| Identification | Back Directory | [Name]
DISPASE I | [CAS]
42613-33-2 | [Synonyms]
Sarre peptidase
Dispase II protease
Native Bacillus polymyxa Dispase
Dispase from Bacillus polymyxa
Native Bacillus polymyxa Dispase I
Native Bacillus polymyxa Dispase II
Bacillus polymyxa Neutral proteinase
Proteinase, Bacillus polymyxa neutral
Paenibacillus polymyxa neutral protease
Dispase I,Protease from Bacillus polymyxa
Dispase II,Protease from Bacillus polymyxa
protease from bacillus polymyxa cell*culture test
PROTEASE FROM BACILLUS POLYMYXA CELL*CULTURE TESTED | [EINECS(EC#)]
255-914-4 | [Molecular Formula]
NULL | [MDL Number]
MFCD00287245 |
| Hazard Information | Back Directory | [Uses]
Dispase I has been used in a study to assess the effect of amniotic membrane on wound size in the early stages of the healing process. Dispase I has also been used in a study to investigate a dityrosine-based substrate for a protease assay. | [Uses]
The enzyme from Sigma has been used in developing a protocol for ex vivo culture of mouse embryonic mammary buds. It has been used in the treatment of rat heart pieces during the isolation of mitochondria from rat heart. It has also been used for the isolation of dental pulp stem cells (DPSCs) by enzymatic hydrolysis. These cells have been compared with DPSCs isolated by explant method to analyse their stem cell and differentiation properties.
Dispase? II has been used for Fluorescence-Activated Cell Sorting (FACS). It has also been used for separating visceral yolk sac layers. | [Biochem/physiol Actions]
Dispase? II is a neutral protease that hydrolyzes the N-terminal peptide bonds of non-polar amino acid residues. It may be used for separating many tissues and cells grown in vitro. The enzyme is very gentle and does not damage cell membranes. It can also be used to prevent clumping in suspension cultures. This protease cleaves fibronectin and type IV collagen, but not laminin, type V collagen, serum albumin, or transferrin. Dispase? II is specific for the cleavage of Leucine-Phenylalanine bonds. Ca2+, Mg2+, Mn2+, Fe2+, Fe3+ and Al3+ activate the enzyme. EDTA, EGTA, Hg2+ and other heavy metals inhibit the enzyme activity. The enzyme contains 1g-atom of zinc per g-mol of purified enzyme. If this zinc component is removed by chelating agents such as EDTA or EGTA, an inactive apoenzyme is obtained. The enzyme is not inhibited by serum. |
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| Company Name: |
Sigma-Aldrich
|
| Tel: |
021-61415566 800-8193336 |
| Website: |
https://www.sigmaaldrich.cn |
| Company Name: |
Energy Chemical
|
| Tel: |
021-58432009 400-005-6266 |
| Website: |
http://www.energy-chemical.com |
|