Shibue M, Mant C T, Hodges R S
Department of Biochemistry and Molecular Genetics, University of Colorado Health Sciences Center at Fitzsimons, Aurora, CO 80045, USA.
J Chromatogr A. 2005 Jul 1;1080(1):68-75. doi: 10.1016/j.chroma.2005.03.035.
Despite the continuing dominance of trifluoroacetic acid (TFA) as the anionic ion-pairing reagent of choice for peptide separations by reversed-phase high-performance liquid chromatography (RP-HPLC), we believe that a step-by-step approach to re-examining the relative efficacy of TFA compared to other ion-pairing reagents is worthwhile, particularly for the design of separation protocols for complex peptide mixtures, e.g., in proteomics applications. Thus, we applied RP-HPLC in the presence of different concentrations of anionic ion-pairing reagents - phosphoric acid, TFA, pentafluoropropionic acid (PFPA) and heptafluorobutyric acid (HFBA)--to a mixture of three groups of four 10-residue peptides, these groups containing peptides of +1, +3 or +5 net charge. Overall separation of the 12-peptide mixture improved with increasing reagent hydrophobicity (phosphate- < TFA- < PFPA- < HFBA-) and/or concentration of the anion, with reagent hydrophobicity having a considerably more pronounced effect than reagent concentration. HFBA, in particular, achieved an excellent separation at a concentration of just 10 mM, whereby the peptides were separated by charged groups (+1 < +3 < +5) and hydrophobicity within these groups. There was an essentially equal effect of reagent hydrophobicity and concentration on each positive charge of the peptides, a useful observation for prediction of the effect of varying counterion concentration hydrophobicity and/or concentration during optimization of peptide purification protocols. Peak widths were greater for the more highly charged peptides, although these could be decreased significantly by raising the acid concentration; concomitantly, peptide resolution increased with increasing concentration of ion-pairing reagent.
尽管三氟乙酸(TFA)在反相高效液相色谱(RP-HPLC)肽分离中作为首选的阴离子离子对试剂仍占据主导地位,但我们认为,逐步重新审视TFA与其他离子对试剂相比的相对效能是值得的,特别是在设计复杂肽混合物(如蛋白质组学应用中的混合物)的分离方案时。因此,我们在不同浓度的阴离子离子对试剂——磷酸、TFA、五氟丙酸(PFPA)和七氟丁酸(HFBA)存在的情况下,将RP-HPLC应用于三组由四个10肽残基组成的肽混合物,这些组包含净电荷为+1、+3或+5的肽。随着试剂疏水性(磷酸盐<TFA<PFPA<HFBA)和/或阴离子浓度的增加,12肽混合物的整体分离效果得到改善,其中试剂疏水性的影响比试剂浓度更为显著。特别是HFBA,在仅10 mM的浓度下就实现了出色的分离,由此肽按电荷基团(+1<+3<+5)以及这些基团内的疏水性进行分离。试剂疏水性和浓度对肽的每个正电荷的影响基本相同,这一观察结果对于预测在优化肽纯化方案过程中改变抗衡离子浓度、疏水性和/或浓度的效果很有用。电荷较高的肽峰宽更大,不过通过提高酸浓度可显著减小峰宽;同时,肽的分离度随离子对试剂浓度的增加而提高。