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Why do some methods use low pH buffers to separate acidic compounds?

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Why do some methods use low pH buffers to separate acidic compounds?

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By suppressing their ionization at low pH, acids will be more like neutral compounds and will retain on HPLC columns much the same way that neutral compounds will. Another benefit of running on Type A and Type B silica at low pH is that the silanol activity is reduced. This should sharpen your peaks.

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