Amplification of bacterial 16S ribosomal DNA with polymerase chain reaction.

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J Clin Microbiol. 1990 September; 28(9): 1942-1946

Amplification of bacterial 16S ribosomal DNA with polymerase chain reaction.

K H Wilson, R B Blitchington and R C Greene

Department of Medicine, Duke University, Durham, North Carolina.

ABSTRACT

The sequence of small-subunit rRNA varies in an orderly manneracross phylogenetic lines and contains segments that are conservedat the species, genus, or kingdom level. By directing oligonucleotideprimers at sequences conserved throughout the eubacterial kingdom,we amplified bacterial 16S ribosomal DNA sequences with thepolymerase chain reaction. Priming sites were located at theextreme 5' end, the extreme 3' end, and the center of 16S ribosomalDNA. The isolates tested with these primers included membersof the genera Staphylococcus, Coxiella, Rickettsia, Clostridium,Neisseria, Mycobacterium, Bilophila, Eubacterium, Fusobacterium,and Lactobacillus and the family Enterobacteriaceae. Initially,the yields from the reactions were erratic because the primerswere self-complementary at the 3' ends. Revised primers thatwere not self-complementary gave more reproducible results.With the latter primers, 0.4 pg of Escherichia coli DNA consistentlygave a visible band after amplification. This method shouldbe useful for increasing the amounts of bacterial 16S ribosomalDNA sequences for the purposes of sequencing and probing. Itshould have a broad range of applications, including the detectionand identification of known pathogens that are difficult toculture. This approach may make it possible to identify new,nonculturable bacterial pathogens.

J Clin Microbiol. 1990 September; 28(9): 1942-1946

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