QIAEX II Gel Extraction Kit 从琼脂糖凝胶和溶液中批量回收纯化DN**段(40 bp到50 kb) - 40 bp 到50 kb DNA高效纯化
- 在TAE/TBE缓冲液中的标准/低熔点琼脂糖凝胶以及聚丙烯酰胺凝胶中的胶回收
- 无需***化钠处理后续反应
- 避免产生DNA大片段的剪切
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. Batch Gel Extraction | | Size range | No. of samples in parallel | Format | Processing | QIAEX II Gel Extraction Kit | 40 bp – 50 kb | 1–24 | Silica particles | Spin procedure |
PrinciplePurification 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. Quantities of DNA from 10 ng to 10 µg are recovered efficiently (see figure "Consistent Recovery from Different Starting Quantities of DNA Fragment"), and the versatile batch procedure can be easily scaled up for preparative purposes up to 15 µg binding capacity using 30 µl QIAEX II suspension. 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. Size vs recovery with QIAEX II DNA size | Recovery* |
| 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 | Binding capacity: | 5 µg DNA per 10 µl QIAEX II suspension | Recovery: | 60-95% of DNA fragments (40 bp – 50 kb) | Elution volume: | Elution volume: 20 µl |
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Procedure QIAEX II silica-gel particles are added to the solubilized gel slice (see "QIAEX II Procedure" flowchart), and the particles collected by a brief centrifugation step. After washing, the pure DNA fragment is eluted in 20 µl of Tris buffer or water.
Downstream applicationsDNA purified with the QIAEX II system can be used directly in most applications, including: - Restriction digestion
- Labeling
- Ligation
- PCR
For a list of references citing uses of the QIAEX II Gel Extraction System, visit the QIAGEN Reference Database online or contact QIAGEN Technical Services or your local distributor. Images Consistent Recovery from Different Starting Quantities of DNA Fragment pH Indicator Dye QIAEX II Procedure - Role for nonstructural protein 1 of severe acute respiratory syndrome coronavirus in chemokine dysregulation
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- Role for nonstructural protein 1 of severe acute respiratory syndrome coronavirus in chemokine dysregulation
Law AH, Lee DC, Cheung BK, Yim HC, Lau AS - Effects of the chemotherapeutic agent doxorubicin on the protein C anticoagulant pathway
Woodley-Cook J, Shin LY, Swystun L, Caruso S, Beaudin S, Liaw PC - Additional freeze hardiness in wheat acquired by exposure to -3 degreesC is associated with extensive physiological, morphological, and molecular changes
Herman EM, Rotter K, Premakumar R, Elwinger G, Bae R, Ehler-King L, Chen S, Livingston DP - New functions of XPC in the protection of human skin cells from oxidative damage
D'Errico M, Parlanti E, Teson M, de Jesus BM, Degan P, Calcagnile A, Jaruga P, Bjørås M, Crescenzi M, Pedrini AM, Egly JM, Zambruno G, Stefanini M, Dizdaroglu M, Dogliotti E - Expression and genomic status of EGFR and ErbB-2 in alveolar and embryonal rhabdomyosarcoma
Ganti R, Skapek SX, Zhang J, Fuller CE, Wu J, Billups CA, Breitfeld PP, Dalton JD, Meyer WH, Khoury JD - Exportin-5 orthologues are functionally divergent among species
Shibata S, Sasaki M, Miki T, Shimamoto A, Furuichi Y, Katahira J, Yoneda Y - A variable immunoreceptor in a subpopulation of human neutrophils
Puellmann K, Kaminski WE, Vogel M, Nebe CT, Schroeder J, Wolf H, Beham AW - Polyamine-regulated unproductive splicing and translation of spermidine/spermine N1-acetyltransferase
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