ParB spreading on DNA requires cytidine triphosphate<i>in vitro</i>

Jalal, Adam S. B.; Tran, Ngat T.; Le, Tung B. K.

doi:10.1101/2019.12.11.865972

Cited by 11 publications

(52 citation statements)

References 60 publications

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“…CTP hydrolysis is not required for loading but might instead assist ParB recycling and control ParB spreading, as shown in vitro for C. crescentus ParB [140]. Spreading may also be restricted by road blocks formed by NAPs [122,140]. The role of CTP binding and hydrolysis in ParB-driven partition complex formation was also shown for M. xanthus ParB [141].…”

Section: The Structure Of the Parb-pars Complexmentioning

confidence: 80%

“…The steric hindrance between parS bound HTH motifs was suggested to promote the detachment of the ParB dimers in a closed conformation from parS, as well as sliding away (spreading). CTP hydrolysis is not required for loading but might instead assist ParB recycling and control ParB spreading, as shown in vitro for C. crescentus ParB [140]. Spreading may also be restricted by road blocks formed by NAPs [122,140].…”

Section: The Structure Of the Parb-pars Complexmentioning

confidence: 97%

“…The observation that ParB loading at parS and sliding on DNA requires CTP binding [122,140,141], a key metabolite in DNA and phospholipids synthesis, adds CTP to the players possibly regulating the ParB-DNA interactions. The motif containing amino acid residues responsible for CTP binding and ParB CTPase activity is one of the most conserved elements within the ParB protein sequences [122,141].…”

Section: Conclusion and Future Perspectivesmentioning

confidence: 99%

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Rules and Exceptions: The Role of Chromosomal ParB in DNA Segregation and Other Cellular Processes

et al. 2020

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The segregation of newly replicated chromosomes in bacterial cells is a highly coordinated spatiotemporal process. In the majority of bacterial species, a tripartite ParAB-parS system, composed of an ATPase (ParA), a DNA-binding protein (ParB), and its target(s) parS sequence(s), facilitates the initial steps of chromosome partitioning. ParB nucleates around parS(s) located in the vicinity of newly replicated oriCs to form large nucleoprotein complexes, which are subsequently relocated by ParA to distal cellular compartments. In this review, we describe the role of ParB in various processes within bacterial cells, pointing out interspecies differences. We outline recent progress in understanding the ParB nucleoprotein complex formation and its role in DNA segregation, including ori positioning and anchoring, DNA condensation, and loading of the structural maintenance of chromosome (SMC) proteins. The auxiliary roles of ParBs in the control of chromosome replication initiation and cell division, as well as the regulation of gene expression, are discussed. Moreover, we catalog ParB interacting proteins. Overall, this work highlights how different bacterial species adapt the DNA partitioning ParAB-parS system to meet their specific requirements.

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Section: The Structure Of the Parb-pars Complexmentioning

confidence: 80%

Section: The Structure Of the Parb-pars Complexmentioning

confidence: 97%

Section: Conclusion and Future Perspectivesmentioning

confidence: 99%

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Rules and Exceptions: The Role of Chromosomal ParB in DNA Segregation and Other Cellular Processes

et al. 2020

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“…The ParB DNA-binding protein recognizes its target parS, present in one or several copies in the Ori region of bacterial chromosomes (Livny et al, 2007). ParB is a CTP hydrolase whose activity is critical for its interaction with parS (Jalal et al, 2020;Osorio-Valeriano et al, 2019;Soh et al, 2019). The resulting ParB/parS nucleoprotein complex encompasses several kbs of DNA and interacts with the ParA ATPase that drives its segregation (Kawalek et al, 2020).…”

Section: Introductionmentioning

confidence: 99%

Distinct activities of bacterial condensins for chromosome management inPseudomonas aeruginosa

Lioy

Junier

Lagage

et al. 2020

Preprint

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Bacteria encompass three types of structurally related SMC complexes referred to as condensins. Smc-ScpAB is present in most bacteria while MukBEF is found in enterobacteria and MksBEF is scattered over the phylogenic tree. The contributions of these condensins to chromosome management were characterized in Pseudomonas aeruginosa that carries both Smc-ScpAB and MksBEF. In this bacterium, SMC-ScpAB controls chromosome disposition by juxtaposing chromosome arms. In contrast, MksBEF is critical for chromosome segregation in the absence of the main segregation system and affects the higher-order architecture of the chromosome by promoting DNA contacts in the megabase range.Strikingly, our results reveal a prevalence of Smc-ScpAB over MksBEF involving a coordination of their activities with the DNA replication process. They also show that E. coli MukBEF can substitute for MksBEF in P. aeruginosa while prevailing over Smc-ScpAB. Altogether, our results reveal a hierarchy between activities of bacterial condensins on the same chromosome.

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“…In most bacteria, Smc-ScpAB complexes start DNA translocation from predefined entry sites, the 16-bp parS DNA sequences, which are generally found near the replication origin and are specifically recognized by the Smc-loader protein ParB (Gruber & Errington, 2009; Sullivan et al, 2009). ParB dimers form DNA clamps that self-load onto DNA at a parS site (Jalal et al, 2020; Osorio-Valeriano et al, 2019; Soh et al, 2019). As Smc complexes translocate away from the parS loading site in both directions (two-sided), they co-align the left and the right chromosome arms that flank the replication origin (Minnen et al, 2016; Tran et al, 2017; Wang et al, 2015, 2017).…”

Section: Introductionmentioning

confidence: 99%

Fine-tuning of the Smc flux facilitates chromosome organization inB. subtilis

Anchimiuk

Lioy

Minnen

et al. 2020

Preprint

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SMC complexes are widely conserved ATP-powered loop extrusion motors indispensable for the faithful segregation of chromosomes during cell division. How SMC complexes translocate along DNA for loop extrusion and what happens when two complexes meet on the same DNA molecule is largely unknown. Revealing the origins and the consequences of SMC encounters is crucial for understanding the folding process not only of bacterial, but also of eukaryotic chromosomes. Here, we uncover several factors that influence bacterial chromosome organization by modulating the probability of such clashes. These factors include the number, the strength and the distribution of Smc loading sites, the residence time on the chromosome, the translocation rate, and the cellular abundance of Smc complexes. By studying various mutants, we show that these parameters are fine-tuned to reduce the frequency of encounters between Smc complexes, presumably as a risk mitigation strategy. Mild perturbations hamper chromosome organization by causing Smc collisions, implying that the cellular capacity to resolve them is rather limited. Altogether, we identify mechanisms that help to avoid Smc collisions and their resolution by Smc traversal or other potentially risky molecular transactions.

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ParB spreading on DNA requires cytidine triphosphatein vitro

Cited by 11 publications

References 60 publications

Rules and Exceptions: The Role of Chromosomal ParB in DNA Segregation and Other Cellular Processes

Rules and Exceptions: The Role of Chromosomal ParB in DNA Segregation and Other Cellular Processes

Distinct activities of bacterial condensins for chromosome management inPseudomonas aeruginosa

Fine-tuning of the Smc flux facilitates chromosome organization inB. subtilis

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