GENOPURE PLASMID MIDI KIT

Not available outside of the UK & Ireland.

Analysis Note

Sample:E. coli culture that contains a high-copy number plasmid: 5 to 30 mL bacterial cultureE. coli culture that contains a low-copy number plasmid: 10 to 100 mL bacterial culturePlasmid Size: The isolation procedure is suitable for all sizes of plasmid. Note: Lysates of larger constructs (up to 100 kb) should be cleared by filtration rather than centrifugation to avoid shearing the plasmid.Time Required: 60 minutes (including filtration of the lysate)Typical Yield:High-copy number plasmid: 3 to 5 µg/mL cultureLow-copy number plasmid: 0.2 to 1 µg/mL cultureProduct Purity: Isolated plasmid DNA is free of other bacterial components, including RNA.

Application

The Genopure Plasmid Midi Kit prepares transfection-grade plasmid DNA in medium quantities (up to 100 µg plasmid) from bacterial cultures. Isolated plasmid is suitable for most molecular biology applications: Transfection Southern blotting Sequencing PCR Restriction analysis Cloning

Components

Suspension Buffer RNase A Lysis Buffer Neutralization Buffer Equilibration Buffer Wash Buffer Elution Buffer, NucleoBond AX 100 Columns Folded Filters (150 mm diameter) Sealing Rings

Features and Benefits

The Genopure Plasmid Midi Kit prepares highly purified plasmid DNA in medium quantities using a modified alkaline lysis method. Save time with ready-to-use reagents.Purify up to 20 samples (10 minutes hands-on-time/75 minutes overall). Purify all sizes and types of plasmid,even BAC DNA, since the crude lysate can be filtered to avoid plasmid shearing. Process multiple samples in parallelusing high speed gravity-flow columns. Eliminate the use of hazardous organic compoundssuch as cesium chloride, phenol, chloroform, and ethidium bromide. Obtain higher purity plasmid DNAover plasmid prepared by 2 x cesium chloride gradient centrifugation.

General description

Plasmid recovery was tested with 50 µg purified plasmid. The recovery was >90%, with more than 80% in supercoiled form. The yield of plasmid DNA was determined by isolating pBS from DH5a cells. From 30 mL culture volume with a density of A600 between 3 and 6, >85 µg of plasmid DNA was obtained. The purity (checked by the ratio of A260/A280) is 1.8 + 0.2. No RNA is detectable. The kit components have been tested for the absence of nucleases according to current quality control procedures.

Other Notes

For life science research only. Not for use in diagnostic procedures.

Ion Exchange Chromatography

Preparation Note

The isolation procedure is based on a modified alkaline lysis protocol and can be divided into the following steps:The bacteria are partially lysed, allowing the plasmid DNA to escape the cell wall into the supernatant. The larger E. coli chromosomal DNA is trapped in the cell wall. The lysate is cleared of cellular debris by filtration or centrifugation, and the plasmid DNA-containing fraction is loaded onto a pre-equilibrated column. Since the cleared lysate is applied to the column in a low-salt buffer, plasmid DNA binds to the macroporous anion-exchange material in the column. Cellular impurities are eluted from the column with a high-salt wash. Finally, the plasmid DNA is eluted from the column. Recovered DNA is precipitated from the eluate to remove salt and concentrate the plasmid.

Quality

Plasmid DNA purified by this kit has been tested for restriction digestion; pUC 19 was isolated from transformed HB101 as described in the protocol. 1 µg of plasmid was completely digested with 1 U Msp I for 2 hours at +37°C, as shown by agarose gel analysis.Plasmid recovery was tested with 50 µg purified plasmid. The recovery was >90%, with more than 80% in supercoiled form. The yield of plasmid DNA was determined by isolating pBS from DH5a cells. From 30 ml culture volume with a density of A600 between 3 and 6, >85 µg of plasmid DNA was obtained.The purity (checked by the ratio of A₂₆₀/A₂₈₀) is 1.8 + 0.2.RNA contamination was analyzed with 3 µg pBS purified with the standard procedure and checked by electrophoresis on an agarose gel. No RNA was detected.The kit components have been tested for the absence of nucleases according to current Quality Control procedures.