QIAEX II Gel Extraction Kit

For purification of DNA fragments (40 bp to 50 kb) from gels and solutions
  • Efficient extraction of DNA from 40 bp to 50 kb
  • Gel extraction from TAE or TBE agarose gels and polyacrylamide gels
  • No sodium iodide to interfere with subsequent reactions
  • No shearing of large DNA fragments
The QIAEX II Gel Extraction Kit provides a suspension of silica particles to which DNA fragments bind in the presence of chaotropic salts. QIAEX II Suspension is added to solutions or solubilized agarose gel slices and binds DNA. The particles are collected by a brief centrifugation, washed, and DNA from 40 bp to 50 kb is eluted in Tris buffer or water.
製品名 Cat. no. List price:
QIAEX II Gel Extraction Kit (150)
For 150 extractions: 3 x 0.5 ml QIAEX II Suspension, Buffers
20021
¥30,500
QIAEX II Gel Extraction Kit (500)
For 500 extractions: 5 x 1.0 ml QIAEX II Suspension, Buffers
20051
¥69,000

QIAEX II Gel Extraction Kit  は分子生物学実験用です。疾病の診断、治療または予防の目的には使用することはできません。


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QIAEX II操作手順|pH指示薬|一定した回収率|
|溶解および結合バッファー中のpH指示薬により、DNA吸着に最適なpHが簡単に分かります(pH ≤7.5)。アガロースゲル電気泳動バッファーを繰り返し使用したり、間違って調製した場合に、結合混合液のpHが不適切となる可能性があります。このような場合は、3M酢酸ナトリウム、pH 5.0を10 µl添加してpHを簡単に調整することが可能です。
|2.9 kb DNAフラグメントの様々な量を1 %アガロースゲルからQIAEX II Gel Extraction Kit を用いて抽出した際の回収率を示した。|
パフォーマンス

Using the QIAEX II Gel Extraction Kit, 10 ng to 10 µg DNA are recovered efficiently (see figure "Consistent recovery"). The versatile batch procedure can be easily scaled up to a binding capacity of 15 µg using 30 µl QIAEX II suspension.

The QIAEX II Gel Extraction Kit provides silica particles for purifying 60–95% DNA fragments (40 bp – 50 kb). A volume of 10 µl QIAEX II suspension binds up to 5 µg DNA, which is subsequently eluted in 20 µl.

Recovery according to size
DNA sizeRecovery, percent*
44 bp 75
75 bp 75
500 bp 95
7.5 kb 85
23.5 kb 75
48.5 kb 60
* From 2 µg loaded on a 1% TAE agarose gel.
原理

Purification of DNA fragments with the QIAEX II system is based on solubilization of agarose and selective adsorption of nucleic acids onto QIAEX II silica-gel particles in the presence of chaotropic salt. QIAEX II separates DNA from salts, agarose, polyacrylamide, dyes, proteins, and nucleotides without phenol extraction or ethanol precipitation. QIAEX II is effective for any type of agarose in either TAE or TBE buffers.

QIAEX II particles ensure efficient recovery without shearing, even for large DNA fragments. Optimized buffers permit DNA recovery without sodium iodide, which is difficult to remove from DNA samples, and may affect subsequent reactions.

The solubilization and binding buffer used with the QIAEX II system contains a unique pH indicator. A simple color change indicates whether the pH of the binding mixture is optimal for efficient adsorption of DNA to QIAEX II silica particles (see figure "pH indicator dye"). The colored dye also allows easy visualization of any unsolubilized agarose in the binding mixture, ensuring complete solubilization for maximum yield.

操作手順

QIAEX II silica-gel particles are added to the solubilized gel slice, and the particles collected by a brief centrifugation step (see flowchart "QIAEX II procedure"). After washing, the pure DNA fragment is eluted in 20 µl of Tris buffer or water.

The QIAEX II Gel Extraction Kit provides QIAEX II suspension together with binding and wash buffers, and a comprehensive handbook. QIAEX II Suspension is also sold separately. Protocols are provided for purification of DNA from agarose gels, solutions, and polyacrylamide gels.

アプリケーション

DNA purified with the QIAEX II system can be used directly in most applications, including:

Restriction digestion
Labeling
Ligation
PCR
Feature
Specifications
Binding capacity 5 µg/10 µl
Elution volume 20 µl
Format Tube
Fragment size 40 bp – 50 kb
Processing Manual
Recovery: oligonucleotides dsDNA Recovery: dsDNA fragments
Removal <10mers 17–40mers dye terminator proteins Removal <40mers
Sample type: applications DNA: PCR reactions
Technology Silica technology

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QIAEX II Procedure
QIAEX II操作手順
ILLU_0104_MinElute
pH指示薬
溶解および結合バッファー中のpH指示薬により、DNA吸着に最適なpHが簡単に分かります(pH ≤7.5)。アガロースゲル電気泳動バッファーを繰り返し使用したり、間違って調製した場合に、結合混合液のpHが不適切となる可能性があります。このような場合は、3M酢酸ナトリウム、pH 5.0を10 µl添加してpHを簡単に調整することが可能です。
Consistent Recovery from Different Starting Quantities of DNA Fragment
一定した回収率
2.9 kb DNAフラグメントの様々な量を1 %アガロースゲルからQIAEX II Gel Extraction Kit を用いて抽出した際の回収率を示した。