Acta Naturae

2075-8251

Acta Naturae Ltd

10767

10.32607/20758251-2010-2-1-82-87

Articles

Статьи

Research Article

A Novel High-resolving Method for Genomic PCR-fingerprinting of Enterobacteria

Isaeva

A S

Kulikov

E E

Tarasyan

K K

Letarov

A V

letarov@gmail.com

Winogradsky Institute of Microbiology, Russian Academy of Sciences

15032010

VOL 2, NO1 (2010)

ТОМ 2, №1 (2010)

828717012020

2010

Isaeva A.S., Kulikov E.E., Tarasyan K.K., Letarov A.V.

https://creativecommons.org/licenses/by/4.0

https://actanaturae.ru/2075-8251/article/view/10767

We developed a novel PCR-fingerprinting system for differentiation of enterobacterial strains using a single oligonucleotide primer IS1tr that matches the inverted terminal repeats of the IS1 insertion element. Compared to widely used BOX-PCR and ribotyping methods, our system features higher resolution allowing differentiation of closely related isolates that appear identical in BOX-PCR and ribotyping but differ in their phage sensitivity. The IS1-profiling system is less sensitive to the quality of the material and equipment used. At the same time, BOX-PCR is more universal and suitable for bacterial strain grouping and reconstruction of the low-distance phylogeny. Thus, our system represents an important supplement to the existing set of tools for bacterial strain differentiation; it is particularly valuable for a detailed investigation of highly divergent and rapidly evolving natural bacterial populations and for studies on coliphage ecology. However, some isolates could not be reliably differentiated by IS1-PCR, because of the low number of bands in their patterns. For improvement of IS1-fingerprinting characteristics, we offer to modify the system by introducing the second primer TR8834 hybridizing to the sequence of a transposase gene that is widely spread in enterobacterial genomes.

genomic fingerprintingwhole-cell PCR fingerprintinginsertion elementEnterobacterial diversitystrain differentiation

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