The XbaI-BlnI-CeuI genomic cleavage map of Salmonella typhimurium LT2 determined by double digestion, end labelling, and pulsed-field gel electrophoresis.

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J Bacteriol. 1993 July; 175(13): 4104-4120

research-article

The XbaI-BlnI-CeuI genomic cleavage map of Salmonella typhimurium LT2 determined by double digestion, end labelling, and pulsed-field gel electrophoresis.

S L Liu, A Hessel and K E Sanderson

Department of Biological Sciences, University of Calgary, Alberta, Canada.

ABSTRACT

Endonuclease digestion of the 4,800-kb chromosome of Salmonellatyphimurium LT2 yielded 24 XbaI fragments, 12 BlnI fragments,and 7 CeuI fragments, which were separated by pulsed-field gelelectrophoresis. The 90-kb plasmid pSLT has one XbaI site andone BlnI site. The locations of the fragments around the circularchromosome and of the digestion sites of the different endonucleaseswith respect to each other were determined by excision of agaroseblocks containing fragments from single digestion, redigestionwith a second enzyme, end labelling with 32P by using T7 DNApolymerase, reelectrophoresis, and autoradiography. Forty-threecleavage sites were established on the chromosome, and the fragmentsand cleavage sites were designated in alphabetical order andnumerical order, respectively, around the chromosome. One hundrednine independent Tn10 insertions previously mapped by geneticmeans were located by pulsed-field gel electrophoresis on thebasis of the presence of XbaI and BlnI sites in Tn10. The genomiccleavage map was divided into 100 units called centisomes; theendonuclease cleavage sites and the genes defined by the positionsof Tn10 insertions were located by centisome around the map.There is very good agreement between the genomic cleavage map,defined in centisomes, and the linkage map, defined in minutes.All seven rRNA genes were located on the map; all have the CeuIdigestion site, all four with the tRNA gene for glutamate havethe XbaI and the BlnI sites, but only four of the seven havethe BlnI site in the 16S rRNA (rrs) gene. Their inferred orientationof transcription is the same as in Escherichia coli. A rearrangementof the rrnB and rrnD genes with respect to the arrangement inE. coli, observed earlier by others, has been confirmed. Thesites for all three enzymes in the rrn genes are strongly conservedcompared with those in E. coli, but the XbaI and BlnI sitesoutside the rrn genes show very little conservation.

J Bacteriol. 1993 July; 175(13): 4104-4120

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