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I cleaned up my peptide sample using C18 or desalting columns, but I lost most of my peptides. What went wrong?

Peptides do not bind well to reversed phase resins at neutral pH or in the presence of organic solvents (e.g., acetonitrile). Acidify protein digest samples using formic acid or trifluoroacetic acid (TFA) to pH <3 before desalting. Ensure that samples do not contain organic solvents before and after clean-up by drying them down using a SpeedVac concentrator or equivalent.

I still have detergent present in my sample after protein digestion. Is there anything I can do?

Some detergents can be removed from peptide samples using Pierce Detergent Removal Resin or HiPPR Detergent Removal Spin Columns in the HIPPR (High Protein and Peptide Recovery) format. However, detergents are more easily removed at the protein level using acetone precipitation, dialysis, or affinity capture using Pierce Detergent Removal ResinHiPPR Detergent Removal Spin Columns before protein digestion.

I have a low number of protein identifications from my protein digest sample. What can I do?

We recommend checking your mass spectrometry system performance using the Pierce HeLa Protein Digest Standard (Cat. No. 88328) to help determine if the problem is from the sample preparation or the LC-MS system.

I’m seeing a peak in my mass spectrometry analysis results that seems to always be present in my system. What can I do?

The peak most likely represents PEG or a similar contaminant. Clean your MS system and/or perform sample clean-up using Pierce Peptide Desalting Spin Columns (Cat. No. 89851 or 89852) or Pierce C18 Resin. In addition, ensure that LC-MS pre-blended solvents are being used (formic acid/water, formic acid/acetonitrile, etc.)

I’m seeing extra peaks in my mass spectrometry chromatogram that do not appear to come from my protein sample or the system. Where did they come from and what should I do?

Extra peptides in the sample may be introduced during digestion from self-cleavage of the protease or contaminate proteases. We recommend using LC-MS grade proteases which are purer and modified to reduce the number of autolytic peaks in the sample.

A database search of my peptide samples shows low and/or no identifications, but I have excellent signal in my chromatograph. What might be the problem?

Your mass spectrometry instrument may require calibration. We recommend calibrating using one of our Pierce Calibration Solutions. Additionally, verify that correct search parameters were used for database searching (e.g., species, enzyme, fragment ions, mass tolerance, etc.).

My mass spectrometry system is performing well but my digested peptide sample results are poor. What should I do?

This indicates poor peptide digestion due to improper pH, or incompatible salts (e.g., urea, guanidine etc.).

I have varying amounts of peptide in my samples. Is there a way to determine peptide yield after sample clean-up?

Peptide concentration can be measured using our Pierce Quantitative Fluorometric Peptide Assay (Cat. No. 23290) or Pierce Quantitative Colorimetric Peptide Assay (Cat. No. 23275).

I’m struggling with mass spectrometry sample clean-up and feel that I’m losing peptides. Can you help me verify?

We recommend using the Pierce HeLa Protein Digest Standard (Cat. No. 88328) to test your sample clean-up method. Use it directly and also as a control, co-treated with the sample to check for any loss of peptides.

After TMT reagent labeling, I still see a lot of excess TMT tags in my sample. How should I remove it?

We offer EasyPep MS sample preparation kits (EasyPep Maxi Sample Prep KitEasyPep Mini MS Sample Prep KitEasyPep 96 MS Sample Prep Kit) that contain wash buffers specifically formulated to clean up TMT-labeled protein digests. To remove excess TMT reagent from samples prepared using other sample preparation methods, we recommend using Pierce Peptide Desalting Spin Columns with extra washes using 5% methanol. The Pierce High pH Reversed-Phase Peptide Fractionation Kit can also be used to remove excess unreacted TMT tags before collecting fractions. 

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