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合成寡核苷酸n-1产物的序列同一性。

Sequence identity of the n-1 product of a synthetic oligonucleotide.

作者信息

Temsamani J, Kubert M, Agrawal S

机构信息

Hybridon, Inc., Worcester, MA 01605, USA.

出版信息

Nucleic Acids Res. 1995 Jun 11;23(11):1841-4. doi: 10.1093/nar/23.11.1841.

Abstract

After synthesis and purification of an oligonucleotide, the final product usually contains a low level of n-1 congeneric species. We have sequenced the n-1 population of a 25mer phosphodiester oligonucleotide. The n-1 band was cut from the gel and eluted. Oligonucleotides were tailed with dA and annealed to a dT-tailed plasmid. The recombinant plasmid was ligated and used to transform competent bacteria. Our results show that the n-1 population was heterogeneous. The frequency of truncated nucleotides at the 3'-end was much higher than at the 5'-end of the oligomer. No truncated nucleotides were found in the last four nucleotides at the 5'-end. Our results also show that the chain of oligonucleotides can grow on unreacted sites of a controlled-pore glass support.

摘要

在寡核苷酸合成和纯化后,最终产物通常含有低水平的n-1同系物。我们对一个25聚体磷酸二酯寡核苷酸的n-1群体进行了测序。从凝胶上切下n-1条带并洗脱。寡核苷酸用dA加尾并与dT加尾的质粒退火。连接重组质粒并用于转化感受态细菌。我们的结果表明,n-1群体是异质的。寡聚物3'-末端截短核苷酸的频率远高于5'-末端。在5'-末端的最后四个核苷酸中未发现截短核苷酸。我们的结果还表明,寡核苷酸链可以在可控孔玻璃支持物的未反应位点上生长。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a2fa/306952/cac07c79c057/nar00011-0012-a.jpg

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