DNA methylation at the CfrBI site is involved in expression control in the CfrBI restriction-modification system

doi:10.1093/nar/28.19.3817

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Nucleic Acids Research, 2000, Vol. 28, No. 19 3817-3822
© 2000 Oxford University Press

DNA methylation at the CfrBI site is involved in expression control in the CfrBI restriction–modification system

Irina V. Beletskaya^*, Marina V. Zakharova, Michael G. Shlyapnikov, Lidiya M. Semenova and Alexander S. Solonin

Institute of Biochemistry and Physiology of Microorganisms, Russian Academy of Sciences, Pushchino, Moscow Region 142290, Russia

We have previously found that genes of the CfrBI restriction–modification(R-M) system from Citrobacter freundii are oriented divergentlyand that their promoter regions overlap. The overlapping promoterssuggest regulation of gene expression at the transcriptionallevel. In this study the transcription regulation of CfrBI R-Mgenes was analyzed in vivo and in vitro in Escherichiacoli. It was shown that in the presence of CfrBI methyltransferase(M·CfrBI), cell galactokinase activity decreases 10-foldwhen the galactokinase gene (galK) is under the control of thecfrBIM promoter and increases 20-fold when galK is under thecontrol of the cfrBIR promoter. The CfrBI site, proven to beunique for the entire CfrBI R-M gene sequence, is located inthe –35 cfrBIM promoter region and is in close vicinityof the –10 cfrBIR promoter region. A comparison of thecfrBIM and the cfrBIR promoter activities in the in vitro transcriptionsystem using methylated and unmethylated DNA fragments as templatesdemonstrated that the efficiency of CfrBI R-M gene transcriptionis regulated by enzymatic modification at the N-4-position ofcytosine bases of the CfrBI site by M·CfrBI. From theresults of the in vivo and in vitro experiments we suggest anew model of gene expression regulation in type II R-M systems.

^* To whom correspondence should be addressed. Tel: +7 095 9257448; Fax: +7 095 956 3370; Email: irina@ibpm.serpukhov.su

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