公开(公告)号：US07846703B2

公开(公告)日：2010-12-07

申请号：US11866148

申请日：2007-10-02

申请人： Eiji Kobayashi ,  Yuki Ueda ,  Yoshimi Sato ,  Takashi Uemori ,  Hiroyuki Mukai ,  Ikunoshin Kato

发明人： Eiji Kobayashi ,  Yuki Ueda ,  Yoshimi Sato ,  Takashi Uemori ,  Hiroyuki Mukai ,  Ikunoshin Kato

IPC分类号： C12N9/10 ,  C12N9/96 ,  C07K14/00 ,  C12Q1/66 ,  C12P19/34

CPC分类号： C12N9/1241

摘要： A polymerase activity is effectively enhanced by adding an anionic surfactant, in particular an anionic surfactant having a polyethoxyl group, to a reaction mixture containing a polymerase.

摘要翻译： 通过向含有聚合酶的反应混合物中加入阴离子表面活性剂，特别是具有聚乙氧基的阴离子表面活性剂，可有效提高聚合酶活性。

公开(公告)号：US06218150B1

公开(公告)日：2001-04-17

申请号：US09446504

申请日：1999-12-23

申请人： Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C12P1934

CPC分类号： C12N9/1252

摘要： The present invention relates to a thermostable DNA polymerase-associated factor capable of enhancing DNA synthesizing-activity of a DNA polymerase; a thermostable DNA polymerase-associated factor possessing an activity of binding to a DNA polymerase and a method for producing the same; a gene encoding the DNA polymerase-associated factor; a method of DNA synthesis by using a DNA polymerase in the presence of the DNA polymerase-associated factor; and a kit comprising the DNA polymerase-associated factor. According to the present invention, there can be provided in vitro DNA synthesis and a DNA amplification system which are more excellent than conventional techniques by utilizing the DNA polymerase-associated factor of the present invention.

公开(公告)号：US07521178B1

公开(公告)日：2009-04-21

申请号：US09673884

申请日：1999-04-21

申请人： Kiyozo Asada ,  Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroyuki Mukai ,  Ikunoshin Kato

发明人： Kiyozo Asada ,  Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroyuki Mukai ,  Ikunoshin Kato

IPC分类号： C12Q1/68 ,  C12P19/34 ,  C07H21/02

CPC分类号： C12P19/34 ,  C12N9/1252 ,  C12N9/96 ,  C12Q1/6806 ,  Y10S435/975 ,  C12Q2521/107

摘要： A DNA synthesis reaction-enhancer comprising at least one kind selected from the group consisting of acidic substances and cationic complexes; a DNA synthesis method in which during a DNA synthesis reaction a reaction is carried out in the presence of the above enhancer by using DNA polymerase; a DNA synthesis reaction composition comprising the above enhancer; a DNA synthesis reaction composition comprising two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity; a DNA synthesis method in which during a DNA synthesis reaction two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity are used; a kit for use in in vitro DNA synthesis, comprising two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity; and a kit for use in in vitro DNA synthesis, wherein the kit comprises the DNA synthesis reaction-enhancer and DNA polymerase. According to the present invention, DNA synthesis can be carried out at an efficiency more excellent as compared to conventional DNA synthesis reaction.

摘要翻译： 一种DNA合成反应增强剂，其包含选自酸性物质和阳离子配合物中的至少一种; DNA合成方法，其中在DNA合成反应中，通过使用DNA聚合酶在上述增强剂的存在下进行反应; 包含上述增强剂的DNA合成反应组合物; 包含两种或更多种各自具有3'→5'核酸外切酶活性的DNA聚合酶的DNA合成反应组合物; 一种DNA合成方法，其中在DNA合成反应中使用两种或更多种具有3'→5'核酸外切酶活性的DNA聚合酶; 用于体外DNA合成的试剂盒，其包含两种或更多种各自具有3'→5'核酸外切酶活性的DNA聚合酶; 和用于体外DNA合成的试剂盒，其中试剂盒包含DNA合成反应增强剂和DNA聚合酶。 根据本发明，与常规DNA合成反应相比，可以以更优异的效果进行DNA合成。

公开(公告)号：US06673578B1

公开(公告)日：2004-01-06

申请号：US09786684

申请日：2001-05-22

申请人： Takashi Uemori ,  Yoshimi Sato ,  Mariko Okawa ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroaki Sagawa ,  Michio Hagiya ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Takashi Uemori ,  Yoshimi Sato ,  Mariko Okawa ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroaki Sagawa ,  Michio Hagiya ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C12P1934

CPC分类号： C12N15/1003 ,  C12Q1/686 ,  C12Q2527/125

摘要： A DNA synthesis method with a shortened time period required for DNA synthesis by polymerase chain reaction (PCR), characterized in that a DNA polymerase is used in an amount effective for providing more than 10 ng of amplified DNA fragments of about 2 kb per 50 &mgr;l of a reaction mixture, when PCR is carried out under the following conditions (A) and (B): (A) reaction mixture: 50 &mgr;l volume of a reaction mixture comprising DNA polymerase, 1 ng of genomic DNA from Escherichia coli, and 10 pmol each of primers Eco-1 and Eco-2 (nucleotide sequences of the primers Eco-1 and Eco-2 being shown in SEQ ID NOs: 10 and 11 of Sequence Listing, respectively); and having a composition suitable for the DNA polymerase; and (B) reaction conditions: 35 cycles of PCR, wherein one cycle consists of 99° C., 1 second-66° C., 7 seconds; a kit for DNA synthesis usable for the DNA synthesis method; and an article of manufacture of a PCR agent. According to the present invention, the procedures in the genetic engineering studies and industries involved with PCR can be speeded up.

摘要翻译： 一种DNA合成方法，其通过聚合酶链式反应（PCR）进行DNA合成所需的时间缩短，其特征在于使用DNA聚合酶，其量有效提供超过10ng每50ul约2kb的扩增DNA片段 的反应混合物，当在以下条件（A）和（B）下进行PCR时：（A）反应混合物：将50体积的包含DNA聚合酶的反应混合物，1ng来自大肠杆菌的基因组DNA和10ng 各引物Eco-1和Eco-2（引物Eco-1和Eco-2的核苷酸序列分别示于序列表的SEQ ID NO：10和11中） 并具有适合于DNA聚合酶的组合物; 和（B）反应条件：35个循环的PCR，其中一个循环由99℃，1秒-66℃，7秒; 用于DNA合成方法的DNA合成试剂盒; 以及PCR试剂的制造。 根据本发明，可以加快基因工程研究和涉及PCR的行业的程序。

公开(公告)号：US20090098613A1

公开(公告)日：2009-04-16

申请号：US12285866

申请日：2008-10-15

申请人： Kiyozo Asada ,  Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroyuki Mukai ,  Ikunoshin Kato

发明人： Kiyozo Asada ,  Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Osamu Takeda ,  Hiroyuki Mukai ,  Ikunoshin Kato

IPC分类号： C12P19/34

CPC分类号： C12P19/34 ,  C12N9/1252 ,  C12N9/96 ,  C12Q1/6806 ,  Y10S435/975 ,  C12Q2521/107

摘要： A DNA synthesis reaction-enhancer comprising at least one kind selected from the group consisting of acidic substances and cationic complexes; a DNA synthesis method in which during a DNA synthesis reaction a reaction is carried out in the presence of the above enhancer by using DNA polymerase; a DNA synthesis reaction composition comprising the above enhancer; a DNA synthesis reaction composition comprising two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity; a DNA synthesis method in which during a DNA synthesis reaction two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity are used; a kit for use in in vitro DNA synthesis, comprising two or more kinds of DNA polymerases each having 3′→5′ exonuclease activity; and a kit for use in in vitro DNA synthesis, wherein the kit comprises the DNA synthesis reaction-enhancer and DNA polymerase. According to the present invention, DNA synthesis can be carried out at an efficiency more excellent as compared to conventional DNA synthesis reaction.

公开(公告)号：US20050239100A1

公开(公告)日：2005-10-27

申请号：US10973919

申请日：2004-10-27

申请人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C07H21/04 ,  C12N9/22 ,  C12P19/34 ,  C12Q1/68

CPC分类号： C12N9/1252 ,  C12P19/34 ,  C12Q1/6853 ,  C12Q2531/119 ,  C12Q2525/121 ,  C12Q2521/301

摘要： A convenient and effective method for amplifying a nucleic acid sequence characterized by effecting a DNA synthesis reaction in the presence of chimeric oligonucleotide primers; a method for supplying a large amount of DNA amplification fragments; an effective method for amplifying a nucleic acid sequence by combining the above method with another nucleic acid sequence amplification method; a method for detecting a nucleic acid sequence for detecting or quantitating a microorganism such as a virus, a bacterium, a fungus or a yeast; and a method for detecting a DNA amplification fragment obtained by the above method in situ.

摘要翻译： 一种用于扩增核酸序列的方法和方法，其特征在于在嵌合寡核苷酸引物存在下进行DNA合成反应; 提供大量DNA扩增片段的方法; 通过将上述方法与另一种核酸序列扩增方法结合来​​扩增核酸序列的有效方法; 用于检测用于检测或定量微生物如病毒，细菌，真菌或酵母的核酸序列的方法; 以及通过上述方法原位检测DNA扩增片段的方法。

公开(公告)号：US20050123950A1

公开(公告)日：2005-06-09

申请号：US10929759

申请日：2004-08-31

申请人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C07H21/04 ,  C12N9/22 ,  C12P19/34 ,  C12Q1/68

CPC分类号： C12N9/1252 ,  C12P19/34 ,  C12Q1/6853 ,  C12Q2531/119 ,  C12Q2525/121 ,  C12Q2521/301

摘要： A convenient and effective method for amplifying a nucleic acid sequence characterized by effecting a DNA synthesis reaction in the presence of chimeric oligonucleotide primers; a method for supplying a large amount of DNA amplification fragments; an effective method for amplifying a nucleic acid sequence by combining the above method with another nucleic acid sequence amplification method; a method for detecting a nucleic acid sequence for detecting or quantitating a microorganism such as a virus, a bacterium, a fungus or a yeast; and a method for detecting a DNA amplification fragment obtained by the above method in situ.

公开(公告)号：US06333158B1

公开(公告)日：2001-12-25

申请号：US09712266

申请日：2000-11-15

申请人： Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Takashi Uemori ,  Yoshimi Sato ,  Tomoko Fujita ,  Kazue Miyake ,  Hiroyuki Mukai ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C12Q168

CPC分类号： C12N9/1252

摘要： The present invention relates to a thermostable DNA polymerase-associated factor capable of enhancing DNA synthesizing-activity of a DNA polymerase; a thermostable DNA polymerase-associated factor possessing an activity of binding to a DNA polymerase and a method for producing the same; a gene encoding the DNA polymerase-associated factor; a method of DNA synthesis by using a DNA polymerase in the presence of the DNA polymerase-associated factor; and a kit comprising the DNA polymerase-associated factor. According to the present invention, there can be provided in vitro DNA synthesis and a DNA amplification system which are more excellent than conventional techniques by utilizing the DNA polymerase-associated factor of the present invention.

摘要翻译： 本发明涉及能够增强DNA聚合酶的DNA合成活性的热稳定的DNA聚合酶相关因子; 具有与DNA聚合酶结合的活性的热稳定DNA聚合酶相关因子及其制备方法; 编码DNA聚合酶相关因子的基因; 在DNA聚合酶相关因子存在下使用DNA聚合酶进行DNA合成的方法; 以及包含DNA聚合酶相关因子的试剂盒。 根据本发明，通过利用本发明的DNA聚合酶相关因子，可以提供比常规技术更优异的体外DNA合成和DNA扩增系统。

公开(公告)号：US06951722B2

公开(公告)日：2005-10-04

申请号：US09935338

申请日：2001-08-23

申请人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

发明人： Hiroyuki Mukai ,  Hiroaki Sagawa ,  Takashi Uemori ,  Junko Yamamoto ,  Jun Tomono ,  Eiji Kobayashi ,  Tatsuji Enoki ,  Osamu Takeda ,  Kazue Miyake ,  Yoshimi Sato ,  Mariko Moriyama ,  Haruhisa Sawaragi ,  Michio Hagiya ,  Kiyozo Asada ,  Ikunoshin Kato

IPC分类号： C07H21/04 ,  C12N9/22 ,  C12P19/34 ,  C12Q1/68

CPC分类号： C12N9/1252 ,  C12P19/34 ,  C12Q1/6853 ,  C12Q2531/119 ,  C12Q2525/121 ,  C12Q2521/301

摘要： A convenient and effective method for amplifying a nucleic acid sequence characterized by effecting a DNA synthesis reaction in the presence of chimeric oligonucleotide primers; a method for supplying a large amount of DNA amplification fragments; an effective method for amplifying a nucleic acid sequence by combining the above method with another nucleic acid sequence amplification method; a method for detecting a nucleic acid sequence for detecting or quantitating a microorganism such as a virus, a bacterium, a fungus or a yeast; and a method for detecting a DNA amplification fragment obtained by the above method in situ.

公开(公告)号：US07572617B2

公开(公告)日：2009-08-11

申请号：US10526073

申请日：2003-08-26

申请人： Shigekazu Hokazono ,  Takashi Uemori ,  Tetsuki Tanaka ,  Ikunoshin Kato

发明人： Shigekazu Hokazono ,  Takashi Uemori ,  Tetsuki Tanaka ,  Ikunoshin Kato

IPC分类号： C07K14/00 ,  C12N9/16 ,  C12Q1/14 ,  C12N15/00 ,  C12N5/10 ,  C12N1/21 ,  C12P21/00 ,  C07H21/00

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。