The capacity of origins to load MCM establishes replication timing patterns
Authors:
Livio Dukaj aff001; Nicholas Rhind aff001
Authors place of work:
Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Medical School Worcester, Massachusetts, United States of America
aff001
Published in the journal:
The capacity of origins to load MCM establishes replication timing patterns. PLoS Genet 17(3): e1009467. doi:10.1371/journal.pgen.1009467
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1009467
Summary
Loading of the MCM replicative helicase at origins of replication is a highly regulated process that precedes DNA replication in all eukaryotes. The stoichiometry of MCM loaded at origins has been proposed to be a key determinant of when those origins initiate replication during S phase. Nevertheless, the genome-wide regulation of MCM loading stoichiometry and its direct effect on replication timing remain unclear. In order to investigate why some origins load more MCM than others, we perturbed MCM levels in budding yeast cells and, for the first time, directly measured MCM levels and replication timing in the same experiment. Reduction of MCM levels through degradation of Mcm4, one of the six obligate components of the MCM complex, slowed progression through S phase and increased sensitivity to replication stress. Reduction of MCM levels also led to differential loading at origins during G1, revealing origins that are sensitive to reductions in MCM and others that are not. Sensitive origins loaded less MCM under normal conditions and correlated with a weak ability to recruit the origin recognition complex (ORC). Moreover, reduction of MCM loading at specific origins of replication led to a delay in their replication during S phase. In contrast, overexpression of MCM had no effects on cell cycle progression, relative MCM levels at origins, or replication timing, suggesting that, under optimal growth conditions, cellular MCM levels are not limiting for MCM loading. Our results support a model in which the loading capacity of origins is the primary determinant of MCM stoichiometry in wild-type cells, but that stoichiometry is controlled by origins’ ability to recruit ORC and compete for MCM when MCM becomes limiting.
Keywords:
Auxins – DNA replication – Genomic signal processing – Genomics – Helicases – Hyperexpression techniques – Stoichiometry – Synthesis phase
Introduction
The initiation of DNA replication is an exquisitely orchestrated and highly conserved process. Although the molecular biochemistry of initiation at individual origins continues to be elucidated in great detail [1,2], the mechanism governing the time at which different regions of the genome replicate has remained largely elusive [3]. Nonetheless, replication timing has been implicated in a number of important processes, including gene expression, mutation rates, and chromatin structure [4–7]. Which molecular mechanisms underlie the replication timing patterns, how they establish it, and what the consequences are when those mechanisms go awry is still a matter of active research [8].
Origin licensing, the establishment of potential origins of replication in G1, is separated from replication initiation through a variety of biochemical mechanisms, which are particularly well-understood in budding yeast [1,9]. In late M and G1, the Minichromosome Maintenance (MCM) complex, the heterohexameric catalytic core of the replicative helicase, composed of Mcm2-7, is shuttled into the nucleus with the help of Cdt1 [10]. In the nucleus, the Origin Recognition Complex (ORC), which loads MCM at origins, recognizes and binds origins at their ARS Consensus Sequence (ACS) [11,12]. After binding of its Cdc6 subunit, ORC recruits MCM-Cdt1 to the origins and loads MCM onto double stranded DNA (dsDNA), at which point Cdt1 is released and a second MCM is coordinately loaded [13]. The resulting MCM double hexamer (MCM-DH) establishes an origin that can be activated for replication through the action of the replication kinases CDK and DDK and accessory initiation factors [14].
Although the biochemical mechanisms of MCM activation appear to be uniform across origins, the timing of MCM activation varies from origin to origin. The observation that MCM activation is regulated by limiting initiation factors [15] has led to the model that the competition between origins for these limiting initiators establishes the relative efficiency of MCM activation, which in turn determines the average firing time for each origin. This model raises the question of why some origins compete more efficiently for the limiting factors. Heterochromatin reduces origin activation efficiency, perhaps by restricting access to limiting initiators, but also by recruiting phosphatases that antagonize the required S-phase kinases [16]. Conversely, origins can by programed for early activation by recruiting limiting factors. An early example was the demonstration that fission yeast recruits DDK to centromeres to advance their activation [17].
Although the simplest models of origin function posit exactly one MCM-DH loaded at each origin, many studies have reported that the levels of MCM signal at origins vary by over ten fold [12,18–21]. Moreover, MCM stoichiometry (that is, the average MCM loading at an origin, relative to other origins) has been proposed as an important determinant of replication timing [20–22]. In particular, if MCMs are activated stochastically, then an origin that has higher MCM stoichiometry has a greater probability of firing and thus, on average, will fire earlier in S phase [23]. Combining evidence for the regulation of origin activation efficiency by trans-acting factors with evidence for the effect of MCM stoichiometry on origin activation efficiency leads to a unified model in which the probability of an origin firing, and thus its average firing time in S phase, is a product of an origin’s MCM stoichiometry and the activation efficiency of that MCM, regulated by trans-acting factors.
There are two ways in which MCM stoichiometry could vary at origins. In the one-MCM scenario, an origin either has one or zero MCM-DH loaded. Therefore, the population-based average can range from 0 to 1, a parameter that has been referred to as competency [24–26]. In the multiple-MCM scenario, more than one MCM can be loaded at an origin and so MCM stoichiometry can range from 0 to many [20,22]. As elaborated in the Discussion, distinguishing between the one-MCM and many-MCM scenarios is an area of active research. However, the hypotheses tested here—regarding whether variable MCM stoichiometry affects replication timing and how variable MCM stoichiometry is established—are independent of whether the range of variation is from 0 to 1 or 0 to many.
Regardless of the absolute stoichiometry of MCM loading at origins, it remains unclear how relative loading dynamics are regulated at individual origins genome-wide. In order to investigate the mechanisms regulating the level of MCM loading and to determine the effect that such changes in levels have on replication timing, we performed experiments under conditions in which cellular MCM levels were either increased or decreased. We aimed to test two general models of the regulation of MCM loading: the ORC Activity model, in which the relative activity of ORC at individual origins regulates MCM occupancy, and the Origin Capacity model, in which the intrinsic capacity of each origin for MCM loading regulates MCM occupancy. Importantly, we performed both MCM ChIP-seq and replication timing assays in the same experiments, such that the density of MCM loaded in late G1 could be directly correlated to replication timing at specific origins. Furthermore, we used MNase ChIP-seq, which produces much higher resolution data than standard ChIP-seq, allowing us to localize where MCMs are loaded within origins with close to base-pair resolution. Using genome-wide MNase ChIP-seq and replication timing assays, we found that lowering cellular MCM levels caused differential loading of MCM, with MCM loading at some origins being sensitive to intermediate reductions of cellular MCM levels and loading at other origins being largely resistant. Importantly, reduction in MCM levels correlated with delays in replication timing. Conversely, increasing the MCM levels in budding yeast had no effects on MCM loading onto DNA or replication timing in S phase, indicating that MCM loading under normal conditions is saturated. These results suggest that loading of MCM at origins in G1 is a dynamic process and that relative levels of helicase at origins are dependent on the origins’ abilities to recruit MCM as well as the levels of MCM pools in the cells. In particular, as described in the Discussion, our results are consistent with a hybrid model combining regulation by both ORC activity and origin capacity.
Results
Auxin-induced reduction in cellular MCM levels causes a dose-dependent reduction in viability and slower progression through S phase
To test the effects of reduced MCM pools on helicase loading and replication timing we employed the auxin-inducible degron (AID) system optimized for budding yeast [27,28]. In order to reduce the cellular pool of MCM, we tagged the endogenous copy of Mcm4 with the AID degron cassette (IAA17) followed by GFP at its C terminus. The MCM hexamer requires all six components for nuclear localization [29]. In addition, degradation of any single component of the hexamer causes destabilization of the rest [29]. Therefore, degradation of Mcm4 is expected to reduce the total cellular pool of MCM. As previously reported, continual exposure to increasing amounts of auxin caused a dose-dependent lethality in cells harboring degron-tagged Mcm4 (S2A Fig) [27]. However, cells maintain viability under our specific experimental conditions (S2B Fig).
We determined the effect of lowered MCM levels on genome-wide loading and replication timing in synchronized cells. We synchronized the cells and reduced MCM levels prior to G1 in order ensure that MCM was not removed from active replisomes or pre-loaded origins. We first synchronized cells in metaphase using nocodazole, followed by release into α-factor for a G1 arrest (S1 Fig). Mcm4 was degraded through the addition of auxin, first for 30 minutes during nocodazole arrest, then during the majority of the α-factor arrest. Following a 30 minute period of equilibration in the absence of auxin at the G1/S boundary, samples were collected for MCM ChIP-seq analysis, and the rest of the culture was released into S phase (Fig 1A). Immunoblots monitoring the levels of Mcm4-IAA17-GFP revealed that Mcm4 is efficiently degraded after addition of auxin in a dose-dependent manner (Fig 1B). Quantification of Mcm4 levels revealed that, compared to untreated cells, 30 μM auxin reduced Mcm4 levels to 14% of the endogenous levels, whereas 500 μM auxin reduced those levels to 7%. The observation that cells released onto plates containing the replication stress drug hydroxyurea (HU) showed an auxin dose-dependent increase in sensitivity to HU suggests that lowered Mcm4 levels reduce MCM function and cell viability (S2B Fig). We performed flow cytometry analysis on S-phase-synchronized cells treated with 0 μM, 30 μM, and 500 μM auxin and found that degradation of Mcm4 also causes a dose-dependent delay in progression through S phase (Figs 1C and S1). Together, this data show that the AID system can be used to reduce Mcm4 levels in a dose-dependent manner and that reduction of Mcm4 causes reduced viability, slower progression through S phase, and lower resistance to replication stress.
Reduced MCM levels cause a reduction in helicase loading at many, but not all origins of replication
Previous studies using ChIP have shown that MCM abundance at origins of replication varies throughout the genome [12,18–21]. To test how lowered MCM pools affect the dynamics of helicase loading and abundance at origins of replication, we used α-factor-arrested cells to perform ChIP-seq using a polyclonal antibody against the full MCM hexamer on micrococcal nuclease- (MNase) digested chromatin [30]. MNase digestion has the advantage, relative to the standard ChIP approach of shearing by sonication, of cleaving the chromatin into much smaller fragments. Because the MCM-DH complex protects about 70 bp of DNA, using MNase ChIP-seq, we can map MCM footprints with almost nucleotide resolution.
Fragments of the genome associated with MCM were pulled down, sequenced, and their abundance was normalized to read depth and no-immunoprecipitation input controls. Using this method, we found that MCM peaks localize to known origins of replication (Fig 1D), are reproducible (r = 0.97–0.99, S3A Fig) and correlate well with previously reported levels (r = 0.78–0.82, S3B Fig). Quantitation of origin peaks revealed changes to MCM loading throughout the genome in response to reduction of MCM levels (Fig 2 and S1 Table). Many origins exhibited a reduction in MCM abundance in auxin-treated cells, as seen by a shift away from the diagonal line in Fig 2A. The level of reduction was dose-dependent, as cells treated with 500 μM auxin showed greater reduction in MCM abundance than those treated with 30 μM auxin. Plotting the percent of MCM abundance that is lost in response to auxin treatment showed that some origins lose most of their MCM signal after 30 μM auxin treatment, while others are resistant to the changes in MCM levels even after 500 μM auxin treatment (Fig 2B). Origins that have lower levels of MCM in control cells are more prone to lose MCM signal in response to even intermediate levels of auxin treatment compared to origins that have high levels of MCM (Fig 2B). These results indicate that levels of MCM pools in cells affect loading at origins of replication throughout the genome in significant and dissimilar ways.
To investigate the reason that reduced MCM levels delayed bulk S-phase progression, we examined we examined the distribution of MCM signal and inter-origin distances in the three conditions. We calculated the smallest number of origins required to account for 50% of the total MCM signal for each condition and measured the inter-origin distances between these major origins. If MCM pools are reduced and loading is decreased significantly for some origins, others would be expected to replicate larger tracts of the genome, leading to an increase in the time required to complete S phase (Fig 1C). As seen in S2 Table, the smallest number of origins required to make up 50% of the MCM signal in each condition decreases as MCM pools are decreased (0 μM = 110, 30 μM = 85, 500 μM = 72), consistent with the observation that origins which load less MCM under control conditions lose a higher fraction of their MCM signal in response decreases in MCM pools. The in-silico-calculated average inter-origin distance between these top origins increases from 96 kb for 0 μM, to 118 kb for 30 μM, and to 136 kb for 500 μM auxin treatment, suggesting that they need to replicate larger tracts of the genome. In addition, a larger portion of origins replicate shorter tracts at 0 μM auxin, while a larger portion replicates longer tracts for 30 μM and 500 μM auxin treatments (S4 Fig). Overall, this data indicates that, in response to reduced MCM pools, origins that load higher levels of MCM are responsible for replicating larger tracts of DNA, leading to an increase in the amount of time required to complete DNA replication.
‘Weak’ origins are more prone to reduced MCM loading
Previous analysis of various replication origins in budding yeast classified origins based on their affinity for ORC in vivo, as measured by ChIP-seq, and in vitro, as measured by gel shift assays [31]. Origins for which high in vitro ORC affinity explained their high in vivo affinity were classified as DNA-dependent. Origins whose high in vivo affinity could not be explained by their in vitro affinity were classified as Chromatin-dependent. Origins that displayed low ORC affinity both in vivo and in vitro were classified as Weak. Importantly, the three classes of origins have similar distributions of efficiency (0.64±20, 0.69±19, 0.66±17, respectively) [32] and replication timing (21.8±2.1’, 20.6±2.7’, 21.4±2.1’, this paper), showing that all three classes can support early/efficient and late/inefficient origins. To gauge the effect of lowered MCM pools on loading dynamics between these origin classes, we compared MCM levels for cells treated with 0 μM auxin to those treated with 30 μM or 500 μM auxin (Fig 2C). The comparison shows that DNA-dependent and Chromatin-dependent origins maintain most of their endogenous levels of loading in response to auxin treatment and therefore are more resistant to changes in MCM pools compared to Weak origins. As expected, Weak origins lose more of their signal in response to reductions in MCM pools compared to DNA- and Chromatin-dependent origins (Fig 2D). This analysis suggests that origins with low ORC affinity are outcompeted by origins with higher ORC affinity (due to sequence or chromatin differences) when the pool of available MCM is reduced.
MCM associates with flanking nucleosomes and the nucleosome-free region (NFR) of origins
Studies using MNase footprinting indicate that MCM associates with well-positioned nucleosomes flanking the ACS at origins of replication [19]. To assess the location of MCM signal in our data, we constructed strand-specific V plots centered at the ARS consensus sequence (ACS) [11]. V plots map the abundance of reads and their length relative to their genomic location. Mapping MCM ChIP-seq reads from control cultures shows that MCM is mostly found within 2–3 nucleosomes from the ACS, with signal decreasing with distance away form the ACS (Fig 3A). Examination of individual origins shows a similar distribution of MCMs (S5A Fig). The signal includes MCM-DH-sized reads (~68bp) as well as larger, nucleosome-sized reads (~146bp) (Fig 3A). Although most of the MCM ChIP-seq signal is associated with nucleosomes, as previously reported [19], the increased resolution of our approach also allowed us to detect MCM signal in the nucleosome-free region (NFR) of origins, as predicted by recent in-vitro cryo-EM structures [33]. In particular, the smaller, MCM-sized fragments, populate the NFR (Figs 3A and S5B). This observation was dependent on the degree of MNase digestion, as Replicate #1, which had a lower degree of digestion, lacked the smaller fragments, in agreement with similar studies involving transcription factors (S6 Fig)[34].
In order to gauge changes in MCM signal around origins in response to reduction in MCM levels we constructed read density profiles. To do so, we used the midpoint of ACS-annotated origins and quantified read densities based on their genomic location around these origins [11]. As expected, there was a reduction in MCM ChIP-seq read density at origins in response to both 30 μM and 500 μM auxin (Fig 3B). In contrast, there was a much smaller but reproducible increase in read density for the +1 and -1 nucleosome positions for input DNA, indicating a possible increase in nucleosome occupancy as MCM loading is reduced at these origins (S7A Fig). However, in a 1kb window around the origins there was no significant difference in read density for input samples (r = 0.96–0.98, S7B Fig). Given the differential response of origins in response to auxin, we separated origins in quartiles based on the percent of MCM signal that they lost in response to 500 μM auxin. As seen in Fig 3C, origins which are least affected by MCM pool reduction tend to have higher levels of MCM loaded under control conditions and do not lose any signal in response to intermediate levels of auxin. On the other hand, origins which are most affected by reduced MCM pools tend to have less MCM loaded under control conditions and upon intermediate auxin treatment lose most of their signal. This data elucidates sets of origins that are distinct in how they are affected by MCM levels, identifying origins that are resistant to intermediate reductions in MCM levels and others that are sensitive.
ORC binding to the ACS and subsequent MCM loading is a directional process dependent on an ACS-site and a similar but inverted nearby sequence [12,35]. To determine whether the directionality of MCM loading is maintained throughout G1 in relation to the dominant annotated ACS sites, we separated origins based on the magnitude of signal upstream or downstream of the ACS. The 253 origins tested were split nearly evenly between higher signal upstream or downstream of the annotated ACS (129 to 124, respectively; S8 Fig). The MCM signal was largely independent of ACS directionality, as a previously noted [19]. Only 50% of higher-upstream-signal origins and 44% of higher-downstream-signal origins correlated with ACS directionality. This data supports a model where, once loaded, MCM is able to passively slide in either direction on double stranded DNA, consistent with previous in vitro findings [33,36].
Auxin-induced reduction in MCM loading causes significant delays in replication timing at corresponding origins
Reduction of MCM pools via auxin-induced Mcm4 degradation caused significant changes to MCM loading at origins. To test whether these changes in MCM abundance have an effect on replication timing, we measured replication timing in cells released into S phase after treatment with 0 μM, 30 μM, or 500 μM auxin, using the same cultures as those used for our ChIP-seq experiments. Briefly, using the sync-seq approach, we measured replication timing by measuring genome-wide copy number at multiple points after synchronous release into S phase [37]. From this data, we extracted the parameter Trep, the time at which 50% of cells have replicated a specific locus. Fig 4A shows the Trep profile of Chromosome V along with the corresponding ChIP-seq profiles for treated and untreated cells. Trep values for cells expressing control levels of MCM correlate well with values obtained from previously published studies (r = 0.91, S3C Fig) [37]. A comparison of Trep values between untreated and auxin-treated conditions indicates that reduction of MCM levels leads to delays in replication timing across the genome and that these delays increase with higher auxin concentrations (Fig 4B). Together, this data demonstrates that reduction of cellular pools of MCM and subsequent reduction of MCM levels loaded at origins has direct implications for replication timing at specific origins in yeast.
Overlaying the Trep profiles reveals that some origins that are active in untreated cells become inactive in auxin-treated cells. Loss of origin activity from these origins correlates with a decrease in MCM signal by ChIP, as is evident for ARS512 and ARS520 (Fig 4A, black boxes). In contrast, other origins, such as ARS511 and ARS16, are less affected by auxin treatment (Fig 4A, gray boxes). To investigate the extent of this correlation, we examined it genome wide (Fig 4C and 4D). The replication timing of many origins throughout the budding yeast genome is controlled by specific mechanisms involving trans-acting factors and chromosomal location, such as Rif1, Rpd3, Fkh1, and Ctf19 binding, or telomere proximity, [16,38–41]. We measured Trep values and MCM abundance for the 46% of origins of replication that exclude those known to be affected by specific mechanisms of origin regulation [20]. Comparison of Trep values and MCM abundance for these origins under endogenous conditions indicated a small negative correlation between MCM abundance and timing of replication, suggesting that origins with higher MCM levels replicate earlier in S phase (Fig 4C, 0 μM auxin). The correlation increased and the slope became more negative in conditions where MCM levels were reduced via auxin (Fig 4C, 30 μM and 500 μM auxin). Furthermore, comparing changes in Trep with changes in MCM abundance as a result of auxin treatment revealed a positive correlation, indicating that larger decreases in MCM loading correlate with stronger delays in replication timing (Fig 4D). The analysis is complicated by the fact that Trep convolves origin firing time and passive replication. For instance, the MCM signal at ARS501 is greatly reduced and its replication-timing peak is lost (Fig 4A). However, its Trep value does not change much, because it is passively replicated by ARS511, which remains early-firing. Such passive replication reduces the effect seen in Fig 4C and 4D. Nonetheless, taken together, these results suggest that decreases in MCM loading lead to delays in replication timing at origins of replication. The 54% of origins that are known to be affected by trans-acting factors display a much weaker correlation between MCM signal and replication timing (r = 0.08, S9A Fig), but that correlation becomes stronger upon MCM depletion (r = 0.25–0.30, S9B and S9C Fig), suggesting that MCM loading affects the timing of these origins, as well.
Cells overexpressing MCM are viable
Reduction of MCM pools leads to significant changes in MCM loading and replication timing. In order to investigate the effects of the converse condition of increased MCM pools, we employed the galactose overexpression system. The six genes encoding MCM were expressed from bidirectional Gal-1,10 promoters integrated into the genome, in addition to their endogenous copies [13]. The overexpressed copy of Mcm7 was tagged at its C terminus with GFP in order to monitor its overexpression levels. To test whether cells overexpressing MCM are viable, we performed serial dilution assays on YP-Raffinose and YP-Galactose plates. Overexpression of the complete hexamer, with or without the added GFP tag on Mcm7, did not affect cell viability (S10A Fig). However, overexpression of the MCM hexamer in conjunction with the loading factor Cdt1, but not overexpression of Cdt1 alone, reduced viability. This data shows that Mcm2-7 overexpression by itself is not lethal and can be used to increase cellular pools of MCM helicase.
Overexpression of MCM during a G1 arrest does not affect progression through S phase
We assayed whether overexpression of MCM leads to changes in helicase loading prior to S phase, and whether such changes affect replication timing. We synchronized cells in metaphase using nocodazole then released them into media containing α-factor for synchronization at the G1/S boundary (Figs 5A and S1). In addition to α-factor, the media was supplemented with galactose or raffinose, to induce Mcm2-7 overexpression or not, respectively. Induction of MCM was monitored via western blot using a polyclonal antibody against MCM. After two hours, a ~5-fold overexpression of the hexamer was observed (Fig 5B). A portion of the α-factor arrested culture was collected for ChIP-seq analysis while the rest was released into S phase to monitor replication timing. As seen in Fig 5C, cells overexpressing MCM during a G1 arrest show a slight delay in replication initiation in S phase. However, a control strain that did not overexpress MCM showed similar results, indicating that the delay was likely due to the switch in carbon source (S10B Fig). Therefore, overexpression of MCM does not appear to cause any significant changes to cell cycle progression.
Increased MCM levels do not alter relative levels of helicase loading at origins
In order to measure MCM loading in cells overexpressing the full hexamer, we performed MNase ChIP-seq on α-factor arrested cells as outlined in Fig 5A. Fragments of the genome that were associated with MCM were pulled down, sequenced, and their abundance was normalized to an S. pombe spike-in control, resulting in peaks that correspond to previously annotated origins of replication (Fig 5D). In addition, the signal of MCM peaks correlates well with data from the MCM-depletion experiments, as well as previous publications (r = 0.78–0.93, S11A and S11B Fig).
To gauge whether increased cellular pools of MCM helicase lead to changes in loading during G1, we compared MCM abundance at origins of replication in cells overexpressing MCM and those that did not (S1 Table). MCM signal at origins in cultures overexpressing MCM show a ~41% decrease in abundance compared to cultures with endogenous MCM levels (Fig 6A and 6E). However, this difference is almost perfectly uniform throughout all origins assayed (r = 0.99, Fig 6A), and shows no apparent difference in MCM ChIP-seq reads (Fig 6D), pointing to technical reasons involving ChIP or non-MCM-specific biological consequences of the overexpression. This result was not due to an insufficient amount of time allowed for loading, as three hours of MCM overexpression in α-factor produced similar loading levels (r = 0.99, S12A Fig). As a result, we conclude that overexpression of Mcm2-7 does not alter relative helicase loading in G1.
MCM requires Cdt1 to enter the nucleus and to be loaded onto origins of replication [10]. Although Cdt1 disassociates from the MCM complex after it is loaded onto DNA, it doesn’t fully exit the nucleus until late G1/early S phase. Therefore, although Cdt1 likely shuttles in and out of the nucleus in some equilibrium during the α-factor arrest in our experiments, it may not be able to accommodate nuclear import for all of the overexpressed MCM2-7 hexamers. To address the possibility that overexpressed MCM is not imported into the nucleus and therefore not loaded onto DNA due to substoichiometric levels of Cdt1, we overexpressed MCM2-7 along with Cdt1. However, we did not observe any significant changes in relative MCM loading (r = 0.98, S12C Fig). Furthermore, the lack of any changes was not due to the inability of the overexpressed hexamer to enter cell nuclei, as microscopy confirmed the presence of overexpressed Mcm7 in cell nuclei (S13 Fig). All together, these results indicate that overexpression of MCM helicase does not cause altered loading dynamics in G1.
Overexpression of MCM does not affect replication timing
To test whether the increase in cellular MCM abundance led to changes in the replication timing program, we performed sync-seq experiments. Trep values for cells expressing endogenous levels of MCM correlate well with values obtained from the MCM-depletion experiments as well as previously published data (r = 0.92, S11C Fig) [37]. Moreover, origin replication times for cells overexpressing MCM do not significantly differ from control cells, beyond a brief and global delay attributed to the switch in carbon source (Figs 6B and 5C). Moreover, changes in replication timing do not correlate with changes in MCM signal (Fig 6C). Altogether, this data shows that overexpression of the MCM helicase does not affect replication timing.
Discussion
A unifying model of the mechanisms involved in establishing replication timing in eukaryotes remains elusive. Numerous cis- and trans-acting factors have been shown to affect timing, but the mechanism by which they do so is unclear [8]. Since replication timing is primarily determined by the timing of origin firing, these factors are thought to affect the timing of MCM activation. However, it has also been noted that regulating MCM occupancy at origins would affect replication timing, because higher MCM occupancy at an origin would lead to a higher probability of it firing and thus an earlier average firing time [22,23,26]. Variable MCM occupancy could occur in one of two scenarios. The first is the single-MCM scenario, in which an origin can either be loaded with an MCM-DH complex or not. MCM occupancy at a specific origin would, in this scenario, be the fraction, from 0 to 1, of cells in which an MCM complex is loaded at that origin, a parameter that has been referred to as origin competency [21,24–26]. Alternatively, in the multiple-MCM scenario, more than one MCM-DH complex could be loaded at a single origin, so MCM occupancy could range from 0 to many [20,22,42].
Quantification of MCM components in budding yeast using a variety of techniques has yielded a wide range of values for the number of MCMs in each cell [43–45]. A meta-study using data from 21 publications reported median value estimates for MCM components that ranged from 2774–5360 molecules per cell for each of the components of the MCM helicase [46]. This analysis suggests that MCM is present in cells at levels that allow for loading of many more than one MCM at each of the 400 or so origins that are present in the genome. Moreover, measurements of in vivo chromatin binding in budding yeast indicate that MCM is loaded at a much higher number than accounted by the loading of a single MCM-DH at known origins [44].
Indeed, studies from various eukaryotic organisms have shown that MCM is loaded onto the genome at levels that are higher than necessary for replication under optimal conditions [47,48]. However, the excess of loaded MCM appears to be necessary under conditions that lead to elevated levels of replication stress. In Xenopus egg extracts, excess MCM loading becomes essential for successful replication under conditions of replication stress, indicating that dormant, excess MCM molecules are activated to salvage stalled replication forks that result from replication stress [49]. In C. elegans, worms only become susceptible to low doses of HU when their MCM levels are reduced [49]. Similarly, studies using human cells have suggested a mechanism where excess MCM hexamers that are loaded and not used during unperturbed replication become vital for successful replication after treatment with replication-stress-inducing agents [50,51]. Finally, MCMs were originally isolated based on the fact that reducing MCM number causes loss of minichromosomes, which are more sensitive to origin function than regular chromosomes [52,53]. Altogether, this data suggests that eukaryotes load more MCM onto DNA in G1 than is needed during an unperturbed S phase.
Although excess loading of MCM is important for a successful S phase under conditions of replication stress, it has also been implicated in contributing to the replication timing program under normal conditions. Genome-wide MCM mapping experiments in budding yeast have shown that MCM is loaded at origins in different amounts, and that the level of MCM loading correlates with the time in S phases at which an origin fires [20,21]. In addition, mutation of the B2 element in ARS1, which has been shown to be important for MCM loading at that origin, causes reduced MCM loading and a delay in replication timing [20,54]. This data points to a model where the more MCMs that are available for activation at an origin in S phase, the higher the likelihood that the specific origin will initiate early. Indeed, this MCM-stoichiometry model fits well with kinetic modeling of replication, which predicts that stochastic firing arising from differences in the availability of MCM in the presence of limiting initiation factors can give rise to the observed replication kinetics seen in budding yeast cells [21,22,26]. It is important to note that the MCM-stoichiometry models are equally valid whether MCM stoichiometry varies from 0 to 1 or 0 to many.
Our previous work supports a model in which multiple MCMs are loaded at origins [20,22]. Furthermore, overexpression of origin-activating factors in S phase causes most all origins to fire early in S phase, consistent with most origins having at least one MCM loaded [55]. Our MNase approach to MCM ChIP-seq reported here further supports the multiple-MCM model by producing high-resolution maps of MCM locations that identify MCMs at multiple locations across origins. We find MCM ChIP-seq signal distributed around origins up to three nucleosomes away from the ACS, similar to previous lower resolution results [19], in addition to signal inside the origin NFR (Fig 3A). The location of MCMs in the NFR and the surrounding nucleosomes support a model in which MCMs are mobile after being loaded and can slide past nucleosomes during nucleosome exchange. Indeed, this data is consistent with observations that early origins, which tend to have more MCM signal by ChIP-seq ([20] and Fig 4C), display higher rates of nucleosome exchange [56]. Furthermore, the fact that we find MCM with equal frequency upstream and downstream of origins suggests that ORC does not prevent MCM from diffusing past the ACS, consistent with ORC having a short dwell time at origins [13,57]. Nonetheless, because our current ChIP-seq data only represents an average of MCM locations, it cannot formally exclude the possibly that no more that one MCM-DH complex is ever loaded at a single origin—albeit at varying locations—and thus our current data does not discriminate between the single- and multiple-MCM scenarios. However, for all the analyses presented here, the two scenarios are formally equivalent and make the same predictions about how competition between origins for MCM loading affects replication timing.
Regardless of stoichiometry, the possibility of variable MCM occupancy raises interesting questions about how MCM occupancy is regulated and how it affects replication timing. We considered two hypotheses for how varying MCM occupancy between origins could be regulated. The first hypothesis, which we refer to as the ORC Activity model, posits that the rate at which ORC loads MCM varies among origins. ORC activity at an origin could vary due to ORC occupancy, which could be affected by ORC affinity for the ACS or by the local chromatin environment [31], or due to local regulation of ORC specific activity, which could be affected by local activators or repressors. The second hypothesis, which we refer to as the Origin Capacity model, posits that origins have an intrinsic capacity for MCM loading that varies among origins, and that once that capacity is achieved, no more MCMs can be loaded. To distinguish between these models, we varied cellular MCM levels, reasoning that changes in cellular MCM levels would lead to predictable changes in the level of MCM loaded at origins, depending on the mechanism that regulates origin loading. In particular, in response to a reduction in cellular MCM levels, the Origin Activity model predicts that all origins would be proportionally reduced in MCM occupancy, because origins will load at the same relative rates but the MCM pool will be depleted sooner. On the other hand, the Origin Capacity model predicts that origins with low capacities will fill up as normal, but that origins with higher capacities will fail to reach regular capacities if the MCM pool is depleted (Fig 7A).
Our results are not consistent with either the simple ORC Activity or Origin Capacity model (Figs 2A and 7A). Instead, we propose a hybrid model, in which both ORC activity and origin capacity vary at each origin (Fig 7B). In the hybrid model, origin capacity is the primary effector of MCM occupancy in wild-type cells. ORC activity does vary among origins, but because neither time during G1 nor MCM amount is limiting, all origins are loaded to their full capacity. However, when MCM levels become limiting, not all origins can be fully occupied. In this case, origins with high ORC activity (bright red in Fig 7B) outcompete other origins and are still loaded to their full capacity, whereas origins with progressively lower ORC activity (light red and pink in Fig 7B) load MCM to progressively lower proportions of their full capacity before the MCM pool is exhausted. Therefore, although origin competition does not appear to play a decisive role in MCM loading in wild-type cells, its appearance when MCMs become limiting offers insight into the dynamics of MCM loading.
Our hybrid model is consistent with the behavior of three classes of origins previously characterized by ORC affinity and origin activity ([31] and Fig 2C). These three classes—DNA-dependent, chromatin-dependent and weak—show the behavior predicted by the hybrid model, with the strong, DNA-dependent origins maintaining close to full MCM loading (109–94%), the somewhat less strong, chromatin-dependent origins showing an intermediate reduction (100–77%), and the weak origins showing the greatest reduction in MCM loading (74–48%). Our hybrid model is also consistent with our MCM over-expression experiments. We find no change in the relative MCM ChIP-seq signal at origins in response to a five-fold increase in cellular MCM levels (r = 0.99, Fig 6A). This result is consistent with the conclusion that origins in wild-type cells are loaded to their full capacity and that MCM is normally in excess in budding yeast [44].
Although we find no relative difference in MCM ChIP-seq signal in our MCM overexpression experiments, we find an absolute reduction of 41% (Fig 6A). This result was dependent on overexpression constructs being present in the cells, because a control strain with no overexpressing genes did not display any reduction in MCM ChIP-seq signal in response to galactose (S12B Fig). This result does not appear to be due to a uniform increase in background signal, which might be expected if excess MCM was loaded with low specificity at many sites across the genome, because the data was normalized to an S. pombe spike-in to allow for absolute quantitation. It could be that the overexpression of MCM titrates away an interacting component that is crucial for MCM loading or nuclear import. However, in that case we would expect to see an effect similar to reducing MCM levels, which does not affect all origins uniformly (Fig 2A). Alternatively, although the antibody is added in saturating amounts, antibody-binding dynamics of chromatin-bound MCM could be altered due to the presence of excess MCM. In any case, given the lack of a plausible biological and mechanistic explanation for reduced MCM loading in response to MCM overexpression, and the nearly perfect correlation between plus and minus overexpression conditions, we conclude that increased MCM levels do not cause altered MCM loading in yeast.
In addition to the lack of changes in MCM loading, overexpression of MCM did not affect cell viability, bulk S-phase progression, or replication timing (Fig 6). In contrast, overexpression of MCM along with Cdt1, but not Cdt1 alone, was lethal if constitutively expressed (S8A Fig), resulting in dumbbell-shaped terminal phenotype and suggesting a metaphase arrest. This result does not appear to be related to MCM loading or replication timing (at least in the window of one cell cycle) as levels of MCM loading and replication timing remained largely unchanged in MCM/Cdt1-overexpressing cells (S11C Fig). Although this points to a synergistic effect between MCM and Cdt1 in causing cell death, the exact mechanism for the lethality remains unclear.
Reduction of MCM levels caused a delay in progression through bulk S phase (Figs 1C and 4A). The slower progression through S phase is consistent with less MCM being loaded onto some origins, resulting in fewer origins being activated in S phase. If MCM levels at all origins were uniformly reduced, we would not expect any change in replication timing because replication initiation in budding yeast is regulated by competition for a limited a set of initiation factors [15,58]. If MCM loading were lowered in uniform proportions, the relative competition for initiation factors, and thus replication timing, would be maintained. However, because the reduction of MCM loading is not uniform, and because low MCM origins tend to lose more MCM than high efficiency ones (Fig 2B), the distribution of MCM is more heterogeneous, leading to larger distances between efficient origins and thus longer S phase (S4 Fig and S2 Table).
Our combination of MCM ChIP-seq and replication timing data also allow us to directly confirm in a single experiment previous conclusions, drawn from comparing data collected in different studies, that replication timing correlates with levels of MCM loading [20,21]. Although the correlation between MCM levels and replication timing is robust (Fig 4C, p > 10−5), it is clearly not the only determining factor (r = 0.29–0.52). Therefore, we conclude that MCM loading is a significant effector of replication timing, but one that is modulated by other factors that affect the specific activity of loaded MCMs. Nonetheless, by manipulating MCM levels and showing that replication changes concomitantly, we confirm genome-wide that MCM levels directly regulate replication timing (Fig 4D), an experiment that had previously been done only at a single locus [20].
In this study, we show that some origins are efficient at recruiting MCM, while others depend on excess levels of the helicase to display the loading observed in wild type cells. These results indicate that the relative levels of MCM loaded at origins are not simply static, but rather a dynamic balance dependent on cellular MCM levels, origin MCM recruiting ability, and origin MCM capacity. In addition, our data suggests that wild-type MCM abundance is saturating, such that increasing levels further does not lead to increased loading. Altogether, this work suggests that MCM loading homeostasis in wild type cells, and subsequently replication timing, is dependent on MCM being in excess. In future studies, it will be interesting to dissect the specific cis- and trans-acting factors that make origins sensitive or resistant to changes in MCM levels. The rapid evolution of origins within the Saccharomyces sensu stricto clade provides a rich resource for a genome-wide approach to such studies [59,60]
Materials and methods
Strains used are listed in Table 1. Standard techniques were used for strain constructions. Cultures were grown in YP-Dextrose (YPD) at 30°C, unless otherwise noted.
Auxin degradation experiments
S. cerevisiae strain yFS1059 (MCM4-AID-GFP) was grown to an OD of ~0.2. Nocodazole was added to a final concentration of 7.5 μg/ml for two hours. 1.5 hours into the nocodazole arrest, cultures were supplemented with auxin (Indole-3-acetic acid sodium salt, Sigma I5948) to final concentrations of 500 μM, 30 μM, or 0 μM. After two hours total in nocodazole, cultures were vacuum-filtered and cells were resuspended in fresh YPD supplemented with 5 μg/ml α-factor (Biomatik) and auxin to a final concentration of 500 μM, 30 μM, or 0 μM, as before filtration. After 1.5 hours, cultures were vacuum filtered and cells were resuspended in fresh YPD supplemented with 500 μM, 30 μM, or 0 μM, as before filtration, for 30 minutes. Cultures were vacuum-filtered a final time and cells were resuspended in fresh YPD for S phase progression.
For ChIP sample collection, α-factor-arrested cells were crosslinked with formaldehyde and collected as previously described (Wal & Pugh 2012).
Galactose overexpression experiments
S. cerevisiae strains yFS1075 (GAL-MCM), yFS1021 (GAL-MCM, GAL-CDT1), and yFS1020 (WT) were grown in YP-Raffinose (YP-Raf) at 30°C to an OD of ~0.2. Nocodazole was added to a final concentration of 10 μg/ml. After two hours, cultures were vacuum-filtered and cells were resuspended in fresh YP-Raf supplemented with α-factor (Biomatik) to a final concentration of 25 nM, as well as either galactose to a final concentration of 2% or an equal volume of water. Cells were allowed to arrest in α-factor for either two or three hours, followed by release via vacuum filtration into fresh YPD supplemented with 0.2 mg/ml pronase (Sigma P6911).
For ChIP sample collection, α-factor arrested cells were crosslinked with formaldehyde and collected as previously described (Wal & Pugh 2012). After formaldehyde quenching, S. cerevisiae cells were combined with log-phase wild-type S. pombe cells (yFS105, also crosslinked) at a 9:1 ratio.
Fluorescence microscopy
Cultures were grown and supplemented with 2% final galactose as in Fig 5A. At the α-factor-arrest point, 1ml cells were fixed by the addition of 10ml methanol which was pre-chilled in dry ice, then stored at -80°C until imaging. To prepare for imaging, fixed cells were equilibrated to 4°C from their -80°C storage, centrifuged, and all but 1ml supernatant was removed. The remaining mix was washed 2x with 2 ml ice cold PBS. Cells were then resuspended in 150 μl Vectashield+DAPI (Vector Laboratories H-1200) and imaged using a Zeiss Axioskop 2 Plus microscope fitted with DIC, GFP, and DAPI filters.
Spot assays
Yeast was grown in YPD (auxin strains) or YP-Raf (Galactose-overexpression strains) overnight at 30°C. Log phase cells were collected by brief centrifugation, washed twice with PBS, serially diluted five-fold starting with 4x106 cells, then spotted onto the specified medium. Plates were incubated at 30°C for at least 36 hours before imaging.
Western blots and quantitations
Standard western blot techniques were used [61]. Mcm2-7 was probed with polyclonal UM174 (gift from Bell lab, MIT—[62]) and anti-rabbit HRP conjugate secondary (Promega W401B), tubulin was probed with monoclonal anti-tubulin antibody (Sigma T5168) and anti-mouse HRP conjugate secondary (Promega W402B), and GFP was probed with the monoclonal JL8 antibody (Takara) and anti-mouse HRP conjugate secondary (Promega W401B). Probing of Mcm2-7 using UM174 antibody was performed using 12% gels in order to compress signal from the six MCMs into a compact region to facilitate quantification. Signal was detected using SuperSignal West Dura chemiluminescent HRP substrate (Thermo 34076) and GE Amersham Imager 600. Quantitation of gel images was carried out using ImageJ (NIH, Maryland, USA).
ChIP experiments
ChIP experiments were carried out as described previously with modifications noted below (Wal & Pugh 2012). MNase was titrated for each sample to determine concentrations that would yield ~80–90% mononucleosomal digestion. Immunoprecipitation was carried out using 95% of the MNase digested sample (v/v) and 4 μl of anti-MCM2-7 polyclonal antibody (UM174, gift from Bell lab, MIT—[62]). The remaining 5% of MNase digested sample was processed as ‘input’ and was treated with Proteinase K and RNase A to prepare libraries for deep sequencing.
Flow cytometry
0.25 ODs of fixed cells (see below) were washed once with water, resuspended in 250 μl RNase A solution (100 μg/ml RNase A, 50 mM Tris pH 8.0, 15 mM NaCl), and incubated overnight at 37°C. Cells were then collected and resuspended in Proteinase K solution (125 μg/ml Proteinase K, 50 mM Tris pH 8.0) for 1 hour at 50°C. The samples were then collected by centrifugation, resuspended in 1 ml staining solution (1 μM Sytox green–ThermoFisher S7020, 50 mM Tris pH8.0), sonicated briefly using a microtip sonicator, and analyzed for flow cytometry using a Guava easyCyte instrument.
Sync-seq replication timing experiments
Experiments to monitor replication timing consisted of measuring population movement through S phase by flow cytometry and measuring genome-wide replication timing by deep sequencing [37]. To do so, 3 ODs of cells were collected for each time point and arrested by the addition of sodium azide to 0.1% and EDTA to 20mM. From these samples, 0.25 ODs were used for flow cytometry and the rest was used for genome-wide copy number analysis by deep sequencing.
To prepare genomic DNA for deep sequencing, cells were lysed as for ChIP experiments. Lysates were treated with proteinase K and RNase A, followed by two consecutive extractions with phenol-chloroform-IAA (25:24:1, Fisher). DNA was purified by ethanol precipitation and resuspended in 135 μl water in preparation for shearing. A Covaris machine was used to shear the DNA to an average size of ~200bp, following manufacturer’s instructions. DNA was then purified by DNA Clean and Concentrator Columns (Zymo Research) before making libraries.
Library preparation and sequencing
Libraries were prepared using NEBNext Ultra II kits (NEB) following the manufacturer’s protocol. Following library preparation, ChIP samples were purified as described [30], while input samples were purified using a 2:1 ratio of AmpureXP (GE) beads to library. Following PCR amplification, all samples were purified using AMpure XP beads with 0.9:1 beads to PCR ratio. Samples were sequenced using the Illumina NextSeq 500 platform with paired ends. See S3 and S4 Tables for library statistics.
Data analysis
The sequencing data from this study have been submitted to the NCBI Sequence Read Archive under accession number PRJNA663099. For MNase-ChIP experiments, sequencing reads were mapped to SacCer3 using Bowtie1, a 650bp upper limit cutoff, and exclusion of reads mapping to more than one genomic location. Duplicates were removed using Samtools 1.4.1. ACS-centered density profiles were constructed using coverage files normalized as indicated in the paragraph below. V plot intensities were normalized to counts per million (CPM) and generated by taking into account strand specificity of the ACSs [11] using R and modified in-house scripts (courtesy of Nils Krietenstein). Heatmaps were generated using Deeptools 3.0.2 without taking strand specificity into account. Quantification of MCM signal at origins of replication was done using a 1 kb window centered at the origin or ACS midpoints. Correlation coefficients and slopes were calculated for origins displaying normalized MCM signal greater than zero for untreated cells. The set of origins displaying ARS activity in plasmid assays from OriDB [63] was used for all quantitations, unless otherwise stated. For the MCM depletion experiments, all analyses were preformed on both replicates with similar results. Results from Replicate #1 are presented for all analyses because it displayed a better separation between the 30 and 500 μm datasets. The exception is the V plots, for which the higher resolution Replicate #2 is presented.
Coverage files for auxin degradation experiments were normalized to CPM and to the non-origin background signal in 25 bp windows. Input signal was then subtracted from the normalized ChIP coverage files to account for MNase digest-induced background oscillations. For galactose induction experiments, ChIP coverage files were normalized in 25 bp windows to the total number of reads mapped to the S. pombe spike-in control. Normalized input signal was then subtracted from the normalized ChIP coverage to account for background oscillations in the data.
For replication timing experiments, coverage files were generated using LocalMapper scripts and Trep was calculated in 1000 bp bins genome wide using Repliscope. Both packages were shared by Dzmitry Batrakou of the Nieduszynski Lab and are available at https://github.com/DzmitryGB/ [64]. Trep data generated from Repliscope was LOESS-smoothed in windows of ~50kb using Igor (Wavemetrics, Lake Oswego, OR, USA). Trep data for subtelomeric origins residing within 15 kb of chromosome ends was discarded due to large amount of noise. At least seven samples covering S phase progression were used to estimate Trep.
Supporting information
S1 Fig [pdf]
Progression of synchronized cultures through S phase as monitored by flow cytometry.
S2 Fig [pdf]
Auxin-induced degradation of Mcm4 causes reduced viability.
S3 Fig [pdf]
MNase-ChIP-seq and replication timing results from the MCM reduction experiments are reproducible.
S4 Fig [pdf]
Genome-wide reduction in MCM loading leads to larger inter-origin distances.
S5 Fig [pdf]
Effects of MCM depletion on MCM loading at origins.
S6 Fig [pdf]
Fragment analyzer results for the two MCM reduction replicates shows different degrees of MNase digestion.
S7 Fig [pdf]
Input density profiles and origin coverage quantitations do not change significantly after auxin-induced Mcm4 degradation.
S8 Fig [pdf]
ACS-annotated origins separated by magnitude of signal upstream or downstream of ACS.
S9 Fig [pdf]
Correlation of MCM signal and replication timing for origins that are affected by specific timing mechanisms.
S10 Fig [gfp]
MCM overexpression does not affect cell viability.
S11 Fig [pdf]
MNase-ChIP-seq and replication timing results from the MCM overexpression experiments are reproducible.
S12 Fig [pdf]
Overexpression of MCM for longer times or along with Cdt1 does not alter loading levels at origins or replication timing.
S13 Fig [pdf]
Overexpressed MCM is able to enter the nucleus during α-factor arrest.
S1 Table [xls]
Quantification of MCM signal at origins of replication and Trep data for ARS-annotated origins (OriDB).
S2 Table [xls]
Smallest number of origins that make up 50% of total MCM signal for each condition, as well as the interorigin distances between those sets of origins.
S3 Table [xls]
Mnase-ChIP Sequencing Statistics.
S4 Table [xls]
Replication Timing Sequencing Statistics.
S5 Table [xls]
Numerical data for all figures.
Zdroje
1. Bell SP, Labib K. Chromosome Duplication in Saccharomyces cerevisiae. Genetics. 2016;203: 1027–1067. doi: 10.1534/genetics.115.186452 27384026
2. Bleichert F. Mechanisms of replication origin licensing: a structural perspective. Curr Opin Struct Biol. 2019;59: 195–204. doi: 10.1016/j.sbi.2019.08.007 31630057
3. Boos D, Ferreira P. Origin Firing Regulations to Control Genome Replication Timing. Genes (Basel). 2019;10: doi: 10.3390/genes10030199 30845782
4. Gilbert DM, Takebayashi SI, Ryba T, Lu J, Pope BD, Wilson KA et al. Space and time in the nucleus: developmental control of replication timing and chromosome architecture. Cold Spring Harb Symp Quant Biol. 2010;75: 143–153. doi: 10.1101/sqb.2010.75.011 21139067
5. Goren A, Cedar H. Replicating by the clock. Nat Rev Mol Cell Biol. 2003;4: 25–32. doi: 10.1038/nrm1008 12511866
6. Lang GI, Murray AW. Mutation rates across budding yeast chromosome VI are correlated with replication timing. Genome Biol Evol. 2011;3: 799–811. doi: 10.1093/gbe/evr054 21666225
7. Müller CA, Nieduszynski CA. DNA replication timing influences gene expression level. J Cell Biol. 2017;216: 1907–1914. doi: 10.1083/jcb.201701061 28539386
8. Rhind N, Gilbert DM. DNA replication timing. Cold Spring Harb Perspect Biol. 2013;5: a010132. doi: 10.1101/cshperspect.a010132 23838440
9. Nguyen VQ, Co C, Li JJ. Cyclin-dependent kinases prevent DNA re-replication through multiple mechanisms. Nature. 2001;411: 1068–1073. doi: 10.1038/35082600 11429609
10. Tanaka S, Diffley JF. Interdependent nuclear accumulation of budding yeast Cdt1 and Mcm2-7 during G1 phase. Nat Cell Biol. 2002;4: 198–207. doi: 10.1038/ncb757 11836525
11. Eaton ML, Galani K, Kang S, Bell SP, MacAlpine DM. Conserved nucleosome positioning defines replication origins. Genes Dev. 2010;24: 748–753. doi: 10.1101/gad.1913210 20351051
12. Xu W, Aparicio JG, Aparicio OM, Tavaré S. Genome-wide mapping of ORC and Mcm2p binding sites on tiling arrays and identification of essential ARS consensus sequences in S. cerevisiae. BMC Genomics. 2006;7: 276. doi: 10.1186/1471-2164-7-276 17067396
13. Ticau S, Friedman LJ, Ivica NA, Gelles J, Bell SP. Single-Molecule Studies of Origin Licensing Reveal Mechanisms Ensuring Bidirectional Helicase Loading. Cell. 2015 doi: 10.1016/j.cell.2015.03.012 25892223
14. Labib K. How do Cdc7 and cyclin-dependent kinases trigger the initiation of chromosome replication in eukaryotic cells. Genes Dev. 2010;24: 1208–1219. doi: 10.1101/gad.1933010 20551170
15. Mantiero D, Mackenzie A, Donaldson A, Zegerman P. Limiting replication initiation factors execute the temporal programme of origin firing in budding yeast. EMBO J. 2011;30: 4805–4814. doi: 10.1038/emboj.2011.404 22081107
16. Hiraga S, Alvino GM, Chang F, Lian HY, Sridhar A, Kubota T et al. Rif1 controls DNA replication by directing Protein Phosphatase 1 to reverse Cdc7-mediated phosphorylation of the MCM complex. Genes Dev. 2014;28: 372–383. doi: 10.1101/gad.231258.113 24532715
17. Hayashi MT, Takahashi TS, Nakagawa T, Nakayama J, Masukata H. The heterochromatin protein Swi6/HP1 activates replication origins at the pericentromeric region and silent mating-type locus. Nat Cell Biol. 2009;11: 357–362. doi: 10.1038/ncb1845 19182789
18. De Piccoli G, Katou Y, Itoh T, Nakato R, Shirahige K, Labib K. Replisome stability at defective DNA replication forks is independent of S phase checkpoint kinases. Mol Cell. 2012;45: 696–704. doi: 10.1016/j.molcel.2012.01.007 22325992
19. Belsky JA, MacAlpine HK, Lubelsky Y, Hartemink AJ, MacAlpine DM. Genome-wide chromatin footprinting reveals changes in replication origin architecture induced by pre-RC assembly. Genes Dev. 2015;29: 212–224. doi: 10.1101/gad.247924.114 25593310
20. Das SP, Borrman T, Liu VW, Yang SC, Bechhoefer J, Rhind N. Replication timing is regulated by the number of MCMs loaded at origins. Genome Res. 2015;25: 1886–1892. doi: 10.1101/gr.195305.115 26359232
21. Foss EJ, Sripathy S, Gatbonton-Schwager T, Kwak H, Thiesen AH, Lao U et al. Chromosomal Mcm2-7 distribution is the primary driver of the genome replication program in species from yeast to humans. bioRxiv. 2020737742. doi: 10.1101/737742
22. Yang SC, Rhind N, Bechhoefer J. Modeling genome-wide replication kinetics reveals a mechanism for regulation of replication timing. Mol Syst Biol. 2010;6: 404. doi: 10.1038/msb.2010.61 20739926
23. Rhind N, Yang SC, Bechhoefer J. Reconciling stochastic origin firing with defined replication timing. Chromosome Res. 2010;18: 35–43. doi: 10.1007/s10577-009-9093-3 20205352
24. Stillman B. Origin recognition and the chromosome cycle. FEBS Letters. 2005;579: 877–884. doi: 10.1016/j.febslet.2004.12.011 15680967
25. McCune HJ, Danielson LS, Alvino GM, Collingwood D, Delrow JJ, Fangman WL et al. The temporal program of chromosome replication: genomewide replication in clb5{Delta} Saccharomyces cerevisiae. Genetics. 2008;180: 1833–1847. doi: 10.1534/genetics.108.094359 18832352
26. de Moura AP, Retkute R, Hawkins M, Nieduszynski CA. Mathematical modelling of whole chromosome replication. Nucleic Acids Res. 2010;38: 5623–5633. doi: 10.1093/nar/gkq343 20457753
27. Nishimura K, Fukagawa T, Takisawa H, Kakimoto T, Kanemaki M. An auxin-based degron system for the rapid depletion of proteins in nonplant cells. Nat Methods. 2009;6: 917–922. doi: 10.1038/nmeth.1401 19915560
28. Nishimura K, Kanemaki MT. Rapid Depletion of Budding Yeast Proteins via the Fusion of an Auxin-Inducible Degron (AID). Curr Protoc Cell Biol. 2014;64: 20.9.1–16. doi: 10.1002/0471143030.cb2009s64 25181302
29. Labib K, Kearsey SE, Diffley JF. MCM2-7 proteins are essential components of prereplicative complexes that accumulate cooperatively in the nucleus during G1-phase and are required to establish, but not maintain, the S-phase checkpoint. Mol Biol Cell. 2001;12: 3658–3667. doi: 10.1091/mbc.12.11.3658 11694596
30. Wal M, Pugh BF. Genome-wide mapping of nucleosome positions in yeast using high-resolution MNase ChIP-Seq. Methods Enzymol. 2012;513: 233–250. doi: 10.1016/B978-0-12-391938-0.00010-0 22929772
31. Hoggard T, Shor E, Müller CA, Nieduszynski CA, Fox CA. A Link between ORC-origin binding mechanisms and origin activation time revealed in budding yeast. PLoS Genet. 2013;9: e1003798. doi: 10.1371/journal.pgen.1003798 24068963
32. McGuffee SR, Smith DJ, Whitehouse I. Quantitative, genome-wide analysis of eukaryotic replication initiation and termination. Mol Cell. 2013;50: 123–135. doi: 10.1016/j.molcel.2013.03.004 23562327
33. Miller TCR, Locke J, Greiwe JF, Diffley JFX, Costa A. Mechanism of head-to-head MCM double-hexamer formation revealed by cryo-EM. Nature. 2019;575: 704–710. doi: 10.1038/s41586-019-1768-0 31748745
34. Henikoff JG, Belsky JA, Krassovsky K, MacAlpine DM, Henikoff S. Epigenome characterization at single base-pair resolution. Proc Natl Acad Sci U S A. 2011;108: 18318–18323. doi: 10.1073/pnas.1110731108 22025700
35. Coster G, Diffley JFX. Bidirectional eukaryotic DNA replication is established by quasi-symmetrical helicase loading. Science. 2017;357: 314–318. doi: 10.1126/science.aan0063 28729513
36. Remus D, Beuron F, Tolun G, Griffith JD, Morris EP, Diffley JF. Concerted loading of Mcm2-7 double hexamers around DNA during DNA replication origin licensing. Cell. 2009;139: 719–730. doi: 10.1016/j.cell.2009.10.015 19896182
37. Müller CA, Hawkins M, Retkute R, Malla S, Wilson R, Blythe MJ et al. The dynamics of genome replication using deep sequencing. Nucleic Acids Res. 2014;42: e3. doi: 10.1093/nar/gkt878 24089142
38. Knott SR, Viggiani CJ, Tavaré S, Aparicio OM. Genome-wide replication profiles indicate an expansive role for Rpd3L in regulating replication initiation timing or efficiency, and reveal genomic loci of Rpd3 function in Saccharomyces cerevisiae. Genes Dev. 2009;23: 1077–1090. doi: 10.1101/gad.1784309 19417103
39. Lian HY, Robertson ED, Hiraga S, Alvino GM, Collingwood D, McCune HJ et al. The effect of Ku on telomere replication time is mediated by telomere length but is independent of histone tail acetylation. Mol Biol Cell. 2011;22: 1753–1765. doi: 10.1091/mbc.E10-06-0549 21441303
40. Knott SR, Peace JM, Ostrow AZ, Gan Y, Rex AE, Viggiani CJ et al. Forkhead transcription factors establish origin timing and long-range clustering in S. cerevisiae. Cell. 2012;148: 99–111. doi: 10.1016/j.cell.2011.12.012 22265405
41. Natsume T, Müller CA, Katou Y, Retkute R, Gierliński M, Araki H et al. Kinetochores coordinate pericentromeric cohesion and early DNA replication by Cdc7-Dbf4 kinase recruitment. Mol Cell. 2013;50: 661–674. doi: 10.1016/j.molcel.2013.05.011 23746350
42. Das SP, Rhind N. How and why multiple MCMs are loaded at origins of DNA replication. Bioessays. 2016;38: 613–617. doi: 10.1002/bies.201600012 27174869
43. Ghaemmaghami S, Huh WK, Bower K, Howson RW, Belle A, Dephoure N et al. Global analysis of protein expression in yeast. Nature. 2003;425: 737–741. doi: 10.1038/nature02046 14562106
44. Donovan S, Harwood J, Drury LS, Diffley JF. Cdc6p-dependent loading of Mcm proteins onto pre-replicative chromatin in budding yeast. Proc Natl Acad Sci U S A. 1997;94: 5611–5616. doi: 10.1073/pnas.94.11.5611 9159120
45. Lei M, Kawasaki Y, Tye BK. Physical interactions among Mcm proteins and effects of Mcm dosage on DNA replication in Saccharomyces cerevisiae. Mol Cell Biol. 1996;16: 5081–5090. doi: 10.1128/mcb.16.9.5081 8756666
46. Ho B, Baryshnikova A, Brown GW. Unification of Protein Abundance Datasets Yields a Quantitative Saccharomyces cerevisiae Proteome. Cell Syst. 2018;6: 192–205.e3. doi: 10.1016/j.cels.2017.12.004 29361465
47. Bowers JL, Randell JC, Chen S, Bell SP. ATP hydrolysis by ORC catalyzes reiterative Mcm2-7 assembly at a defined origin of replication. Mol Cell. 2004;16: 967–978. doi: 10.1016/j.molcel.2004.11.038 15610739
48. Edwards MC, Tutter AV, Cvetic C, Gilbert CH, Prokhorova TA, Walter JC. MCM2-7 complexes bind chromatin in a distributed pattern surrounding the origin recognition complex in Xenopus egg extracts. J Biol Chem. 2002;277: 33049–33057. doi: 10.1074/jbc.M204438200 12087101
49. Woodward AM, Göhler T, Luciani MG, Oehlmann M, Ge X, Gartner A et al. Excess Mcm2-7 license dormant origins of replication that can be used under conditions of replicative stress. J Cell Biol. 2006;173: 673–683. doi: 10.1083/jcb.200602108 16754955
50. Ge XQ, Jackson DA, Blow JJ. Dormant origins licensed by excess Mcm2-7 are required for human cells to survive replicative stress. Genes Dev. 2007;21: 3331–3341. doi: 10.1101/gad.457807 18079179
51. Ibarra A, Schwob E, Méndez J. Excess MCM proteins protect human cells from replicative stress by licensing backup origins of replication. Proc Natl Acad Sci U S A. 2008;105: 8956–8961. doi: 10.1073/pnas.0803978105 18579778
52. Li N, Lam WH, Zhai Y, Cheng J, Cheng E, Zhao Y et al. Structure of the origin recognition complex bound to DNA replication origin. Nature. 2018;559: 217–222. doi: 10.1038/s41586-018-0293-x 29973722
53. Maine GT, Sinha P, Tye BK. Mutants of S. cerevisiae defective in the maintenance of minichromosomes. Genetics. 1984;106: 365–385. 6323245
54. Zou L, Stillman B. Assembly of a complex containing Cdc45p, replication protein A, and Mcm2p at replication origins controlled by S-phase cyclin-dependent kinases and Cdc7p-Dbf4p kinase. Mol Cell Biol. 2000;20: 3086–3096. doi: 10.1128/mcb.20.9.3086-3096.2000 10757793
55. Lynch KL, Alvino GM, Kwan EX, Brewer BJ, Raghuraman MK. The effects of manipulating levels of replication initiation factors on origin firing efficiency in yeast. PLoS Genet. 2019;15: e1008430. doi: 10.1371/journal.pgen.1008430 31584938
56. Dion MF, Kaplan T, Kim M, Buratowski S, Friedman N, Rando OJ. Dynamics of replication-independent histone turnover in budding yeast. Science. 2007;315: 1405–1408. doi: 10.1126/science.1134053 17347438
57. Sonneville R, Querenet M, Craig A, Gartner A, Blow JJ. The dynamics of replication licensing in live Caenorhabditis elegans embryos. J Cell Biol. 2012;196: 233–246. doi: 10.1083/jcb.201110080 22249291
58. Tanaka S, Nakato R, Katou Y, Shirahige K, Araki H. Origin association of Sld3, Sld7, and Cdc45 proteins is a key step for determination of origin-firing timing. Curr Biol. 2011;21: 2055–2063. doi: 10.1016/j.cub.2011.11.038 22169533
59. Müller CA, Nieduszynski CA. Conservation of replication timing reveals global and local regulation of replication origin activity. Genome Res. 2012;22: 1953–1962. doi: 10.1101/gr.139477.112 22767388
60. Nieduszynski CA, Knox Y, Donaldson AD. Genome-wide identification of replication origins in yeast by comparative genomics. Genes Dev. 2006;20: 1874–1879. doi: 10.1101/gad.385306 16847347
61. Green MR (2012) Molecular cloning: a laboratory manual. Fourth edition. Cold Spring Harbor, N.Y.: Cold Spring Harbor Laboratory Press.
62. Chen S, Bell SP. CDK prevents Mcm2-7 helicase loading by inhibiting Cdt1 interaction with Orc6. Genes Dev. 2011;25: 363–372. doi: 10.1101/gad.2011511 21289063
63. Siow CC, Nieduszynska SR, Müller CA, Nieduszynski CA. OriDB, the DNA replication origin database updated and extended. Nucleic Acids Res. 2012;40: D682–6. doi: 10.1093/nar/gkr1091 22121216
64. Batrakou DG, Müller CA, Wilson RHC, Nieduszynski CA. DNA copy-number measurement of genome replication dynamics by high-throughput sequencing: the sort-seq, sync-seq and MFA-seq family. Nat Protoc. 2020;15: 1255–1284. doi: 10.1038/s41596-019-0287-7 32051615
65. Huh WK, Falvo JV, Gerke LC, Carroll AS, Howson RW, Weissman JS et al. Global analysis of protein localization in budding yeast. Nature. 2003;425: 686–691. doi: 10.1038/nature02026 14562095
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