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Research Paper |
Laboratorio de Bioingeniería, Instituto de Nutrición y Tecnología de los Alimentos, Universidad de Chile, Macul 5540, Santiago, Chile1
Author for correspondence: Romilio T. Espejo. Tel: +56 2 6781426. Fax: +56 2 2214030. e-mail: respejo{at}uec.inta.uchile.cl
Analysis of the 16S rDNAs obtained from cultures of single colonies of either type collection strains or environmental strains of the genus Vibrio revealed the presence of polymorphism in every one of the strains examined. Polymorphism was detected by visualization of heteroduplexes produced after 16S rDNA PCR amplification, a procedure that allows for the screening of a large number of isolates. Amplified 16S rDNAs obtained from both Vibrio parahaemolyticus and an environmental strain were cloned. Their nucleotide sequences revealed differences of up to 2% among 16S rDNAs from the same strain. Polymorphic sites were concentrated in a recognized variable stemloop of bacterial 16S rRNA that contained in some cases up to 83% of the total mismatches observed. Most of the substitutions present in the stemloop region showed compensating base covariation. The accumulation of so many compensating changes in the stemloop region implies that the divergence of the different versions of this stemloop is relatively ancient. This divergence could be the result of either a selection process or a lateral transfer of independently evolved genes.
Keywords: marine, 16S rDNA, rrn
The GenBank accession numbers for the sequences reported in this paper are AF388386 (Vp23), AF388387 (Vp16), AF388388 (F44), AF388389 (Vp27), AF388390 (F6), AF388391 (3d2), AF388392 (3d4), AF388393 (3d7) and AF388394 (3d8).
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