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    • 2. 再颁专利
    • Method of detecting or quantitatively determining mitochondrial DNA 3243 variation, and kit therefor
    • 检测或定量测定线粒体DNA 3243变异的方法及其试剂盒
    • USRE44894E1
    • 2014-05-13
    • US13234907
    • 2011-09-16
    • Mitsuharu Hirai
    • Mitsuharu Hirai
    • C12Q1/68C12P19/34
    • A method for detecting a DNA having the mitochondrial DNA 3243 mutation is disclosed. Quantitative PCR is used with a primer having a nucleotide sequence complementary to the nucleotide sequence starting from the nucleotide number 243 in SEQ ID NO: 2 and having a length of 12 to 30 nucleotides. A method is also disclosed for detecting a DNA having the mitochondrial DNA 3243 mutation by using a nucleic acid probe which is end labeled with a fluorescent dye. The fluorescence of the fluorescent dye decreases upon hybridization. The nucleic acid probe has a nucleotide sequence complementary to the nucleotide sequence starting from nucleotide number 230 in the nucleotide sequence of SEQ ID NO: 2 and a length of 14 to 40 nucleotides. The 3′ end of the probe is labeled with the fluorescent dye.
    • 公开了一种用于检测具有线粒体DNA 3243突变的DNA的方法。 定量PCR与具有与核苷酸序列互补的核苷酸序列的引物使用,其核苷酸序列以SEQ ID NO:2的核苷酸编号243开始,长度为12〜30个核苷酸。 还公开了通过使用用荧光染料末端标记的核酸探针来检测具有线粒体DNA 3243突变的DNA的方法。 荧光染料的荧光在杂交时降低。 核酸探针具有与SEQ ID NO:2的核苷酸序列中的核苷酸230号开始的核苷酸序列互补的核苷酸序列,长度为14〜40个核苷酸。 探针的3'末端用荧光染料标记。
    • 7. 发明授权
    • Probes for detecting obesity gene
    • 检测肥胖基因的探针
    • US08021845B2
    • 2011-09-20
    • US12306417
    • 2007-11-30
    • Mitsuharu HiraiSatoshi Majima
    • Mitsuharu HiraiSatoshi Majima
    • C12Q1/68C07H21/04
    • C12Q1/6883C12Q2600/156C12Q2600/16
    • Primer sets for amplifying target regions containing sites to be detected in the obesity gene (the β2AR gene, the β3AR gene, and the UCP1 gene) by a gene amplification method are provided, wherein the primer sets can amplify the regions specifically. Three pairs of primer sets are used including forward primers composed of the base sequences of SEQ ID NO: 9 or SEQ ID NO: 109, SEQ ID NO: 25, and SEQ ID NO:43 as well as reverse primers composed of the base sequences of SEQ ID NO: 18, SEQ ID NO: 30, and SEQ ID NO: 63, respectively. The use of these primer sets makes it possible to specifically amplify a target region including a site where a polymorphism to be detected is generated in the β2AR gene, the β3AR gene, and the UCP1 gene, in the same reaction solution at the same time.
    • 提供了通过基因扩增方法扩增含有在肥胖基因中检测到的位点(“bgr2AR基因”,“3AR基因”,“UCP1基因”)的靶区域的引物组,其特征在于, 。 使用三对引物组,包括由SEQ ID NO:9或SEQ ID NO:109,SEQ ID NO:25和SEQ ID NO:43的碱基序列组成的正向引物,以及由碱基序列组成的反向引物 分别为SEQ ID NO:18,SEQ ID NO:30和SEQ ID NO:63。 这些引物组的使用使得可以特异性地扩增包含在第2AR基因,第3AR基因和UCP1基因中产生待检测多态性的位点的靶区域,在同一反应溶液中 同一时间。
    • 8. 发明申请
    • PROBE FOR DETECTING MUTATION IN JAK2 GENE AND USE THEREOF
    • 用于检测JAK2基因中的突变的探针及其用途
    • US20100068713A1
    • 2010-03-18
    • US12513642
    • 2008-07-11
    • Mitsuharu HiraiSatoshi MajimaTaira MaekawaShinya Kimura
    • Mitsuharu HiraiSatoshi MajimaTaira MaekawaShinya Kimura
    • C12Q1/68G01N33/53C07H21/04
    • C12Q1/6883C12Q2600/156Y10T436/143333
    • A probe for detecting a mutation in the JAK2 gene is provided that can detect a target sequence containing a mutation even when the target sequence containing the mutation and a non-target sequence containing no mutation coexist, which are different only in a single base from each other. The probe to be used is an oligonucleotide that is at least one oligonucleotide having a sequence identical to that of a region extending from a cytosine base (C) at position 84 to be considered as the first base to any one of the 17th to 22nd bases in the direction toward the 5′ end in exon 12 of the JAK2 gene consisting of the base sequence of SEQ ID NO: 1, with the cytosine base (C) being the 3′ end. Even in the case of a sample containing both the JAK2 genes with a mutation that has occurred and without a mutation that has occurred, the use of such a probe in, for example, Tm analysis allows the former mutation to be detected. Preferably, the probe is labeled with a fluorescent dye.
    • 提供了用于检测JAK2基因突变的探针,即使当含有突变的靶序列和不含突变的非靶序列共存时也可以检测到含有突变的靶序列,其仅在单个碱基中不同 其他。 要使用的探针是至少一种寡核苷酸,其具有与从第84位的胞嘧啶碱基(C)延伸的区域的序列相同的寡核苷酸,被认为是第17位至第22位碱基的第一碱基 在由SEQ ID NO:1的碱基序列组成的JAK2基因的外显子12的5'端的方向上,胞嘧啶碱基(C)为3'末端。 即使在含有具有发生突变且没有发生突变的JAK2基因的样品的情况下,在例如Tm分析中使用这种探针也可以检测到前述突变。 优选地,探针用荧光染料标记。