Pregled bibliografske jedinice broj: 1260311
Genetic analysis of transductional recombination in Escherichia coli reveals differences in the postsynaptic stages of RecBCD and RecFOR pathways
Genetic analysis of transductional recombination in Escherichia coli reveals differences in the postsynaptic stages of RecBCD and RecFOR pathways // Periodicum biologorum, 124 (2022), 3-4; 97-106 doi:10.18054/pb.v124i3-4.23604 (međunarodna recenzija, članak, znanstveni)
CROSBI ID: 1260311 Za ispravke kontaktirajte CROSBI podršku putem web obrasca
Naslov
Genetic analysis of transductional recombination
in Escherichia coli reveals differences in the
postsynaptic stages of RecBCD and RecFOR pathways
Autori
Zahradka, Ksenija ; Repar, Jelena ; Đermić, Damir ; Zahradka, Davor
Izvornik
Periodicum biologorum (0031-5362) 124
(2022), 3-4;
97-106
Vrsta, podvrsta i kategorija rada
Radovi u časopisima, članak, znanstveni
Ključne riječi
recombination pathways ; transduction ; RuvABC ; RecG ; RadA ; PriA ; recombination-dependent replication
Sažetak
Background and purpose: Homologous recombination in Escherichia coli proceeds via two pathways, RecBCD and RecFOR, which use different enzymes for DNA end resection and loading of RecA recombinase. The postsynaptic reactions following RecA-mediated homologous pairing have mostly been studied within the RecBCD pathway. They involve RuvABC helicase/resolvase complex, RecG and RadA helicases that process recombination intermediates to produce recombinant DNA molecules. Also, RecG functionally interacts with the PriA protein in initiation of recombination-dependent replication. Here, we studied the individual and combined effects of ruvABC, recG and radA null mutations on transductional recombination in both pathways. The effect of the priA300 mutation, which acts as a suppressor of the recG mutation, was also tested. The goal was to characterize the postsynaptic stage of transductional recombination in more details, especially in the RecFOR pathway, which is less well-studied. Materials and methods: Phage P1vir-mediated transduction was used to measure recombination efficiency in a series of recombination mutants. The proA+ marker was used for selection in transductional crosses with various ΔproA recipients. Results: The ruvABC mutation moderately decreased recombination in both recombination pathways, while radA had no effect. The recG mutation reduced recombination in the RecBCD pathway but not in the RecFOR pathway. The strong recombination defect of recG radA double mutants in both pathways was completely suppressed by the priA300 mutation, and this suppression depended on the functional RuvABC complex. Conclusions: RecG and RadA proteins have a redundant role in transductional recombination via RecFOR pathway. In both recombination pathways, RecG and RadA functionally interact with PriA, probably during initiation of recombination- dependent replication.
Izvorni jezik
Engleski
Znanstvena područja
Biologija
POVEZANOST RADA
Projekti:
IP-2013-11-2978 - Rekombinacija, popravak DNA i očuvanje integriteta genoma: novi putevi (RECNEWPATH) (Zahradka, Davor, HRZZ - 2013-11) ( CroRIS)
HRZZ-IP-2019-04-3790 - Regulacija popravka dvolančanog loma u genomu bakterije Escherichia coli (DNARegPop) (Đermić, Damir, HRZZ - 2019-04) ( CroRIS)
Ustanove:
Institut "Ruđer Bošković", Zagreb
Citiraj ovu publikaciju:
Časopis indeksira:
- Web of Science Core Collection (WoSCC)
- Science Citation Index Expanded (SCI-EXP)
- SCI-EXP, SSCI i/ili A&HCI
- Scopus
