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1. 发明授权

US5654190A Process for producing plant belonging to the section leuce 失效
标题翻译：生产属于断面的植物的过程
公开(公告)号：US5654190A
公开(公告)日：1997-08-05
申请号：US443161
申请日：1995-05-17
申请人： Etsuko Matsunaga , Ayako Todate , Hiroyasu Ebinuma
发明人： Etsuko Matsunaga , Ayako Todate , Hiroyasu Ebinuma
IPC分类号： A01H4/00 , C12N5/04 , C12N5/00
CPC分类号： C12N5/04 , A01H4/001
摘要： A process for producing a plant is described, which comprises the step of culturing a tissue of a plant belonging to the genus Populus, the section Leuce, thereby regenerating the plant via an adventitious bud, wherein the adventitious bud is differentiated from the cultured tissue using an adventitious bud differentiation medium having nitrogen source concentrations of from 1 to 15 mM as ammonia-nitrogen and from 15 to 50 mM as nitrate-nitrogen.
摘要翻译：描述了一种用于生产植物的方法，其包括培育属于杨属的植物的组织，Leuce部分的步骤，从而通过不定芽再生植物，其中不定芽与培养的组织分化，使用具有氮源浓度为1至15mM的氮源和15至50mM作为硝酸盐 - 氮的不定芽分化培养基。

2. 发明授权

US06326192B1 Vector for gene transfer into plant allowing optional deletion of marker gene 失效
标题翻译：用于基因转移到植物中的载体，允许标记基因的任选缺失
公开(公告)号：US06326192B1
公开(公告)日：2001-12-04
申请号：US09147241
申请日：1998-11-09
申请人： Koichi Sugita , Mikiko Uesugi , Etsuko Matsunaga , Hiroyasu Ebinuma
发明人： Koichi Sugita , Mikiko Uesugi , Etsuko Matsunaga , Hiroyasu Ebinuma
IPC分类号： C12N1582
CPC分类号： C12N15/8205 , C12N15/8201 , C12N15/8209 , C12N15/8213 , C12N15/8242
摘要： The present invention relates to a vector for introducing a desired gene into a plant, wherein a selectable marker gene introduced into a plant cell along with a desired gene is optionally removable from the DNA such as chromosome or the like where it exists and functions, then disappeared the function thereof after its expression, and the expression of the selectable marker gene and the disappearance of the function thereof are detectable by morphological change of the tissue derived from the plant cell into which the selectable marker gene is introduced. Also, the present invention constitutes a vector using a morphological abnormality induction gene as a selectable marker gene, while putting a removable DNA element under control of an inducible promoter, wherein the morphological abnormality induction gene is positioned such that it behaves integrally with the removable DNA element, and wherein a desired gene is positioned such that it does not behave integrally with the removable DNA element.
摘要翻译：本发明涉及用于将期望的基因导入植物中的载体，其中与所需基因一起导入植物细胞的选择性标记基因可任选地从其存在并起作用的染色体等DNA脱除，然后其表达后的功能消失，并且可选择标记基因的表达及其功能的消失可以通过导入选择性标记基因的植物细胞衍生的组织的形态学变化来检测。此外，本发明构成使用形态异常诱导基因作为选择性标记基因的载体，同时将可移除的DNA元件置于诱导型启动子的控制下，其中形态异常诱导基因定位成使其与可除去的DNA整体地起作用元件，并且其中将期望的基因定位成使得其不与可移除的DNA元件整体表现。

3. 发明授权

US5965791A Vector for introducing a gene into a plant, and methods for producing transgenic plants and multitudinously introducing genes into a plant using the vector 失效
标题翻译：用于将基因导入植物的载体，以及使用载体生产转基因植物并将基因大量引入植物的方法
公开(公告)号：US5965791A
公开(公告)日：1999-10-12
申请号：US555760
申请日：1995-11-09
申请人： Hiroyasu Ebinuma , Koichi Sugita , Etsuko Matsunaga , Mikiko Yamakado
发明人： Hiroyasu Ebinuma , Koichi Sugita , Etsuko Matsunaga , Mikiko Yamakado
IPC分类号： A01H1/00 , A01H5/00 , C07H21/04 , C12N1/21 , C12N5/00 , C12N5/10 , C12N15/09 , C12N15/29 , C12N15/52 , C12N15/82 , C12R1/01 , C12R1/91 , A01H4/00
CPC分类号： C12N15/821 , C12N15/8201 , C12N15/8209 , C12N15/8213 , C12N15/8242
摘要： A vector for introducing a desired gene into a planet, which comprises the desired gene and at least one morphological abnormally induction (MAI) gene as a marker gene, or which comprises the desired gene, at least one MAI gene and a removable element. A method for producing a transgenic plant free from the influence of a marker gene. A method for multitudinously introducing desired genes into one plant.
摘要翻译：用于将期望的基因引入行星的载体，其包含所需基因和至少一种形态异常诱导（MAI）基因作为标记基因，或包含所需基因，至少一种MAI基因和可移除元件。一种不受标记基因影响的转基因植物的制备方法。将所需基因大量引入一种植物的方法。

4. 发明授权

US07294761B2 Method for efficiently producing transgenic plant using auxin precursor 失效
标题翻译：使用生长素前体有效生产转基因植物的方法
公开(公告)号：US07294761B2
公开(公告)日：2007-11-13
申请号：US10626609
申请日：2003-07-25
申请人： Etsuko Matsunaga , Koichi Sugita , Hiroyasu Ebinuma
发明人： Etsuko Matsunaga , Koichi Sugita , Hiroyasu Ebinuma
IPC分类号： C12N15/82 , C12N15/83 , C12N15/84 , C12N15/31 , C12N15/54 , C12N15/55
CPC分类号： C12N15/821
摘要： A method for producing a transgenic plant, which comprises: (A) introducing a vector into a plant cell, wherein the vector is a vector for gene introduction into a plant and comprises: a desired gene, and a selectable marker gene comprising a gene encoding an enzyme which synthesizes auxin from an auxin precursor; (B) culturing the plant cell into which the genes are introduced by the vector, in the presence of an auxin precursor and/or an analogue thereof to thereby prepare a redifferentiated tissue, and detecting and selecting the redifferentiated tissues; and (C) culturing the redifferentiated tissue selected in (B) to redifferentiate a plant individual, and a vector for gene introduction into a plant, which comprises: a desired gene, and a selectable marker gene comprising an indoleacetamide hydrolase, iaaH, gene and an isopentenyl transferase, ipt, gene and being free of an tryptophan monooxygenase, iaaM, gene.
摘要翻译：一种生产转基因植物的方法，其包括：（A）将载体导入植物细胞，其中所述载体是用于将基因导入植物的载体，并且包含：所需基因和选择标记基因，所述选择标记基因包含编码从生长素前体合成生长素的酶; （B）在生长素前体和/或其类似物的存在下培养载体引入基因的植物细胞，由此制备再分化组织，并检测并选择再分化组织; （C）培养在（B）中选择的再分化组织以重新分化植物个体和将基因导入植物的载体，其包含：所需基因和包含吲哚乙酰胺水解酶，iaaH基因和异戊烯基转移酶，ipt，基因，并且不含色氨酸单加氧酶，iaaM基因。

5. 发明授权

US06294714B1 Method for introducing a gene into a plant using an adventitious bud redifferentiation gene under the control of a light-inducible promoter as a selectable marker gene, and vector for introducing a gene into a plant using the same 失效
标题翻译：使用在光诱导型启动子作为选择性标记基因的控制下的不定芽再分化基因将基因引入植物的方法，以及使用其将基因导入植物的载体
公开(公告)号：US06294714B1
公开(公告)日：2001-09-25
申请号：US09354305
申请日：1999-07-16
申请人： Etsuko Matsunaga , Takehide Kasahara , Koichi Sugita , Hiroyasu Ebinuma
发明人： Etsuko Matsunaga , Takehide Kasahara , Koichi Sugita , Hiroyasu Ebinuma
IPC分类号： C12N504
CPC分类号： A01H4/005 , C12N15/8205 , C12N15/8209
摘要： A method for introducing a gene into a plant, which comprises introducing a gene into a plant cell using a vector containing an adventitious shoot redifferentiation gene as a selectable marker gene under the control of a light-inducible promoter, and a vector for introducing a gene into a plant, which comprises a desired gene, an adventitious shoot redifferentiation gene as a selectable marker gene under the control of a light-inducible promoter, and a removable DNA element, wherein the selectable marker gene is positioned such that it behaves integrally with the removable DNA element, and wherein the desired gene is positioned such that it does not behave integrally with the removable DNA element.
摘要翻译：将基因导入植物的方法，其特征在于，在光诱导型启动子的控制下，使用含有不定芽再分化基因的载体作为选择性标记基因，将基因引入植物细胞，以及用于引入基因的载体包含所需基因的植物，作为在光诱导型启动子控制下的选择性标记基因的不定芽再分化基因和可除去的DNA元件，其中所述选择标记基因定位成使其与可去除的DNA元件，并且其中所需基因定位成使其不与可移除的DNA元件整体地表现。

6. 发明申请

US20090320164A1 METHOD FOR PRODUCTION OF PLANT CELL HAVING CHROMOSOME LOSS 审中-公开
标题翻译：用于生产染色体损失的植物细胞的方法
公开(公告)号：US20090320164A1
公开(公告)日：2009-12-24
申请号：US11721273
申请日：2005-12-08
申请人： Kazuya Nanto , Hiroyasu Ebinuma
发明人： Kazuya Nanto , Hiroyasu Ebinuma
IPC分类号： A01H5/00 , C12N15/82 , C12N5/10
CPC分类号： C12N15/8213 , C12N15/82
摘要： The present invention provides a simple aneuploid production process, applicable to all species, without producing unexpected damage to chromosomes other than a chromosome which is to be disappeared. A vector comprising two site-specific recognition sequences oriented in the opposite direction, or one site-specific recombinase recognition sequence comprising a point-symmetric nucleotide sequence, and a recombinase gene is introduced into a plant cells or a vector comprising two site-specific recognition sequences oriented in the opposite directions or one site-specific recombinase recognition sequence comprising a point-symmetric nucleotide sequence is introduced into a plant cell; a recombinase is allowed to act transiently in the cell during at least growth of the cell; and the cell is cultured and grown; and a cell in which a predetermined chromosome is disappeared is selected.
摘要翻译：本发明提供了一种适用于所有物种的简单的非整倍体生产方法，而不会对将要消失的染色体以外的染色体产生意外的损害。将包含相反方向取向的两个位点特异性识别序列或包含点对称核苷酸序列的一个位点特异性重组酶识别序列和重组酶基因的载体导入植物细胞或包含两个位点特异性识别的载体将指向相反方向的序列或包含点对称核苷酸序列的一个位点特异性重组酶识别序列引入植物细胞中; 允许重组酶在细胞的至少生长期间暂时在细胞中起作用; 并培养和培养细胞; 并且选择其中预定染色体消失的细胞。

7. 发明申请

US20070169224A1 Novel vector and method of constructing transformant plant using the vector 审中-公开
标题翻译：使用载体构建转化体植物的新型载体和方法
公开(公告)号：US20070169224A1
公开(公告)日：2007-07-19
申请号：US10552146
申请日：2004-04-07
申请人： Akiyoshi Kawaoka , Kazuya Nanto , Hiroyasu Ebinuma
发明人： Akiyoshi Kawaoka , Kazuya Nanto , Hiroyasu Ebinuma
IPC分类号： A01H1/00 , C12N15/82
CPC分类号： C12N15/8216
摘要： Gene introduction to a plant is carried out by using a vector which comprises the following constitutional units A and B: A: a DNA sequence comprising P1, an expression inhibitory sequence and a desired gene which is controlled by P1 and the expression inhibitory sequence; B: a DNA sequence comprising P2, an expression inhibitory gene which is controlled by P2, P3, the expression inhibitory sequence, and a gene of a removal reaction-catalyzing enzyme which is controlled by P3 and the expression inhibitory sequence, wherein the DNA sequence is removed by expression of the gene of a removal reaction-catalyzing enzyme, wherein P1 is a promoter which shows its activity in at least a callus and a plant tissue where a desired gene should be expressed, P2 is a promoter which shows its activity in at least a callus, and P3 is a promoter which shows its activity in at least a plant tissue where P1 and P2 do not show their activities.
摘要翻译：通过使用包含以下结构单元A和B的载体进行植物的基因导入：A：包含P1，表达抑制性序列和由P1控制的所需基因的DNA序列和表达抑制性序列; B：包含P2，由P2，P3控制的表达抑制基因，表达抑制性序列和由P3控制的去除反应催化酶的基因和表达抑制性序列的DNA序列，其中所述DNA序列通过去除反应催化酶的基因的表达除去，其中P1是至少在愈伤组织中显示其活性的启动子和其中应该表达所需基因的植物组织，P2是显示其活性的启动子至少一个愈伤组织，P3是在P1和P2不显示其活性的至少一种植物组织中显示其活性的启动子。

8. 发明申请

US20110203016A1 PROCESS FOR PRODUCING PLANT STORAGE ORGAN WITH HIGH PRODUCTION OF RECOMBINANT PROTEIN AND NOVEL RECOMBINANT PROTEIN 审中-公开
标题翻译：生产重组蛋白和新型重组蛋白的植物储存制剂的生产工艺
公开(公告)号：US20110203016A1
公开(公告)日：2011-08-18
申请号：US12765711
申请日：2010-04-22
申请人： Koichi SUGITA , Saori Kasahara , Hiroyasu Ebinuma , Fumio Takaiwa
发明人： Koichi SUGITA , Saori Kasahara , Hiroyasu Ebinuma , Fumio Takaiwa
IPC分类号： A01H1/00 , A01H5/00 , C12N15/63
CPC分类号： C12N15/8257 , C07K14/605 , C12N15/8216
摘要： The present invention provides a method for highly producing a recombinant protein in a plant storage organ and a GLP-1 derivative. The plant storage organ in which the recombinant protein is highly produced is obtained by transformation with the use of a vector which comprises a recombinant protein gene, a cytokinin-related gene, a drug-resistant gene and a removable DNA element, in which the cytokinin-related gene and the drug-resistant gene exist in the positions so that they can behave together with the DNA element, while the recombinant protein to be expressed in the plant storage organ exists in the position so that it would not behave together with the DNA element. The GLP-1 is produced by using the method, and a derivative having been stabilized against enzymatic digestion is further provided.
摘要翻译：本发明提供了在植物贮藏器官和GLP-1衍生物中高度产生重组蛋白的方法。通过使用包含重组蛋白基因，细胞分裂素相关基因，耐药性基因和可移除DNA元件的载体转化获得重组蛋白质高度产生的植物贮藏器官，其中细胞分裂素相关基因和耐药基因存在于可以与DNA元件一起表现的位置，而在植物储存器官中表达的重组蛋白存在于与DNA不一致的位置元件。通过使用该方法制备GLP-1，进一步提供了稳定的酶促消化的衍生物。

9. 发明申请

US20080292732A1 Plant and Plant Storage Organ Having Glp-1 Derivative Accumulated Therein and Method of Producing the Same 失效
标题翻译：含有Glp-1衍生物的植物和植物储存器官及其生产方法
公开(公告)号：US20080292732A1
公开(公告)日：2008-11-27
申请号：US11662650
申请日：2004-09-14
申请人： Koichi Sugita , Saori Kasahara , Hiroyasu Ebinuma , Fumio Takaiwa , Hiroshi Yasuda , Takahito Jomori , Yuji Hayashi , Akira Tashita
发明人： Koichi Sugita , Saori Kasahara , Hiroyasu Ebinuma , Fumio Takaiwa , Hiroshi Yasuda , Takahito Jomori , Yuji Hayashi , Akira Tashita
IPC分类号： A61K36/00 , C12N15/82 , A01H5/00 , A61P31/10
CPC分类号： A61K38/26 , A23L33/105 , C12N15/8257
摘要： The present invention is to provide a plant and a plant storage organ thereof in which GLP-1 derivatives are accumulated, and a method of producing them in order to develop a method for ingesting orally GLP-1 derivatives at a low cost and to make use of it in diabetic treatment. A transgenic plant or a plant storage organ thereof in which GLP-1 derivatives are accumulated cleavable with a digestive enzyme is produced by a method comprising: integrating into a vector a linked GLP-1s-DNA which comprises tandem repeated “n” DNAs (“n” being an integer of 3 or more) encoding a GLP-1 derivative consisting of GLP-1 (7-36) or of an amino acid sequence of GLP-1 (7-36) in which one or a few amino acids are deleted, substituted and/or added, and C-terminal consists of Arg or Lys, and having GLP-1 activity; introducing the vector into a plant cell; and redifferentiating the obtained transformant. The transgenic plant and the plant storage organ are useful as a pharmaceutical composition or a food or drink for treating or preventing diabetes.
摘要翻译：本发明提供一种其中积聚有GLP-1衍生物的植物和植物贮藏器官及其生产方法，以便开发低成本摄取口服GLP-1衍生物的方法并使用的糖尿病治疗。 GLP-1衍生物可以用消化酶积聚可切割的转基因植物或植物贮藏器官是通过以下方法产生的：将连接的GLP-1s-DNA整合到载体中，所述连接的GLP-1s-DNA包含串联重复的“n”DNA（“ 编号由GLP-1（7-36）或GLP-1（7-36）的氨基酸序列组成的GLP-1衍生物的n“为3以上的整数，其中一个或几个氨基酸为缺失，取代和/或添加，C-末端由Arg或Lys组成，具有GLP-1活性; 将载体导入植物细胞; 并对所得转化体进行重新分化。转基因植物和植物贮藏器官可用作药物组合物或用于治疗或预防糖尿病的食物或饮料。

10. 发明申请

US20070277264A1 Novel Vector 审中-公开
标题翻译：小说矢量
公开(公告)号：US20070277264A1
公开(公告)日：2007-11-29
申请号：US10559072
申请日：2004-06-03
申请人： Kazuya Nanto , Keiko Watanabe , Hiroyasu Ebinuma
发明人： Kazuya Nanto , Keiko Watanabe , Hiroyasu Ebinuma
IPC分类号： A01H5/00 , C12N15/82
CPC分类号： C12N15/8213 , C12N15/8209 , C12N15/821
摘要： In order to provide a vector and a method for introducing one copy of a desired gene to a predetermined position of a host DNA at a high frequency without any bad influences upon the host cell and a vector and a method for deleting or inverting a host DNA at a predetermined position without a crossing step and without any bad influences upon the host cell. A vector which has an introduction cassette inserted between two site-specific recombinase recognition sequences and a site-specific recombinase gene which recognizes these site-specific recombinase recognition sequences, wherein the recombinase gene is positioned outside the introduction cassette, is used, and this is introduced into a host cell having a DNA in which one or two site-specific recombinase recognition sequences are present. A recombinant of interest can be efficiently obtained by positioning a lethal induction gene or a morphological abnormality induction gene outside the introduction cassette, together with the site-specific recombinase gene.
摘要翻译：为了提供一种将所需基因的一个拷贝以高频率引入宿主DNA的预定位置的载体和方法，对宿主细胞和载体没有任何不良影响，以及用于删除或翻译宿主DNA的方法在没有交叉步骤的预定位置处，并且对宿主细胞没有任何不良影响。使用具有插入两个位点特异性重组酶识别序列之间的引物盒和识别这些位点特异性重组酶识别序列的位点特异性重组酶基因的载体，其中重组酶基因位于引入盒外部，这是引入具有其中存在一个或两个位点特异性重组酶识别序列的DNA的宿主细胞。通过将导入盒外的致死诱导基因或形态异常诱导基因与位点特异性重组酶基因一起定位，可以有效地获得感兴趣的重组体。

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