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21.发明申请公开(公告)号:US20100113566A1
公开(公告)日:2010-05-06
申请号:US12064185
申请日:2006-08-10
申请人: Hideto Chono , Kazuya Matsumoto , Junichi Mineno , Ikunoshin Kato
发明人: Hideto Chono , Kazuya Matsumoto , Junichi Mineno , Ikunoshin Kato
IPC分类号: A61K31/7088 , C07H21/00 , C12N15/74 , C12N5/0783 , A61P31/18
CPC分类号: C12N15/86 , A61K31/7088 , A61K35/17 , A61K38/00 , A61K38/465 , A61K48/00 , C07K14/4702 , C12N5/0636 , C12N9/22 , C12N15/85 , C12N2510/00 , C12N2830/002 , Y02A50/473
摘要: A nucleic acid comprising a transcription regulation sequence whose transcription is induced by a trans-acting factor of a human immunodeficiency virus and a gene encoding a polypeptide having an endoribonuclease activity specific to single-stranded RNA, wherein the gene is located in such a position that the expression of the gene can be regulated by the transcription regulation sequence; a method for production of a cell showing an inhibited replication of a human immunodeficiency virus therein, the method comprising the step of introducing the nucleic acid into a cell; and a method for treatment or prevention of a human immunodeficiency virus infection.
摘要翻译: 一种核酸,其包含其转录由人免疫缺陷病毒的反式作用因子诱导的转录调控序列和编码具有对单链RNA特异性的内切核糖核酸酶活性的多肽的基因,其中所述基因位于 该基因的表达可以通过转录调控序列来调节; 一种在其中显示抑制人体免疫缺陷病毒复制的细胞的制备方法,所述方法包括将核酸引入细胞的步骤; 以及用于治疗或预防人类免疫缺陷病毒感染的方法。
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22.发明授权Thermostable ribonuclease H obtained from Archeoglobus profundus 有权从Archeoglobus profundus获得的热稳定性核糖核酸酶H公开(公告)号:US07572617B2
公开(公告)日:2009-08-11
申请号:US10526073
申请日:2003-08-26
CPC分类号: C12N9/22
摘要: An isolated polypeptide having a thermostable ribonuclease H activity from Archaeoglobus profundus is highly useful in genetic engineering, as well as a gene encoding this polypeptide and a genetic engineering process for producing the polypeptide.
摘要翻译: 具有来自古细丝虫的热稳定核糖核酸酶H活性的分离的多肽在遗传工程中是非常有用的,以及编码该多肽的基因和用于产生多肽的基因工程方法。
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公开(公告)号:US07491405B2
公开(公告)日:2009-02-17
申请号:US11116371
申请日:2005-04-28
申请人: Kazutoh Takesako , Takashi Okada , Tomoko Yagihara , Masanobu Kuroda , Yoshimi Onishi , Ikunoshin Kato , Kazuo Akiyama , Hiroshi Yasueda , Hideyo Yamaguchi
发明人: Kazutoh Takesako , Takashi Okada , Tomoko Yagihara , Masanobu Kuroda , Yoshimi Onishi , Ikunoshin Kato , Kazuo Akiyama , Hiroshi Yasueda , Hideyo Yamaguchi
CPC分类号: A61K39/0002 , A61K38/00 , A61K39/00 , C07K14/37 , C07K16/14 , Y10S530/858
摘要: A substantially pure, isolated, antigenic protein from fungi of the genus Malassezia, characterized in that said antigenic protein has a binding ability to IgE antibodies from patients with allergoses; an antigenic fragment derived from the antigenic protein; and an antibody against the antigenic protein or fragments thereof. According to the present invention, there can be provided an isolated and purified antigenic protein having high purity from Malassezia, antigenic fragments thereof, and a specific antibody against those antigenic protein or fragments thereof. In addition, there can be provided a diagnostic agent, a therapeutic agent, or a prophylactic drug for Malassezia allergoses, wherein the agent includes, as an active ingredient, the antigenic protein or fragments thereof.
摘要翻译: 从马拉色氏菌属真菌的基本上纯的,分离的抗原性蛋白质,其特征在于所述抗原蛋白质具有与过敏原患者的IgE抗体的结合能力; 衍生自抗原蛋白的抗原片段; 和针对抗原蛋白或其片段的抗体。 根据本发明,可以提供从马拉色霉属,其抗原性片段和针对那些抗原性蛋白质或其片段的特异性抗体具有高纯度的分离和纯化的抗原性蛋白质。 此外,可以提供用于马拉色氏菌过敏原的诊断剂,治疗剂或预防药物,其中所述药剂包含抗原蛋白或其片段作为活性成分。
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公开(公告)号:US07485448B2
公开(公告)日:2009-02-03
申请号:US11519775
申请日:2006-09-13
申请人: Hirofumi Yoshioka , Yasushi Katayama , Daisuke Tomura , Masao Funakoshi , Kazuya Matsumoto , Junichi Mineno , Kazutoh Takesako , Ikunoshin Kato
发明人: Hirofumi Yoshioka , Yasushi Katayama , Daisuke Tomura , Masao Funakoshi , Kazuya Matsumoto , Junichi Mineno , Kazutoh Takesako , Ikunoshin Kato
CPC分类号: C12N5/0037 , C12N2500/84 , C12N2510/02
摘要: A method for obtaining a virus vector free of a serum, and a serum-free medium for cultivation of a virus producer cell which can be used for the method are provided. By cultivating a virus producer cell using a serum-free medium containing serum albumin, it is possible to cultivate the cell in a state equivalent to that in a serum-containing medium to produce a virus vector at a sufficient titer. The virus vector prepared from the virus producer cell cultivated in the medium exhibits gene transfer efficiency comparable to that of a conventional vector. The medium is useful for gene therapy and studies thereof.
摘要翻译: 本发明提供了获得不含血清的病毒载体的方法和用于培养可用于该方法的病毒生产细胞的无血清培养基。 通过使用含有血清白蛋白的无血清培养基培养病毒生成细胞,可以以与含有血清的培养基相同的状态培养细胞以产生足够滴度的病毒载体。 从培养基中培养的病毒生产细胞制备的病毒载体表现出与常规载体相当的基因转移效率。 该培养基可用于基因治疗及其研究。
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25.发明申请公开(公告)号:US20080166325A1
公开(公告)日:2008-07-10
申请号:US11790025
申请日:2007-04-23
申请人: Hiroaki Sagawa , Mitsuko Ideno , Ikunoshin Kato
发明人: Hiroaki Sagawa , Mitsuko Ideno , Ikunoshin Kato
CPC分类号: C12N5/0636 , A61K39/0011 , A61K39/12 , A61K39/145 , A61K2039/5158 , A61K2039/55583 , C12N2501/515 , C12N2501/90 , C12N2760/16134
摘要: The present invention provides methods for inducing, maintaining and expanding CTL (cytotoxic T cell) having an antigen-specific cytotoxic activity at a high level, which is useful in the adoptive immunotherapy, by using as an effective ingredient at least one compound selected from the group consisting of acidic polysaccharides, acidic oligosaccharides, acidic monosaccharides, and salts thereof. The above-mentioned compounds include fucoidans, heparins, alginic acid, chondroitin sulfate A, chondroitin sulfate B, pectic acid, hyaluronic acid, degradation products of fucoidans, sulfated glucose, sulfated fucose and salts thereof.
摘要翻译: 本发明提供用于诱导,维持和扩增具有高水平的抗原特异性细胞毒性活性的CTL(细胞毒性T细胞)的方法,其可用于过继性免疫治疗,通过使用至少一种选自以下的化合物作为有效成分: 由酸性多糖,酸性寡糖,酸性单糖及其盐组成的组。 上述化合物包括岩藻多糖,肝素,海藻酸,硫酸软骨素A,硫酸软骨素B,果胶酸,透明质酸,岩藻多糖的降解产物,硫酸化葡萄糖,硫酸岩藻糖及其盐。
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公开(公告)号:US20070218524A1
公开(公告)日:2007-09-20
申请号:US10573381
申请日:2004-09-29
申请人: Jun Tomono , Harumi Ueno , Hiroaki Sagawa , Ikunoshin Kato
发明人: Jun Tomono , Harumi Ueno , Hiroaki Sagawa , Ikunoshin Kato
CPC分类号: C12N15/111 , C12N9/22 , C12N2310/14 , C12N2330/30 , C12Y301/26003
摘要: A polypeptide having an RNase III activity with which the length of a dsRNA degradation product can be easily controlled depending on reaction conditions and, in preparing a dsRNA having a length allowing it to serve as an siRNA in RNA interference, a low-molecular weight product having little RNA interferring effect is scarcely formed; a method of degrading a dsRNA with the use of the above polypeptide; and a composition and a kit for the above method.
摘要翻译: 可以根据反应条件容易地控制dsRNA降解产物的长度的具有RNase III活性的多肽,并且在制备具有允许其在RNA干扰中作为siRNA的长度的dsRNA时,低分子量产物 几乎没有形成RNA干扰效果; 使用上述多肽降解dsRNA的方法; 以及用于上述方法的组合物和试剂盒。
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公开(公告)号:US20070105113A1
公开(公告)日:2007-05-10
申请号:US10567731
申请日:2004-08-10
申请人: Hiroaki Sagawa , Jun Tomono , Harumi Ueno , Ikunoshin Kato
发明人: Hiroaki Sagawa , Jun Tomono , Harumi Ueno , Ikunoshin Kato
摘要: A protein having an activity of degrading a dsRNA, namely, being capable of acting on a long-chain dsRNA to form a dsRNA of a definite length; a method of efficiently preparing a dsRNA of a definite length which comprises treating a dsRNA with the protein having an activity of degrading a dsRNA in the coexistence of a protein having an activity of binding to a nucleic acid such as a protein having an RNA-binding activity; and a method of using the protein having an activity of binding to a nucleic acid to elevate the efficiency in an RNA synthesis reaction typified by dsRNA synthesis.
摘要翻译: 具有降解dsRNA活性的蛋白质,即能够作用于长链dsRNA以形成一定长度的dsRNA; 一种有效制备一定长度的dsRNA的方法,该方法包括在具有与核酸如具有RNA结合性的蛋白质结合的蛋白质共存的蛋白质共同存在下具有降解dsRNA活性的蛋白质对dsRNA进行处理 活动; 以及使用具有与核酸结合的活性的蛋白质以提高以dsRNA合成为代表的RNA合成反应中的效率的方法。
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公开(公告)号:US20070065854A1
公开(公告)日:2007-03-22
申请号:US11519775
申请日:2006-09-13
申请人: Hirofumi Yoshioka , Yasushi Katayama , Daisuke Tomura , Masao Funakoshi , Kazuya Matsumoto , Junichi Mineno , Kazutoh Takesako , Ikunoshin Kato
发明人: Hirofumi Yoshioka , Yasushi Katayama , Daisuke Tomura , Masao Funakoshi , Kazuya Matsumoto , Junichi Mineno , Kazutoh Takesako , Ikunoshin Kato
CPC分类号: C12N5/0037 , C12N2500/84 , C12N2510/02
摘要: A method for obtaining a virus vector free of a serum, and a serum-free medium for cultivation of a virus producer cell which can be used for the method are provided. By cultivating a virus producer cell using a serum-free medium containing serum albumin, it is possible to cultivate the cell in a state equivalent to that in a serum-containing medium to produce a virus vector at a sufficient titer. The virus vector prepared from the virus producer cell cultivated in the medium exhibits gene. transfer efficiency comparable to that of a conventional vector. The medium is useful for gene therapy and studies thereof.
摘要翻译: 本发明提供了获得不含血清的病毒载体的方法和用于培养可用于该方法的病毒生产细胞的无血清培养基。 通过使用含有血清白蛋白的无血清培养基培养病毒生成细胞,可以以与含有血清的培养基相同的状态培养细胞以产生足够滴度的病毒载体。 从培养基中培养的病毒生产细胞制备的病毒载体表现出基因。 转移效率与常规载体相当。 该培养基可用于基因治疗及其研究。
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公开(公告)号:US20060269999A1
公开(公告)日:2006-11-30
申请号:US11500480
申请日:2006-08-08
IPC分类号: C12P21/06 , C07K14/195 , C12N15/74 , C07H21/04 , C12N1/21
CPC分类号: C07K14/195
摘要: Isolated DNAs which are DNAs having a base sequence represented by any of SEQ ID NOS:1 to 6 in Sequence Listing or fragments thereof and showing a stationary phase-specific promoter activity in gram positive bacteria.
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公开(公告)号:US07135291B2
公开(公告)日:2006-11-14
申请号:US10468128
申请日:2002-02-14
申请人: Hiroaki Sagawa , Eiji Kobayashi , Ikunoshin Kato
发明人: Hiroaki Sagawa , Eiji Kobayashi , Ikunoshin Kato
CPC分类号: C12Q1/683 , C12Q2521/101
摘要: A Nucleotide useful for detecting a base substitution in a gene, a method for detecting a base substitution in a gene using said Nucleotide, and a kit for the same.
摘要翻译: 用于检测基因中碱基取代的核苷酸,使用所述核苷酸检测基因中的碱基取代的方法及其用途。
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