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Contribution of various types of liquid chromatography-mass spectrometry instruments to band broadening in fast analysis

机译:各种类型的液相色谱质谱仪在快速分析中对谱带扩展的贡献

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When performing fast LC with 50mm narrow-bore columns packed with small particles, the LC instrumentation can give rise to non-negligible band broadening. In the present study, the loss in chromatographic efficiency attributed to nine different mass spectrometers of various brands, ionization source geometries and types of analyzers was assessed. In their standard configurations, the extra-column variance of these UHPLC-MS systems was estimated to vary from 20 to >100μL~2. However, it was demonstrated that these differences arise exclusively from the chromatographic system (i.e., injector, tubing, valves, heater) and from the tubing employed to interface the UHPLC instrument with the MS device. By minimizing the tubing used for each UHPLC system, the extra-column variance was reduced to approximately 17-19μL~2 at 600μL/min, for all types of configurations. To achieve optimal chromatographic performance, it is therefore of prime importance to optimize the UHPLC configuration prior to conducting MS. The tubing located between the UHPLC system and the ionization source entrance was found to be particularly critical, as it contributes to band broadening even in the gradient mode. Using an optimized UHPLC-MS configuration, the loss in efficiency with a 50×2.1mm I.D. column was negligible for k>7. However, the efficiency loss with 1mm I.D. columns remained non-negligible for all current instrumentation, even for solutes with a value of k>20. Indeed, for a mixture of isobaric substrates and metabolites analyzed in gradient mode, the peak widths decreased by approximately 50% between a standard and optimized UHPLC-MS configuration, considering a 50×2.1mm, 1.7μm column. The peak broadening was changed by 230% on a 50×1mm, 1.7μm stationary phase, for the same system configurations.
机译:当使用填充有小颗粒的50mm窄口径色谱柱进行快速LC色谱分析时,LC仪器会引起不可忽略的谱带展宽。在本研究中,评估了归因于不同品牌的九种不同质谱仪,电离源几何形状和分析仪类型的色谱效率损失。在其标准配置中,这些UHPLC-MS系统的柱外差异估计在20至>100μL〜2之间变化。但是,事实证明,这些差异完全是由色谱系统(即进样器,管路,阀门,加热器)以及用于将UHPLC仪器与MS设备连接的管路引起的。通过最小化每个UHPLC系统使用的管路,对于所有类型的配置,柱外差异均以600μL/ min的速度减小到大约17-19μL〜2。因此,要获得最佳的色谱性能,在进行MS之前优化UHPLC配置至关重要。发现位于UHPLC系统和电离源入口之间的管道特别关键,因为即使在梯度模式下,它也有助于谱带展宽。使用优化的UHPLC-MS配置,内径50×2.1mm时效率损失。对于k> 7,该列可忽略不计。但是,内径为1mm时的效率损失对于所有当前的仪器,即使对于k> 20的溶质,色谱柱仍然不可忽略。的确,对于以梯度模式分析的等压底物和代谢物的混合物,考虑到50×2.1mm,1.7μm的色谱柱,在标准配置和优化的UHPLC-MS配置之间,峰宽降低了约50%。对于相同的系统配置,在50×1mm,1.7μm固定相上,峰展宽变化了230%。

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