Novagen: 70664: Benzonase? Nuclease, Purity ? 99%

Tech Resources
	TB261 Benzonase^� Nuclease
	MSDS - English
	Other Languages
	Selected Citations

Store
	-20�C
Ship
	Blue ice
Note: Store and Ship conditions may differ.
See Key

Also available in:

Request a Quote!

��	Benzonase^� Nuclease, Purity > 99%

Cat. No. 70664��

All Categories � Novagen � Protein Expression, Purification, and Detection � Protein Extraction � Benzonase� Nuclease

Benzonase� Nuclease

Effective viscosity reduction and removal of nucleic acids from protein solutions

�

Benzonase� Nuclease is a genetically engineered endonuclease from Serratia marcescens. It degrades all forms of DNA and RNA (single stranded, double stranded, linear and circular) while having no proteolytic activity. It is effective over a wide range of conditions and possesses an exceptionally high specific activity. The enzyme completely digests nucleic acids to 5′-monophosphate terminated oligonucleotides 2 to 5 bases in length (below the hybridization limit), which is ideal for removal of nucleic acids from recombinant proteins, enabling compliance with FDA guidelines for nucleic acid contamination. The ability of Benzonase to rapidly hydrolyze nucleic acids makes the enzyme an excellent choice for viscosity reduction to reduce processing time and increase yields of protein. For example, the enzyme is compatible with BugBuster� and PopCulture� Protein Extraction Reagents and can therefore be added along with these reagents to eliminate viscosity and remove nucleic acids from E. coli extracts.

The enzyme consists of two subunits of 30 kDa each. It is functional between pH 6 and 10 and from 0-42�C and requires 1-2 mM Mg²⁺ for activation. The enzyme is also active in the presence of ionic and non-ionic detergents, reducing agents, PMSF (1 mM), EDTA (1 mM) and urea (relative activity depends on specific conditions). Activity is inhibited by > 150 mM monovalent cations, > 100 mM phosphate, > 100 mM ammonium sulfate, or > 100 mM guanidine HCl.

Benzonase Nuclease is available in ultrapure (> 99% by SDS-PAGE) and pure (> 90%) grades at a standard concentration of 25 U/�l and at a high concentration (HC) of 250 U/�l. Both preparations are free of detectable protease and have specific activity > 1 � 10⁶ U/mg protein. The > 99% purity grade is tested for endotoxins and contains < 0.25 EU/1000 units. The product is supplied as a 0.2 �m filtered solution in 50% glycerol. Store at -20�C.

�

Product Description

Purity: > 99% by SDS-PAGE.
Total endotoxin: < 0.25 EU/1,000 units.

Unit Activity: One unit is defined as the amount of enzyme that causes a DA₂₆₀ of 1.0 in 30 minutes, which corresponds to complete digestion of 37 �g DNA. �

Need additional information about this product? Email our Technical Service department at: novatech@novagen.com

� Related information for this product is available:
Additional information is available from the "Tech Resources"
box in the upper left panel of this page.

Merck Chemicals list price is displayed (pricing with local distributors may vary). NOTE: In Stock status is based on item availability worldwide.

Sales Office Contact Details

Cat. No.
Size
In Stock
Select Country Above
For Pricing Information

70664-3 10 KU Y N/A

E. coli cells BL21(DE3) containing a pET construct were suspended in BugBuster reagent (5 ml/g wet weight). Aliquots of the suspension were treated with the indicated amounts of Benzonase for 10 min at room temperature, centrifuged at 350 � g for 3 min and photographed.

Material Safety Data Sheets:
70664: Benzonase^� Nuclease, Purity > 99% - English
Bulgarian
Danish
Dutch
Finnish
French
German
Greek
Hungarian
Italian
Korean
Norwegian
Polish
Portuguese
Spanish
Swedish

Selected Citations:
Maria Cecilia Huaman, et al. (2008) Ex vivo cytokine and memory T cell responses to the 42-kDa fragment of Plasmodium falciparum merozoite surface protein-1 in vaccinated volunteers. Journal of Immunology 180, 1451-1461.
Lluis Masip, et al. (2008) Laboratory evolution of Escherichia coli thioredoxin for enhanced catalysis of protein oxidation in the periplasm reveals a phylogenetically conserved substrate specificity determinant. Journal of Biological Chemistry 283, 840-848.
Chikako Suzuki, et al. (2008) PDCD4 inhibits translation initiation by binding to eIF4A using both its MA3 domains. Procedings of the National Academy of Science 105, 3274-3279.
Sandra Hervas-Stubbs, et al. (2007) Insect baculoviruses strongly potentiate adaptive immune responses by inducing type I IFN. Journal of Immunology 178, 2361-2369.
Lisa Kercher, et al. (2007) Prion protein (PrP) expression differences in microglia and astroglia influence scrapie-induced neurodegeneration in retina and brain of transgenic mice. Journal of Virology 81, 10340-10351.
Shogo Kobayashi, et al. (2007) Serine 64 phosphorylation enhances the antiapoptotic function of Mcl-1. Journal of Biological Chemistry 282, 18407-18417.
Samantha M. Lloyd-Burton, et al. (2007) Regulation of Ins(1,4,5)P3 3-kinases by calcium and localization in cells. Journal of Biological Chemistry 282, 9526-9535.
Federico Mingozzi, et al. (2007) Modulation of tolerance to the transgene product in a nonhuman primate model of AAV-mediated gene transfer to liver. Blood 110, 2334-2341.
Hisashi Nishiwaki, et al. (2007) Cloning, functional characterization, and mode of action of a novel insecticidal pore-forming toxin, sphaericolysin, produced by Bacillus sphaericus. Applied and Enviornmental Microbiology 73, 3404-3411.
Elizabeth E. Norgett, et al. (2007) V1 and V0 domains of the human H+-ATPase are linked by an interaction between the G and a subunits. Journal of Biological Chemistry 282, 14421-14427.
...see all selected citations...

Change Country | Contact Us | Privacy Policy | Terms and Conditions

©2008 Calbiochem, Novabiochem, & Novagen

are brands of EMD Chemicals Inc., an Affiliate of Merck KGaA, Darmstadt, Germany.