 minutes as elongation. PCR product was cleaved with SnaBI restriction enzyme, a partial GUS fragment (fragment I) of 387 bp in length was recovered and stored at 4° C. for use. 
     Step 3: Obtaining Banana Polyubiquitin Gene Mh-UBQ1 Promoter (MhUBQ1p) Sequence 
     Banana genomic DNA extracted as described in Example 1 was used as template, amplification of the sequence of 3,093 bp (SEQ ID No: 3) ahead of the translation start site of banana polyubiquitin gene Mh-UBQ1 promoter was carried out by polymerase chain reaction (PCR), as shown in  FIG. 1C . 
     Primers used in the PCR had following sequences: 
     
       
         
               
               
             
           
               
                 forward primer M1: 
                   
               
               
                 5′-ggatccacatgttctgcagatagatag-3′ 
                 (SEQ ID No: 10) 
               
               
                   
               
               
                 reverse primer M2: 
               
               
                 5′-ctgatcaaagagataaaagaagaaagg-3′ 
                 (SEQ ID No: 11) 
               
             
          
         
       
     
     Total reaction volume of PCR was 50 μl (comprising: 1 μl genomic DNA, 10 μl 5× Phusion HF buffer solution, 1 μl of 10 mM dNTP, 1 μl of 20 μM forward primer, 1 μl of 20 μM reverse primer, 35.5 μl sterile water, 0.5 μl Phusion DNA polymerase). PCR reaction conditions were: after reaction at 98° C. for 30 seconds, performing total of 35 cycles of: 98° C. 10 seconds, 65° C. 30 seconds, and 72° C. 60 seconds, and finally, 72° C. for 10 minutes as elongation. PCR product (fragment MhUBQ1p) of full length was recovered and stored at 4° C. for use. 
     Step 4: DNA Ligation 
     The  Agrobacterium tumefaciens  transformation vector pGKU prepared in step 1 was cleaved with SmaI+SnaBI double restriction enzymes (as shown in  FIG. 1D ), and after purification, a cleaved pGKU vector was obtained. 
     Referring to  FIG. 1E , this cleaved pGKU vector was ligated with the partial GUS DNA fragment (fragment I) prepared in the step 2 and the banana polyubiquitin gene MhUBQ1 promoter (fragment MhUBQ1p, SEQ ID No: 3) prepared in the step 3 to obtain a plasmid pMhUBQ1p-GUS containing banana polyubiquitin gene MhUBQ1 promoter sequence (SEQ ID No: 3). In said pMhUBQ1p-GUS plasmid, the 3′terminal of the banana polyubiquitin gene MhUBQ1 promoter was ligated with DNA sequence (MhUBQ1p::GUS-NOS) of the reporter gene β-glucuronidase (GUS). Consequently, by transferring said pMhUBQ1p-GUS plasmid into a plant body through  Agrobacterium tumefaciens  transformation, the pattern as banana polyubiquitin gene MhUBQ1 promoter initiating the expression of reporter gene β-glucuronidase (GUS) gene could be analyzed. 
     Example 3 
     Analysis of the Transient Expression of Banana Polyubiquitin Gene Promoter with Gene Gun 
     1. Preparation of Micro-Particle and DNA Packaging 
     To 60 mg of metal tungsten particle with a diameter of 1.7 □m, 1 mL of 70% EtOH was added and after shaking for 3-5 minutes, the mixture was allowed to stand for 15 minutes. After a short centrifuge to settle the particles, the supernatant was discarded. 1 mL sterile water was added thereto, shaken for 1 minute, short centrifuged again, and discarded the supernatant. These treatments were repeated several times. Finally, 1 mL sterile 50% glycerol was added thereto. To 50 □g glycerol suspension containing metal micro-particles, 5 □L plasmid DNA (1 □g/□L), 50 □L of 2.5 M CaCl 2 , 20 □L of 0.1 M spermidine were added successively, and the mixture was vortexed for 2-3 minutes. The mixture was allowed to stand for 1 minute. After settling by centrifuge, the supernatant was discarded. After washed with 140 □L 70% EtOH and 100% EtOH, respectively, the supernatant was aspirated off, and finally, 48 □L of 100% EtOH was added thereto, and the mixture was stored for use. Each gun hit used 6 □L. 
     2. Conditions for Gene Gun Transformation 
     Banana cell suspension, banana pericarp and Phalaenopsis petal were used as materials and treated with pressure-accelerated particle gene gun, PDS-1000/He particle gun, from Bio-Rad under conditions: Gap: ⅜ inches; micro-carrier flight distance: 8 mm; vacuum: 25 inches-Hg; pressure sheets used: 900, 1350 and 1100 Psi, respectively; and distance from material to stop screen: 6 cm. 
     3. GUS Histochemical Staining 
     Materials to be tested were incubated in pre-treatment buffer solution [50 mM Na 3 PO 4  (pH6.8), 1% TritonX-100] at 37° C. for 2 hours, and then rinsed 2-3 times with buffer solution (50 mM Na 3 PO 4 , pH6.8) containing no Triton X-100. Thereafter, buffer solution (1 mM X-Gluc dissolved in 50 mM Na 3 PO 4 , pH 6.8) containing X-Gluc (5-Bromo-4-chloro-3-indoxyl-beta-D-glucuronic acid) was added thereto. The mixture was evacuated at 25 inches-Hg for 5 minutes, and then returned to atmospheric pressure for 5 minutes. This process was repeated once more. The mixture was then placed at 37° C., reacted for 2 days, and finally, 70% ethanol was added to terminate and reaction and tissue discoloration, where coloration was to be observed. 
       FIG. 3  shows the results of GUS activity analysis, where conventional CaMV 35S promoter was used as the control group ( FIGS. 3  A, B, and C); reporter gene GUS activated with banana polyubiquitin gene MhUBQ1 promoter was test groups ( FIGS. 3  D, E, and F), wherein reporter gene GUS activated with banana polyubiquitin gene MhUBQ1 promoter, either for suspended banana cell, banana pericarp or Phalaenopsis petal, their transient expressions in monocotyledon plant materials were analyzed as good activation ability ( FIGS. 3  D, E, and F), and especially, suspended banana cell and banana pericarp exhibited significant genetic bombardment results ( FIGS. 3  E and F). Within banana tissues, CaMV 35S promoter exhibited extreme low activation ability for GUS ( FIGS. 3  B and C), where only few cells presented coloration response. In contrast, banana polyubiquitin gene MhUBQ1 promoter exhibited significant activation ability for downstream GUS gene, indicating that banana polyubiquitin gene MhUBQ1 promoter did have high expression ability in monocotyledon plants. Accordingly, if this promoter could be applied in the gene transfer of monocotyledon plants, the development of the biotechnical industry of monocotyledon plants (for example: paddy rice, corn, banana, orchid and the like) should be improved. 
     Example 4 
     Gene Transfer of  Arabidopsis thialana  Through  Agrobacterium tumefaciens  Transformation 
     In this example,  Arabidopsis thialana  was used as a model material. By means of  Agrobacterium tumefaciens  floral dip transformation, pMhUBQ1p-GUS plasmid prepared in Example 2 was transferred into  Arabidopsis thialana  so as to change the genomic constitution of the transgenic plant such that the banana polyubiquitin gene MhUBQ1 promoter could activate effectively the expression of reporter gene GUS in the objective transgenic plant and the progeny thereof. In addition, the expression sites of reporter gene GUS on  Arabidopsis thialana  transformant as well as the expression strength of the banana polyubiquitin gene MhUBQ1 promoter were analyzed by means of GUS active histochemical staining. 
     1. Growth Condition of  Arabidopsis thialana  Plant Material 
     Seeds of  Arabidopsis thialana  were wet and cold stratified at 4° C. for 2-4 days and sowed then in a medium consisting of peat:Perlite:vermiculite in a ratio of 10:1:1. Cultivation conditions were: 22-25° C., 16 hours light cycle, and 75% relative humidity. After about 4-6 weeks, the plant was pruned. As the rachis had grown to a length of about 3 inches on 4-8 days after pruning, the plant was subjected to transformation. 
     2. Preparation of  Agrobacterium tumefaciens  Liquor and Infiltration 
       Agrobacterium tumefaciens  LBA4404 strain was inoculated in YEB solid medium (0.5% beef extract, 0.1% yeast extract, 0.5% peptone, 0.5% mannitol, 0.05% MgSO 4 , 1.25% agar, pH 7.5) containing suitable antibiotics (50 μg/ml of kanamycin, 50 μg/ml of ampicillin), and cultivated at 28° C. for 2 days. Then, single colony was picked, inoculated in 20 ml YEB liquid medium containing suitable antibiotics (50 μg/ml of kanamycin, 50 μg/ml of ampicillin) and cultivated by shaking at 28° C. and 240 rpm for 1 day. 5 ml bacteria liquor thus obtained was added in 200 ml YEB liquid medium and cultivated at 28° C. and 240 rpm for 9 hours. The culture suspension was centrifuged at 4° C. and 4,200 rpm for 20 minutes (Beckman J2-MC, JA-10 rotor). The supernatant was discarded, and the pellet was suspended in 20 ml pre-cooled YEB medium. The resulted suspension was centrifuged again at 4° C. and 4,200 rpm for 20 minutes. The pellet was re-suspended in 20 ml pre-cooled YEB medium and was stored at 4° C. till used.  Agrobacterium tumefaciens  transformation was performed by employing frozen-thaw method. 500 μl suspension of  Agrobacterium tumefaciens  to be transformed was well mixed with 1 μg pMhUBQ1p-GUS plasmid DNA prepared in Example 2, and the mixture was treated successively on ice, in liquid nitrogen and at 37° C., each for 5 minutes. The bacteria liquor was then mixed with 1 ml YEB medium and cultivated by shaking at 28° C. and 240 rpm for 3˜4 hours. The bacterial liquor was applied over medium containing suitable antibiotics (50 μg/ml of kanamycin, 100 μg/ml rifamycin, and 20 μg/ml streptomycin), and cultivated at 28° C. for 2 days. 
       Agrobacterium tumefaciens  that had been transformed to contain plasmid pMhUBQ1p-GUS prepared in example 2 was used to inoculate single colony of the above-described  Agrobacterium tumefaciens  on 5 ml YEB medium (0.5% beef extract, 0.1% yeast extract, 0.5% peptone, 0.5% mannitol, 0.05% MgSO 4 , pH 7.5) containing suitable antibiotics (50 μg/ml kanamycin, 100 μg/ml rifamycin, and 20 μg/ml streptomycin) and cultivated by shaking at 28° C. and 240 rpm for 2 days. Then, it was poured in 250 ml YEB medium containing suitable antibiotics (50 μg/ml kanamycin, 100 μg/ml rifamycin, 20 μg/ml streptomycin), and cultivated again by shaking at 28° C. and 240 rpm for more than 24 hours. It was then centrifuged at 4° C. and 6,000 rpm for 10 minutes. The supernatant was discarded, and the pellet was suspended in 200 ml infiltration medium (½ MS, 5% sucrose, 0.044 μM ABA, 0.01% Silwet L-77, pH 5.7).  Arabidopsis thialana  plants to be transformed were placed upside down in the  Agrobacterium tumefaciens  suspension, and soaked there for 20 seconds.  Arabidopsis thialana  plants were taken off and kept wet for 24 hours. Seeds could be harvested after about 3˜4 weeks. 
     3. Sowing and Selection of Transformant 
     The transformed  Arabidopsis thialana  seeds thus-collected was rinsed several times with sterile water, treated with 70% ethanol for 2 minutes, treated with sterile water containing 1% Clorox and 0.1% Tween-20 for 20 minutes, and then rinsed 4-5 times with sterile water for 5 minutes each time. Thereafter, these seeds thus-treated were sown in germinating medium (½MS, 1% sucrose, 0.7% agar, 50 μg/ml of kanamycin, 50 μg/ml of ampicillin) to carry out segregation assay of anti-antibiotic progeny. Homozygote transformant progeny thus obtained could be used in assay of promoter activity. 
     4. GUS Histochemical Staining 
     The procedure described in Example 3 was repeated. 
       FIG. 4  shows the result of GUS activity analysis. As shown in  FIG. 4 , reporter gene GUS activated by banana polyubiquitin gene MhUBQ1 promoter could be expressed in every tissue of  Arabidopsis thialana , including root, stem, leaf, pod and pollinia (as shown in  FIG. 4 ); wherein,  FIG. 4A : GUS histochemical staining results of  Arabidopsis thialana  transformant whole plants grown for different number of days;  FIG. 4B : GUS histochemical staining results of  Arabidopsis thialana  transformant flower organ at different developmental stages, where non-transformed flower organs at each stage (stages 1-4) were used as the control groups;  FIG. 4C : GUS histochemical staining results of siliques of  Arabidopsis thialana  transformant at different developmental stages, where non-transformed siliques at each stage (stage 1-4) were used as the control groups. From results of GUS activity analysis, it indicated that banana polyubiquitin gene MhUBQ1 promoter did have high expression strength, and could be over-expressed in various tissues of the transformant progeny. 
     Example 5 
     Transformation of  Nicotiana tabacum  L. via  Agrobacterium tumefaciens -Mediated Transformation Process 
     Separately,  Nicotiana tabacum  L. cv Wisc. 38 was used as the material, and similarly,  Agrobacterium tumefaciens -mediated transformation was employed to transform plasmid pMhUBQ1p-GUS prepared in Example 2 into  Nicotiana tabacum  L. to alter genomic constitution in the transgenic plant such that banana polyubiquitin gene MhUBQ1 promoter could activate effectively the expression of reporter gene GUS at objective transgenic  Nicotiana tabacum  L. plant and progeny thereof. Furthermore, GUS histochemical staining was used to analyze expression patterns of reporter gene GUS in  Nicotiana tabacum  L. transformant to detect whether banana polyubiquitin gene MhUBQ1 promoter exhibited likewise activation ability with high strength. 
     1. Preparation of  Agrobacterium tumefaciens  Liquor 
     The same procedure described in Example 4 was followed in this example. 
     2. Transformation of  Agrobacterium tumefaciens    
     The same procedure described in Example 4 was followed in this example. 
     3. Small Amount Preparation of Transformed  Agrobacterium tumefaciens  Plasmid 
     The same procedure described in Example 4 was followed in this example. 
     4. Transformation and Selection of  Nicotiana tabacum  L. 
     Leaves of  Nicotiana tabacum  L. cv Wisc. 38 plants sterile seeded were cut into square of 1.5 cm×1.5 cm in a bacteria liquor, placed on N01B1 solid medium (MS, adding 0.1 mg/L of 1-naphthyl acetic acid, 1 mg/L of BA, 3% sucrose, pH 5.7, 0.7% agar) and cultivated at 25° C., 16-hour lighting environment for 3 days. Then, the square leaves were rinsed by dipping in N01B1 liquid medium containing 250 mg/L cefotaxime for 1 minute. Next, they were placed on N01B1 solid medium containing 250 mg/L cefotaxime and 100 mg/L kanamycin, and selected at 25° C., 16-hour lighting environment for 3 weeks. Thereafter, those square leaves were soaked and washed in 20 mL N01B1 liquid medium containing 250 mg/L of cefotaxime for 1 minute. Subsequently, they were transferred on N01B1 solid medium containing 250 mg/L of cefotaxime and 100 mg/L of kanamycin, and were selected at 25° C., 16-hour lighting environment for about 3 weeks. Upon germination of adventitious buds from square leaves, those leaves were moved onto N01B1 solid medium containing 250 mg/l of cefotaxime and 200 mg/l of kanamycin. Selection was carried out at 25° C., 16-hour lighting environment. As shoots had grown to longer than 1 cm, shoots without etiolation could be cut and cottage cultivated in MS solid medium containing 250 mg/L of cefotaxime and 200 mg/L of kanamycin at 25° C. and 16-hour lighting environment till rooting. The plants were used in GUS activity assay. 
     5. GUS Histochemical Staining 
     The  Nicotiana tabacum  L. transformant survived in the above selection was subjected to GUS histochemical staining analysis followed the procedure described in example 4. 
     Results of GUS activity analysis were shown in  FIG. 5 ; wherein  FIG. 5A : GUS histochemical staining results of  Nicotiana tabacum  L. transformant whole plants grown for different number of days, and non-transformed flower organs at each stage (stages 1-5) were used as control groups. Here, as shown, reporter gene GUS activated with banana polyubiquitin gene MhUBQ1 promoter could be expressed likewise at all sites of the  Nicotiana tabacum  L. transformant. Accordingly, double analyses of GUS activity in  Arabidopsis thialana  and  Nicotiana tabacum  L. transformants revealed that the inventive banana polyubiquitin gene MhUBQ1 promoter did exhibit significant high expression strength in different spices, as well as could be over-expressed in various tissues of the transgenic plant and progeny thereof. 
     The promoter that has high expression strength and can be over-expressed in various tissues of a plant as well as its application provided according to the invention has following advantages over other conventional techniques: 
     1. The inventive promoter can activate the expression of the gene behind its 3′terminal in all tissues of a plant, thereby the high expression strength of said promoter makes possible the over-expression of a target gene in an objective plant so as to increase the product of said target gene. 
     2. The inventive promoter can be transferred as a vector into a plant, and either a monocotyledon or dicotyledon plants, it exhibits strong activation ability. In a dicotyledon plant, it can be expressed in all sites and tissues, while in monocotyledon plant, its activation ability is higher than that of conventional CaMV 35S promoter; consequently, a common problem as insufficient expression of a transferred gene in a monocotyledon plant can be thus overcome. 
     While the detailed description provided above is directed to a possible embodiment of invention, it should be understood that said embodiment is not construed to limit the scope of the invention as defined in the appended claims, and those embodiments or alteration that can be made without departing from the spirit and scope of the invention are intended to fall within the scope of the appended claims. 
     Accordingly, the invention has indeed not only an innovation on the species gene, but also has particularly an expression uniqueness, and therefore, the application should meet sufficiently requirements of patentability on novelty and non-obviousness, and should deserve an invention patent right. 
     Many changes and modifications in the above described embodiment of the invention can, of course, be carried out without departing from the scope thereof. Accordingly, to promote the progress in science and the useful arts, the invention is disclosed and is intended to be limited only by the scope of the appended claims.