The 99% Standard:
Advanced Purity Analysis

In the unregulated landscape of research peptides, “purity” is often a marketing buzzword rather than a scientific metric. Vendors frequently claim “>99% purity” without providing raw data, or provide chromatograms that obscure impurities.

For serious research, reagent quality matters. A peptide at 95% may look fine, but the remaining 5%—truncations, deletion peptides, and residual solvents—can alter binding, introduce confounds, and quietly wreck your experiment.

This guide helps you audit Certificates of Analysis (COA) and interpret core purity / identity data.

1. High-Performance Liquid Chromatography (HPLC)

HPLC separates mixture components based on interaction with the stationary phase (column) and mobile phase (solvent). The elution time is the Retention Time (R_t).

Methodology & Parameters

Analytical peptide testing commonly uses Reverse-Phase (RP-HPLC): non-polar stationary phase and polar mobile phase.

Interpreting the Chromatogram

The output is Absorbance (mAU) vs. Time (min).

• Main Peak: target peptide; should be sharp and symmetric.
• Baseline: should be stable; drift suggests contamination or equilibration issues.
• Side Peaks: impurities; peaks before/after main peak indicate different species.

2. Mass Spectrometry (MS) & Identity

HPLC tells you how clean the sample is; MS tells you what it is by measuring m/z (mass-to-charge).

Peptides are commonly run by ESI-MS (electrospray ionization), a “soft” ionization method that preserves intact molecular ions.

Understanding Charge States

Peptides often pick up multiple protons, creating multiple charge-state peaks.

• [M+H]⁺: MW + 1
• [M+2H]²⁺: (MW + 2) / 2
• [M+3H]³⁺: (MW + 3) / 3

A clean spectrum shows dominant peaks matching the theoretical MW. Extra unexplained peaks suggest byproducts or co-eluting impurities.

3. The Impurity Library: What Hides in the Data

Impurities in SPPS generally fall into a few categories—each one tells a story about synthesis quality.

A. Deletion Sequences (Truncated Peptides)

Missing one or more residues due to incomplete coupling. A 30-mer might include a 29-mer impurity.

Cause: incomplete coupling / steric hindrance.
Detection: often better seen in MS (mass lower by the missing residue).

B. Diastereomers (Racemization)

L→D epimerization during harsh coupling can create same-mass species with different 3D structure.

Impact: potency changes; MS may not reveal it.
Detection: specialized chiral methods.

C. Oxidation Products

Met/Cys/Trp can oxidize during processing/storage. Methionine oxidation often shows a +16 Da shift and may change retention.

D. Dimerization

Cysteine-containing peptides can form disulfide-linked dimers (2× MW), often inactive and potentially confounding.

4. Counter-Ion Analysis: Acetate vs. TFA

Peptides are commonly isolated as salts. After TFA cleavage, many arrive as [Peptide]⁺ [TFA]⁻.

Why it matters: counter-ions can impact downstream work. Many labs prefer exchanging TFA for acetate or chloride depending on application requirements.

5. Residual Moisture & Karl Fischer Titration

Lyophilized peptides are hygroscopic. Even good freeze-drying leaves some bound water.

Purity vs. content: “99% purity” does not mean 99% of the vial weight is peptide. Powder weight includes salts (counter-ions) and water.

Example:
10 mg powder
− 15% counter-ions
− 5% residual water
= 80% net peptide content (8 mg peptide)

Karl Fischer titration is commonly used to quantify residual water for accurate dosing calculations.

6. The Researcher’s Checklist

Before running experiments, verify:

1. HPLC trace: peak symmetry, baseline stability, integrated purity target met.
2. MS spectrum: major ions match theoretical MW; no suspicious extra peaks.
3. Counter-ion: salt form matches your assay needs (e.g., acetate vs. TFA).
4. Net content: account for salts + moisture for molar-accurate work.
5. Appearance: consistent lyophilized cake; discoloration can indicate degradation.

“Data is only as good as the reagent it is derived from.”