Preparative-scale endotoxin-free plasmid DNA purification—NucleoBond PC Prep100
NucleoBond PC EF kits use anion exchange for purification of endotoxin-free plasmid DNA. Endotoxin removal is achieved in a unique washing step—no extra incubations are necessary. NucleoBond PC Prep100 is used to purify 80–100 mg of endotoxin-free plasmid DNA.
NucleoBond PC EF kits use anion exchange for purification of endotoxin-free plasmid DNA. Endotoxin removal is achieved in a unique washing step—no extra incubations are necessary. NucleoBond PC Prep100 is used to purify 80–100 mg of endotoxin-free plasmid DNA.
Endotoxins (lipopolysaccharides, or LPS) are a major component of the Gram-negative bacterial cell wall. The LPS molecule is an extremely potent stimulator of the mammalian immune system, and a number of mechanisms exist to detect LPS and to respond to the presence of either this molecule or Gram-negative bacteria. LPS is a common contaminant of plasmid DNA preparations grown in E. coli. The negative charges associated with lipid A and the inner core of LPS cause the LPS molecule to behave like DNA on anion exchange chromatography resins.
Obtaining endotoxin-free plasmid DNA is an important prerequisite for transfections and gene therapy applications. For this reason Macherey-Nagel developed a specific patented procedure that reduces endotoxins to a very low level. Unlike competitor kits, there is no need for a time-consuming incubation step to remove the endotoxins. The working procedure for the endotoxin-free plasmid preparation is identical to the standard protocol, and each prep yields up to 100 mg of endotoxin-free plasmid DNA.
NucleoBond EF kits employ a modified alkaline/SDS lysis procedure to prepare the bacterial cell pellet for plasmid purification. The bacterial lysate is cleared by filtration and loaded onto the equilibrated column. No additional incubation step is required for endotoxin removal. After efficient washing of the column, the purified plasmid DNA is eluted from the column.
Overview
- Endotoxins are efficiently removed (<0.1 EU/µg DNA)
- No additional incubation is required for endotoxin removal
- Purify up to 100 mg from 5–20 L of overnight E. coli culture
- Patented procedure
More Information
| Technology | Anion exchange |
| Format | Preparative scale |
| Lysate clarification | Folded filters |
| Starting material | 5–20 L |
| Vector size | <300 kb |
| Typical yield | 80–100 mg |
| A260/280 | 1.80–1.95 |
| Endotoxin level | <0.1 EU/µg |
| Preparation time | 20 hr/prep |
Applications
Purified DNA is suitable for:
- Transfection of highly sensitive cells
- Lentivirus production
Additional product information
Please see the product's Certificate of Analysis for information about storage conditions, product components, and technical specifications. Please see the Kit Components List to determine kit components. Certificates of Analysis and Kit Components Lists are located under the Documents tab.
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