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    • 1. 发明申请
      US20060188881A1 Dna amplification method and kit therefor 失效
    • Dna amplification method and kit therefor
    • Dna扩增方法及其试剂盒
    • US20060188881A1
    • 2006-08-24
    • US10547354
    • 2004-03-05
    • Satoshi HashiguchiKen Inose
    • Satoshi HashiguchiKen Inose
    • C12Q1/68C12P19/34
    • C12Q1/6853C12Q1/686C12Q2525/155
    • In a method for amplifying a DNA, comprising performing PCR using a sense primer and an antisense primer, PCR is performed in the presence of an additional sense primer comprising the sense primer and an oligodeoxyribonucleotide having a first additional sequence and ligated to the 5′ end of the sense primer and an additional antisense primer comprising the antisense primer and an oligodeoxyribonucleotide having a second additional sequence complementary to the first additional sequence and ligated to the 5′ end of the antisense primer; a Tm value of the additional sequences is lower than Tm values of the sense primer and the antisense primer; and annealing temperature in PCR is initially set to be a temperature at which the additional sequences do not anneal and changed in the course of PCR to a temperature at which the additional sequences anneal to each other.
    • 在扩增DNA的方法中,包括使用有义引物和反义引物进行PCR,在包含有义引物和具有第一附加序列的寡脱氧核糖核苷酸的另外的有义引物的存在下进行PCR,并连接到5'末端 的正义引物和另外的反义引物,其包含反义引物和具有与第一附加序列互补的第二附加序列并连接到反义引物的5'末端的寡脱氧核糖核苷酸; 附加序列的Tm值低于有义引物和反义引物的Tm值; 并且PCR中的退火温度最初设定为附加序列在PCR过程中不退火并且在附加序列彼此退火的温度下的温度。
    • 基本信息 添加关注 加入工作空间 PDF全文 PDF下载 全文下载 相似专利 双屏查看 权利要求书 说明书全文 Global Dossier Espacenet 法律信息 同族专利 专利引用
    • 3. 发明申请
      US20080035482A1 Method Of Concentrating And Purifying Nucleic Acid And Apparatus Therefor 审中-公开
    • Method Of Concentrating And Purifying Nucleic Acid And Apparatus Therefor
    • 浓缩和纯化核酸的方法及其设备
    • US20080035482A1
    • 2008-02-14
    • US10578770
    • 2004-11-09
    • Satoshi HashiguchiKen Inose
    • Satoshi HashiguchiKen Inose
    • C12N15/00C12M1/00C12Q1/68G01N27/447
    • C12N15/1017B01D57/02B01D61/145B01D61/42B01D61/425B01D61/46B01L3/502753C12N15/101G01N27/44747
    • The conventional method of purifying and concentrating nucleic acids, because of dangerous chemicals, requires elaborate chemical equipment to result in restriction of environment available. Further, time-consuming operation is inevitable and high-speed centrifugation, etc. are needed to cause automation to be difficult and to cause high purification degree to be unattainable. Still further, in the purification method using a column/filter, application of dusty samples tends to invite clogging to lead to a drop of purification efficiency, and centrifugation or suction operation is needed to cause automation to be difficult. In this invention, surfactants (3,4) are adsorbed on impurity (2) contained in a sample, so that the impurity (2) conducts behavior different from that of nucleic acid (1) to thereby attain separation of the impurity (2) from the nucleic acid (1). Impurity (2) other than nucleic acid (1) is energized with cationic surfactant (4) and nonionic surfactant (3) and placed in an electric field to thereby effect separation and purification of the nucleic acid (1) for an analyte containing the impurity (2). Thus, the nucleic acid (1) is brought into the state of being concentrated or easily concentrated.
    • 由于危险化学品,纯化和浓缩核酸的常规方法需要精心设计的化学设备来限制可用的环境。 此外,耗时的操作是不可避免的,需要高速离心等来引起自动化困难,并且导致高的净化程度是不可实现的。 此外,在使用柱/过滤器的净化方法中,灰尘样品的施用往往会引起堵塞,导致净化效率降低,需要离心或抽吸操作以使自动化变得困难。 在本发明中,表面活性剂(3,4)被吸附在样品中所含的杂质(2)上,使得杂质(2)的导电性质与核酸(1)不同,从而使杂质(2)分离, 来自核酸(1)。 核酸(1)以外的杂质(2)用阳离子表面活性剂(4)和非离子表面活性剂(3)通电,并放置在电场中,从而对含有杂质的分析物(1)进行分离和纯化 (2)。 因此,使核酸(1)进入浓缩或容易浓缩的状态。
    • 基本信息 添加关注 加入工作空间 PDF全文 PDF下载 全文下载 相似专利 双屏查看 权利要求书 说明书全文 Global Dossier Espacenet 法律信息 同族专利 专利引用
    • 4. 发明申请
      US20090311770A1 Method of collecting microorganisms using fine particles, method of collecting nucleic acids using fine particles, and kits for use in the these methods 审中-公开
    • Method of collecting microorganisms using fine particles, method of collecting nucleic acids using fine particles, and kits for use in the these methods
    • 使用细颗粒收集微生物的方法,使用细颗粒收集核酸的方法,以及用于这些方法的试剂盒
    • US20090311770A1
    • 2009-12-17
    • US11919475
    • 2006-05-19
    • Satoshi HashiguchiMitsuharu HiraiToshiya Hosomi
    • Satoshi HashiguchiMitsuharu HiraiToshiya Hosomi
    • C12N1/02C12N7/02C12N1/20C12N5/06
    • C12N7/00C12N1/02C12N15/1013C12N2730/10151C12N2740/16051C12N2770/24251C12Q1/24
    • The present invention provides a method of collecting microorganisms and a method of collecting nucleic acids, which both can be carried out easily and can achieve a high collection rate. A method of collecting microorganisms according to the present invention includes a microorganism adsorption step of bringing a sample into contact with fine particles so as to cause microorganisms contained in the sample to be adsorbed onto the fine particles. In this method, the fine particles have a particle diameter of 6 μm or less and a specific surface area of 50 m2/g or less. Furthermore, a method of collecting nucleic acids according to the present invention includes: a microorganism adsorption step of causing microorganisms to be adsorbed onto fine particles; and a nucleic acid elution step of eluting nucleic acids from the microorganisms that have been adsorbed onto the fine particles. The microorganism adsorption step in this method is the microorganism collection method of the present invention. According to the collection methods of the present invention, microorganisms and nucleic acids can be collected easily and efficiently. Preferably, the fine particles are magnetic silica particles.
    • 本发明提供收集微生物的方法和收集核酸的方法,这两者都可以容易地进行并且可以实现高收集率。 根据本发明的收集微生物的方法包括微生物吸附步骤,使样品与细颗粒接触,以使样品中所含的微生物吸附到微粒上。 在该方法中,微粒的粒径为6μm以下,比表面积为50m 2 / g以下。 此外,根据本发明的收集核酸的方法包括:使微生物吸附在细颗粒上的微生物吸附步骤; 以及从已经吸附到微粒上的微生物中洗脱核酸的核酸洗脱步骤。 该方法中的微生物吸附步骤是本发明的微生物收集方法。 根据本发明的收集方法,可以容易且有效地收集微生物和核酸。 优选地,微粒是磁性二氧化硅颗粒。
    • 基本信息 添加关注 加入工作空间 PDF全文 PDF下载 全文下载 相似专利 双屏查看 权利要求书 说明书全文 Global Dossier Espacenet 法律信息 同族专利 专利引用
    • 6. 发明授权
      US07365187B2 DNA amplification method and kit therefor 失效
    • DNA amplification method and kit therefor
    • DNA扩增方法及试剂盒
    • US07365187B2
    • 2008-04-29
    • US10547354
    • 2004-03-05
    • Satoshi HashiguchiKen Inose
    • Satoshi HashiguchiKen Inose
    • C07H21/04C12Q1/68C12P19/34
    • C12Q1/6853C12Q1/686C12Q2525/155
    • In a method for amplifying a DNA, comprising performing PCR using a sense primer and an antisense primer, PCR is performed in the presence of an additional sense primer comprising the sense primer and an oligodeoxyribonucleotide having a first additional sequence and ligated to the 5′ end of the sense primer and an additional antisense primer comprising the antisense primer and an oligodeoxyribonucleotide having a second additional sequence complementary to the first additional sequence and ligated to the 5′ end of the antisense primer; a Tm value of the additional sequences is lower than Tm values of the sense primer and the antisense primer; and annealing temperature in PCR is initially set to be a temperature at which the additional sequences do not anneal and changed in the course of PCR to a temperature at which the additional sequences anneal to each other.
    • 在扩增DNA的方法中,包括使用有义引物和反义引物进行PCR,在包含有义引物和具有第一附加序列的寡脱氧核糖核苷酸的另外的有义引物的存在下进行PCR,并连接到5'末端 的正义引物和另外的反义引物,其包含反义引物和具有与第一附加序列互补的第二附加序列并连接到反义引物的5'末端的寡脱氧核糖核苷酸; 附加序列的Tm值低于有义引物和反义引物的Tm值; 并且PCR中的退火温度最初设定为附加序列在PCR过程中不退火并且在附加序列彼此退火的温度下的温度。
    • 基本信息 添加关注 加入工作空间 PDF全文 PDF下载 全文下载 相似专利 双屏查看 权利要求书 说明书全文 Espacenet 法律信息 同族专利 专利引用
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