Regulation of endonuclease activity by proteolysis prevents breakage of unmodified bacterial chromosomes by type I restriction enzymes

Abstract: ClpXP-dependent proteolysis has been implicated in the delayed detection of restriction activity after the acquisition of the genes (hsdR, hsdM, and hsdS) that specify EcoKI and EcoAI, representatives of two families of type I restriction and modification (R-M) systems. Modification, once established, has been assumed to provide adequate protection against a resident restriction system. However, unmodified targets may be generated in the DNA of an hsd ؉ bacterium as the result of replication errors or recombin… Show more

“…The expected consequence of this mutation in vivo would be fragmentation of the bacterial chromosome. However, recent experiments contradict this expectation (Makovets et al, 1999 ;Doronina & Murray, 2001 ;Cromie & Leach, 2001). It would appear that when modification fails, the bacterial cell is endowed with the means of causing the restriction pathway to abort before the enzymes break the DNA.…”

“…10), or directly by mutations that create target sequences. The original genetic evidence for the creation of vulnerable target sequences by mutation (Makovets et al, 1999) is now supported by the demonstration of breaks in the bacterial chromosome when E. coli K-12 is treated with 2-AP. The breaks are dependent on EcoKI and, as predicted if they arise by base substitutions, their generation requires two rounds of replication (Cromie & Leach, 2001).…”

“…A similar response has been demonstrated for a variety of agents that damage DNA, including mutagens such as the base analogue 2-aminopurine (2-AP), and defects in some genes that affect DNA metabolism, e.g. dam, topA and mutD (dnaQ) (Efimova et al, 1988a, b ;Thoms & Wackernagel, 1984 ;Makovets et al, 1999). DNA damage may generate unmodified target sequences as a consequence of the repair of double-strand breaks by homologous recombination (see Fig.…”

“…One simple solution is to delay production of the restriction enzyme until the modification enzyme has had time to modify all the targets in the bacterial chromosome . This process, however, takes many generations following the acquisition of the genes specifying EcoKI, because unmethylated DNA is a very poor substrate for modification (Makovets, 1999). For type II R-M systems, transcriptional control of gene expression is well documented (see Raleigh & Brooks, 1998), but transcriptional control has not been found to be relevant for any type I or type III system that has been investigated (Loenen et al, 1987 ;Kulik & Bickle, 1996 ;Redaschi & Bickle, 1996).…”

“…Some data will challenge our long-established belief that modification of DNA is essential to distinguish whether the DNA is ' self or foreign '. Experiments show that while modification of DNA is sufficient, it is not always essential to identify resident DNA as self (Makovets et al, 1999 ;Doronina & Murray, 2001). …”

Immigration control of DNA in bacteria: self versus non-self

“…The expected consequence of this mutation in vivo would be fragmentation of the bacterial chromosome. However, recent experiments contradict this expectation (Makovets et al, 1999 ;Doronina & Murray, 2001 ;Cromie & Leach, 2001). It would appear that when modification fails, the bacterial cell is endowed with the means of causing the restriction pathway to abort before the enzymes break the DNA.…”

“…10), or directly by mutations that create target sequences. The original genetic evidence for the creation of vulnerable target sequences by mutation (Makovets et al, 1999) is now supported by the demonstration of breaks in the bacterial chromosome when E. coli K-12 is treated with 2-AP. The breaks are dependent on EcoKI and, as predicted if they arise by base substitutions, their generation requires two rounds of replication (Cromie & Leach, 2001).…”

“…A similar response has been demonstrated for a variety of agents that damage DNA, including mutagens such as the base analogue 2-aminopurine (2-AP), and defects in some genes that affect DNA metabolism, e.g. dam, topA and mutD (dnaQ) (Efimova et al, 1988a, b ;Thoms & Wackernagel, 1984 ;Makovets et al, 1999). DNA damage may generate unmodified target sequences as a consequence of the repair of double-strand breaks by homologous recombination (see Fig.…”

“…One simple solution is to delay production of the restriction enzyme until the modification enzyme has had time to modify all the targets in the bacterial chromosome . This process, however, takes many generations following the acquisition of the genes specifying EcoKI, because unmethylated DNA is a very poor substrate for modification (Makovets, 1999). For type II R-M systems, transcriptional control of gene expression is well documented (see Raleigh & Brooks, 1998), but transcriptional control has not been found to be relevant for any type I or type III system that has been investigated (Loenen et al, 1987 ;Kulik & Bickle, 1996 ;Redaschi & Bickle, 1996).…”

“…Some data will challenge our long-established belief that modification of DNA is essential to distinguish whether the DNA is ' self or foreign '. Experiments show that while modification of DNA is sufficient, it is not always essential to identify resident DNA as self (Makovets et al, 1999 ;Doronina & Murray, 2001). …”

Immigration control of DNA in bacteria: self versus non-self

Localization of the Type I Restriction–Modification Enzyme EcoKI in the Bacterial Cell

The DNA translocation and ATPase activities of restriction-deficient mutants of EcoKI