SOME MODIFICATIONS IN THE PROCEDURE OF DIRECT SEQUENCING OF PCR AMPLIFIED 16S-RDNA

被引：170

作者：

DORSCH, M ^{[1
]}

STACKEBRANDT, E ^{[1
]}

机构：

[1] UNIV QUEENSLAND,CTR BACTERIAL DIVERS & IDENTIFICAT,DEPT MICROBIOL,ST LUCIA,QLD 4072,AUSTRALIA

来源：

JOURNAL OF MICROBIOLOGICAL METHODS | 1992年 / 16卷 / 04期

关键词：

16S-RIBOSOMAL-RNA GENE AMPLIFICATION; DNA SEQUENCING; PHYLOGENETIC STUDIES;

D O I：

10.1016/0167-7012(92)90017-X

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A method for the analysis of PCR-amplified 16S ribosomal (r)DNA has been developed that generates sequences of excellent quality. In order to avoid time consuming purification and cloning steps and to reduce the number of non-specific terminations that frequently occur during direct sequencing of 16S rDNA, we developed a strategy that combines the advantages of several procedures described previously for different purposes, such as purification of amplified DNA via the Prep-A-Gene method and the snap-freeze technique in the sequencing protocol. Using 40-400 ng DNA per PCR reaction the amount of PCR product was sufficient to subsequently generate a complete 16S rDNA sequence. The primary structures of these genes were determined fast and reliably, yielding sequences in which the rate of unidentified positions usually did not exceed 0.2%.

引用

页码：271 / 279

页数：9

共 25 条

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