You searched for: Enzymes

Supplier: VWR Chemicals

10,000 units is that quantity of enzyme which will degrade 2 cm² of cellulose filter paper (17 mg) in 1 minute in 0,1 M acetate buffer at pH 4,0.

Supplier: VWR Chemicals

VWR® Pepsin

Supplier: VWR Chemicals

From bovine pancreas.

Supplier: VWR Chemicals

Source is Fig Latex. Fine, light beige powder

Supplier: VWR Chemicals

Off-white to light brown powder from Streptomyces griseus.

Supplier: VWR Chemicals

Beta-D-glucose oxidase with high purity grade and storage in frozen condition.

Supplier: VWR Chemicals

Ribonuclease A is an endoribonuclease that efficiently hydrolyses RNA from tissue or bacterial cell cultures.

Supplier: VWR Chemicals

Catalyses the decomposition of hydrogen peroxide in solution causing the oxidation of a number of substrates. Used extensively as a label for immunohistological assays and ELISA. Its exceptional stability in powdered and solution form enhances its desirability as an enzyme conjugate.

Supplier: VWR Chemicals

A freeze-dried product with >3000 ß-l units per vial.
One unit of ß-l activity is defined as the amount of enzyme that will catalyse the hydrolysis of 1,0 µm of benzylpenicillin per minute at 25 °C and pH 7,0.

Supplier: VWR Chemicals

VWR® Life Science's DNase, Double-Strand Specific, Heat-Labile is a recombinant endonuclease that cleaves phosphodiester bonds in DNA to yield 2 to 8 bp oligonucleotides with 5’-phosphate and 3’-hydroxyl termini.

Supplier: VWR Chemicals

Uracil-DNA glycosylase (UNG), cod is a thermolabile recombinant enzyme produced in E. coli (ung-) using a modified ung gene derived from Atlantic cod. It degrades uracil-containing single- and double-stranded DNA, but not RNA or thymidine-containing DNA, by hydrolysing the N-glycosidic bond between deoxyribose sugar and the base in uracil. This generates alkaline-sensitive apyramidinic sites in the DNA that will be cleaved upon a combination of alkaline conditions and high temperature.

Supplier: Avantor

J.T.Baker® Endonuclease Biotech Reagent meets the strictest cGMP standards and is designed for the degradation of both single stranded and double stranded DNA and RNA. J.T.Baker® Endonuclease Biotech Reagent is used to ensure host cell DNA impurities are removed; driving process efficiency by lowering viscosity and preventing aggregation. J.T.Baker® Endonuclease Biotech Reagent is an enzyme based upon the native endonuclease of Serratia marcescens, enabling rapid clearance of residual DNA and RNA during the production and purification of both recombinant proteins and viral vectors. Non-animal origin. Absence of proteolytic activity. The purity of materials in non-negotiable. J.T.Baker® Endonuclease Biotech Reagent acts to degrade and eliminate extraneous genetic material, ensuring the pristine quality of your final product.

Supplier: Avantor

J.T.Baker® Endonuclease Ultrapure Bioreagent is designed for the degradation of both single stranded and double stranded DNA and RNA. J.T.Baker® Endonuclease Ultrapure Bioreagent is used to ensure host cell DNA impurities are removed; driving process efficiency by lowering viscosity and preventing aggregation. J.T.Baker® Endonuclease is an enzyme based upon the native endonuclease of Serratia marcescens, enabling rapid clearance of residual DNA and RNA during the production and purification of both recombinant proteins and viral vectors. Non-animal origin. The purity of materials in non-negotiable. J.T.Baker® Endonuclease Ultrapure Bioreagent acts to degrade and eliminate extraneous genetic material, ensuring the pristine quality of your final product.