Determine the necessary mass, volume, or concentration for preparing a solution.
Bioactive,ActiBioPure™,Native,High Performance,EnzymoPure™,≥450 U/mg enzyme powder ActiBioPure™,Bioactive,High Performance,Native,EnzymoPure™ for sensitive chromatographic and analytical workflows requiring minimal baseline interference.
Store at -20°C,Avoid repeated freezing and thawing Ships Ice chest + Ice pads Check lot-specific COA for exact specifications.
SDS, COA, datasheet, and spec sheet available for download. Lot-specific COA accessible via lot number lookup.
Cited in 1 peer-reviewed publications across chromatography, organic synthesis, and cross-coupling reactions.
Creatinine Amidohydrolase catalyzes the hydrolytic reaction converting creatinine to creatine. The enzyme is purified from a microorganism. The molecular size of the enzyme is approximately 175,000. The enzyme is useful for the enzy-matic assay of creatinine when coupled with other related enzymes.
Reaction formula: Creatinine + H₂O → Creatine
PREPARATION and SPECIFICATION
| Appearance: | White amorphous powder, lyophilized |
| Activity: | ≥450 U/mg powder |
| Contaminants: | NADH oxidase ≤5.0×10⁻²%; Catalase ≤2.0% |
| Stabilizers: | Sucrose, BSA |
PROPERTIES
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APPLICATIONS
This enzyme is useful for enzymatic determination of creatinine when coupled with creatine amidinohydrolase (CRH-211, CRH-221, CRH-229) and sarcosine oxidase (SAO-351) in clinical analysis.
ASSAY
Principle:

The appearance of creatinine-picrate (orange dye based on Jaffe's reaction) is measured at 520nm by spectrophotometry.
Unit definition:
One unit causes the formation of one micromole of orange dye per minute under the conditions described below.
Method:
Reagents
A. Creatine solution: 0.1M [1.49g creatine (Nacalai tesque)/100ml of 50mM phosphate buffer, pH 7.5] (Should be prepared fresh)
B. NaOH solution: 0.5N
C. Picric acid solution: 1.0% (W/V)
D. Enzyme diluent: 50mM phosphate buffer, pH 7.5
Procedure
1. Pipette 1.0ml of the substrate solution (A) into a test tube and equilibrate at 37℃ for about 5 minutes.
2. Add 0.1ml of the enzyme solution* and mix.
3. After exactly 10 minutes at 37℃, immediately transfer an aliquot (0.1ml) (1/11 volume) of the reaction solution to 2.0ml of NaOH solution (B).
4. Add 1.0ml of picric acid solution (C) and incubate at 25℃ for 20 minutes.
5. Measure the optical density at 520nm against water (OD test).
At the same time, prepare the blank by transferring an aliquot (0.1ml) of the reaction solution into NaOH solution (2.0ml) just after the addition of the enzyme solution into ice-cold substrate solution, and carry out the same procedure as the test (procedure 4 and 5) (OD blank).
*Dissolve the enzyme preparation in ice-cold 50mM phosphate buffer, pH 7.5 and dilute to 1.8−2.4U/ml with the same buffer, immediately before assay.
Concentration in assay mixture
Phosphate buffer 45mM
Creatine 90mM
Calculation
Activity can be calculated by using the following formula:

Vt: Total volume (3.1ml)
Vs: Sample volume (0.1ml)
4.65: Millimolar extinction coefficient of creatinine-picrate (orange dye) (cm²/micromole)
11: Volume of reaction solution (1.1ml)/Sampling volume (0.1ml)
1.0: Light path length (cm)
t: Reaction time (10 minutes)
df: Dilution factor of enzyme solution
C: Enzyme concentration in dissolution (mg/ml)
Table 1. Effect of Various Metals on Creatinine amidohydrolase
[The enzyme dissolved in 50mM K-phosphate buffer, pH 7.5 was incubated with each metal (0.2mM) for 30 minutes at 25℃.]
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Ac, CH₃CO.

Comprehensive hazard, handling, storage, and regulatory compliance document.
Download SDS →Lot-specific quality data. Enter your lot number to retrieve the exact COA.
Look up COA →Full quality attributes and acceptance criteria for this grade.
View spec sheet →| 1. Fangbing Wang, Qiwen Peng, Yongheng Zhang, Min Zhang, Guoyue Shi. (2026) Five-in-one colorimetric multiplexed point-of-care testing of blood biomarkers via Janus separation-sensing membrane. CHEMICAL ENGINEERING JOURNAL, [PMID:] [10.1016/j.cej.2026.174104] |
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