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    • 3. 发明授权
    • Method and kit for quantitative analysis of protein
    • 蛋白质定量分析方法和试剂盒
    • US07354996B2
    • 2008-04-08
    • US11028322
    • 2005-01-04
    • Eiichi MatsuoMakoto WatanabeChikako TodaOsamu Nishimura
    • Eiichi MatsuoMakoto WatanabeChikako TodaOsamu Nishimura
    • A61K38/00
    • G01N33/6842G01N33/6851
    • The present invention provides a method for global quantitative analysis of protein that is effectively applied also for unpurified samples such as biological samples, and achieves better detection sensitivity and quantitativeness than the conventional NBS method. A method for global quantitative analysis of protein comprising: preparing two states of protein samples, a Protein sample I for analysis and a control Protein sample II; solubilizing the Protein sample I and II by urea or guanidine hydrochloride; subjecting the solubilized Protein sample I and II to modification using 2-nitro[13C6]benzenesulfenyl chloride and 2-nitro[12C6]benzenesulfenyl chloride; mixing and desalting the modified Protein sample I and II; resolubilizing by urea or guanidine hydrochloride; reducing and alkylating; subjecting to trypsin digestion in the presence of urea or guanidine hydrochloride; separating the obtained peptide mixture using a media having a phenyl group; and subjecting the enriched modified peptide fragments to mass spectrometry preferably using 3CHCA, 3H4NBA or mixture of 3H4NBA and 4CHCA as a matrix.
    • 本发明提供了一种全球定量分析蛋白质的方法,该方法也有效应用于未纯化的样品如生物样品,并且比常规NBS方法获得更好的检测灵敏度和定量性。 一种用于蛋白质全球定量分析的方法,包括:制备蛋白质样品的两种状态,用于分析的蛋白质样品I和对照蛋白质样品II; 通过尿素或盐酸胍溶解蛋白质样品I和II; 将溶解的蛋白质样品I和II用2-硝基[13 C 6]苯硫基氯和2-硝基[12β] 亚苯基氯; 混合和脱盐改性蛋白质样品I和II; 用尿素或盐酸胍重新溶解; 还原和烷基化; 在尿素或盐酸胍存在下进行胰蛋白酶消化; 使用具有苯基的介质分离得到的肽混合物; 并将富集的经修饰的肽片段进行质谱,优选使用3CHCA,3H4NBA或3H4NBA和4CHCA的混合物作为基质。
    • 5. 发明申请
    • Method and kit for quantitative analysis of protein
    • 蛋白质定量分析方法和试剂盒
    • US20060051831A1
    • 2006-03-09
    • US11028322
    • 2005-01-04
    • Eiichi MatsuoMakoto WatanabeChikako TodaOsamu Nishimura
    • Eiichi MatsuoMakoto WatanabeChikako TodaOsamu Nishimura
    • C12Q1/37
    • G01N33/6842G01N33/6851
    • The present invention provides a method for global quantitative analysis of protein that is effectively applied also for unpurified samples such as biological samples, and achieves better detection sensitivity and quantitativeness than the conventional NBS method. A method for global quantitative analysis of protein comprising: preparing two states of protein samples, a Protein sample I for analysis and a control Protein sample II; solubilizing the Protein sample I and II by urea or guanidine hydrochloride; subjecting the solubilized Protein sample I and II to modification using 2-nitro[13C6]benzenesulfenyl chloride and 2-nitro[12C6]benzenesulfenyl chloride; mixing and desalting the modified Protein sample I and II; resolubilizing by urea or guanidine hydrochloride; reducing and alkylating; subjecting to trypsin digestion in the presence of urea or guanidine hydrochloride; separating the obtained peptide mixture using a media having a phenyl group; and subjecting the enriched modified peptide fragments to mass spectrometry preferably using 3CHCA, 3H4NBA or mixture of 3H4NBA and 4CHCA as a matrix.
    • 本发明提供了一种全球定量分析蛋白质的方法,该方法也有效应用于未纯化的样品如生物样品,并且比常规NBS方法获得更好的检测灵敏度和定量性。 一种用于蛋白质全球定量分析的方法,包括:制备蛋白质样品的两种状态,用于分析的蛋白质样品I和对照蛋白质样品II; 通过尿素或盐酸胍溶解蛋白质样品I和II; 将溶解的蛋白质样品I和II用2-硝基[13 C 6]苯硫基氯和2-硝基[12β] 亚苯基氯; 混合和脱盐改性蛋白质样品I和II; 用尿素或盐酸胍重新溶解; 还原和烷基化; 在尿素或盐酸胍存在下进行胰蛋白酶消化; 使用具有苯基的介质分离得到的肽混合物; 并将富集的经修饰的肽片段进行质谱,优选使用3CHCA,3H4NBA或3H4NBA和4CHCA的混合物作为基质。