Nucleic Acids Research, Vol 25, Issue 18 3629-3635, Copyright © 1997 by Oxford University Press
RT Pon and S Yu
When hydroquinone-O,Ooffiacetic acid is used as a linker arm in solid phase
oligonucleotide synthesis, the time for NH4OH cleavage of oligodeoxy- or
oligoribonucleotides is reduced to only 2 min. This allows increased
productivity on automated DNA synthesizers without requiring any other
modifications to existing reagents or synthesis and deprotection methods.
The Q-linker may also be rapidly cleaved by milder reagents such as 5%
NH4OH, potassium carbonate, anhydrous ammonia, t-butylamine or fluoride
ion. However, the Q-linker is sufficiently stable for long-term storage at
room temperature without degradation and no loss of material occurs during
synthesis. The linker is also reasonably resistant to 20% piperidine/DMF,
0.5 M DBU/pyridine and 1:1 triethylamine/ethanol. The Q-linker can
therefore serve as a general replacement for both succinyl and oxalyl
linker arms.
ARTICLES
Hydroquinone-O,O'-diacetic acid ('Q-linker') as a replacement for succinyl and oxalyl linker arms in solid phase oligonucleotide synthesis
Department of Medical Biochemistry, The University of Calgary, Calgary, Alberta T2N 4N1, Canada. rtpon@acs.ucalgary.ca
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