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The RuvABC Resolvase Is Indispensable for Recombinational Repair in sbcB15 Mutants of Escherichia coli
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ABSTRACT
The RuvABC proteins of
Escherichia coli
play an important role in the processing of Holliday junctions during homologous recombination and recombinational repair. Mutations in the
ruv
genes have a moderate effect on recombination and repair in wild-type strains but confer pronounced recombination deficiency and extreme sensitivity to DNA-damaging agents in a
recBC sbcBC
background. Genetic analysis presented in this work revealed that the Δ
ruvABC
mutation causes an identical DNA repair defect in UV-irradiated
recBC sbcBC
,
sbcBC
, and
sbcB
strains, indicating that the
sbcB
mutation alone is responsible for the extreme UV sensitivity of
recBC sbcBC ruv
derivatives. In experiments with gamma irradiation and in conjugational crosses, however,
sbcBC
Δ
ruvABC
and
sbcB
Δ
ruvABC
mutants displayed higher recombination proficiency than the
recBC sbcBC
Δ
ruvABC
strain. The frequency of conjugational recombination observed with the
sbcB
Δ
ruvABC
strain was quite similar to that of the Δ
ruvABC
single mutant, indicating that the
sbcB
mutation does not increase the requirement for RuvABC in a recombinational process starting from preexisting DNA ends. The differences between the results obtained in three experimental systems used suggest that in UV-irradiated cells, the RuvABC complex might act in an early stage of recombinational repair. The results of this work are discussed in the context of recent recombination models which propose the participation of RuvABC proteins in the processing of Holliday junctions made from stalled replication forks. We suggest that the mutant SbcB protein stabilizes these junctions and makes their processing highly dependent on RuvABC resolvase.
American Society for Microbiology
Title: The RuvABC Resolvase Is Indispensable for Recombinational Repair in
sbcB15
Mutants of
Escherichia coli
Description:
ABSTRACT
The RuvABC proteins of
Escherichia coli
play an important role in the processing of Holliday junctions during homologous recombination and recombinational repair.
Mutations in the
ruv
genes have a moderate effect on recombination and repair in wild-type strains but confer pronounced recombination deficiency and extreme sensitivity to DNA-damaging agents in a
recBC sbcBC
background.
Genetic analysis presented in this work revealed that the Δ
ruvABC
mutation causes an identical DNA repair defect in UV-irradiated
recBC sbcBC
,
sbcBC
, and
sbcB
strains, indicating that the
sbcB
mutation alone is responsible for the extreme UV sensitivity of
recBC sbcBC ruv
derivatives.
In experiments with gamma irradiation and in conjugational crosses, however,
sbcBC
Δ
ruvABC
and
sbcB
Δ
ruvABC
mutants displayed higher recombination proficiency than the
recBC sbcBC
Δ
ruvABC
strain.
The frequency of conjugational recombination observed with the
sbcB
Δ
ruvABC
strain was quite similar to that of the Δ
ruvABC
single mutant, indicating that the
sbcB
mutation does not increase the requirement for RuvABC in a recombinational process starting from preexisting DNA ends.
The differences between the results obtained in three experimental systems used suggest that in UV-irradiated cells, the RuvABC complex might act in an early stage of recombinational repair.
The results of this work are discussed in the context of recent recombination models which propose the participation of RuvABC proteins in the processing of Holliday junctions made from stalled replication forks.
We suggest that the mutant SbcB protein stabilizes these junctions and makes their processing highly dependent on RuvABC resolvase.
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