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- Posts: 2
- Joined: Fri Sep 13, 2024 6:20 am
- Location: Paris
I am currently having trouble fine-tuning my HPLC gradient approach in order to achieve better separation because I am working with a complicated mixture of peptides. A C18 column (150 x 4.6 mm, 5 µm) with a 0.1% formic acid mobile phase and a conventional water/acetonitrile gradient is what I'm using. Getting decent resolution is challenging because the hydrophobicity of the peptides in my combination varies a lot in this community.
The details of my current approach are as follows:
- Column dimensions: 150 x 4.6 mm / 5 µm
- Phase A of mobility: Water plus 0.1% formic acid
- Phase B mobile: 0.1% formic acid + acetonitrile
- Gradient: 30 minutes, 5–50% B
- One millilitre per minute of flow
- UV light detected at 214 nm
Has anyone else worked with peptide mixes and encountered problems comparable to these? Would switching to a different column (perhaps one with a shorter or lower particle size) or modifying the pH of the mobile phase be helpful? I'm not sure if using ion-pairing reagents—which I've read some people use—would be appropriate in this situation.
I would be grateful for any guidance on gradient optimisation, choosing a mendix rapid column, or other possible tactics!
Thank you in advance.