Next Article in Journal
Enhanced Treatment of Swine Farm Wastewater Using an O3/Fe2+/H2O2 Process: Optimization and Performance Evaluation via Response Surface Methodology
Previous Article in Journal
CoFeNi-Layered Double Hydroxide Combined Activation of PMS and Ozone for the Degradation of Rhodamine B in Water
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Separations
Volume 12
Issue 10
10.3390/separations12100275
separations-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Investigation of Ethanol and Isopropanol as Greener Alternatives to Acetonitrile in the RP-HPLC Purification of Histone Tail Peptides Bearing Acylation-Type Post-Translational Modifications

by
Yordan Hayat
1,2 and
Zeynep Kanlidere
3,*
1
Department of Medical Biotechnology, Institute of Health Sciences, Acibadem Mehmet Ali Aydinlar University, Istanbul 34752, Türkiye
2
Bioligomer Kimya ve Biyoteknoloji, Istanbul 34776, Türkiye
3
Department of Pharmaceutical Basic Sciences, Faculty of Pharmacy, Acibadem Mehmet Ali Aydinlar University, Istanbul 34752, Türkiye
*
Author to whom correspondence should be addressed.
Separations 2025, 12(10), 275; https://doi.org/10.3390/separations12100275
Submission received: 1 September 2025 / Revised: 24 September 2025 / Accepted: 30 September 2025 / Published: 9 October 2025
Browse Figures
Review Reports Versions Notes

Abstract

Background: Histone post-translational modifications (PTMs) play a pivotal role in the regulation of chromatin structure and gene expression, making them key targets in structural and epigenetic research. Synthetic histone peptides bearing specific PTMs are essential tools for elucidating the molecular mechanisms of histone function and protein–histone interactions. Methods: We synthesized histone H4 tail peptides containing site-specific lysine modifications using solid-phase peptide synthesis (SPPS). The correct synthesis of the peptides was confirmed by their molecular weights using a mass spectrometer. Results: An improved high-performance liquid chromatography (HPLC) method was developed to efficiently separate peptides with one modification difference. In alignment with green chemistry principles, we evaluated ethanol and isopropanol as an alternative organic solvent to acetonitrile in the mobile phase. The optimized HPLC method using acetonitrile enabled effective resolution of closely related peptide species, providing peptides suitable for downstream applications requiring high purities such as structural biology. Conclusions: This study presents a strategy for the purification of histone PTM peptides, emphasizing both analytical performance and sustainability. Further investigation must be undergone to develop high-precision purification using green chemicals.

Graphical Abstract

1. Introduction

Histone proteins and their post-translational modifications (PTMs) play a central role in regulating chromatin structure and gene expression, making them key targets of study in structural biology [1]. More precisely, modifications such as methylation, acylations, and phosphorylation modulate interactions between nucleosomes and associated proteins, thereby influencing cellular processes ranging from transcription to DNA repair [2,3]. To investigate the structural basis of the interaction with these modifications and their impact on chromatin architecture, synthetic histone peptides bearing specific PTMs are widely employed as molecular tools [4,5,6,7,8].
The chemical synthesis of modified histone peptides and their purification are essential for producing homogeneous samples suitable for biochemical and structural studies. In particular, high-purity histone peptides are a prerequisite for successful crystallization and high-resolution structural analysis, such as X-ray crystallography or cryo-EM, where sample quality critically determines experimental outcomes [9]. Obtaining synthetic histone peptides with post-translational modifications in high purity is crucial for advancing PTM-related research.
When the desired PTM containing building blocks are commercially available, the corresponding modification can be directly incorporated during solid-phase peptide synthesis (SPPS). However, in the absence of such modified building blocks, post-synthesis chemical modification strategies become inevitable. In frame of these post-synthesis approaches, optimization of both the incorporation conditions and the purification processes are of paramount importance. For instance, the post-synthesis incorporation of acylations such as an acetyl or a crotonyl group on the lysine side chain would potentially yield two results, one with the desired modification and one unreacted side-product. In these cases, the differences between the unmodified peptide and its PTM-bearing variants are minor. The two sequences differ by only 43 and 70 Daltons, respectively (Figure 1). Furthermore, it is currently difficult to assess quantity by mass spectrometry thus, a heterogeneous sample including these two products would have an uncertain purity level. Even though the mass shift is minor, the differences can significantly influence downstream applications. That is why it would be ideal to obtain 100% yield during the modification and approve the absence of the unreacted side product by mass spectrometry, but this cannot be always achieved. The only remaining option to obtain high-purity product is to be able to elute those two species separately. Therefore, precise and efficient purification is essential to ensure the homogeneity of the final PTM-modified histone product. The study of PTM-bearing peptide purification has not been extensively elaborated in the literature.
Peptides are commonly purified using high-performance liquid chromatography (HPLC), a crucial step to obtain high-purity products for research and therapeutic applications. In HPLC, acetonitrile is widely used as an organic solvent due to its polarity character, low viscosity, and miscibility with water. It offers an effective elution capability with minimal UV absorbance above 190 nm, and low system backpressure. These characteristics make acetonitrile particularly well-suited for high-resolution separations and fractionations in biomolecular analysis, but it is toxic and harmful. Moreover, according to the International Council for Harmonisation (ICH) guidelines, acetonitrile (ACN) is designated as a Class 2 solvent that should be limited in pharmaceutical products because of its inherent toxicity [10]. Therefore, in recent years, academia and industry have started searching for greener alternatives for both synthesis and purification of peptides [11,12,13]. The physical properties of some green solvents that could be alternatives to the frequently used acetonitrile and methanol are summarized in Table 1. However, not all green solvents are suitable for peptide purification, as some may not dissolve peptides well or offer proper separation or simply not compatible with the current purification instrumentations. Therefore, separation efficiency is influenced by the physicochemical properties of the solvent alongside those of the peptide, column, stationary phase, and the purification setup. So far, in HPLC studies, solvents like methanol, ethanol, and isopropanol, which are less harmful and mix well with water, have been tested as alternatives to acetonitrile [14,15,16,17,18]. Employing these greener solvents not only minimizes the environmental footprint but also promotes safer working conditions in the laboratory.
In this study, we focus on the separation of histone H4 tail peptides bearing different site-specific lysine modifications. Specifically, we examine two peptide sequences that differ solely by the presence of a crotonyl group. To address this subtle difference, which corresponds to only a few additional atoms, we aim to optimize a HPLC method capable of efficiently resolving such closely related peptide species. The current literature lacks references on the purification of PTM-bearing histone peptides. Researching efficient methods for this purpose will inevitably accelerate PTM-related discoveries in molecular biology. More generally, the development of an HPLC method that can accurately distinguish modified peptides from their unmodified counterparts is particularly critical for the analysis of a multitude of peptides generated through post synthetic modifications. On the other hand, metabolomics and proteomics studies can benefit from this research for the isolation and identification of different PTM-bearing molecules present in the cell. Furthermore, in alignment with green chemistry principles, we have chosen to investigate the use of ethanol and isopropanol based on their UV cut-off and polarity (Table 1) as an alternative mobile phase component to acetonitrile to ensure a reduced environmental impact while conducting basic research.

2. Materials and Methods

2.1. Reagents and Chemicals

All chemicals and reagents used were of analytical grade, unless otherwise specified. For peptide synthesis, Fmoc-amino acids, coupling reagents, Rink amide resin, DMF, DCM, piperidine, and TFA were obtained from Merck (Darmstadt, Germany). HPLC-grade solvents were purchased from Merck (Darmstadt, Germany).

2.2. Peptide Synthesis, Purification and Characterization

Histone H4 tail peptides (residues 1–18) were synthesized on a fully automated peptide synthesizer (Aapptec, Louisville, KY, USA) at 0.1 mmol scale using Fmoc chemistry on Rink amide resin. Site-specific lysine modifications were incorporated using commercially available Fmoc-Lys(Ac)-OH or Fmoc-Lys(Cro)-OH derivatives. Following synthesis, peptides were cleaved from the resin using a cleavage cocktail composed of TFA/TIS/H2O in a ratio of 95:2.5:2.5 for 1 h at room temperature. After cleavage, the crude peptides were precipitated in cold diethyl ether, collected by centrifugation, and dried under nitrogen flow. Crude products were then dissolved in water and purified on a reversed-phase C18 column (5 μm; 250 × 4.6 mm, Shim-pack GISS, Shimadzu, Kyoto, Japan) using a high-performance liquid chromatography system equipped with DAD detector (Shimadzu Nexera Prep, Kyoto, Japan). Gradient elution was performed using different combinations of two mobile phases, both including 0.05% TFA: solvent A was water in all cases and solvent B was either acetonitrile, ethanol, or isopropanol. Purified peptides were analyzed by liquid chromatography–tandem mass spectrometry (LC-MS/MS) using an Agilent 6420 Triple Quadrupole (Agilent Technologies, Santa Clara, CA, USA) and a Q Exactive Hybrid Quadrupole-Orbitrap mass spectrometer (Thermo Fisher Scientific, Waltham, MA, USA).

2.3. Mathematical Formulas Used for the Analysis of Chromatograms

2.3.1. Theoretical Plates

The number of theoretical plates (N) is calculated to assess column efficiency using Equation (1), where tR is the retention time of the peptide (in minutes) and W0.5 is the peak width at half-height (in minutes).
N = 5.54 × t R W 0.5 2

2.3.2. Height Equivalent to a Theoretical Plate (HETP)

The column efficiency is evaluated by calculating the Height Equivalent to a Theoretical Plate (HETP) using Equation (2), where L is the length of the chromatographic column and N is the number of theoretical plates.
H = L × 1000 N   ( μ m )

2.3.3. Tailing Factor

Peak symmetry is assessed by calculating the tailing factor (Tf) using Equation (3), where W0.05 is the width of the peak at 5% of the peak height and Q0.05 is the distance from the peak maximum to the front of the peak at 5% of the peak height.
T f = W 0.05 2 × Q 0.05

2.3.4. Resolution

The resolution (R) between two adjacent peaks was calculated with Equation (4) to evaluate the separation efficiency, where tR and tRP are the retention times of the first and second eluting peaks, and W0.5 and WP0.5 are the respective baseline peak widths of the two compounds.
R = 1.18 × t R t R P W 0.5 + W P 0.5

2.3.5. The Capacity Factor k’

The capacity factor (k′) was calculated to assess the retention of the peptides under the chromatographic conditions, using Equation (5) where t is the retention time of the peptide and t0 is the column void time.
k = t t 0 1

3. Results

We synthesized two different peptides derived from the same histone H4 sequence (Table 2). One peptide contained a single post-translational modification (PTM), an acetylated lysine, while the other carried two distinct PTMs: one acetylated lysine and one crotonylated lysine.
Following synthesis, the peptides were subjected to purification by high-performance liquid chromatography (HPLC). The conventional HPLC peptide purification protocol uses elution on a C18 column with an increasing gradient of acetonitrile in water. Several parameters must be considered while choosing a C18 column, including particle and pore size, carbon loading, and column dimensions. Due to pressure limits, we could choose 5 μm particle size at best. Additionally, we decided to use a 200 Å pore size based on the peptides’ molecular weights. Finally, we took a 250 mm long column to ensure the best resolution possible. HPLC profile of crude peptides are given in Supplementary Figures S1 and S2 for H4K5ac and H4K5acK8cro, respectively.
The molecular weight of the synthesized peptides were verified by LC-MS/MS, and their spectra are provided in the Supplementary Files (Figures S3–S10). The calculated monoisotopic m/z values for the fragment ions of peptides H4K5ac and H4K5acK8cro are listed in Table 3. The detection of molecular ion peaks with +2, +3, and +4 charge states in the MS spectra of the peptide H4K5ac confirmed its proper synthesis. Likewise, the synthesis of the peptide H4K5acK8cro was confirmed with the presence of +2, +3, +4 charge states in its MS spectra.
Once we obtained our two peptides of interest, we first wanted to validate the maximum concentration of acetonitrile that would elute the peptides. We first tested a run with the 5 to 80% in 30 min protocol that translated to an increment of 2.5% acetonitrile per minute. Finding the maximum concentration that elutes the peptides helps in shortening the HPLC method to gain time for the following runs but also limits solvent consumption. In that sense, we individually ran peptide H4K5acK8cro (Figure 2A), which was more hydrophobic and should elute later than peptide H4K5ac. That result indicated that peptide H4Kac5K8cro already eluted by minute 20. This led us to shorten the method by finishing it at 52% acetonitrile instead of 80%. To validate the percentage of elution, both peptides were run individually with the new 5 to 52% in 19 min. Peptide H4K5acK8cro eluted at minute 20 (Figure 2B) and H4K5ac eluted at minute 15 (Figure 2C). Since the elution times of these two peptides differed significantly with this gradient, the method was deemed suitable for subsequent tests aimed at separating the two molecules. To validate the method, we prepared a mixture of the two peptides and co-injected them. As expected, the two peptides eluted separately (Figure 2D). We evaluated the separation efficiency with the respective number of theoretical plates and resolution parameters summarized in Table 4.
Having demonstrated that these two peptides eluted separately with acetonitrile on our C18 column, we next explored the use of alternative solvents more aligned with green chemistry principles. In this context, ethanol was selected as the first candidate. Although ethanol is considered a greener solvent, its higher viscosity compared to acetonitrile (Table 1) results in increased backpressure on the column. One common strategy to mitigate this issue is to increase the mobile phase temperature using a column oven. However, as our HPLC system was not equipped with a column oven, we instead reduced the flow rate to avoid exceeding the 200 bar pressure limit of the column. Upon co-injection of the peptide mixture and analysis using a 5% to 52% gradient method, only a single peak was observed at 30 min, indicating co-elution of the peptides (Figure 3A). To assess whether ethanol could achieve separation of the peptides using the existing column, we opted to reduce the gradient to 1% per minute (Figure 3B), as opposed to the 2.5% per minute previously applied with acetonitrile, prior to evaluating alternative columns. Despite the modified gradient, both peptides still co-eluted as a single peak.
Before pursuing further optimization with ethanol, we decided to also evaluate isopropanol as a substitute for acetonitrile, given that its polarity is more similar to that of acetonitrile. However, like ethanol, isopropanol presents challenges due to its higher viscosity. Consequently, it was necessary to also reduce the flow rate when using this solvent. Using the 5% to 52% gradient method, we observed that the peptides did not bind to the column, as a single peak appeared in the unbound fraction (Figure 4A). To promote peptide adsorption, we modified the method to start the gradient from 0% instead of 5%. As anticipated, initiating the gradient at 0% allowed the peptides to bind to the column, as evidenced by their elution occurring after the unbound fraction. However, despite improved retention, the peptides continued to co-elute as a single peak (Figure 4B).

4. Discussion

Using an increasing gradient of acetonitrile, we successfully achieved the separation of two peptide molecules differing by only 70 Da. Having such a precise purification method is crucial for accurately assessing purity levels when incorporating post-translational modifications (PTMs) after peptide synthesis. To align with green chemistry principles, we first developed a shorter method, recognizing that minimizing solvent consumption is as important as selecting environmentally friendly solvents. Furthermore, we explored ethanol and isopropanol as alternative solvents to acetonitrile. We limited our study to these two solvents because their UV cut-off permitted peptide monitoring by UV at 214nm. Indeed, the solvent’s UV cut-off value must be below the UV absorption maxima of the studied molecule. At the same time, the solvent’s viscosity must be low to avoid generating high column backpressure. For example, glycerol has a UV cut-off below 214 nm but its high viscosity (Table 1) makes it almost impossible to use in HPLC studies. Alternatively, a mass detector could be used instead of a UV detector; however, this setup is less common in laboratories and thus difficult to access. Even so, there are applications in the literature, for example, some research has been conducted with acetone, demonstrating that it can successfully replace acetonitrile in RP-HPLC when mass spectrometry detectors are used for peptide analysis [19,20,21]. However, as stated above, UV detectors are still the most commonly used in pharmaceutical analysis, meaning acetone is not a favored green solvent to substitute acetonitrile in RP-HPLC. Another green solvent, dimethyl carbonate (DMC), is considered a promising alternative for industrial use. Recently, a study by Bozza et al. [22] showed that DMC could be used in the mobile phase for preparative chromatography to purify a therapeutic peptide (Icatibant). However, its use in liquid chromatography is still very limited [23], which might be due to the lack of commercially available HPLC-grade DMC. In frame with the objective of our study, it might be promising to also test DMC in the future, when HPLC-grade DMC will become available.
For the reasons mentioned above, our study was limited to only three solvents. Among them, acetonitrile remained the most effective, as it was the only one that enabled the separation of peptides differing by just 70 Da in molecular weight using our C18 column (5 μm, 4.6 × 250 mm). At present, we were unable to achieve baseline separation of these peptides using ethanol or isopropanol. A plausible reason could be the molecular interactions between the mobile phase, the peptide and the stationary phase. Ethanol and isopropanol are polar protic solvents, whereas acetonitrile misses hydrogen atoms, making it aprotic but still polar. Thus, compared to acetonitrile, the greener solvents evaluated in this study might have stronger interactions with the peptides due to hydrogen bonds formed with the solvent’s alcohol groups. Additionally, compared to acetonitrile, ethanol and isopropanol should have fewer interactions with the C18 column. The protic solvents’ higher affinity towards the peptides relative to the stationary phase could be eluting the peptides more rapidly from the C18 stationary phase; thus, it would decrease the elution sensitivity for closely similar moieties. Similarly, the protic solvents’ weaker affinity towards the C18 hydrophobic stationary phase may lead to heterogeneous interactions between the solvent, column, and peptides. Achieving a more homogeneous distribution between the mobile and stationary phases could improve the separation of similar peptides. As the two peptides in this study differ by only a single charge on the lysine residue, it might be difficult to separate them based on hydrogen interactions. The addition of acylation on lysine residues removes their charge. It would be more suitable to have significant charge differences between the peptides to separate them when working with protic solvents. Furthermore, a hydrophilic stationary phase might give more promising results for separations based on hydrogen interactions. This kind of alternative stationary phase screening should also be tested in the future for the investigation of ethanol and isopropanol in the purification of PTM-bearing peptides. In conclusion, our findings should not be interpreted as a definitive limitation of these solvents for the purification of PTM-bearing peptides. Other post-translational modifications, which were not examined in this study, may respond differently to these solvents. Moreover, the absence of a column oven in our setup hindered full optimization, as elevated temperatures could reduce solvent viscosity and improve chromatographic performance. However, with industrial applications in mind, a green solvent capable of separating these two peptides without heating would be more suitable, since column ovens are rarely used at industrial scale.
In summary, an RP-HPLC method capable of separating PTM-bearing peptides was found. Additionally, for future greener approaches, testing different HPLC columns, both hydrophobic but also hydrophilic, alongside broader solvent screening is necessary.

Supplementary Materials

The following supporting information can be downloaded at https://www.mdpi.com/article/10.3390/separations12100275/s1, Figure S1: HPLC profile of crude peptide H4K5ac; Figure S2: HPLC profile of crude peptide H4K5acK8cro; Figure S3: Full mass spectra for H4K5ac; Figure S4: H4K5ac mass spectra region at m/z 1100; Figure S5: H4K5ac mass spectra region at m/z 734; Figure S6: H4K5ac mass spectra region at m/z 550; Figure S7: Full mass spectra for H4K5acK8cro; Figure S8: H4K5acK8cro mass spectra region at m/z 1135; Figure S9: H4K5acK8cro mass spectra region at m/z 757; Figure S10: H4K5acK8cro mass spectra region at m/z 568.

Author Contributions

Conceptualization, Z.K. and Y.H.; methodology, Z.K. and Y.H.; investigation, Z.K. and Y.H.; resources, Z.K. and Y.H.; data curation, Z.K. and Y.H.; writing— original draft preparation, Z.K. and Y.H.; writing—review and editing, Z.K. and Y.H.; visualization, Z.K. and Y.H.; All authors have read and agreed to the published version of the manuscript.

Funding

No direct funding was received for this study.

Data Availability Statement

Data will be made available on reasonable request.

Conflicts of Interest

Author Y.H. is director of company Bioligomer. The authors declare the research was conducted in the absence of any influence that could be construed as a potential conflict of interest.

References

  1. Millán-Zambrano, G.; Burton, A.; Bannister, A.J.; Schneider, R. Histone post-translational modifications—Cause and consequence of genome function. Nat. Rev. Genet. 2022, 23, 563–580. [Google Scholar] [CrossRef] [PubMed]
  2. McDermott, C.; Gaona-Gamboa, A.; Lee, S.H.; Sesco, E.; Deppmann, C. The Role of Posttranslational Modification in Cellular Function. In eLS; John Wiley & Sons: Hoboken, NJ, USA, 2025. [Google Scholar]
  3. Liu, R.; Wu, J.; Guo, H.; Yao, W.; Li, S.; Lu, Y.; Jia, Y.; Liang, X.; Tang, J.; Zhang, H. Post-translational modifications of histones: Mechanisms, biological functions, and therapeutic targets. MedComm 2023, 4, e292. [Google Scholar] [CrossRef] [PubMed]
  4. Wu, D.; Liu, T. Studying Reversible Protein Post-translational Modification through co-translational Modification. ChemBioChem 2023, 24, e202200716. [Google Scholar] [CrossRef] [PubMed]
  5. Müller, M.M.; Muir, T.W. Histones: At the Crossroads of Peptide and Protein Chemistry. Chem. Rev. 2015, 115, 2296–2349. [Google Scholar] [CrossRef]
  6. Merx, J.; Hintzen, J.C.J.; Proietti, G.; Elferink, H.; Wang, Y.; Porzberg, M.R.B.; Sondag, D.; Bilgin, N.; Park, J.; Mecinović, J.; et al. Investigation of in vitro histone H3 glycosylation using H3 tail peptides. Sci. Rep. 2022, 12, 19251. [Google Scholar] [CrossRef]
  7. Papini, A.M. The use of post-translationally modified peptides for detection of biomarkers of immune-mediated diseases. J. Pept. Sci. 2009, 15, 621–628. [Google Scholar] [CrossRef]
  8. Nuti, F.; Peroni, E.; Real-Fernández, F.; Bonache, M.A.; Le Chevalier-Isaad, A.; Chelli, M.; Lubin-Germain, N.; Uziel, J.; Rovero, P.; Lolli, F.; et al. Posttranslationally modified peptides efficiently mimicking neoantigens: A challenge for theragnostics of autoimmune diseases. Pept. Sci. 2010, 94, 791–799. [Google Scholar] [CrossRef]
  9. Tsunaka, Y.; Furukawa, A.; Nishimura, Y. Histone tail network and modulation in a nucleosome. Curr. Opin. Struct. Biol. 2022, 75, 102436. [Google Scholar] [CrossRef]
  10. International Council for Harmonisation (ICH). Q3C(R9) Impurities: Guideline for Residual Solvents. EMA/CHMP/ICH/82260/2006. 29 April 2024. Available online: https://www.ema.europa.eu/en/ich-q3c-r9-residual-solvents-scientific-guideline (accessed on 30 August 2025).
  11. Al Musaimi, O.; de la Torre, B.G.; Albericio, F. Greening Fmoc/tBu solid-phase peptide synthesis. Green Chem. 2020, 22, 996–1018. [Google Scholar] [CrossRef]
  12. Mthethwa, N.; Nandhini, K.P.; Kumar, A.; Sharma, A.; de la Torre, B.G.; Albericio, F. Toward sustainable solid-phase peptide synthesis strategy—In situ Fmoc removal. Green Chem. Lett. Rev. 2024, 17, 2325993. [Google Scholar] [CrossRef]
  13. Pacini, L.; Muthyala, M.; Aguiar, L.; Zitterbart, R.; Rovero, P.; Papini, A.M. Optimization of peptide synthesis time and sustainability using novel eco-friendly binary solvent systems with induction heating on an automated peptide synthesizer. J. Pept. Sci. 2024, 30, e3605. [Google Scholar] [CrossRef]
  14. Brettschneider, F.; Jankowski, V.; Günthner, T.; Salem, S.; Nierhaus, M.; Schulz, A.; Zidek, W.; Jankowski, J. Replacement of acetonitrile by ethanol as solvent in reversed phase chromatography of biomolecules. J. Chromatogr. B 2010, 878, 763–768. [Google Scholar] [CrossRef]
  15. Gaudin, K. Potential of green solvents as mobile phases in liquid chromatography. J. Chromatogr. A 2025, 1750, 465810. [Google Scholar] [CrossRef] [PubMed]
  16. Ferrazzano, L.; Corbisiero, D.; Catani, M.; Cavazzini, A.; Martelli, G.; Cantelmi, P.; Fantoni, T.; Mattellone, A.; De Luca, C.; Felletti, S.; et al. Sustainability in peptide chemistry: Current synthesis and purification technologies and future challenges. Green Chem. 2022, 24, 975–1020. [Google Scholar] [CrossRef]
  17. Maráková, K. Greening Separation and Purification of Proteins and Peptides. J. Sep. Sci. 2024, 47, e202400554. [Google Scholar] [CrossRef] [PubMed]
  18. Panjwani, D.; Patel, A.; Mishra, D.; Patel, S.; Patel, V.; Yadav, M.R.; Singh, B. Green RP-HPLC method for the estimation of carfilzomib in bulk, protein nanocarriers and human plasma: Application of chemometrics and Monte-Carlo simulations. J. Chromatogr. B 2024, 1249, 124350. [Google Scholar]
  19. Yabré, M.; Ferey, L.; Somé, I.T.; Gaudin, K. Greening Reversed-Phase Liquid Chromatography Methods Using Alternative Solvents for Pharmaceutical Analysis. Molecules 2018, 23, 1065. [Google Scholar] [CrossRef]
  20. Fritz, R.; Ruth, W.; Kragl, U. Assessment of acetone as an alternative to acetonitrile in peptide analysis by liquid chromatography/mass spectrometry. Rapid Commun. Mass Spectrom. 2009, 23, 2139–2145. [Google Scholar] [CrossRef]
  21. Keppel, T.R.; Jacques, M.E.; Weis, D.D. The use of acetone as a substitute for acetonitrile in analysis of peptides by liquid chromatography/electrospray ionization mass spectrometry. Rapid Commun. Mass. Spectrom. 2010, 24, 6–10. [Google Scholar] [CrossRef]
  22. Bozza, D.; De Luca, C.; Felletti, S.; Spedicato, M.; Presini, F.; Giovannini, P.P.; Carraro, M.; Macis, M.; Cavazzini, A.; Catani, M.; et al. Dimethyl carbonate as a green alternative to acetonitrile in reversed-phase liquid chromatography Part II: Purification of a therapeutic peptide. J. Chromatogr. A 2024, 1713, 464530. [Google Scholar] [CrossRef]
  23. Felletti, S.; Spedicato, M.; Bozza, D.; De Luca, C.; Presini, F.; Giovannini, P.P.; Carraro, M.; Macis, M.; Cavazzini, A.; Catani, M.; et al. Dimethyl carbonate as a green alternative to acetonitrile in reversed-phase liquid chromatography. Part I: Separation of small molecules. J. Chromatogr. A 2023, 1712, 464477. [Google Scholar] [CrossRef]
Separations 12 00275 g001
Figure 1. Structures of lysine bearing acylation type of post-translational modifications.
Figure 1. Structures of lysine bearing acylation type of post-translational modifications.
Separations 12 00275 g001
Separations 12 00275 g002
Figure 2. HPLC chromatogram obtained using acetonitrile with 1 mL/min flow rate and, respectively, gradients of (A) 5 to 80% in 30 min for peptide H4K5acK8cro; (B) 5 to 52% in 19 min for peptide H4K5acK8cro; (C) 5 to 52% in 19 min for peptide H4K5ac; (D) 5 to 52% in 19 min for co-injection of peptides H4K5ac and H4K5acK8cro.
Figure 2. HPLC chromatogram obtained using acetonitrile with 1 mL/min flow rate and, respectively, gradients of (A) 5 to 80% in 30 min for peptide H4K5acK8cro; (B) 5 to 52% in 19 min for peptide H4K5acK8cro; (C) 5 to 52% in 19 min for peptide H4K5ac; (D) 5 to 52% in 19 min for co-injection of peptides H4K5ac and H4K5acK8cro.
Separations 12 00275 g002
Separations 12 00275 g003
Figure 3. HPLC chromatogram of peptides H4K5ac and H4K5acK8cro co-injection obtained using ethanol with 0.5 mL/min flow rate and, respectively, gradients of (A) 5 to 52% in 38 min; (B) 5 to 52% in 76 min.
Figure 3. HPLC chromatogram of peptides H4K5ac and H4K5acK8cro co-injection obtained using ethanol with 0.5 mL/min flow rate and, respectively, gradients of (A) 5 to 52% in 38 min; (B) 5 to 52% in 76 min.
Separations 12 00275 g003
Separations 12 00275 g004
Figure 4. HPLC chromatogram of peptides H4K5ac and H4K5acK8cro co-injection obtained using isopropanol with 0.35 mL/min flow rate and, respectively, gradients of (A) 5 to 52% in 100 min; (B) 0 to 35% in 100 min.
Figure 4. HPLC chromatogram of peptides H4K5ac and H4K5acK8cro co-injection obtained using isopropanol with 0.35 mL/min flow rate and, respectively, gradients of (A) 5 to 52% in 100 min; (B) 0 to 35% in 100 min.
Separations 12 00275 g004
Table 1. Physical properties of different solvents [15].
Table 1. Physical properties of different solvents [15].
SolventUV Cut-Off (nm)Polarity (K-T π)Viscosity (MPa.s)HPLC Grade
Acetonitrile1900.750.35yes
Ethanol2100.541.07yes
Isopropanol2100.482.04yes
Acetone3300.710.32yes
Dimethyl carbonate2800.770.66no
Ethyl lactate2550.602.53no
Propylene carbonate2550.902.51no
Glycerol2070.92954no
Table 2. Synthesized histone H4 peptides and their modifications.
Table 2. Synthesized histone H4 peptides and their modifications.
Peptide NameSequenceModificationsMW (Da)
H4K5acSGRGK(ac)GGKGLGKGGAKRHGSGSYAcetylation2200.46
H4K5acK8croSGRGK(ac)GGK(cro)GLGKGGAKRHGSGSYAcetylation,
Crotonylation		2268.53
Table 3. Calculated and found m/z values for the ion fragments of peptides H4K5ac and H4K5acK8cro.
Table 3. Calculated and found m/z values for the ion fragments of peptides H4K5ac and H4K5acK8cro.
H4K5acH4K5acK8cro
CalculatedFoundCalculatedFound
M2199.170-2267.200-
[M+1H]+2200.177-2268.207-
[M+2H]2+1100.5921100.5921134.6071134.609
[M+3H]3+734.064734.064756.741756.740
[M+4H]4+550.800550.800567.807567.809
[M+5H]5+440.841-454.447-
Table 4. Performance parameters * obtained during the separation of H4K5ac and H4K5acK8cro using acetonitrile (Figure 2D).
Table 4. Performance parameters * obtained during the separation of H4K5ac and H4K5acK8cro using acetonitrile (Figure 2D).
Retention TimeNHTfRk
H4K5ac16.5485330.93.067-0.000
H4K5acK8cro19.7544027.64.4143.2510.199
* Abbreviations, definitions and formulas are detailed in Section 2.3.
Disclaimer/Publisher’s Note: The statements, opinions and data contained in all publications are solely those of the individual author(s) and contributor(s) and not of MDPI and/or the editor(s). MDPI and/or the editor(s) disclaim responsibility for any injury to people or property resulting from any ideas, methods, instructions or products referred to in the content.

Share and Cite

MDPI and ACS Style

Hayat, Y.; Kanlidere, Z. Investigation of Ethanol and Isopropanol as Greener Alternatives to Acetonitrile in the RP-HPLC Purification of Histone Tail Peptides Bearing Acylation-Type Post-Translational Modifications. Separations 2025, 12, 275. https://doi.org/10.3390/separations12100275

AMA Style

Hayat Y, Kanlidere Z. Investigation of Ethanol and Isopropanol as Greener Alternatives to Acetonitrile in the RP-HPLC Purification of Histone Tail Peptides Bearing Acylation-Type Post-Translational Modifications. Separations. 2025; 12(10):275. https://doi.org/10.3390/separations12100275

Chicago/Turabian Style

Hayat, Yordan, and Zeynep Kanlidere. 2025. "Investigation of Ethanol and Isopropanol as Greener Alternatives to Acetonitrile in the RP-HPLC Purification of Histone Tail Peptides Bearing Acylation-Type Post-Translational Modifications" Separations 12, no. 10: 275. https://doi.org/10.3390/separations12100275

APA Style

Hayat, Y., & Kanlidere, Z. (2025). Investigation of Ethanol and Isopropanol as Greener Alternatives to Acetonitrile in the RP-HPLC Purification of Histone Tail Peptides Bearing Acylation-Type Post-Translational Modifications. Separations, 12(10), 275. https://doi.org/10.3390/separations12100275

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop