Terminal-phosphate-labeled nucleotides with new linkers
    1.
    发明授权
    Terminal-phosphate-labeled nucleotides with new linkers 有权
    末端磷酸酯标记的核苷酸与新的接头

    公开(公告)号:US07393640B2

    公开(公告)日:2008-07-01

    申请号:US10772996

    申请日:2004-02-05

    IPC分类号: C12Q1/68 C12P19/34

    摘要: The present invention describes methods of using terminal-phosphate-labeled nucleotides in the presence of a manganese salt to enhance their substrate properties towards various enzymes. Particularly described are methods of detecting a nucleic acid in a sample, based on the use of terminal-phosphate-labeled nucleotides as substrates for nucleic acid polymerases, in the presence of a manganese salt. Further provided are manganese complexes of terminal-phosphate-labeled nucleotides as well as terminal-phosphate-labeled nucleotides with new linkers with enhanced substrate properties.

    摘要翻译: 本发明描述了在锰盐存在下使用末端磷酸酯标记的核苷酸以增强其对各种酶的底物性质的方法。 特别描述的是在锰盐存在的情况下,基于使用末端磷酸酯标记的核苷酸作为核酸聚合酶的底物,检测样品中的核酸的方法。 还提供了末端磷酸酯标记的核苷酸的锰络合物以及具有增强的底物性质的新接头的末端磷酸酯标记的核苷酸。

    Allele specific primer extension
    2.
    发明授权
    Allele specific primer extension 有权
    等位基因特异性引物延伸

    公开(公告)号:US07560254B2

    公开(公告)日:2009-07-14

    申请号:US10651558

    申请日:2003-08-29

    摘要: A method of characterizing a nucleic acid sample is provided that includes the steps of: (a) conducting a DNA polymerase reaction that includes the reaction of a template, an allele specific primer, at least one terminal phosphate-labeled nucleotide, DNA polymerase, and optionally an enzyme having 3′→5′ exonuclease activity when the primer is non-hydrolyzable, which reaction results in the production of labeled polyphosphate; (b) permitting the labeled polyphosphate to react with a phosphatase to produce a detectable species; (c) detecting the detectable species; and (d) characterizing the nucleic acid sample based on such detection.

    摘要翻译: 提供了表征核酸样品的方法,其包括以下步骤:(a)进行DNA聚合酶反应,其包括模板,等位基因特异性引物,至少一个末端磷酸酯标记的核苷酸,DNA聚合酶和 任选地当引物不可水解时具有3'→5'核酸外切酶活性的酶,该反应导致标记的多磷酸盐的产生; (b)允许标记的多磷酸酯与磷酸酶反应以产生可检测的物质; (c)检测可检测物种; 和(d)基于这种检测来表征核酸样品。

    Nucleic acid amplification with terminal-phosphate labeled nucleotides
    4.
    发明授权
    Nucleic acid amplification with terminal-phosphate labeled nucleotides 有权
    用磷酸末端标记的核苷酸扩增核酸

    公开(公告)号:US07125671B2

    公开(公告)日:2006-10-24

    申请号:US10651362

    申请日:2003-08-29

    IPC分类号: C12Q1/68 C12P19/34

    摘要: The present invention relates generally to the use of terminal-phosphate-labeled nucleotides having three or more phosphates as substrates for nucleic acid polymerases and their use in DNA amplification. The labels employed are chemiluminescent, fluorescent, electrochemical and chromogenic moieties as well as mass tags and include those that are directly detectable, detectable after enzyme activation or feed into other processes to generate a different signal. The signal generated from the attached dyes may also be used to quantify the amount of amplification. Further provided are stabilizers that enhance the stability of terminal-phosphate labeled nucleoside polyphosphates in aqueous solutions and are useful for reducing non-enzymatic hydrolysis of these nucleotides, hence decrease background.

    摘要翻译: 本发明一般涉及具有三种或更多种磷酸盐的末端磷酸酯标记的核苷酸作为核酸聚合酶的底物及其在DNA扩增中的应用。 使用的标记是化学发光,荧光,电化学和显色部分以及质量标签,并且包括直接可检测的标记,可在酶活化后进行或进入其它过程以产生不同信号。 从连接的染料产生的信号也可用于量化扩增量。 还提供了增强末端磷酸酯标记的核苷多磷酸酯在水溶液中的稳定性的稳定剂,并且可用于减少这些核苷酸的非酶水解,从而降低背景。

    Terminal-phosphate-labeled nucleotides and methods of use

    公开(公告)号:US07052839B2

    公开(公告)日:2006-05-30

    申请号:US10113030

    申请日:2002-04-01

    IPC分类号: C12Q1/68

    摘要: The present invention describes methods of detecting a nucleic acid in a sample, based on the use of terminal-phosphate-labeled nucleotides as substrates for nucleic acid polymerases. The methods provided by this invention utilize a nucleoside polyphosphate, dideoxynucleoside polyphosphate, or deoxynucleoside polyphosphate analogue which has a colorimetric dye, chemiluminescent, or fluorescent moiety, a mass tag or an electrochemical tag attached to the terminal-phosphate. When a nucleic acid polymerase uses this analogue as a substrate, an enzyme-activatable label would be present on the inorganic polyphosphate by-product of phosphoryl transfer. Cleavage of the polyphosphate product of phosphoryl transfer via phosphatase leads to a detectable change in the label attached thereon. When the polymerase assay is performed in the presence of a phosphatase, there is provided a convenient method for real-time monitoring of DNA or RNA synthesis and detection of a target nucleic acid.

    Analyte detection
    7.
    发明授权
    Analyte detection 有权
    分析物检测

    公开(公告)号:US07244566B2

    公开(公告)日:2007-07-17

    申请号:US10651582

    申请日:2003-08-29

    IPC分类号: C12Q1/68

    CPC分类号: C12P19/34 C12Q1/68

    摘要: A method of characterizing an analyte sample is provided that includes the steps of: (a) anchoring the analyte to a nucleic acid template of known sequence; (b) conducting a DNA polymerase reaction that includes the reaction of a template, a non-hydrolyzable primer, at least one terminal phosphate-labeled nucleotide, DNA polymerase, and an enzyme having 3′→5′ exonuclease activity which reaction results in the production of labeled polyphosphate; (c) permitting the labeled polyphosphate to react with a phosphatase to produce a detectable species characteristic of the sample; (d) detecting the detectable species. The method may include the step of characterizing the nucleic acid sample based on the detection. Also provided are methods of analyzing multiple analytes in a sample, and kits for characterizing analyte samples.

    摘要翻译: 提供表征分析物样品的方法,其包括以下步骤:(a)将分析物锚定到已知序列的核酸模板; (b)进行DNA聚合酶反应,其包括模板,不可水解的引物,至少一个末端磷酸酯标记的核苷酸,DNA聚合酶和具有3'→5'核酸外切酶活性的酶的反应,该反应导致 生产标记多磷酸盐; (c)允许标记的多磷酸酯与磷酸酶反应以产生样品的可检测物种特征; (d)检测可检测物种。 该方法可以包括基于检测来表征核酸样品的步骤。 还提供了分析样品中多种分析物的方法,以及用于表征分析物样品的试剂盒。

    Terminal-phosphate-labeled nucleotides and methods of use
    8.
    发明授权
    Terminal-phosphate-labeled nucleotides and methods of use 有权
    末端磷酸酯标记的核苷酸和使用方法

    公开(公告)号:US07223541B2

    公开(公告)日:2007-05-29

    申请号:US10358818

    申请日:2003-02-05

    IPC分类号: C12Q1/68

    摘要: The present invention relates to improved methods of detecting a target using a labeled substrate or substrate analog. The methods comprise reacting the substrate or substrate analog in an enzyme-catalyzed reaction which produces a labeled moiety with independently detectable signal only when such substrate or substrate analog reacts. The present invention, in particular, describes methods of detecting a nucleic acid in a sample, based on the use of terminal-phosphate-labeled nucleotides as substrates for nucleic acid polymerases. The methods provided by this invention utilize a nucleoside polyphosphate, dideoxynucleoside polyphosphate, or deoxynucleoside polyphosphate analogue which has a colorimetric dye, chemiluminescent, or fluorescent moiety, a mass tag or an electrochemical tag attached to the terminal-phosphate. When a nucleic acid polymerase uses this analogue as a substrate, an enzyme-activatable label would be present on the inorganic polyphosphate by-product of phosphoryl transfer. Cleavage of the polyphosphate product of phosphoryl transfer via phosphatase leads to a detectable change in the label attached thereon. When the polymerase assay is performed in the presence of a phosphatase, there is provided a convenient method for real-time monitoring of DNA or RNA synthesis and detection of a target nucleic acid.

    摘要翻译: 本发明涉及使用标记的底物或底物类似物检测靶的改进方法。 所述方法包括在酶催化的反应中使底物或底物类似物反应,其仅在这种底物或底物类似物反应时产生具有独立可检测信号的标记部分。 本发明特别地描述了基于使用末端磷酸酯标记的核苷酸作为核酸聚合酶的底物来检测样品中核酸的方法。 本发明提供的方法利用了具有比色染料,化学发光或荧光部分的核苷多磷酸,双脱氧核苷多聚磷酸酯或脱氧核苷多聚磷酸酯类似物,连接至末端磷酸酯的质量标签或电化学标签。 当核酸聚合酶使用该类似物作为底物时,酶活性标记将存在于磷酸转移的无机多磷酸盐副产物上。 通过磷酸酶切割磷酸转移的多磷酸盐产物导致附着在其上的标签的可检测的变化。 当在磷酸酶的存在下进行聚合酶测定时,提供了用于实时监测DNA或RNA合成和检测靶核酸的方便的方法。

    Oligonucleotide tagged nucleoside triphosphates (OTNTPs) for genetic analysis
    9.
    发明授权
    Oligonucleotide tagged nucleoside triphosphates (OTNTPs) for genetic analysis 失效
    寡核苷酸标记核苷三磷酸(OTNTP)用于遗传分析

    公开(公告)号:US07109316B2

    公开(公告)日:2006-09-19

    申请号:US10226734

    申请日:2002-08-23

    CPC分类号: C07H19/04

    摘要: Oligonucleotide tagged nucleoside triphosphates, OTNTPs, which are substrates for polymerases and or terminal nucleotidyl transferases are provided as well as methods of making these OTNTPs. Further provided are OTNTPs with fluorescent dyes including energy transfer dyes, attached to the oligonucleotide chain, OTNTPs with unnatural bases incorporated in the oligonucleotide sequence and methods for incorporating these OTNTPs in DNA or RNA. Also provided are methods for using the oligonucleotides on OTNTPs for amplifying the oligo sequence on the OTNTP using an amplification method described above. Further provided are reactive bifunctional amidites, methods of making these compounds and methods for detecting single nucleotide polymorphisms using the above OTNTPs. Methods for detecting differential gene expression using the OTNTPs and methods of separating specifically modified DNA or RNA using the OTNTPs are also provided.

    摘要翻译: 提供了寡聚核苷酸标记的核苷三磷酸酯,OTNTP,其是用于聚合酶和末端核苷酸转移酶的底物,以及制备这些OTNTP的方法。 还提供了含有荧光染料的OTNTP,其包括与寡核苷酸链连接的能量转移染料,掺入寡核苷酸序列中的非天然碱基的OTNTP以及将这些OTNTP引入DNA或RNA中的方法。 还提供了使用寡核苷酸在OTNTP上使用上述扩增方法在OTNTP上扩增寡核苷酸序列的方法。 还提供了反应性双官能脒,制备这些化合物的方法和使用上述OTNTP检测单核苷酸多态性的方法。 还提供了使用OTNTP检测差异基因表达的方法和使用OTNTP分离特异性修饰的DNA或RNA的方法。

    FLUORESCENCE RESONANCE ENERGY TRANSFER ENZYME SUBSTRATES
    10.
    发明申请
    FLUORESCENCE RESONANCE ENERGY TRANSFER ENZYME SUBSTRATES 审中-公开
    荧光共振能量转移酶基质

    公开(公告)号:US20120208223A1

    公开(公告)日:2012-08-16

    申请号:US13183518

    申请日:2011-07-15

    申请人: Shiv Kumar Anup Sood

    发明人: Shiv Kumar Anup Sood

    IPC分类号: G01N21/64 C07H21/00 C07K2/00

    CPC分类号: G01N33/542 C12Q1/34

    摘要: Disclosed are compounds of formula (I) wherein D1 is a first dye moiety whose fluorescence properties may be modulated so as to be suitable as a donor or an acceptor in an energy transfer arrangement; D2 is a second dye moiety suitable as an acceptor or a donor in an energy transfer arrangement with said first dye; L is a linking group comprises 2-200 linked atoms, wherein said linking group optionally includes an enzyme cleavage site; and M is an enzyme cleavable group chosen to modulate the fluorescence properties of D1. The compounds of formula (I) may be used as reporter molecules for detecting biochemical cleavage events in assays that employ fluorescence resonance energy transfer.

    摘要翻译: 公开了式(I)的化合物,其中D1是可以调节其荧光性质以适合作为能量转移装置中的给体或受体的第一染料部分; D2是第二染料部分,其适于作为与所述第一染料的能量转移装置中的受体或供体; L是包含2-200个连接原子的连接基团,其中所述连接基团任选地包括酶切割位点; M是选择调节D1荧光性质的酶切割基团。 式(I)的化合物可以用作用于检测采用荧光共振能量转移的测定中生化裂解事件的报道分子。