Topoisomerase III Can Serve as the Cellular Decatenase in Escherichia coli*

Pearl Nurse, Cindy Levine, Heide Hassing, and Kenneth J. MariansDagger

From the Molecular Biology Program, Memorial Sloan-Kettering Cancer Center, New York, New York 10021

Received for publication, November 3, 2002, and in revised form, December 30, 2002

    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

topB, encoding topoisomerase III, was identified as a high copy suppressor of the temperature-sensitive parC1215 allele, encoding one of the subunits of topoisomerase IV. Overexpression of topoisomerase III at the nonpermissive temperature was shown subsequently to restore timely chromosome decatenation and suppress lethality in strains carrying either temperature-sensitive parE or parC alleles. By developing an assay in vitro for precatenane unlinking, we demonstrated directly that both topoisomerase III and topoisomerase IV were efficient at this task, whereas DNA gyrase was very inefficient at precatenane removal. These observations suggest that precatenane unlinking is sufficient to sustain decatenation of replicating daughter chromosomes in the cell.

    INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Escherichia coli has four DNA topoisomerases, two type IIA DNA gyrase and topoisomerase (Topo)1 IV, and two type IA Topo I and Topo III. The roles in the cell played by three of these proteins is reasonably well defined (1-4). DNA gyrase is the major facilitator of DNA replication, acting to convert the positive supercoils generated directly to negative ones. Mutations in either gyrA or gyrB, encoding the subunits of gyrase, are conditionally lethal, and incubation of such mutated strains at the non-permissive temperature causes a rapid cessation of DNA replication. Topo IV is the cellular decatenase, responsible for unlinking the daughter chromosomes so that chromosome segregation is accomplished in a timely manner. Mutations in either parE or parC, encoding the subunits of Topo IV, are also conditionally lethal. Incubation of either parE or parC temperature-sensitive strains at the non-permissive temperature results in the elaboration of a par phenotype, where a large DNA mass accumulates in the center of an elongated cell. This DNA mass results from repeated initiations of replication on chromosomes that have not segregated. Topo IV appears also to be able to support replication fork progression at about one-half the rate supported by gyrase (5). Topo I acts as a balancing force to gyrase, such that the net negative superhelicity of the chromosome is maintained within an optimal range. Inactivation of Topo I is tolerated only in the presence of compensatory mutations in gyrase that act to reduce its activity. In the case of Topo III, there is more known about its biochemical activities than its role in the cell.

Topo III was detected originally as a superhelical DNA relaxing activity present in extracts prepared from cells deficient in Topo I (6) and as an activity that bound to novobiocin affinity columns (7). We purified Topo III as an activity capable of decatenating replicating daughter chromosomes (8) after we determined that gyrase was inefficient at this task (9). Whereas Topo III was inefficient at superhelical DNA relaxation, requiring high temperature for optimal activity, it was very efficient at decatenating multiply linked daughter chromosomes as long as one of the DNA circles contained a small gap. These observations suggested that the productive binding site for the enzyme was single-stranded DNA (10), which has been borne out by all subsequent studies.

Cloning of the gene for Topo III (topB (10)) indicated that the protein had considerable identity to Topo I, although it lacked the zinc finger region of the latter enzyme. Rothstein and colleagues (11) reported contemporaneously that EDR1, a gene in yeast that, when mutated, caused enhanced deletion of SUP4-o when it was flanked by delta  sequences (the long terminal repeats of the Ty retrotransposon) (12), encoded a protein that had significant similarity to E. coli Topo I and therefore renamed the gene TOP3. TOP3 was actually more homologous to E. coli Topo III than to E. coli Topo I and proved to be the first eukaryotic member of the Topo III family identified.

Disruption of topB was noted originally not to cause any obvious phenotype (10). Subsequently, Schofield et al. (13) showed that mutR, a gene that, when mutated, caused a 5-fold increase in RecA-independent recombination between short directly repeated sequences, was allelic with topB. To date, this observation describes the only known phenotype of topB deficiencies over an otherwise wild-type background. Interestingly, the situation in eukaryotes is very different, where the phenotypes of deficiencies in Top3 clearly indicate that the enzyme plays a significant role in the maintenance of genomic integrity. Deletion of TOP3 in Saccharomyces cerevisiae causes a slow growth phenotype, the hyper-recombination phenotype mentioned above (11), and sensitivity to several DNA-damaging agents as a result of disruption of the intra-S phase checkpoint (14). In Schizosaccharomyces pombe, TOP3 is an essential gene. Cells deleted for TOP3 undergo only a few rounds of abnormal nuclear division before death (15, 16). In this organism, dysregulation of Top3 function has been linked to low Cdc2-cyclin B activity, causing a defect in the late stages of homologous recombination (17). In vertebrates, there are two Top3 isozymes, alpha  (18) and beta  (19). Deletion of the former causes embryonic lethality in mice (20). Many of these effects are thought to be manifested via interaction, or the lack thereof, of Top3 with members of the RecQ-like family of DNA helicases (21).

Here we show that E. coli Topo III can act as the principal cellular decatenase, capable of unlinking replicating daughter chromosomes in vivo, and provide evidence that this decatenation proceeds via the removal of precatenanes.

    EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Enzymes, Reagents, Proteins, and Antibodies-- Restriction enzymes and bacteriophage T4 DNA ligase were from New England Biolabs. Pfu polymerase was from Stratagene. Hybond ECL nitrocellulose membrane and ECL-Western blotting detection reagents were from Amersham Biosciences. DNA polymerase I, RNase H, and E. coli DNA ligase were from Roche Molecular Biochemicals. Topo III was prepared from a topA- strain as described (22). ParE and ParC were purified as described by Peng and Marians (23). DNA gyrase was prepared as described (9). Polyclonal antisera against Topo III was raised in rabbits. Goat anti-rabbit IgG conjugated to horseradish peroxidase was from Bio-Rad.

Standard Microbiological Techniques-- W3110parE10 and C600parC1215, described previously by Kato and colleagues (24, 25), were obtained from the laboratory of N. Cozzarelli (University of California, Berkeley). W3110 was from the E. coli Genetic Stock Center. DH5-alpha , which was used to prepare all plasmid DNAs, was from Invitrogen. Cultures were grown in Luria broth or on Luria agar plates. Antibiotics, when added, were at the following concentrations: 100 µg/ml ampicillin and 50 µg/ml kanamycin. Competent cells were prepared by CaCl2 treatment.

Fluorescence Microscopy-- Cells were grown in LB with appropriate antibiotics to an A600 of 0.5. Equal volumes of cell culture and a solution of 4% paraformaldehyde and 1 µg/ml 4,6-diamidino-2-phenylindole in 1× phosphate-buffered saline were mixed, and the cells were fixed for 30 min at 4 °C on a rotator. Aliquots (40 µl) of the fixed cells were spread on polylysine-coated glass slides and allowed to air-dry. Samples were observed with an Olympus AX-70 microscope. Fluorescence and differential interference contrast images were acquired with an Hamamatsu Orca-ER CCD camera using MetaMorph software (Universal Imaging). Figures were prepared for publication using Adobe Photoshop 7.0 software.

Plasmid Constructions-- The construction of the pBR-kan-inc3 suppressor library has been described (26). pBR-suppressor-6 is a plasmid from the pBR-kan-inc3 suppressor library carrying the genomic insert described under "Results." pBR-suppressor-6(Delta topB) was constructed by digesting pBR-suppressor-6 with HpaI, which cuts the plasmid once in topB about 800 bp downstream of the start codon, and with ScaI, which cuts the plasmid once about 900 bp upstream of the start codon of topB, within the gene encoding beta -lactamase, gel purifying the larger of the two DNA fragments produced, and religating it. pBADtopB was constructed by inserting an NaeI-SmaI DNA fragment from pTBE302 (the gift of R. DiGate, University of Maryland) that contained araC as well as the topB ORF under the control of the ara promoter into the EcoRV site of pBR-kan-inc3. pLEXparE has been described previously (27).

Construction of W3110Delta parE(pLEXparE)-- The technique of Link et al. (28) was used. A DNA fragment was constructed by overlap PCR such that 33 random, coding bp were inserted in-frame between the ATG and TAA codons of parE flanked by about 700 bp of upstream and downstream genomic sequence. The extreme outside primers also contained a BamHI site. The DNA was digested with BamHI and introduced into the BamHI site of pKO3, which carries cat and sacB, and is replicated via a temperature-sensitive pSC101 origin, to give pKO3parEk/o. This plasmid was transformed into W3110, and the transformants were plated at 42 °C. A chloramphenicol-resistant colony was used to grow cells for transformation with pLEXparE (27) at 42 °C. A single chloramphenicol-resistant, ampicillin-resistant (because of pLEXparE) colony was diluted in media and plated at 30 °C on plates containing 80 µM IPTG, 5% sucrose, and ampicillin. These colonies were then replica-plated in the presence and absence of IPTG and also checked for chloramphenicol sensitivity. A chloramphenicol sensitive-, IPTG-dependent colony was then checked by PCR for the presence of the genomic parE deletion that has the sequence Met-His-Ala-Ile-Thr-Leu-Thr-Leu-Gln-Ile-Tyr-Asn replacing the parE ORF.

Purification of ParEC316Y Topo IV and Assays for Activity-- The sequence of the parE gene in W3110parE10 was determined by sequencing a PCR fragment made from the genomic DNA. The only amino acid substitution present was C316Y. The overexpression plasmid pET21a-parE10 was constructed by introducing a PCR fragment made from W3110parE10 genomic DNA carrying the parE ORF flanked by NdeI and BamHI sites. ParEC316Y expressed from this plasmid was insoluble. Therefore, we transferred the expression cassette from pET3C-parC (23) to pBR-kan-inc3, which is compatible with pET21a, to give pBR-kan-inc3-(pET)parC, and we co-overexpressed the mutant ParE with wild-type ParC. This proved effective and yielded soluble Topo IV. ParEC316Y Topo IV was then purified from BL21(DE3)(pET21a-parE10, pBR-kan-inc3-(pET)parC) after soluble lysis by sequential chromatography on Q-Sepharose, phosphocellulose, and Superose 6. In the presence of excess ParC, the specific activities of ParEC316Y and wild-type Topo IV were essentially identical in the superhelical DNA relaxation assay. Titrations were used to determine the amount of Topo IV required to effect either 80% superhelical DNA relaxation or decatenation. Mutant and wild-type Topo IV was then heated (in 5-µl aliquots) at 20-fold this concentration at 50 °C for the times indicated in Fig. 3 and then chilled on ice. Superhelical DNA relaxation assays (27) and kinetoplast DNA decatenation (29) assays were then as described previously with 1 µl of the heat-treated Topo IV being added to 20-µl reaction mixtures. The extent of the reactions was quantitated using Bio-Rad Quantity One software from digital images of the ethidium bromide-stained gels.

Precatenane Unlinking Assay-- Precatenated DNA was prepared in oriC replication reactions increased in volume 40-fold (30) using chi -1 plasmid DNA (31) as a template. This pBR322-based plasmid carries oriC and two Ter sites oriented to block replication forks coming from oriC, one 2 kb downstream from oriC in the counterclockwise direction and the other 3 kb downstream from oriC in the clockwise direction. Thus, when Tus is included in the replication reaction mixture, replication is terminated at the Ter sites, leaving 1 kb of unreplicated DNA. A significant fraction of the excess positive linkages generated during replication persist as precatenanes in this replication product (32). The precatenated DNA was treated with SDS and proteinase K, isolated by gel filtration through Bio-Gel A-5M, and concentrated by lyophilization before use. Standard precatenane unlinking reaction mixtures (5 µl) containing 50 mM HEPES-KOH (pH 8.0), 10 mM MgOAC, 10 mM dithiothreitol, 2 mM ATP, 100 µg/ml bovine serum albumin, 2.8 nM precatenated DNA, and the indicated concentrations of the different topoisomerases were incubated at 37 °C for 5 min. Reactions were terminated by the addition of EDTA to 20 mM, and the DNA products were analyzed by electrophoresis at 1.5 V/cm for 15 h through vertical 1% agarose gels using 50 mM Tris-HCl (pH 7.8 at 23 °C), 40 mM NaOAC, and 1 mM EDTA as the buffer. The gels were dried, exposed to a PhosphorImager screen, and autoradiographed.

    RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Identification of topB as a High Copy Suppressor of parC1215-- We previously conducted a screen for high copy suppressors of the conditional lethality of W3110parE10 (26), which revealed an interaction between Topo IV and the tau  and gamma  subunits of the DNA polymerase III holoenzyme. Further investigation of this observation led to the discovery that the Topo IV activity was temporally regulated during the cell cycle (33). Here we conducted a screen for high copy suppressors of the conditional lethality of C600parC1215 (24). A plasmid library (26) was generated by inserting size-selected E. coli genomic DNA into a pBR322 vector (pBR322-kan-inc3) that carried a mutation giving it a slightly higher copy number than normal. All E. coli genes present in this library were expressed from their natural promoters. Library DNA was transformed into C600parC1215, and about 80,000 transformants were plated at 42 °C. Of the 13 colonies that grew, 6 regrew at both the permissive and nonpermissive temperatures. Plasmid DNA was isolated from these six clones and retransformed into C600parC1215. Plasmid DNA from all six potential suppressor clones conferred to C600parC1215 the ability to grow at 42 °C (Table I). This screen yielded four different genes that functioned as high copy suppressors of the temperature sensitivity of parC1215: parC (two clones), as expected; topB (two clones), as discussed in this report; dnaN (one clone), encoding the beta  subunit of the DNA polymerase III holoenzyme; and spcA (suppressor of parC A) (one clone), an integral membrane protein that links chromosome segregation to cellular architecture. The interaction of the proteins encoded by these latter two genes with Topo IV will be the subject of a separate report.

                              
View this table:
[in this window]
[in a new window]
 
Table I
Rescue of Topo IV temperature-sensitive strains by overexpression of Topo III
Overnight cultures grown at the permissive temperature were diluted to an A600 of 0.02 and grown in LB broth at the permissive and nonpermissive temperatures to an A600 of 0.5-1.0, diluted by 105, plated (50-100 µl), and grown overnight on LB agar plates. All solid and liquid media contained antibiotics and arabinose (30 mM), as required.

The ends of the genomic DNA insert in pBR-suppressor-6 were determined using primers flanking the BamHI insertion site in the vector. These sequence data were then used to position the genomic insert on the sequence of the E. coli chromosome (34). The genomic insert was found to be 5,769 bp long, spanning nucleotides 1,842,971-1,848,740 of the E. coli chromosome. This chromosomal region included the genes topB, selD, ydjA, and sppA. Given that topB was, of this group of genes, the most likely candidate for the suppressor, we digested pBR-suppressor-6 with both ScaI and HpaI and religated to form pBR-suppressor-6 (Delta topB). HpaI cuts the suppressor clone once within topB about 800 bp downstream from the start of the gene and ScaI cuts once about 900 bp upstream of the 5'-end of the genomic insert, within the previously disrupted gene encoding beta -lactamase. pBR-suppressor-6(Delta topB) failed to rescue the temperature-sensitive phenotype of C600parC1215 (Table I), supporting the argument that topB was the suppressor gene. To confirm that this was the case, the topB ORF was introduced to the suppressor vector under the control of an arabinose-inducible promoter, giving plasmid pBADtopB. Interestingly, in the presence of 30 mM arabinose, this plasmid effected a better rescue of the parC1215 allele at 42 °C than the original suppressor clone (Table I). This observation suggested that the efficiency of rescue by Topo III was dose-dependent, an issue that is explored below.

If rescue by Topo III was a result of substitution of its topoisomerase activity for that of Topo IV, it seemed reasonable to expect that the various suppressor plasmids would also rescue the temperature sensitivity of W3110parE10. This was the case (Table I). For reasons that are unclear, rescue was more complete for each plasmid in the parE mutant strain compared with the parC mutant strain.

Characterization of the Rescue of W3110parE10 by Overexpression of Topo III-- Stationary overnight cultures grown at 42 °C of W3110(pBADtopB) and W3110parE10(pBADtopB) were diluted to an A600 of 0.02 in fresh media, and the growth of the cultures were followed at 42 °C (Fig. 1A). The wild-type culture commenced growth immediately; on the other hand, the mutant culture exhibited a pronounced lag but then grew at a rate that was roughly the same as the wild-type culture. It should be noted that under the conditions described, W3110parE10 itself will not grow at all, all cells having reached a terminal phenotype during the original overnight incubation at the non-permissive temperature. Furthermore, examination of the cell and nucleoid morphology under conditions of topB rescue demonstrated that Topo III was acting to decatenate the daughter chromosomes (Fig. 1, B and C).


View larger version (67K):
[in this window]
[in a new window]
 
Fig. 1.   Characterization of rescue of W3110parE10 by overexpression of topB. A, growth curves of W3110(pBADtopB) and W3110parE10(pBADtopB) at 42 °C. Overnight cultures grown in rich medium were diluted to an A600 of 0.02, and their growth in rich medium was followed at 42 °C. B, cell and nucleoid morphologies of W3110(pBADtopB), W3110parE10(pBADtopB), and W3110parE10(pBR-kan-inc3) growing at 30 and 42 °C. Samples were taken from cultures of the former two strains at an A600 of 0.7. The latter strain was grown as an overnight culture at 30 °C; fresh media were inoculated to an A600 of 0.02, and the culture was then grown for 2 h at 42 °C. Preparation of cells and fluorescence microscopy were as described under "Experimental Procedures." C, comparison of the types of cells present in the three different cultures at 42 °C. Roughly 300-400 cells from each culture were examined at random and assigned, based on cell and nucleoid morphology, to the six cell types illustrated in the figure. Type 1 cells were wild type in appearance. Type 2 cells were small but contained condensed nucleoids. Type 3 cells were anucleates. Type 4 cells were normal-sized but had nucleoids that appeared connected by DNA. Type 5 cells were filaments with non-condensed nucleoids, whereas type 6 cells were filaments with condensed nucleoids.

Wild-type and mutant parE10 cells grown at 30 °C in the presence of pBADtopB and arabinose gave essentially indistinguishable morphologies with about 95% of the population appearing as small cells with either two or four nucleoids. The other 5% of the population was made up of an assortment of abnormally appearing cells (Fig. 1, B and C). When these two strains were grown at the non-permissive temperature as described above, the fraction of wild-type appearing cells in the W3110(pBADtopB) culture decreased to 83%, and there was a significant fraction of small cells with condensed, non-separated nucleoids (type 2, Fig. 1C). In addition, filaments could be observed that contained nucleoids that either were condensed (type 6, Fig. 1C) or appeared normal (type 5, Fig. 1C); anucleates were observed as well (type 3, Fig. 1C). Interestingly, the largest population of abnormally appearing cells were small cells clearly containing two nucleoids that were linked together by DNA (type 4, Fig. 1C), suggesting that either chromosome decatenation or segregation was delayed at 42 °C compared with 30 °C. On the other hand, whereas the culture of W3110parE10(pBADtopB) grown at the non-permissive temperature contained a significant fraction of wild-type appearing cells (43%, Fig. 1C), the proportion of type 2 and type 3 cells was elevated, suggesting that the rescue by overexpression of Topo III was not completely penetrant. However, when compared with the cellular morphologies present in a culture of W3110parE10 grown at the non-permissive temperature, it was clear that overexpression of Topo III resulted in rescue of the Topo IV defect and effected decatenation of the daughter chromosomes. W3110par10(pBR-kan-inc3) cells grown overnight at 30 °C, diluted by 100-fold, and then shifted to 42 °C for 2 h exhibited a classic par phenotype (Fig. 1B). Half the cells in the population were long filaments with either a central very large, dense nucleoid or two symmetrically placed, somewhat smaller dense nucleoids. The other half of the population consisted of anucleate cells (Fig. 1C). No wild-type cells were observed at all.

pBR-suppressor-6 and pBADtopB exhibited different efficiencies of rescue of C600parC1215, suggesting that there was a certain minimal level of Topo III needed to effect chromosome decatenation. We therefore examined the levels of Topo III produced from these plasmids in W3110parE10 growing at 42 °C (Fig. 2). We used the parE10 strain, rather than C600parC1215, because in the former strain both plasmids rescued to the same extent, suggesting that we would obtain an unbiased value for the extent of overproduction. The pBRsuppressor-6 plasmid produced about 60-fold more Topo III at 42 °C than was present in W3110parE10 at 30 °C, whereas the pBADtopB overproduced Topo III by about 180-fold. The level of Topo III in wild-type cells is very low, having been estimated at about 10 copies per cell. Our current estimate for Topo IV is about 1000 copies per cell (33); thus, Topo III works effectively as the cellular decatenase when it is present at roughly the same concentration as Topo IV.


View larger version (12K):
[in this window]
[in a new window]
 
Fig. 2.   Levels of expression of Topo III from the different suppressor plasmids in W3110parE10 and W3110Delta parE(pLEX-parE). Cultures of W3110parE10 growing at 30 °C, W3110parE10(pBR-suppressor-6) growing at 42 °C, W3110parE10(pBADtopB) growing at 42 °C in the presence of 15 mM arabinose, W3110Delta parE(pLEX-parE) growing at 37 °C in the presence of IPTG, W3110Delta parE(pLEX-parE, pBR-suppressor-6) growing at 37 °C in the presence of IPTG, and W3110Delta parE(pLEX-parE, pBADtopB) growing at 37 °C in the presence of IPTG and 15 mM arabinose were sampled at an A600 of 1.0. The cells were pelleted, resuspended in loading dye for SDS-PAGE, and heated at 100 °C, and the resulting extract was electrophoresed through a 10% SDS-PAGE. The gel was then Western-blotted using polyclonal antibody to Topo III. Each lane contains the equivalent of 37.5 µl of culture.

Topo III Is Substituting for the Decatenation Activity of Topo IV-- If the observed rescue by Topo III was a result of it substituting completely for the activity of Topo IV, then overexpression of Topo III should also rescue E. coli in the complete absence of Topo IV. To assess this issue, we constructed a conditional parE null strain. W3110Delta parE(pLEXparE) carries a precise deletion of the chromosomal parE covered by an expression plasmid (pLEX5BA (35)) where the parE ORF is under the tightly regulated control of a modified lac operator. Consequently, growth of this strain at any temperature is dependent on the presence of IPTG to induce ParE expression. pBADtopB could not rescue growth of this strain at 37 °C in the presence of arabinose when IPTG was omitted from the culture medium. In the presence and absence of arabinose to induce Topo III expression, the plating efficiency of W3110Delta parE(pLEXparE, pBADtopB) was 0.96 (with arabinose/without arabinose) when IPTG was also present. In the absence of IPTG, no growth was observed at all in either the presence or absence of arabinose. We considered three explanations for the lack of rescue of the parE deletion strain. The first relates to the possibility that the observed rescue by overexpression of Topo III in the temperature-sensitive parE and parC strains was dependent on a partial level of Topo IV decatenation activity, and therefore, because the ParE deletion strain had no Topo IV, higher levels of Topo III were required to effect rescue.

To address this possibility, we constructed a modified topB expression vector that could produce higher levels of Topo III than pBADtopB; however, we found that even modest increases in the levels of Topo III expression over those produced by pBADtopB were toxic to wild-type cells. Thus, we probed the nature of the Topo IV activity present in W3110parE10 by purifying the mutant protein (the amino acid substitution is C316Y) and assaying its activity in vitro (Fig. 3). Both the superhelical DNA relaxation and the decatenation activity of ParEC316Y Topo IV was exquisitely temperature-sensitive compared with the wild-type protein, which showed only minimal heat inactivation even after 20 min at 50 °C. It thus seems unlikely that there is any residual available topoisomerase activity of Topo IV under the conditions of Topo III rescue of the temperature-sensitive strains described above. We also note that W3110parE10 was completely rescued by the pBR-suppressor-6 plasmid. pBADtopB produced 3-fold more Topo III than pBR-suppressor-6, a relationship that was maintained in W3110Delta parE(pLEXparE) (Fig. 2), yet still could not rescue the null strain. We therefore conclude that overexpression of Topo III to levels roughly comparable with those of Topo IV in wild-type cells allow it to substitute completely for the chromosome decatenation activity of the latter enzyme.


View larger version (20K):
[in this window]
[in a new window]
 
Fig. 3.   ParEC316Y Topo IV is temperature-sensitive. ParEC316Y Topo IV was overexpressed and purified as described under "Experimental Procedures." The temperature sensitivity of the ParEC316Y and wild-type Topo IV was compared. The enzymes were first heated at 50 °C for the time indicated and then chilled on ice. The activity of the heat-treated enzyme was then assessed in standard assays for either superhelical DNA relaxation (A) or decatenation of kinetoplast DNA (B) as described under "Experimental Procedures."

The second possibility is that W3110Delta parE(pLEXparE) cannot be rescued in the absence of IPTG because the presence of ParC in the cell unfettered by association with ParE is toxic. This possibility is difficult to discount; however, we note that overexpression of Topo III did, in fact, rescue the temperature-sensitive parE strain, where, presumably, because the ParEC316Y mutation is likely to cause folding defects, at the nonpermissive temperature the same situation holds, i.e. there is a surfeit of free ParC in the cell. On the other hand, our experience with various parC expression constructs is consistent with high level, overexpression of ParC being toxic to wild-type cells.

A third possibility is that the failure of Topo III overexpression to rescue the parE deletion strain reflects a physical requirement for ParE at some stage of the cell cycle and that this requirement is distinct from the requirement for ParE to form Topo IV that is active for decatenation.

Topo III Is Very Efficient at Removing Precatenanes-- Under most circumstances, Topo III will be a very poor superhelical DNA relaxing enzyme. This is because of its strong dependence on single-stranded DNA for activity and an apparently poor ability to bind and partially denature double-stranded DNA to create its substrate. Thus, maximal relaxation activity in vitro requires elevated temperature to increase the single-stranded character of negatively supercoiled substrates (8). Consequently, the enzyme is essentially inactive in removing positive supercoils (36). How then can Topo III operate on the topology of replicating chromosomes if during DNA replication the only possible position for Topo III action is behind the replication fork (where nicks and gaps presumably exist because of the process of sealing Okazaki fragments)? The most likely answer to this question is that Topo III works by removing precatenanes, an alternative form that can be taken by the positive linkages that arise between the daughter chromosomes during replication.

As noted originally by Champoux and Been (37), the positive linkages between replicating daughter chromosomes that arise as a result of unwinding of the parental duplex can distribute either ahead of the replication fork as positive supercoils or behind the replication fork as precatenanes, torus-like topological linkages that, if replication were completed, would become catenanes. This equilibrium is governed by the extent of DNA that is replicated: with positive supercoils predominating when the majority of the template is unreplicated and precatenanes predominating when the majority of the template is replicated (38). The differential action of Topo IV and DNA gyrase in the cell can be explained, at least in part, by their preference for positive supercoils or catenanes as substrates (36, 39). We demonstrated previously that Topo III can support both nascent strand progression (40) and daughter chromosome decatenation (22) in vitro. In addition, we have argued, based on indirect evidence, that Topo III probably functions by removing precatenanes (36). Given the observations reported here, we developed an assay to explore this issue directly.

A replication system reconstituted with purified proteins was used to replicate a plasmid DNA template carrying oriC (30). The template DNA, which was 6 kb long, also carried replication terminator Ter sites 2 kb clockwise and 3 kb counterclockwise from the origin. Both Ter sites were oriented to stop replication fork progression. Thus, when the replication reaction is performed in the presence of Tus, the forks formed at oriC will be terminated and complete replication of the plasmid prevented. We showed previously, using neutral agarose gel electrophoresis and electron microscopy, that the partially replicated daughter duplexes in these molecules are intertwined in precatenanes. The precatenanes take the form of a ladder of bands during neutral agarose gel electrophoresis, the mobility and spacing of which almost precisely matches that of complete catenanes (32). The steps in the ladder differ by one precatenane. Such a ladder can be observed in the partially replicated DNA that we prepared (Fig. 4A, lane 1). Removal of the precatenanes will yield a classic theta -type late replication intermediate (LRI) where the two partially replicated daughters are held together by the region of unreplicated parental DNA. This species has a very low mobility during agarose gel electrophoresis (9).


View larger version (39K):
[in this window]
[in a new window]
 
Fig. 4.   Topo III and Topo IV, but not gyrase, can remove precatenanes. A, standard precatenane unlinking reaction mixtures containing the indicated concentrations of either DNA gyrase (Gyr) (lanes 2-4), Topo III (lanes 5-7), Topo IV (lanes 8-10), or no topoisomerase (lane 1) were incubated and analyzed as described under "Experimental Procedures." B and C, comparison of the precatenane-removing activities of Topo III and Topo IV. B, standard precatenane unlinking reaction mixtures containing the indicated concentrations of either Topo III (lanes 2-7), Topo IV (lanes 8-13), or no topoisomerase (lane 1) were incubated and analyzed as described under "Experimental Procedures." C, the extent of precatenane unlinking in the reactions displayed on the gel in B was quantitated by using a PhosphorImager to determine the amount of radioactivity present on the gel as LRI. LRI, late replication intermediate; precats, precatenanes; PSL, photo-stimulated luminescence.

The precatenated DNA substrate was treated with either DNA gyrase, Topo III, or Topo IV (Fig. 4A). Both Topo III and Topo IV could clearly remove the precatenanes, as evinced by the disappearance of the DNA ladder and the accumulation of LRI DNA. On the other hand, gyrase was very inefficient at precatenane removal, even at concentrations 25-fold greater than those at which Topo III and Topo IV were effective. These data are consistent with previous observations that address the substrate specificity of Topo IV and gyrase (36, 39).

Topo III and Topo IV were powerful precatenane-removing enzymes, with activity detectable at sub-nanomolar concentrations (Fig. 4, B and C). The specific activities of the two enzymes in this reaction were comparable (Fig. 4C). The DNA replication reaction used to prepare the precatenated substrate lacked DNA ligase; thus there are nicks present between the Okazaki fragments that could represent the sites of Topo III action. To assess if this was the case, the precatenated substrate was treated with a combination of DNA polymerase I, DNA ligase, and RNase H to remove the RNA primers and seal the Okazaki fragments, resulting in the conversion of all the nascent DNA to a long linear strand equal in length to the distance between the two Ter sites (Fig. 5A). Interestingly, this treatment had no effect on the ability of Topo III to remove the precatenanes (Fig. 5B). However, this process does not eliminate all the single-stranded gaps on the lagging strand. We showed previously that when a replication fork collides with the Tus-Ter complex, the site of leading-strand arrest is within a nucleotide or two of the edge of Ter site, whereas the site of the last primer on the lagging strand is about 60 nucleotides upstream, leaving a gap at the fork in the partially replicated molecule (41). This arrangement represents a snapshot of the disposition of the nascent strands at the growing point of a replication fork. This gap cannot be sealed by the treatment described above and thus represents a probable position for the site of Topo III action.


View larger version (49K):
[in this window]
[in a new window]
 
Fig. 5.   The precatenane unlinking activity of Topo III does not require gaps between Okazaki fragments in the nascent daughter chromosomes. A, treatment of the precatenated DNA with RNase H, DNA ligase, and DNA polymerase I (RLP) seals all the Okazaki fragments. The denaturing alkaline-agarose gel shows the nascent DNA present in the precatenated DNA before (lane 1) and after (lane 2) treatment with RLP. Because the plasmid replicates bidirectionally, when sealed, all the Okazaki fragments synthesized by the clockwise-moving fork will be joined to the leading strand synthesized by the counterclockwise-moving fork and vice versa, resulting in a continuous linear nascent DNA product that spans the distance between the two Ter sites (5 kb). B, treatment of the precatenated DNA with RLP does not inhibit precatenane removal by Topo III. Precatenane unlinking by 3.2 nM Topo III was compared using precatenated substrate that either had (lanes 3 and 4) or had not (lanes 1 and 2) been treated with RLP.

These studies demonstrate directly that Topo III can remove precatenanes. It is thus likely that the ability demonstrated here of Topo III to substitute for the decatenation activity of Topo IV in vivo is a manifestation of this capacity.

    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Although the biochemical properties of Topo III are well established, the manner in which these activities are expressed in the cell are far from clear. The purified protein is capable of relaxing supercoiled DNA and decatenating linked DNA circles (8). Its activity is strongly dependent on single-stranded DNA to provide a productive binding site on the substrate. Thus, negatively supercoiled DNA serves as a substrate because of its underwound character, but positively supercoiled DNA, with its overwound character, is not a substrate. Similarly, Topo III-catalyzed decatenation requires that the DNA rings contain discontinuities in the strands and is stimulated when actual gaps are provided (8). We have shown that Topo III can support both nascent strand progression (40) and daughter chromosome decatenation (22) in oriC replication systems in vitro. However, deletion of topB is of little consequence to the cell (8).

Here we report a genetic system where survival of E. coli is dependent on overexpression of Topo III. Increasing the level of Topo III in the cell by about 70-fold was sufficient to allow cells with temperature-sensitive mutations in either parC or parE, the genes encoding the subunits of Topo IV, to grow at the nonpermissive temperature. Although, as indicated by the cellular and nucleoid morphologies, rescue was not complete, it was clear that Topo III was decatenating the replicating daughter chromosomes, allowing them to be partitioned and thus permitting successful cytokinesis.

There are two possible modes of strand unlinking during theta -type DNA replication (36): removal of positive supercoils ahead of the replication fork and removal of positive precatenanes behind the fork. Execution of the latter mode is ultimately required for complete removal of all topological linkages between daughter chromosomes. The biochemical properties of Topo III suggested that it likely acts behind the fork, removing precatenanes. In support of this, we demonstrated that the rate of Topo III-supported fork progression from early replication intermediates where replication forks had stalled because of accumulation of positive supercoils actually increased as the extent of the template replicated increased. In contrast, the rate of gyrase-supported fork progression decreased as the extent of the template replicated increased. We interpreted these observations to mean that at the beginning of the reaction, when only about 20% of the DNA was replicated, most of the positive windings existed as positive supercoils, substrates for DNA gyrase, not Topo III. As replication proceeded, precatenanes, substrates for Topo III and not gyrase, accumulated.

Where is Topo III acting in vivo? In support of the previous observations, we have demonstrated directly in this report that Topo III and Topo IV, but not gyrase, can efficiently remove precatenanes. We therefore think it likely that the observed ability of Topo III to support daughter chromosome decatenation arises as a result of it working behind the fork to unlink precatenanes. However, the actual sites on the chromosome that can be occupied successfully by Topo III to accomplish this task is limited because of its requirement for single-stranded DNA. Topo III could be acting in one of two general locations: at gaps produced on the lagging strand during the process of sealing of Okazaki fragments or at the replication fork itself, in the gap on the lagging strand between the 3'-end of the nascent leading strand and the 5'-end of the last primer for Okazaki fragment synthesis. We favor the latter as the likely preferred location of Topo III because chromosome segregation requires that the topological linkage between the daughters be reduced to zero. Thus, in order for Topo III to support daughter chromosome unlinking, it must be able to act after the last parental duplex turn is unwound and before all gaps in the daughters are sealed. The gap on the lagging strand at the forks will persist after complete unwinding of the parental duplex until the leading strand from the clockwise-moving fork meets up with the 5'-end of the last Okazaki fragment from the counterclockwise-moving fork, for example (Fig. 6). The gaps between Okazaki fragments may be too transient to provide a site at which Topo III can complete its task. This competition between sealing of gaps in the daughter chromosomes and productive Topo III binding provides a possible explanation for the incomplete penetrance of the rescue by Topo III, because once all the gaps are sealed, Topo III will not be able to work.


View larger version (12K):
[in this window]
[in a new window]
 
Fig. 6.   Lagging strand gaps can persist at the replication fork after complete unwinding of the parental template at the termination of replication. (i) Two replication forks approaching each other at the termination of replication. Gaps exist between the 3'-end of the leading strand and the 5'-end of the last Okazaki fragment on the lagging strand at each replication fork. (ii) The gaps on the lagging strand persist as the parental template becomes completely unwound. (iii) The gaps are sealed only after complete unwinding of the parental template, when the leading strand from one direction extends to the 5'-end of the last Okazaki fragment from the opposite fork. (iv) Completely replicated sisters. Arrowheads correspond to 3'-ends.

Topo III could not, when expression of the ParE was shut down, rescue growth of a strain that had been deleted for parE and was dependent on expression of ParE from an IPTG-inducible promoter. We do not think that this observation reflects the fact that some residual Topo IV activity was required for the rescue of the temperature-sensitive parE and parC strains by Topo III. At least in the case of the parE strain, we could demonstrate that the endogenous Topo IV was clearly temperature-sensitive for both its superhelical DNA relaxation and decatenation activities, and the expression of a 3-fold greater level of Topo III than was sufficient to rescue the temperature-sensitive parE strain was still insufficient to rescue the Delta parE strain in the absence of IPTG. The simplest explanation for the lack of rescue of the null is that free ParC is toxic to the cell. ParC must be complexed with ParE for its DNA cleavage and religation activity to be manifested; however, ParC alone is a DNA-binding protein, and its indiscriminate binding to the chromosome could interfere with processes such as replication and transcription. Although this is the most likely possibility, it is interesting to note that both the Delta parE strain in the absence of IPTG and the temperature-sensitive parE strain at the nonpermissive temperature presumably both have free ParC, yet Topo III overexpression rescued the latter and not the former. This observation suggests another, admittedly speculative, possibility that ParE, and possibly Topo IV, has two distinct roles in the cell, only one of which (decatenating the daughter chromosomes) depends on the formation of catalytically active Topo IV. What this second task could be is obscure. Additional studies are required to resolve this issue.

In eukaryotic cells, Topo III and the RecQ-like DNA helicases appear to cooperate to preserve genomic integrity, perhaps by processing some types of recombination intermediates that can form at stalled replication forks (21). Little evidence of such cooperation exists in E. coli, although our observation that Topo III can remove precatenanes in vivo supports its potential involvement in such reactions. Harmon et al. (42) have reported that the combination of E. coli RecQ and Topo III can catenate covalently closed, superhelical DNAs in vitro. These authors proposed that a functional interaction between these two proteins allowed Topo III to execute the required two sequential strand passage events by exploiting the ability of RecQ to unwind the superhelical DNA. The existence of such a mechanism in E. coli would obviate the issue discussed above with respect to the requirement for a single-stranded gap for Topo III action in decatenating the replicating daughter chromosomes. Accordingly, we asked whether disruption of recQ affected the ability of Topo III to rescue the parE temperature-sensitive strain. Interestingly, it did not (data not shown). Of course, this experiment may not be an accurate test of the hypothesis given the requirement for overproduction of Topo III to effect rescue of the parE strain.

    FOOTNOTES

* This work was supported by National Institutes of Health Grant GM34558.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Dagger To whom correspondence should be addressed: Molecular Biology Program, Memorial Sloan-Kettering Cancer Center, 1275 York Ave., New York, NY 10021. Tel.: 212-639-5890; Fax: 212-717-3627; E-mail: k-marians@ski.mskcc.org.

Published, JBC Papers in Press, December 31, 2002, DOI 10.1074/jbc.M211211200

    ABBREVIATIONS

The abbreviations used are: Topo, topoisomerase; IPTG, isopropyl-1-thio-beta -D-galactopyranoside; ORF, open reading frame; LRI, late replication intermediates.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

1. Levine, C., Hiasa, H., and Marians, K. J. (1998) Biochim. Biophys. Acta 1400, 29-43[Medline] [Order article via Infotrieve]
2. Postow, L., Peter, B. J., and Cozzarelli, N. R. (1999) Bioessays 21, 805-808[CrossRef][Medline] [Order article via Infotrieve]
3. Champoux, J. J. (2001) Annu. Rev. Biochem. 70, 369-413[CrossRef][Medline] [Order article via Infotrieve]
4. Wang, J. C. (2002) Nat. Rev. Mol. Cell. Biol. 3, 430-440[CrossRef][Medline] [Order article via Infotrieve]
5. Khodursky, A. B., Peter, B. J., Schmid, M. B., DeRisi, J., Botstein, D., Brown, P. O., and Cozzarelli, N. R. (2000) Proc. Natl. Acad. Sci. U. S. A. 97, 9419-9424[Abstract/Free Full Text]
6. Dean, F., Krasnow, M. A., Otter, R., Matzuk, M. M., Spengler, S. J., and Cozzarelli, N. R. (1983) Cold Spring Harbor Symp. Quant. Biol. 47, 769-777[Medline] [Order article via Infotrieve]
7. Srivenugopal, K. S., Lockshon, D., and Morris, D. R. (1984) Biochemistry 23, 1899-1906[Medline] [Order article via Infotrieve]
8. DiGate, R. J., and Marians, K. J. (1988) J. Biol. Chem. 263, 13366-13373[Abstract/Free Full Text]
9. Minden, J. S., and Marians, K. J. (1985) J. Biol. Chem. 260, 9316-9325[Abstract/Free Full Text]
10. DiGate, R. J., and Marians, K. J. (1989) J. Biol. Chem. 264, 17924-17930[Abstract/Free Full Text]
11. Wallis, J. W., Chrebet, G., Brodsky, G., Rolfe, M., and Rothstein, R. (1989) Cell 58, 409-419[Medline] [Order article via Infotrieve]
12. Rothstein, R. (1984) Cold Spring Harbor Symp. Quant. Biol. 49, 629-637[Medline] [Order article via Infotrieve]
13. Schofield, M. A., Agbunag, R., Michaels, M. L., and Miller, J. H. (1992) J. Bacteriol. 174, 5168-5170[Abstract]
14. Chakraverty, R. K., Kearsey, J. M., Oakley, T. J., Grenon, M., de La Torre Ruiz, M. A., Lowndes, N. F., and Hickson, I. D. (2001) Mol. Cell. Biol. 21, 7150-7162[Abstract/Free Full Text]
15. Goodwin, A., Wang, S. W., Toda, T., Norbury, C., and Hickson, I. D. (1999) Nucleic Acids Res. 27, 4050-4058[Abstract/Free Full Text]
16. Maftahi, M., Han, C. S., Langston, L. D., Hope, J. C., Zigouras, N., and Freyer, G. A. (1999) Nucleic Acids Res. 27, 4715-4724[Abstract/Free Full Text]
17. Caspari, T., Murray, J. M., and Carr, A. M. (2002) Genes Dev. 16, 1195-1208[Abstract/Free Full Text]
18. Hanai, R., Caron, P. R., and Wang, J. C. (1996) Proc. Natl. Acad. Sci. U. S. A. 93, 3653-3657[Abstract/Free Full Text]
19. Seki, T., Seki, M., Onodera, R., Katada, T., and Enomoto, T. (1998) J. Biol. Chem. 273, 28553-28556[Abstract/Free Full Text]
20. Li, W., and Wang, J. C. (1998) Proc. Natl. Acad. Sci. U. S. A. 95, 1010-1013[Abstract/Free Full Text]
21. Wu, L., Karow, J. K., and Hickson, I. D. (1999) Curr. Biol. 9, R518-R520[CrossRef][Medline] [Order article via Infotrieve]
22. Hiasa, H., DiGate, R. J., and Marians, K. J. (1994) J. Biol. Chem. 269, 2093-2099[Abstract/Free Full Text]
23. Peng, H., and Marians, K. J. (1993) J. Biol. Chem. 268, 24481-24490[Abstract/Free Full Text]
24. Kato, J., Nishimura, Y., Yamada, M., Suzuki, H., and Hirota, Y. (1988) J. Bacteriol. 170, 3967-3977[Medline] [Order article via Infotrieve]
25. Kato, J., Nishimura, Y., Imamura, R., Niki, H., Hiraga, S., and Suzuki, H. (1990) Cell 63, 393-404[Medline] [Order article via Infotrieve]
26. Levine, C., and Marians, K. J. (1998) J. Bacteriol. 180, 1232-1240[Abstract/Free Full Text]
27. Mossessova, E., Levine, C., Peng, H., Nurse, P., Bahng, S., and Marians, K. J. (2000) J. Biol. Chem. 275, 4099-4103[Abstract/Free Full Text]
28. Link, A. J., Phillips, D., and Church, G. M. (1997) J. Bacteriol. 179, 6228-6237[Abstract]
29. Nurse, P., Bahng, S., Mossessova, E., and Marians, K. J. (2000) J. Biol. Chem. 275, 4104-4111[Abstract/Free Full Text]
30. Hiasa, H., and Marians, K. J. (1994) J. Biol. Chem. 269, 6058-6063[Abstract/Free Full Text]
31. Xu, L., and Marians, K. J. (2002) J. Biol. Chem. 277, 14321-14328[Abstract/Free Full Text]
32. Peter, B. J., Ullsperger, C., Hiasa, H., Marians, K. J., and Cozzarelli, N. R. (1998) Cell 94, 819-827[Medline] [Order article via Infotrieve]
33. Espeli, O., Levine, C., Hassing, H., and Marians, K. J. (2003) Mol. Cell 11, 189-201[Medline] [Order article via Infotrieve]
34. Blattner, F. R., Plunkett, G., III, Bloch, C. A., Perna, N. T., Burland, V., Riley, M., Collado-Vides, J., Glasner, J. D., Rode, C. K., Mayhew, G. F., Gregor, J., Davis, N. W., Kirkpatrick, H. A., Goeden, M. A., Rose, D. J., Mau, B., and Shao, Y. (1997) Science 277, 1453-1474[Abstract/Free Full Text]
35. Diederich, L., Roth, A., and Messer, W. (1994) BioTechniques 16, 916-923[Medline] [Order article via Infotrieve]
36. Hiasa, H., and Marians, K. J. (1996) J. Biol. Chem. 271, 21529-21535[Abstract/Free Full Text]
37. Champoux, J. J., and Been, M. D. (1980) in Mechanistic Studies of DNA Replication and Recombination: ICN-UCLA Symposia on Molecular and Cellular Biology (Alberts, B., ed) , pp. 809-815, Academic Press, Inc., New York
38. Ullsperger, C. J., Vologodskii, A. A., and Cozzarelli, N. R. (1995) in Nucleic Acids and Molecular Biology (Lilly, D. M. J. , and Eckstein, F., eds) , pp. 115-142, Springer-Verlag, Berlin
39. Ullsperger, C., and Cozzarelli, N. R. (1996) J. Biol. Chem. 271, 31549-31555[Abstract/Free Full Text]
40. Hiasa, H., and Marians, K. J. (1994) J. Biol. Chem. 269, 32655-32659[Abstract/Free Full Text]
41. Hill, T. M., and Marians, K. J. (1990) Proc. Natl. Acad. Sci. U. S. A. 87, 2481-2485[Abstract]
42. Harmon, F. G., DiGate, R. J., and Kowalczykowski, S. C. (1999) Mol. Cell 3, 611-620[Medline] [Order article via Infotrieve]


Copyright © 2003 by The American Society for Biochemistry and Molecular Biology, Inc.