CAS 9025-65-4

endonucleasa serratia marcescens,*recombinante 90+

Descripción:

La endonucleasa Serratia marcescens, recombinante 90+ (CAS 9025-65-4) es una enzima derivada de la bacteria Serratia marcescens, conocida por su papel en el metabolismo de ácidos nucleicos. Esta enzima exhibe actividad endonucleasa, lo que significa que puede romper los enlaces fosfodiéster dentro de los ácidos nucleicos, como el ADN y el ARN, facilitando así procesos como la reparación, replicación y degradación del ADN. La designación "recombinante" indica que la enzima se produce a través de la tecnología de ADN recombinante, lo que permite la generación de grandes cantidades con actividad y pureza específicas. La endonucleasa Serratia marcescens se caracteriza por su capacidad para funcionar de manera óptima bajo ciertas condiciones de pH y temperatura, que pueden variar según la cepa recombinante específica utilizada. Se utiliza comúnmente en aplicaciones de biología molecular, incluyendo clonación, secuenciación y la preparación de ácidos nucleicos para varios ensayos. Además, esta enzima es valorada por su especificidad y eficiencia, lo que la convierte en una herramienta crucial en la ingeniería genética y la investigación biotecnológica.

Sinónimos:

• Binuclease(substitute of Benzonase)

Endonuclease (Serratia marcescens) (35 uL)

CAS:

• 9025-65-4

Enzymes and prepared enzymes, nesoi

Forma y color: Clear Liquid

Serratia marcescens nuclease

CAS:

• 9025-65-4

Serratia marcescens nuclease is a non-specific endonuclease used in molecular biology to degrade and remove DNA and RNA.

Forma y color: Solid

HL-Nuclease

CAS:

• 9025-65-4

Ultra nuclease, liquid, recombinant

CAS:

• 9025-65-4

Ultra nuclease (EC 3.1.30.2) is an enzyme that digests DNA and RNA in any form: single- and double-stranded, linear, circular and supercoiled. The ultimate reaction product is 5'-monophosphate oligonucleatides that are mostly three, four and five bases long. Please enquire for more information about Ultra nuclease, liquid, recombinant including the price, delivery time and more detailed product information at the technical inquiry form on this page

Endonuclease, liquid, food grade

CAS:

• 9025-65-4

Endonuclease, liquid, food grade is a biochemical enzyme, which is derived from microbial or bovine sources, with precision in hydrolyzing phosphodiester bonds within nucleic acids. This endonuclease cleaves the internal bonds of DNA and RNA, enabling the breakdown of these molecules into smaller nucleotide fragments. Its catalytic action is particularly useful in the controlled degradation of nucleic acids without affecting other macromolecules in the substrate.

eXrase DNA Endonuclease, research-grade

CAS:

• 9025-65-4

eXrase DNA endonuclease from enGenes is a recombinant endonuclease from Serratia marcescens produced in E. coli. Effectively and efficiently degrades all forms of DNA and RNA, reducing sample viscosity without proteolytic activity. As effective and efficient as other nucleases on the market, eXrase DNA endonuclease is the most cost-effective way to improve proteins yields and improve sample handing. Presented as a ready to use colourless liquid, formulated in Tris buffer at pH 8.0 with 50 % glycerol (v/v).  This research grade eXrase has low endotoxin, max 0.25 EU/kU.eXrase DNA endonuclease is suitable for the effective breakdown of nucleic acids in numerous biotech settings:  • Removal of residual host DNA from biotechnological products to meet regulatory standards • Reduction of viscosity and streamlined purification in downstream processing of fermentation procedures. • Reduction of viscosity in in upstream fermentation processes • Extraction and/or synthesis of flavouring nucleotides • Enhanced bioavailability of nucleotides in specific feed products • DNA degradation for the removal or prevention of biofilm formationeXrase DNA endonuclease from enGenes is made by a proprietary microbial fermentation process utilizing Escherichia coli cells. This enzyme facilitates the hydrolysis of phosphodiester bonds in various forms of DNA and RNA, including single-stranded, double-stranded, linear, circular, or supercoiled configurations, yielding smaller oligonucleotides typically composed of 2-4 base pairs. Unit-Definition: One unit (U) of the enzyme is defined as the amount required to digest calf thymus DNA, yielding acid-soluble oligonucleotides equivalent to a ΔA260nm of 1.0 within a 30-minute timeframe at pH 8.0 and 37°C. This standardization allows for consistent measurement of enzymatic activity across different batches.

eXrase DNA Endonuclease, tech-grade

CAS:

• 9025-65-4

eXrase DNA endonuclease from enGenes is a recombinant endonuclease from Serratia marcescens produced in E. coli. Effectively and efficiently degrades all forms of DNA and RNA, reducing sample viscosity without proteolytic activity. As effective and efficient as other nucleases on the market, eXrase DNA endonuclease is the most cost-effective way to improve proteins yields and improve sample handing. Presented as a ready to use colourless liquid, formulated in Tris buffer at pH 8.0 with 50 % glycerol (v/v). This tech grade version is our most cost effective endonuclease for R&D applications. eXrase DNA endonuclease is suitable for the effective breakdown of nucleic acids in numerous biotech settings:  • Removal of residual host DNA from biotechnological products to meet regulatory standards • Reduction of viscosity and streamlined purification in downstream processing of fermentation procedures. • Reduction of viscosity in in upstream fermentation processes • Extraction and/or synthesis of flavouring nucleotides • Enhanced bioavailability of nucleotides in specific feed products • DNA degradation for the removal or prevention of biofilm formationeXrase DNA endonuclease from enGenes is made by a proprietary microbial fermentation process utilizing Escherichia coli cells. This enzyme facilitates the hydrolysis of phosphodiester bonds in various forms of DNA and RNA, including single-stranded, double-stranded, linear, circular, or supercoiled configurations, yielding smaller oligonucleotides typically composed of 2-4 base pairs. Unit-Definition: One unit (U) of the enzyme is defined as the amount required to digest calf thymus DNA, yielding acid-soluble oligonucleotides equivalent to a ΔA260nm of 1.0 within a 30-minute timeframe at pH 8.0 and 37°C. This standardization allows for consistent measurement of enzymatic activity across different batches.