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Determination of methionine and selenomethionine in yeast by species-specific isotope dilution GC/MS

机译:物种特异性同位素稀释GC / MS法测定酵母中的蛋氨酸和硒代蛋氨酸

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A method for the simultaneous determination of methionine (Met) and selenomethionine (SeMet) in yeast using species-specific isotope dilution (ID) gas chromatography/mass spectrometry (GC/MS) is described. Samples were digested by refluxing for 16 h with 4 M methanesulfonic acid. Analytes were derivatized with methyl chloroformate and extracted into chloroform for GC/MS analysis. In addition to use of commercially available C-13- enriched Met and SeMet spikes for species specific ID analysis, a Se-74-enriched SeMet spike was also available for comparison of results. In selective ion monitoring mode, the intensities of ions at m/z 221, 222, 269, 270, and 263 were used to calculate the 221/222, 269/270, and 269/263 ion ratios for quantification of Met and SeMet. Concentrations of 5959 +/- 33 and 3404 +/- 12 mug g(-1) (one standard deviation, n = 6) with relative standard deviations of 0.55 and 0.36% for Met and SeMet, respectively, were obtained using C-13-enriched spikes. A concentration of 3417 +/- 8 mug g(-1) (one standard deviation, n = 6) was obtained using the Se-74-enriched SeMet spike. The concentration of SeMet measured in the yeast is equivalent to 66.43 +/- 0.24% of total Se and 30.31 +/- 0.11% of total Met is in the form of SeMet. Method detection limits (three times the standard deviation) of 3.4 and 1.0 mug g(-1) were estimated for Met and SeMet, respectively, based on a 0.25-g subsample of yeast with 1 mL of extract used for derivatization. A similar concentration of 5930 +/- 29 mug g(-1) (one standard deviation, n = 4) for Met and a lower concentration of 2787 +/- 49 mug g(-1) (one standard deviation, n = 4) for SeMet were obtained for this yeast sample using species-specific ID analysis based on GC/MS with C-13-enriched Met and SeMet spikes when a 2-h open microwave digestion approach using 8 M methanesulfonic acid was used.
机译:描述了一种使用物种特异性同位素稀释(ID)气相色谱/质谱(GC / MS)同时测定酵母中蛋氨酸(Met)和硒代蛋氨酸(SeMet)的方法。通过与4 M甲磺酸回流16 h消化样品。用氯甲酸甲酯将分析物衍生化,然后萃取到氯仿中进行GC / MS分析。除了使用市售的富含C-13的Met和SeMet尖峰进行物种特异性ID分析外,还可以使用富含Se-74的SeMet尖峰来比较结果。在选择性离子监测模式下,使用m / z 221、222、269、270和263处的离子强度来计算221 / 222、269 / 270和269/263离子比,以定量Met和SeMet。使用C-13获得的Met和SeMet的浓度分别为5959 +/- 33和3404 +/- 12马克杯g(-1)(一个标准偏差,n = 6),相对标准偏差分别为0.55和0.36%。 -丰富的尖峰。使用富含Se-74的SeMet尖峰获得了3417 +/- 8马克杯g(-1)的浓度(一个标准偏差,n = 6)。酵母中测得的SeMet浓度相当于总Se的66.43 +/- 0.24%,而总Met的30.31 +/- 0.11%是SeMet形式。基于0.25 g酵母亚样品和1 mL提取物用于衍生化,分别估算了Met和SeMet的方法检测限(三倍于标准偏差)为3.4和1.0ug g(-1)。大都会的类似浓度为5930 +/- 29马克杯g(-1)(一个标准偏差,n = 4),而更低的浓度为2787 +/- 49马克杯g(-1)(一个标准偏差,n = 4)当使用8 M甲磺酸进行2小时开放式微波消化时,使用基于GC / MS的具有C-13富集的Met和SeMet尖峰的物种特异性ID分析,可对该酵母样品获得SeMet。

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