Table 5.
Summary of collagenase activity assays
| Method | Substrate | Enzyme activity | Benefit | Drawbacks | References |
|---|---|---|---|---|---|
| Rosen assay | Collagen | After a reaction at pH 7.4 and 37 °C (presence of calcium ions) for 5 h, the amount of peptides released from collagen was equal to the amount of color development of 1 μmol of leucine and ninhydrin, which was a CDU (one collagen digestion unit). | Qualitative and quantitative accuracy and reliability | The reaction time is long, and ninhydrin easily fades after color development | [40,89] |
| Synthetic peptide | FALGPA/Pz peptide | One FALGPA unit refers to the hydrolysis of 1 μmol of FALGPA per minute at 25 °C pH 7.5 (calcium ions present). | Rapid reaction, the substrate is stable and invariable, suitable for large-scale inspection | Does not directly reflect the hydrolytic activity of collagenase toward natural collagen | [86,90] |
| Electrophoresis assay | Gelatin | / | Rapid qualitative analysis | Unquantifiable | [86] |
| Azocoll assay | Azocoll | The light absorption value at A520 is increased by 1.0 per minute, which is defined as one unit of enzyme activity. | The operation is simple, the specificity is high, the colored hydrolysate is stable | Does not directly reflect the hydrolytic activity of collagenase toward natural collagen | [57] |
| Isotope labeling | 14C-labeled collagen | Scintillation counting is performed to characterize enzyme activity, and collagenase activity is represented by the dpm value. | The sensitivity is high, suitable for in vivo testing | The equipment is expensive and produces radioactive contamination | [91] |
| Fluorescence labeling | FITC-collagen | / | Qualitative and quantitative accuracy and reliability | The substrate is expensive, the solvent affects the fluorescence intensity | [92,93] |