Unmodified DNA oligonucleotides are synthesised in our high throughput production facility, using highly automated synthesiser technologies in combination with a sophisticated, completely barcode driven LIMS.
Unmodified DNA oligos are available either as Salt Free oligos or as purified oligos. Purifications can be performed either by our proprietary HPSF® purification method, by HPLC or by HYPUR® gel purification.
A chemical reaction never processes completely. Impurities which occur during oligonucleotide synthesis have to be removed.
Using phosphoramidite chemistry, the main side reaction is the formation of n-x products. The longer the sequence, the more n-x products occur. After deprotection, the protecting groups will be part of the raw synthesis product.
| | | |
20mer | 91 | 83 | 75 |
30mer | 86 | 75 | 65 |
40mer | 82 | 68 | 55 |
60mer | 74 | 55 | 41 |
100mer | 61 | 37 | 22 |
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Salt Free Oligos
- Deprotected oligonucleotides
- Quality control of each oligo by MALDI-TOF MS
HPSF® Purification (High Purity Salt Free)
- Proprietary cartridge purification based on reverse phased chromatography
- Cleaned from any toxic chemicals and n-x products
- Quality control of each oligo by MALDI-TOF MS
HPLC Purification (High Performance Liquid Chromatography)
- High purity (> 80%) due to high chromatographic separation
- Standard purification for all modifications (except Amino C6)
- Recommended for RNA oligonucleotides
- Quality control of each oligo by MALDI-TOF MS or CGE (> 60mers)
HYPUR® Purification (Purification by Gel Electrophoresis)
- Highest available quality for longmers: > 90% purity
- Recommended for unmodified oligonucleotides > 60mers
- Quality control of each oligo by MALDI-TOF MS (< 60mers) or CGE (> 60mers)
HPSF® and HYPUR® are registered trademarks of MWG Biotech AG.
