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    • 6. 发明专利
    • Probe sequence determination system for dna array
    • 用于DNA阵列的探针序列测定系统
    • JP2003052385A
    • 2003-02-25
    • JP2002111490
    • 2002-04-15
    • Hitachi Ltd株式会社日立製作所
    • TOMITA HIROYUKISAITO TOSHIRONARAHARA MASATOSHIKATO KOICHI
    • G01N33/48C12N15/09C12Q1/68
    • PROBLEM TO BE SOLVED: To realize a probe sequence without cross-hybridization, having an equalized Tm and slightly assuming a secondary structure in order to assure the assay accuracy and reproducibility as a probe sequence for a DNA array. SOLUTION: The probe sequence determination for the DNA array is carried out by passing the probe design flow through the following at least two steps. A step of preparing a probe candidate list for the DNA probe array composed of a partial sequence of the genome or a cDNA sequence (a listing step) and a step of excluding candidates having the melting temperature deviating from the predetermined range or high stability of the secondary structure or possibility of cross-hybridization (a filtering step). Thereby, a method for designing the sequence of the probe DNA immobilized on the DNA probe array is provided.
    • 要解决的问题:为了实现没有交叉杂交的探针序列,具有均衡的Tm并稍微假设二级结构,以确保作为DNA阵列的探针序列的测定精度和重现性。 解决方案:通过将探针设计流程通过以下至少两个步骤来进行DNA阵列的探针序列测定。 制备由基因组的部分序列或cDNA序列构成的DNA探针阵列的探针候选序列的步骤(列举步骤)和排除具有偏离预定范围或高稳定性的熔解温度的候选物的步骤 二级结构或交叉杂交的可能性(过滤步骤)。 因此,提供了设计固定在DNA探针阵列上的探针DNA序列的方法。
    • 7. 发明专利
    • Comparison analysis method of in vivo polymer
    • 生物聚合物的比较分析方法
    • JP2006194611A
    • 2006-07-27
    • JP2005003832
    • 2005-01-11
    • Hitachi Ltd株式会社日立製作所
    • NARAHARA MASATOSHISAITO TOSHIROKATO KOICHIOTA MASAYUKI
    • G01N33/50C12N15/09G01N33/68
    • PROBLEM TO BE SOLVED: To provide a method for specifying accurately with high reproducibility comparison data of in vivo polymers wherein in vivo polymers having large dispersion between samples exist in great numbers in the comparison data, in the case where the number of the comparison data of the in vivo polymers which are analysis objects is small.
      SOLUTION: In comparison analysis wherein each abundance of in vivo polymers existing in two different kinds of samples is used as an index, a plurality of in vivo polymers wherein dispersion of the abundance between the samples is known to be small are selected, and a correction value of signal intensity showing the abundance is calculated, and the comparison data between the two samples are specified by using the correction value.
      COPYRIGHT: (C)2006,JPO&NCIPI
    • 要解决的问题:为了提供一种精确地指定体内聚合物的高再现性比较数据的方法,其中在比较数据中存在大量样品间的分散体积较大的体内聚合物, 作为分析对象的体内聚合物的比较数据较少。 解决方案:选择使用存在于两种不同种类的样品中的各种丰度的体内聚合物作为指标的比较分析,选择其中已知样品之间丰度的分散小的多种体内聚合物, 并计算显示丰度的信号强度的校正值,并且通过使用校正值来指定两个样本之间的比较数据。 版权所有(C)2006,JPO&NCIPI
    • 8. 发明专利
    • Hybridization method and apparatus
    • 混合方法和装置
    • JP2003339375A
    • 2003-12-02
    • JP2002150446
    • 2002-05-24
    • Hitachi Ltd株式会社日立製作所
    • KATO KOICHISAITO TOSHIROTOMITA HIROYUKINARAHARA MASATOSHI
    • G01N33/53C12M1/00C12N15/09C12Q1/68G01N37/00
    • PROBLEM TO BE SOLVED: To provide a hybridization method and apparatus to improve the hybridization efficiency of a target DNA relative to the probe DNA immobilized on a substrate surface in a DNA chip assay.
      SOLUTION: A hybridization solution containing fine particles is sealed on a DNA chip with a cover glass and a sealing agent. The hybridization chamber holding the DNA chip is rotated on a rotary shaft. Since the fine particles are moved in the direction of the gravitation force, these particles have an effect to stir the hybridization solution. The hybridization efficiency is increased by the increase of the diffusion distance of the DNA target in the hybridization solution. The method is effective for improving the hybridization efficiency in the DNA chip assay and attains a signal having high quantitative accuracy and reproducibility.
      COPYRIGHT: (C)2004,JPO
    • 要解决的问题:提供在DNA芯片测定中提高靶DNA相对于固定在底物表面上的探针DNA的杂交效率的杂交方法和装置。 解决方案:将含有细颗粒的杂交溶液用盖玻片和密封剂密封在DNA芯片上。 保持DNA芯片的杂交室在旋转轴上旋转。 由于微粒在重力方向上移动,所以这些粒子具有搅拌杂交溶液的作用。 通过杂交溶液中DNA靶的扩散距离的增加,增加了杂交效率。 该方法对于提高DNA芯片测定中的杂交效率是有效的,并获得具有高定量精度和重复性的信号。 版权所有(C)2004,JPO
    • 9. 发明专利
    • Navigation apparatus
    • 导航装置
    • JP2008014663A
    • 2008-01-24
    • JP2006183486
    • 2006-07-03
    • Clarion Co LtdHcx:KkHitachi Ltdクラリオン株式会社株式会社 エイチ・シー・エックス株式会社日立製作所
    • KATO KOICHI
    • G01C21/00G08G1/0969
    • PROBLEM TO BE SOLVED: To provide a navigation apparatus that prevents the lowering of detection accuracy due to a setting angle, in the navigation apparatus which detects an angular velocity based on Coriolis force which acts on an oscillator.
      SOLUTION: The navigation apparatus 1 recognizes a setting angle with respect to a standard angle of an angular velocity detection means which outputs voltage as an angular velocity based on Coriolis force which acts on an oscillator (Step S1), leads out an amplification factor according to the setting angle which has been recognized (Step S2), amplifies the output voltage output from the angular velocity detection means by a gain control amplifier based on the led-out amplification factor (Step S3), converts a value of the amplified output voltage to digital data by an A/D conversion circuit, and performs navigation processing based on the digital data which shows the angular velocity.
      COPYRIGHT: (C)2008,JPO&INPIT
    • 要解决的问题:提供一种导航装置,其能够检测基于作用在振荡器上的科里奥利力的角速度的导航装置中防止由于设定角度引起的检测精度的降低。 导航装置1相对于基于作用在振荡器上的科里奥利力作为角速度输出电压的角速度检测装置的标准角度识别出设定角度(步骤S1),导出放大 根据已识别的设定角度(步骤S2),通过基于导出放大系数的增益控制放大器放大从角速度检测单元输出的输出电压(步骤S3),将放大的 通过A / D转换电路将电压输出到数字数据,并且基于显示角速度的数字数据执行导航处理。 版权所有(C)2008,JPO&INPIT