Chromosome architecture undergoes extensive, programmed changes as cells enter meiosis. A highly conserved change is the clustering of telomeres at the nuclear periphery to form the "bouquet" configuration. In the fission yeast Schizosaccharomyces pombe the bouquet and associated nuclear movement facilitate initial interactions between homologs. We show that Bqt2, a meiosis-specific protein required for bouquet formation, is required for wild-type levels of homolog pairing and meiotic allelic recombination. Both gene conversion and crossing over are reduced and exhibit negative interference in bqt2 mutants, reflecting reduced homolog pairing. While both the bouquet and nuclear movement promote pairing, only the bouquet restricts ectopic recombination (that between dispersed repetitive DNA). We discuss mechanisms by which the bouquet may prevent deleterious translocations by restricting ectopic recombination.

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MEIOSIS, the specialized form of nuclear division that reduces the diploid number of chromosomes by half, consists of one round of DNA replication followed by two successive nuclear divisions. At the first meiotic division (MI) homologous chromosomes (homologs), each consisting of two sister chromatids, are segregated to opposite poles, reducing the chromosome number by half. The second meiotic division (MII), like mitosis, segregates sister chromosomes to opposite poles, producing four haploid nuclei.

The elevated rate of recombination characteristic of meiosis is due to a programmed set of meiosis-specific events that includes the formation of DNA double-strand breaks (DSBs) by Spo11, called Rec12 in Schizosaccharomyces pombe (KEENEY et al. 1997; CERVANTES et al. 2000). The DSBs are then repaired via interaction with an intact duplex, giving rise to gene conversions and crossovers (reviewed in ROEDER 1997; KEENEY 2001). At least one crossover per homolog pair is required to promote the proper attachment of each homolog in a pair to spindle microtubules from opposite poles, ensuring segregation of homologs at MI (reviewed in PAGE and HAWLEY 2003; PETRONCZKI et al. 2003). In addition to its critical role in segregation, recombination generates diversity in subsequent generations by creating new combinations of alleles.

An elevated frequency of recombination is not sufficient to promote proper meiotic chromosome segregation; recombination must involve homologs rather than sister chromatids and must frequently produce a crossover. In meiosis, unlike mitosis, gene conversion is frequently associated with crossing over (GRIMM et al. 1994; VIRGIN et al. 2001; CROMIE et al. 2005 and references therein). Consequently, the recombination events that occasionally occur between dispersed repetitive DNA, such as transposons, genes for tRNAs, subtelomeric sequences, and multigene families, may frequently involve crossovers. Such crossovers can produce deleterious chromosomal rearrangements (reviewed in SHAFFER and LUPSKI 2000). However, in both S. pombe and the budding yeast Saccharomyces cerevisiae, recombination between dispersed repetitive DNA is significantly lower than allelic recombination (MUNZ et al. 1982; KOHLI et al. 1984; KUPIEC and PETES 1988a,b; GOLDMAN and LICHTEN 1996, 2000; VIRGIN and BAILEY 1998; SCHLECHT et al. 2004). The restriction of ectopic recombination may, in some cases, result from an insufficient length of sequence identity. The restriction of ectopic recombination may also reflect the recombination-independent propensity of chromosomes to align, in register, along their entire length. In the latter case, if homologs were unable to align, ectopic recombination would not be restricted and dispersed repetitive elements might recombine as efficiently as allelic sequences.

Despite the elevated frequency of recombination in meiosis, in many organisms the number of crossovers per genome is not much larger than the number of chromosomes (reviewed in HILLERS 2004). If these crossovers were placed randomly throughout the genome, a large fraction of meioses would contain at least one homolog pair with no crossovers and therefore be prone to missegregation at MI. However, in many organisms the placement of crossovers is regulated; for instance, the presence of one crossover reduces the likelihood of a second nearby crossover (reviewed in VAN VEEN and HAWLEY 2003; HILLERS 2004). This phenomenon, crossover interference, is manifest as a frequency of double crossovers lower than that expected for two independent events. In S. pombe, which does not have crossover interference, each of its three chromosomes receives 10–20 randomly placed crossovers, resulting in a very low frequency of chromosomes without a crossover (MUNZ 1994).

Before recombination can take place, two DNA molecules must first be in close proximity. Thus, a critical step in meiotic recombination is the juxtaposition of homologous chromosomes. Homologs are brought together in a stepwise process (reviewed in GERTON and HAWLEY 2005). In this process we define homologs as being "aligned" when they are in register along their entire length. Homologs are subsequently defined as being "paired" when they are intimately associated along their entire length. Clustering of telomeres at the nuclear periphery, the bouquet configuration, is a conserved feature of meiosis that is thought to facilitate the alignment of homologs (reviewed in SCHERTHAN 2001; YAMAMOTO and HIRAOKA 2001). In S. pombe the bouquet consists of a tight cluster of all telomeres at the spindle-pole body (SPB). This clustering requires the telomere-binding protein Taz1, the Taz1-binding protein Rap1, and the heterochromatin protein Rik1 (COOPER et al. 1997, 1998; NIMMO et al. 1998; CHIKASHIGE and HIRAOKA 2001; KANOH and ISHIKAWA 2001; TUZON et al. 2004). Telomere- and SPB-led oscillatory nuclear movement ("horsetail" movement) occurs throughout meiotic prophase (CHIKASHIGE et al. 1994) and depends on Dhc1, the microtubule motor protein dynein (DING et al. 1998; YAMAMOTO et al. 1999). Perturbing either the bouquet or horsetail movement reduces pairing and meiotic recombination (SHIMANUKI et al. 1997; COOPER et al. 1998; NIMMO et al. 1998; YAMAMOTO et al. 1999; NIWA et al. 2000; MIKI et al. 2002; DING et al. 2004; SAITO et al. 2005). By providing a physical linkage between chromosomes, recombination stabilizes their initial alignment and pairing promoted by the bouquet and horsetail movement (NABESHIMA et al. 2001; DING et al. 2004). Thus, the initial alignment and pairing of homologs are required for wild-type levels of meiotic recombination, which in turn is required for stable homolog pairing.

The Bqt2 protein of S. pombe is a meiosis-specific SPB component and is required for telomere clustering (MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006). In bqt2 mutant meioses SPB movement still occurs but telomeres are dispersed throughout the nucleus and chromosome movement is diminished. Here we show that, as expected, pairing of homologs in meiotic prophase and allelic recombination are reduced in bqt2 mutants. Furthermore, recombination events in both bqt2 and dhc1 mutants display negative interference: the presence of one recombination event increases the likelihood of a second nearby event. Bqt2, but not Dhc1, restricts ectopic recombination. We suggest a model in which ectopic recombination is restricted by the position of the two repetitive DNA elements relative to their nearest telomere, rather than pairing per se.

Yeast strains, media, and culture conditions:

Solid media were YEA + 4S, YEA + 5S, YEAG, or supplemented EMM2 used at 32° as described previously (DAVIS and SMITH 2003). Liquid cultures were grown at 30° in YEL + 5S. Sporulation was at 25° on supplemented SPA (GUTZ et al. 1974) for 2–4 days. The yeast strains and mutant alleles used are described below or in references in supplemental Table S1 at http://www.genetics.org/supplemental/.

Genetic screen for meiotic segregation mutants:

In the absence of recombination (e.g., in rec12 mutants), S. pombe possesses a residual ability to segregate homologs at MI (DAVIS and SMITH 2003 and references therein). Missegregation of homologs at MI results in an elevated frequency of heterozygous diploid spores. Random segregation at MI is expected to produce 10-fold more heterozygous diploid spores than that observed in rec12 mutant meioses (DAVIS and SMITH 2003, 2005). Heterozygous diploid spore formation in rec12 mutants is thus expected to be increased by loss of the recombination-independent MI homolog segregation ability. To identify gene products required for this process, we enriched for mutants of strain GP2640 (h⁹⁰ ade6-52 leu1-32 ura4-294 his3-D1 fus1::LEU2 rec12-152::LEU2) as follows. Haploid fus1 mutant cells are unable to mate and therefore cannot sporulate; however, fus1 mutant diploids, if heterozygous at the mating-type locus, are able to properly complete meiosis and sporulation (PETERSEN et al. 1995). By coupling the ability of fus1 to prevent sporulation of haploid cells with the ability to selectively kill nonsporulated cells using glusulase treatment (PONTICELLI and SMITH 1989), the meiotic progeny of diploid cells can be efficiently selected.

Strain GP2640 carrying plasmid pDW220 (ura4⁺ fus1⁺; PETERSEN et al. 1995) was mutagenized by random integration of linearized plasmid pAF1 (his3⁺; OHI et al. 1996) into the genome. Pools of mutagenized cells were sporulated, and the vegetative cells were killed and spores liberated from asci by treatment with glusulase. The spore suspensions were allowed to germinate in EMM2 medium, and cells that lost pDW220 were selected on plates containing 5-fluoroorotic acid. The remaining cells, a mixture of haploids and diploids, were phenotypically Fus1^–, and therefore only the diploids could sporulate. Each subsequent round of sporulation of these diploid spores coupled with killing of haploid cells results in a theoretical 10-fold enrichment for mutants with random segregation at MI. Nine pools of His⁺ transformants (totaling 10,000 individual colonies) were carried through two rounds of enrichment. The resulting mutants were screened by testing 25 individual colonies from each pool for those that produced an elevated level of diploid spores (i.e., I₂-staining spore colonies on EMM2 medium), and two mutants were identified. One mutant contained an insertion within the klp6 (SPBC649.01C) coding sequence. Klp6 is a kinesin-like protein that belongs to the kinesin-8 family of microtubule-destabilizing proteins (LAWRENCE et al. 2004; MIKI et al. 2005). The role of Klp6 in mitosis and meiosis has been described by others (WEST et al. 2001, 2002; GARCIA et al. 2002a,b; LI and CHANG 2003; SANCHEZ-PEREZ et al. 2005). The other mutant contained an insertion within the coding sequence of SPAC1002.06C. This gene, recently named bqt2, is required for meiotic bouquet formation (MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006) and is the subject of this study.

Microscopy:

To assay pairing, strains were used in which lacO was integrated near the centromere of chromosome I (ChrI) (NABESHIMA et al. 1998) and bound by a variant of the green fluorescent protein-LacI-nuclear localization signal fusion (GFP13-LacI12-NLS; STRAIGHT et al. 1998), adapted for S. pombe (DAVIS and SMITH 2003). Approximately 10⁷ cells were mated on supplemented SPA and collected after 16–24 hr. Live zygotes, arrested in prophase by the mei4 mutation (SHIMODA et al. 1985; HIRAOKA et al. 2000), were examined by fluorescence microscopy performed on a Nikon Eclipse 600 microscope using a Nikon 60x 1.40 NA Plan Apo objective (Nikon, Melville, NY). Images were captured using MetaMorph software (Molecular Devices, Sunnyvale, CA) and a Cascade 512B CCD camera (Photometrics, Tucson, AZ). GFP foci were counted in two experiments and statistical significance was calculated for each experiment independently using a ²-test.

Deletion constructs:

A complete replacement of the bqt2 coding sequence with 3HA-6His-kanMX6 was constructed using the method of BAHLER et al. (1998). A PCR was performed using as template plasmid pFA6a-3HA-6His-kanMX6 (DAVIS and SMITH 2003). The forward and reverse primers in this reaction contained nucleotides corresponding to the 5' and 3' ends of bqt2⁺ (nucleotides 10,147–10,226 and 9555–9634, respectively, of cosmid SPAC1002; GenBank accession no. AL136078). The resulting PCR product was used to transform S. pombe strain GP363 (h⁺ ade6-M26 ura4-294 arg3-124) to G418 resistance, conferred by kanMX. Deletion of bqt2 (bqt2-168::kanMX) was confirmed by a PCR.

Recombinant frequencies:

Intergenic recombinant frequencies among Ade⁺ viable spores were determined by plating spore suspensions on YEAG to select Ade⁺ spores and, after 3–5 days, colonies were toothpicked to grids on YEAG. After growth overnight, the segregants were replicated to the appropriate test media. Otherwise, recombinant frequencies were determined as previously described (YOUNG et al. 2002). Statistical significance of Ade⁺ recombinant frequencies was calculated using Student's t-test. ²-tests were used for statistical analysis of genetic interference data. For crossover interference in the ura4-aim–tps16–arg1 intervals we determined whether or not the observed frequency of double crossovers was greater than that expected for two independent events. For interference between a conversion and a crossover we determined whether or not the frequency of crossovers was greater among the Ade⁺ spores than among total spores.

Unequal sister-chromatid exchange (SCE) frequencies were determined as follows. Appropriately diluted mitotic cultures of the ade6-Dup-containing strain were plated on YEA + 4S to determine the total number of viable cells and on YEAG to determine the frequency of Ade⁺ recombinants. The ade6-Dup strain and the appropriate ade6-D19 strain were then mated on supplemented SPA. Spores were harvested and spore suspensions were plated on YEA + 4S to determine the total number of viable cells and on YEAG to determine the frequency of Ade⁺ recombinants. The mitotic frequency, which was typically 5–10% of the meiotic frequency and never >27%, was subtracted from the meiotic frequency to give the final meiotic SCE frequency. Ten crosses were performed for each genotype and the statistical significance was calculated using Student's t-test.

Bqt2 is required for homolog pairing in meiotic prophase:

We isolated a mutation in the S. pombe gene SPAC1002.06c in a screen for mutations that increase MI chromosome missegregation in a rec12 background (see MATERIALS AND METHODS for details). SPAC1002.06c was subsequently named bqt2 and reported to encode a meiosis-specific spindle-pole body protein required for telomere clustering and wild-type levels of meiotic recombination (MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006). To determine whether, as expected, the telomere-clustering defect of bqt2 mutants resulted in defective homolog pairing, we examined both wild-type and bqt2 mutants marked with a tandem array of lacO DNA near the centromere of ChrI (NABESHIMA et al. 1998). As a control, we also examined pairing in the absence of Dhc1, the heavy chain of the microtubule motor dynein, which is required for meiotic horsetail movement and efficient homolog pairing (YAMAMOTO et al. 1999; DING et al. 2004). Pairing was visualized by fluorescence microscopy of the GFP-LacI-NLS fusion protein, which binds to the lacO array.

Homolog pairing in S. pombe is a dynamic process (DING et al. 2004). To aid the analysis, we used the mei4 mutation, which arrests cells in meiotic prophase, after horsetail nuclear movement, with paired homologs (YOKOBAYASHI and WATANABE 2005). To the best of our knowledge, the precise position of the mei4 arrest point relative to the dynamics of pairing is unknown. A single-GFP focus indicates pairing of the lacO array, while unpaired arrays generate two GFP foci in a single nucleus. Three or four GFP foci in a single nucleus indicate a defect in sister-chromatid cohesion. Two experiments, each with wild type and mutants on the same SPA plate, were performed, one 16 hr and the other 24 hr after the cells were mated. A single-GFP focus was found in 66, 39, and 43% of prophase nuclei in wild-type, bqt2, and dhc1 cells, respectively, in the first experiment, and 96, 51, and 53% in the second (Table 1). The difference in the absolute level of pairing observed in the two experiments may be due to the degree to which the cells reached the mei4 arrest point in each experiment. The fraction of paired homologs for both bqt2 and dhc1 was statistically different from that in wild type in each experiment (P < 0.0005). This indicates that pairing of the lacO array was significantly reduced in both bqt2 and dhc1 mutants. In all of the strains examined, 2% prophase nuclei contained three or four GFP foci, indicating that sister-chromatid cohesion is not significantly altered in bqt2 and dhc1 mutants.

View this table: In this window In a new window   TABLE 1 Bqt2 is required for pairing of homologous chromosomes in meiotic prophase

 

Telomere clustering is required for wild-type levels of homologous intergenic recombination:

In bqt2 mutants meiotic DSB formation and repair is nearly wild type but recombination is reduced by factors of 3–7 in the three intervals examined (MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006). To better understand this apparent discrepancy between reduced recombination and normal formation and repair of DSBs, which are expected to produce recombinants, we extended the analysis of meiotic recombination. We measured intergenic recombination (crossovers) in four intervals: lys3–met5 on ChrI, pat1–leu1 on ChrII, and ura4-aim–tps16–arg1 on ChrIII (Figure 1A). Recombinant frequency in the bqt2 mutants was reduced by a factor of 2–4 in the regions tested, a reduction similar to that seen in the dhc1 mutant (Tables 2 and 3). The lys3–met5 interval encompasses a region with DSB frequency and kinetics of repair that are nearly wild type in bqt2 mutant meioses (MARTIN-CASTELLANOS et al. 2005). Significantly, recombination in this interval was reduced in the bqt2 mutant by a factor of 4 (Table 2). These data suggest that repair of meiotic DSBs in the bqt2 mutant, and perhaps all pairing mutants, frequently involves the use of either sister chromatids or homologous nonallelic sequences as a template.

View larger version (15K): In this window In a new window Download PPT slide   FIGURE 1.— S. pombe chromosomes. (A) Centromeres, telomeres, rDNA, and relevant genetic markers are indicated. ChS28 is a deletion derivative of ChrIII (NIWA et al. 1989). Drawn to scale. (B) Graphical representation of the sum of insert distances to their nearest telomere (SIDT) and the difference between the distances of each locus from its nearest telomere (DT) for two loci, aaa1 and bbb1, on heterologous chromosomes.

 

View this table: In this window In a new window   TABLE 2 Pairing mutants demonstrate reduced allelic recombination and negative interference between a conversion and a crossover

 

View this table: In this window In a new window   TABLE 3 Pairing mutants demonstrate negative crossover interference

 

Recombination in pairing mutants displays negative interference:

In many organisms the presence of one crossover reduces the likelihood of a second nearby crossover (reviewed in HILLERS 2004). This phenomenon, called crossover interference, is manifest as a lower-than-expected frequency of double crossovers. Interference is defined as I = 1 – C, where C (coefficient of coincidence) = and R₁, R₂, and R_d are the frequencies of crossovers in interval one, interval two, and double crossovers, respectively. When I = 0, double crossovers occur at the frequency expected for two independent events; when I = 1, no double crossovers are observed. In rare instances the opposite situation has been reported whereby the presence of one crossover increases the likelihood of a second nearby crossover: I < 0, a situation called negative interference. In wild-type S. pombe there is no meiotic crossover interference, either positive or negative (MUNZ 1994).

If recombination is limited by inefficient pairing, the presence of a crossover may select for cells in which adjacent chromosomal intervals are necessarily in close proximity and may also stabilize the interaction between homologs. This may increase the likelihood of a second event, resulting in negative interference. We calculated the coefficient of coincidence (C) for the two adjacent intervals, ura4-aim–tps16 and tps16–arg1, on ChrIII (see Figure 1A) using the recombination data from Table 3. In wild-type crosses C = 1.2, not significantly different from 1 (P > 0.3). In bqt2 mutant crosses C = 2.5, significantly >1 (P < 0.05). Similarly, in dhc1 mutant crosses C = 2.9. Although 2.9 was not significantly >1 (0.05 < P < 0.1), we suspect that this reflects the limited number of observed double crossovers (12). These data indicate that bqt2, and perhaps dhc1, mutants exhibit negative crossover interference.

The negative interference described above was between two crossovers. Similarly, positive interference is typically observed between two crossovers; in both S. cerevisiae and the filamentous fungus Neurospora crassa a gene conversion without an associated crossover does not exhibit interference with an adjacent interval (FOGEL and HURST 1967; STADLER and TOWE 1968; MALKOVA et al. 2004). However, if one allelic interaction promotes the interaction of nearby chromosomal regions, negative interference might be observed between a conversion and a crossover. The crosses used to measure homologous intergenic recombination, above, also contained heteroalleles of ade6, allowing us to address this possibility. We measured intergenic recombination among selected ade6⁺ gene convertants in these crosses and calculated C. Here , where and are the frequencies of crossovers among ade6⁺ convertants and among total spores, respectively. For gene convertants at ade6 and crossovers in the tps16–arg1 interval, which is 60–300 kb from ade6 on ChrIII (Figure 1A), C = 0.93 in wild-type crosses, not significantly different from 1 (P > 0.25; Table 2). In bqt2 and dhc1 mutant crosses C = 2.29 and 2.49, respectively, and is significantly >1 (P < 0.0005; Table 2). The data in Table 2 include ade6⁺ gene convertants with and without an associated crossover between ura4⁺-aim and tps16. When only those convertants without an associated crossover are considered, C = 2.45 and 2.51 in bqt2 and dhc1 mutant crosses, respectively, and is significantly >1 (P < 0.0005). These data indicate that both bqt2 and dhc1 mutants exhibit negative interference between a conversion and a crossover.

An alternative explanation for apparent negative interference is a subpopulation of "hot" meiotic cells that are recombinationally more competent than the bulk population. To address this possibility, we determined the recombinant frequency in the lys3–met5 and pat1–leu1 intervals, on ChrI and -II, respectively, among ade6⁺ (ChrIII) convertants. If there is a significant subpopulation of hot cells, then the recombinant frequency in both intervals would be higher among ade6⁺ convertants than among total cells (C > 1), despite the intervals being on different chromosomes. The recombinant frequency in the lys3–met5 interval was not significantly higher among ade6⁺ convertants than among total cells in wild type, bqt2, or dhc1 (C = 0.92, P > 0.3; C = 1.18, P > 0.3; C = 1.02, P > 0.9, respectively; Table 2). These data argue against a subpopulation of hot cells.

In the pat1–leu1 interval the recombinant frequency was modestly higher among ade6⁺ convertants than among total spores in wild type, bqt2, and dhc1 (Table 2). In wild-type crosses C = 1.15, not significantly different from 1 (P > 0.05), but in bqt2 and dhc1 mutant crosses C = 1.31 and 1.46, respectively, and was significantly >1 (P < 0.02 and P < 0.0025, respectively). To determine if the increase in recombinant frequency among ade6⁺ convertants observed in bqt2 and dhc1 mutants was significantly different from the increase observed in wild type, we determined whether or not the observed frequency of crossovers was greater than that expected if C = 1.15, the wild-type value. The increase in recombinant frequency among ade6⁺ convertants observed in the bqt2 mutant was not significantly different from the increase observed in wild type (P > 0.25), but that in the dhc1 mutant was significantly different (P < 0.05). These results indicate that the observed increase of recombinant frequencies among ade6⁺ convertants in the pat1–leu1 interval (ChrII) is independent of the bqt2 mutation but partially dependent on the dhc1 mutation. The reason for this result is unknown, but in light of the results with the lys3–met5 interval (ChrI), it does not indicate that the negative interference observed at the ura4-aim–ade6–tps16–arg1 region of ChrIII in bqt2 and dhc1 mutants is due to hot cells specifically present in the mutant population.

Telomere clustering, but not horsetail movement, restricts ectopic recombination:

To determine whether reduced pairing resulted in excess ectopic (nonallelic) recombination, we first determined the recombinant frequency between the ade6-M26 allele on ChrIII and the ade6-M210 allele on an artificial minichromosome (ChS28; NIWA et al. 1989 and see Figure 1A). In this assay, the frequency of Ade⁺ recombinants was increased, relative to that in wild type, by a factor of 18 in bqt2 mutants but was not affected in dhc1 mutants (Table 4). We infer that the minichromosome is released from its position near the telomeres of ChrI, -II, and -III in the bqt2 mutant and can more readily come into proximity to the ade6 locus on ChrIII and therefore recombine with it.

View this table: In this window In a new window   TABLE 4 Telomere clustering, but not horsetail movement, limits ectopic recombination

 
We next determined the recombinant frequency between the ade6-M26 allele on ChrIII and the ade6-469 allele ectopically transplaced on ChrII (zzz7; VIRGIN and BAILEY 1998 and see Figure 1A). In this assay, the frequency of Ade⁺ recombinants was increased, relative to that in wild type, by a factor of 3.5 in bqt2 mutants but was not significantly affected in dhc1 mutants (P > 0.05; Table 4). In bqt2 mutants, recombinant frequencies increased in both assays of ectopic recombination but decreased by a factor of 4.4 for allelic recombination (at the endogenous locus) between the ade6-M26 and ade6-M210 alleles (Table 4). These data indicate that Bqt2, but not Dhc1, restricts the interaction of ectopic sequences.

The normal frequency of DSB formation and repair (MARTIN-CASTELLANOS et al. 2005), but reduced homolog recombination (Tables 2 and 3), suggested that the bqt2 mutation might increase the frequency of meiotic sister-chromatid exchange. To address this possibility, we determined the frequency of recombination between tandemly duplicated copies of the ade6 gene, one marked with the M26 allele and the other with the 469 allele, flanking ura4⁺ at the endogenous ade6 locus (SCHUCHERT and KOHLI 1988). In this assay, recombination must use the sister as a template, since ade6 is deleted from the homologous chromosome. In bqt2 mutant meioses the Ade⁺ recombinant frequency was modestly but significantly greater than that in wild type (Table 4; P = 0.009). The Ade⁺ recombinant frequency in dhc1 mutant meioses was not significantly different from that in wild type (Table 4; P > 0.9). These data indicate that Bqt2, but not Dhc1, restricts unequal sister-chromatid exchange.

In S. pombe, telomere clustering and horsetail nuclear movement promote the pairing of homologous chromosomes during meiotic prophase (reviewed in BURGESS 2004), perhaps by limiting the space that must be searched for a homologous sequence. Recombination requires homolog proximity but also promotes pairing, perhaps by stabilizing the initial alignment of homologs. To understand the role that each of these processes plays in homolog pairing, we have analyzed mutations that specifically abolish telomere clustering (bqt2; MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006) and horsetail nuclear movement (dhc1; YAMAMOTO et al. 1999). Bqt2 is a meiosis-specific SPB component that, together with Bqt1, tethers the telomere protein Rap1 to the SPB protein Sad1 (MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006). Dhc1, the heavy chain of the microtubule motor dynein, is required for horsetail nuclear movement and, although expression of Dhc1 is not meiosis specific, it has no detected mitotic phenotype (YAMAMOTO et al. 1999). We first showed that Bqt2, as predicted, is required for efficient pairing of homologs in meiotic prophase (Table 1). We then extended the analysis of meiotic recombinant frequencies in bqt2 and dhc1 mutants. In light of our results, we propose that (1) the bouquet promotes the alignment of homologs but not their full pairing, (2) horsetail movement facilitates the transition from alignment to full pairing (Figure 2A), and (3) ectopic recombination is restricted by the alignment of homologs, rather than pairing per se.

View larger version (27K): In this window In a new window Download PPT slide   FIGURE 2.— The role of telomere clustering and "horsetail" nuclear movement in meiotic homolog pairing. (A) Prior to nuclear fusion, telomeres cluster at the SPB (solid circle). In the prophase nucleus, the bouquet promotes alignment of homologs, and horsetail movement facilitates the transition to full pairing. (B) Proposed chromosome configuration in wild-type, dhc1, and bqt2 mutant prophase nuclei. Only two of the three chromosome pairs are shown. The stars represent homologous sites on a pair of homologs.

 

Recombination in homolog-pairing mutants displays negative interference:

Positive crossover interference is widespread in meiotic recombination (reviewed in HILLERS 2004). Negative crossover interference (higher than expected frequency of double crossovers) is less common and has been associated with special chromosomal regions—centromeres in Drosophila melonogaster and several species of plants (GREEN 1975; SINCLAIR 1975; DENELL and KEPPY 1979; PENG et al. 2000; BOYKO et al. 2002; ESCH and WEBER 2002; ESCH 2005) and heterozygous translocations in the mosquito Aedes aegypti and several species of plants (AUGER and SHERIDAN 2001, and references therein). Several proposals have been put forth to explain these cases of negative interference. Apparent negative crossover interference has been attributed to gene conversion of the central marker, i.e., one, not two, events (GREEN 1975). DENELL and KEPPY (1979) suggested that negative interference may be characteristic of chromosomal regions, such as centromeres, that have a low density of recombination events (per unit physical length). AUGER and SHERIDAN (2001) suggested that negative interference is a result of reduced competence for crossover formation near translocation breakpoints. Just as hot cells result in negative interference (GROSSENBACHER-GRUNDER 1985), so would hot regions of chromosomes—the chromosomal regions that do pair in a pairing-deficient mutant. After submission of this article, negative crossover interference was reported in a zip4 mutant of S. cerevisiae using a single-interval assay (nonparental ditype ratio; TSUBOUCHI et al. 2006). Our results suggest that inefficient homolog pairing leads to negative interference in S. pombe.

bqt2 and dhc1 mutants display negative interference, both between two crossovers and between a conversion and a crossover (Tables 2 and 3). This is in contrast to wild-type S. pombe where there is no interference (Tables 2 and 3; KOHLI and BAHLER 1994; MUNZ 1994). The negative crossover interference in the ura4-aim–tps16–arg1 intervals is unlikely to result from gene conversion of the central marker for the following reason. The frequency of conversion at tps16 would have to be 0.9%, the frequency of apparent double crossovers in excess of the expected frequency, in the ura4-aim–tps16–arg1 intervals in bqt2 and dhc1 mutants. This is more than twice the frequency of conversion observed in wild type (0.4%; ZAHN-ZABAL et al. 1995). Given that both mutations reduce all allelic recombination examined by more than a factor of 2 (Tables 2–4), it is unlikely that conversion at tps16 could explain these results. Additionally, to explain the negative interference between ade6⁺ convertants and tps16–arg1 crossovers (Table 2), the frequency of conversion at tps16 would have to be at least 17%, but only among ade6⁺ spores.

Gene conversion in S. pombe meiosis is frequently associated with crossing over between flanking markers (GRIMM et al. 1994; CROMIE et al. 2005). Negative interference between a conversion and a crossover could be explained if the conversion and crossover were not separate events. However, to explain the negative interference between ade6⁺ convertants and apparent tps16–arg1 crossovers, a single recombination event would frequently have to cover more than the 59 kb between ade6 and tps16. While we cannot formally rule out this possibility, it seems unlikely that the frequency of this type of event would be increased in bqt2 and dhc1 mutants.

We propose that negative interference in bqt2 and dhc1 mutants is the consequence of inefficient homolog pairing and an otherwise wild-type ability to repair meiotic DSBs and reflects a propensity for localized proximity of homologs to extend to larger regions—at least 59 kb, the distance between ade6 and tps1 (Figure 1A). The propensity for extended proximity may be related to recombination in two distinct ways. First, an initial recombination event may stabilize the interaction between homologs. This would limit the space that an adjacent chromosomal interval must search for a homologous sequence with which to recombine, thus increasing the likelihood of a second nearby recombination event. In this model, recombination is required to extend localized proximity. Second, when, by chance, one locus is close enough to its homolog to recombine, adjacent chromosomal intervals are necessarily in close proximity, thus increasing the likelihood of a second nearby recombination event. In this model, the first recombination event does not cause local proximity to be extended; rather, extended proximity reflects simply the physical properties of the chromosome. Our genetic data do not differentiate between these models, although a cytological assay for local alignment in a Rec^– mutant may be able to do so.

Telomere clustering, but not horsetail movement, restricts ectopic recombination:

Crossovers between dispersed repetitive DNA such as transposons, genes for tRNA, subtelomeric sequences, and multigene families can produce deleterious chromosomal rearrangements. Endogenous repetitive sequences are unlikely to be identical. At least in S. cerevisiae, the mismatch repair (MMR) pathway, which can detect regions of sequence divergence, restricts recombination between diverged sequences (reviewed in BORTS et al. 2000). Despite this restriction, ectopic recombination (that between nonallelic sequences) does occur. In humans, a significant number of diseases and syndromes are due to chromosomal translocations, duplications, or deletions generated by meiotic recombination between repetitive DNA (reviewed in STANKIEWICZ and LUPSKI 2002). This emphasizes the importance of restricting ectopic recombination. In fact, processes other than MMR must restrict ectopic recombination since the frequency of recombination between nearly identical repeats is significantly lower than that of allelic recombination in both S. cerevisiae and S. pombe (GOLDMAN and LICHTEN 1996, 2000; VIRGIN and BAILEY 1998; SCHLECHT et al. 2004). The mechanisms that limit ectopic recombination have not been well characterized. Our data indicate that the meiotic bouquet plays a critical role in S. pombe, perhaps by promoting the alignment of chromosomes, in register, along their entire length.

We have shown that, in S. pombe, ectopic recombination is predominantly constrained by telomere clustering, not homolog pairing per se. Both bqt2 and dhc1 mutants reduce pairing and allelic recombination, although the meiotic DSB frequency is nearly wild type (Tables 1–4; YAMAMOTO et al. 1999; DING et al. 2004; MARTIN-CASTELLANOS et al. 2005; CHIKASHIGE et al. 2006; C. ELLERMEIER and G. R. SMITH, unpublished data). The high viable spore yield in bqt2 and dhc1 mutants (50% of wild type; our unpublished data) indicates that the meiotic DSBs are repaired. We had initially inferred that DSB repair in both mutants frequently involves the use of either sister chromatids or homologous nonallelic sequences as a template. Instead, we found that unequal sister-chromatid exchange and ectopic recombination were unaffected in the dhc1 mutant (Table 4). Perhaps in dhc1 mutant meioses DSBs are repaired by equal sister-chromatid exchange or by nonhomologous end joining. In bqt2 mutant meioses unequal sister-chromatid exchange was elevated 1.5-fold, relative to wild type (Table 4). If sister-chromatid exchange is more frequent than exchange between homologs in wild-type S. pombe, a reduced ability to repair DSBs using the homolog as template (e.g., in pairing mutants) would result in only a small increase in SCE. Ectopic recombination, measured in two different assays, was elevated 3.5- and 18-fold in bqt2 mutant meioses (Table 4). Both bqt2 and dhc1 mutants reduce homolog pairing and allelic recombination to approximately the same extent (Tables 1–4) while the restriction of meiotic ectopic recombination is eased in bqt2 mutants and maintained in dhc1 mutants. This indicates that the restriction is not dependent on homolog pairing per se. Instead, we suggest that ectopic recombination is restricted predominantly by chromosomal position.

We propose that ectopic recombination between two dispersed repetitive sequences is restricted by their relative positions in the prophase nucleus. Because of telomere clustering, the distance, in base pairs, from the nearest telomere determines the position of a locus within the nucleus (DING et al. 2004). As a result, the frequency of ectopic recombination is inversely proportional to the difference between the distances of each locus from its nearest telomere (DT, Figure 1B). This proposal is supported by the following data. First, in wild type, the frequency of recombinants increases as DT decreases: the frequency of recombinants is highest when DT = 0 (i.e., in allelic recombination) and decreases as DT increases (Table 4). When DT is the highest, the ratio of allelic to ectopic recombinant frequencies is 240 (ade6 x ChS28, Table 4). Second, in bqt2 mutant meioses the effect of DT was nearly eliminated: the ratio of allelic to ectopic recombinant frequencies was never >4 (Table 4). Together, these data suggest that the effect of DT on ectopic recombination reflects the role of telomere clustering in restricting ectopic recombination. Determination of recombinant frequencies at additional pairs of loci is required to establish the generality of the effect of DT on ectopic recombination.

We interpret the different effects of bqt2 and dhc1 mutants on ectopic recombination as follows. Alignment and subsequent pairing of homologs along their entire length are required to ensure wild-type levels of meiotic recombination. Bqt2 (telomere clustering) and Dhc1 (horsetail movement) contribute to this in different ways (Figure 2). Prior to mating, chromosomes in wild-type S. pombe are in the "Rabl" orientation; i.e., the centromeres are clustered at the SPB and telomeres are dispersed (FUNABIKI et al. 1993). When mating is induced, centromeres are released and telomeres move to the SPB (CHIKASHIGE et al. 1994, 1997). After nuclear fusion, the bouquet promotes alignment but not full pairing of homologs. The Dhc1-dependent horsetail movement facilitates the transition to full pairing but is dependent on telomere clustering for this effect. In a dhc1 mutant meiosis telomeres still cluster at the SPB and the bouquet is sufficient to promote alignment of homologs but not full pairing (Figure 2B). In the absence of telomere clustering (bqt2), chromosomes are not able to align (Figure 2B). In this view, both bqt2 and dhc1 mutants are scored as pairing defective, measured cytologically at a single locus, but have distinctly different configurations of homologous chromosomes. One prediction of this model is that meiotic ectopic recombination should be elevated to the same extent in the bqt2 dhc1 double mutant as in bqt2.

We expect that like bqt2, other mutations that disrupt telomere clustering such as bqt1, taz1, rap1, and rik1 would result in elevated meiotic ectopic recombination. Additionally, we expect that mutations that disrupt horsetail nuclear movement without disrupting telomere clustering would have no effect on meiotic ectopic recombination. Like Bqt2, Mcp6 is a meiosis-specific SPB protein in S. pombe. In mcp6 mutant meioses telomere clustering appears normal but horsetail nuclear movement is reduced (SAITO et al. 2005; TANAKA et al. 2005). In contrast to our view above, the frequency of ectopic recombinants is increased modestly in mcp6 mutant meioses (SAITO et al. 2005). Additional experiments may determine whether telomere clustering is fully wild type in mcp6 mutants.

In an extensive analysis of ectopic recombination in S. cerevisiae, the authors concluded that for loci on heterologous chromosomes the efficiency of ectopic recombination is negatively correlated with the sum of insert distances to their nearest telomeres (SIDT) (see Figure 1B; GOLDMAN and LICHTEN 1996; SCHLECHT et al. 2004). In S. cerevisiae, Ndj1 is required for bouquet formation and pairing (CONRAD et al. 1997; TRELLES-STICKEN et al. 2000). The negative correlation of ectopic recombination efficiency with SIDT does not depend on Ndj1 (SCHLECHT et al. 2004). Additionally, ectopic recombination efficiencies are only modestly increased in ndj1 mutants (SCHLECHT et al. 2004). In S. cerevisiae, unlike in S. pombe, the bouquet does not play a major role in restricting ectopic recombination. Perhaps in S. cerevisiae the bouquet is not required for alignment, and the synaptonemal complex promotes alignment and restricts ectopic recombination.

Pairing functions and the distribution of meiotic recombination events:

Our data have several important implications. First, we suggest that by promoting homolog pairing, the bouquet and horsetail movement prevent negative interference in S. pombe. Similarly, in S. cerevisiae, Ndj1 and presumably the bouquet contribute to positive interference (CHUA and ROEDER 1997). In both of these highly diverged species, the bouquet affects the distribution of recombination events. Second, the bouquet functions to restrict ectopic recombination in S. pombe. This function is critical for successful completion of meiosis. Ectopic recombination not only results in deleterious chromosomal rearrangements (reviewed in STANKIEWICZ and LUPSKI 2002), but also disturbs meiotic chromosome segregation in S. cerevisiae (JINKS-ROBERTSON et al. 1997). Understanding the mechanism by which the bouquet functions in S. pombe should contribute to our understanding of how chromosome rearrangements are formed in humans.

We are grateful to Yasushi Hiraoka for providing strains and sharing unpublished data; Chad Ellermeier and Greg Freyer for unpublished data; Olaf Nielsen for strains and plasmids; and Sue Amundsen, Gareth Cromie, Joseph Farah, and Alastair S. H. Goldman for helpful comments on the manuscript. This work was supported by National Institutes of Health research grant GM32194 to G.R.S. and postdoctoral fellowship F32-GM20125 to L.D.

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