Whitehead Institute for Biomedical Research, and the Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02142
![]() |
Abstract |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
The Drosophila MEI-S332 protein has been shown to be required for the maintenance of sister-chromatid cohesion in male and female meiosis. The protein localizes to the centromeres during male meiosis when the sister chromatids are attached, and it is no longer detectable after they separate. Drosophila melanogaster male meiosis is atypical in several respects, making it important to define MEI-S332 behavior during female meiosis, which better typifies meiosis in eukaryotes. We find that MEI-S332 localizes to the centromeres of prometaphase I chromosomes in oocytes, remaining there until it is delocalized at anaphase II. By using oocytes we were able to obtain sufficient material to investigate the fate of MEI-S332 after the metaphase II-anaphase II transition. The levels of MEI-S332 protein are unchanged after the completion of meiosis, even when translation is blocked, suggesting that the protein dissociates from the centromeres but is not degraded at the onset of anaphase II. Unexpectedly, MEI-S332 is present during embryogenesis, localizes onto the centromeres of mitotic chromosomes, and is delocalized from anaphase chromosomes. Thus, MEI-S332 associates with the centromeres of both meiotic and mitotic chromosomes and dissociates from them at anaphase.
![]() |
Introduction |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
COHESION between sister chromatids is essential for
proper segregation of chromosomes during mitosis and meiosis. By counteracting spindle forces
pulling chromosomes towards the poles, cohesive forces
between sister chromatids enable stable bipolar attachments to be established; these in turn allow the sister chromatids to be partitioned appropriately during anaphase.
The consequences of inappropriate partitioning can be severe: aneuploidy is observed in many tumors and also in
individuals with congenital disorders such as Down's syndrome. Defects in sister-chromatid cohesion have been
suggested as an important factor that might be involved in
oncogenesis or meiotic errors (Orr-Weaver, 1996; Lamb et
al., 1996
; Lengauer et al., 1997
).
In both meiosis and mitosis, cohesion exists between the
arms and the centromere regions of the sister chromatids
after their replication, but release of sister-chromatid cohesion occurs differently in these two types of cell division
(Moore and Orr-Weaver, 1998). In mitosis, the sister chromatids segregate from one another in a single cell division,
and thus cohesion is released from both the chromosome
arms and centromere regions at the same time, the onset
of anaphase. Meiosis consists of two cell divisions that follow a single round of replication: the homologues segregate from one another in the first division, the sister chromatids in the second division. The homologues are typically
connected at sites on their arms called chiasmata, and sister-chromatid cohesion along the chromosome arms is believed to be important for the maintenance of chiasmata
(Maguire, 1974
, 1993
). With the onset of anaphase I, this
arm cohesion is lost, but cohesion between the centromeric regions of the sister chromatids is maintained. This
cohesion in the centromeric region is required to align the sister chromatids for metaphase II and is released at the
beginning of anaphase II. Thus, meiosis is a specialized
cell division that requires a two-step release of sister-chromatid cohesion.
The Drosophila protein MEI-S332 has been demonstrated both to be essential for cohesion between sister
chromatids and to be localized to chromosomes (Goldstein, 1980; Kerrebrock et al., 1992
, 1995
). These cytological studies were performed in spermatocytes. In male meiosis, MEI-S332 localizes to the centromeric regions of
meiotic chromosomes and is maintained there through the
metaphase I-anaphase I transition (Kerrebrock et al., 1995
).
MEI-S332 is observed on chromosomes in metaphase II
but is no longer detectable with the commencement of
anaphase II, the time when cohesion between sister chromatids is released. The protein is required primarily for
proper segregation during the second meiotic division, because by genetic assays, mei-S332 mutant males and females have nearly normal segregation during the first meiotic division and high levels of missegregation during the
second meiotic division (Davis, 1971
; Goldstein, 1980
; Kerrebrock et al., 1992
). Precociously separated sister chromatids are observed in mei-S332 spermatocytes in late
anaphase I, suggesting that MEI-S332 is vital for centromeric cohesion after the metaphase I-anaphase I transition
(Goldstein, 1980
; Kerrebrock et al., 1992
). Previous studies have not described the localization of MEI-S332 during
female meiosis.
The structure of the meiotic chromatin and the meiotic
spindle differs between the sexes in Drosophila melanogaster (for review see Orr-Weaver, 1995), so it cannot be
assumed that localization of MEI-S332 is the same in both
spermatocytes and oocytes. In females, but not in males,
synaptonemal complex forms during prophase and reciprocal exchange occurs, resulting in the chiasmata that are
assumed to hold homologues together. In males, pairing
sites hold the homologues together without synaptonemal
complex or reciprocal exchange between the homologues
(for review see McKee, 1996
). Another significant difference is that the oocyte metaphase I spindle is thought to
be organized by the chromatin rather than by centrosomes
(Theurkauf and Hawley, 1992
), and this function could require that the meiotic chromosomes have a different structure in females. Finally, oocytes arrest during metaphase I,
whereas spermatocytes normally do not, thus requiring cohesion to be maintained longer. Differences between meiosis in male and female Drosophila could impact MEI-S332
localization. Moreover, the existence of alleles that affect
male and female meiosis with different severity suggests
that there must be some differences in MEI-S332 mechanism between the sexes (Kerrebrock et al., 1992
). Whereas Drosophila male meiosis has several unusual features, Drosophila female meiosis is more typical of meiosis in most
eukaryotes; thus, localization of MEI-S332 in oocytes is of
particular interest.
Sister chromatids are believed to be held together by
proteins until anaphase (for review see Bickel and Orr-Weaver, 1996). The cohesive proteins that hold sister
chromatids together could dissociate or could be degraded
at the time when the chromatids separate. Studies in both
yeast and Xenopus extracts have shown that release of cohesion is dependent on proteolysis of some substrates by
the cyclin degradation machinery, the anaphase promoting
complex (Holloway et al., 1993
; Irniger et al., 1995
; Funabiki et al., 1996
). This complex could directly proteolyze
the cohesive proteins at the chromosomes, or indirectly
promote sister-chromatid separation by degrading inhibitors of anaphase. Recent work in budding yeast demonstrates that the Pds1p protein, which acts as an inhibitor of
separation, is degraded by the anaphase promoting complex at the initiation of anaphase (Cohen-Fix et al., 1996
;
Yamamoto et al., 1996
). A second protein more integrally
involved in cohesion, the Mcd1p/Scc1p protein, has also
been identified (Guacci et al., 1997
; Michaelis et al., 1997
).
Mcd1p localizes to mitotic chromosomes and dissociates at
the metaphase-anaphase transition, but its degradation is
slow, and the protein persists after anaphase. Thus, both
dissociation and degradation may play important roles in
the release of sister-chromatid cohesion. Although the cohesion protein MEI-S332 is not observed on the chromatids after the sister chromatids separate during meiosis II,
it is not known whether the protein simply dissociates or is
degraded.
In this paper, we look at the localization of MEI-S332
during meiosis in females, and we find that, as in males,
the protein disappears from centromeres at anaphase II.
The fate of MEI-S332 at the metaphase II-anaphase II
transition is examined using Western blots, and we find
that MEI-S332 is not degraded detectably at that time. Because the protein is not degraded, we examine its localization during embryonic mitoses. Although centromeric cohesion also occurs in mitosis, mei-S332 is not essential for
mitotic divisions (Kerrebrock et al., 1992, 1995
). Strikingly, we find that the MEI-S332 protein is localized to the
centromeric regions of mitotic chromosomes in the embryo.
![]() |
Materials and Methods |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Fly Strains
In the studies of MEI-S332green fluorescent protein (GFP)1 localization in oocyte meiosis, females of genotype y w P(+mc 5.6KK mei-S332+::
GFP = GrM)-13; P(w+mc 5.6KK mei-S332+::GFP = GrM)-1, containing
four copies of the fusion transgene mei-S332+::GFP (Kerrebrock et al.,
1995
) and two endogenous copies of mei-S332+, were used. (The insertion
of the transgene on the X chromosome is named P(GrM)-13; the insertion
on chromosome 2 is named P(GrM)-1.) For localization of MEI-S332-GFP in embryos, mothers of the genotype described above or mothers
carrying only two copies of the fusion transgene mei-S332+::GFP in the y;
mei-S3327/Df(2R)X58-6 background were used. The latter flies were generated by crossing y w P(GrM)-13; cn mei-S3327 px sp/SM1 females to y w
P(GrM)-13/y+Y; Df(2R)X58-6 pr cn/SM1 males.
In studying the MEI-S332 levels in oocytes before and after activation
(see Fig. 3 C), y w females were used. Embryos and oocytes from y; pr cn
mei-S3327 bw sp/Df(2R)X58-6, pr cn and y; pr cn mei-S3327 bw sp/cn mei-S3327 px sp females were used as negative controls for the anti-MEI-S332 peptide antibodies (Kerrebrock et al., 1992 and see below). Oregon-R (wild type) was used as the negative control for GFP fluorescence microscopy and positive control for Western blot analysis (see Fig. 3 B). For protein extracts from overexpressing oocytes, oocytes were obtained from females carrying six copies of the mei-S332+ gene (two endogenous copies
and four copies from homozygous insertions of P(w+mc 5.6 KK mei-S332+)
on the second and third chromosomes; Kerrebrock et al., 1995
). In all the
mei-S332 transposons, the gene was expressed from the normal genomic
regulatory regions.
|
Meiosis in Activated Eggs
The cytology of activated eggs was performed essentially as described in
Page and Orr-Weaver (1997) with changes in the fixation conditions to
preserve the GFP fluorescence. 300 females of genotype y w P(GrM)-13;
P(GrM)-1 were fattened on wet yeast for several days. Flies were disrupted in IB (55 mM NaOAc, 40 mM KOAc, 110 mM sucrose, 1.2 mM
MgCl2, 1 mM CaCl2, 100 mM Hepes, final pH 7.4) in a blender, and oocytes were isolated by filtration and gravity settling. This isolation step
took 10-11 min. Oocytes were activated by the addition of AB (3.3 mM
NaH2PO4, 16.6 mM KH2PO4, 10 mM NaCl, 50 mM KCl, 5% PEG 8000, 2 mM CaCl2, final pH 6.4) for a 5-min incubation, and then the buffer was
changed to ZAB (9 mM MgCl2, 10 mM MgSO4, 2.9 mM NaH2PO4, 0.22 mM
NaOAc, 5 mM glucose, 27 mM glutamic acid, 33 mM glycine, 2 mM malic
acid, 7 mM CaCl2, final pH 6.8) for an additional incubation of 10 min (for
anaphase I and metaphase II) or 25 min (for anaphase II and the postmeiotic interphase). Eggs with cross-linked vitelline membranes, a hallmark of activation, were selected by a 3-min incubation in 50% Clorox bleach,
and fixed in 8% EM-grade, MeOH-free formaldehyde (Ted Pella Inc., Irvine, CA) in cacodylate buffer (100 mM cacodylic acid, 100 mM sucrose,
40 mM KOAc, 10 mM NaOAc, 10 mM EGTA, pH to 7.2 with KOH;
Theurkauf, 1994
) for 10-15 min, and washed in PBST (PBS with 0.3% Triton X-100) containing ~1% BSA to prevent sticking to glassware. Vitelline membranes were removed by rolling the fixed eggs between two
microscope slides (Theurkauf, 1994
), again using PBST-BSA as a lubricant. Eggs were incubated in 1% RNase A (boiled to destroy DNase activity) for 20 min, and then incubated with 1 µg/ml propidium iodide
(Sigma Chemical Co., St. Louis, MO) for 30 min. Samples were mounted
in Vectashield containing propidium iodide (Vector Labs Inc., Burlingame, CA).
Tubulin Immunofluorescence
Oocytes were prepared using the protocol described by Theurkauf (1994)
for isolation and fixation of egg chambers. Tubulin was labeled using two
anti-tubulin rat monoclonal antibodies, YL1/2 and YOL1/34 (Sera-Lab
Ltd., Sussex, UK), overnight at room temperature at a dilution of 1:5 in
0.1% BSA in PBST, followed by a 3-h incubation with a Texas red-conjugated donkey anti-rat antibody (Jackson Immunoresearch Laboratories
Inc., West Grove, PA) at room temperature at a dilution of 1:200. The oocytes were further stained with 4',6-diamidino-2-phenylindole (DAPI;
Sigma Chemical Co.) at 1 µg/ml in PBS for 10 min, followed by two 15-min rinses in PBS before mounting in 50% glycerol.
MEI-S332-GFP Localization in Embryos
Embryos were collected for 2.5 h from females of the genotype y w P(GrM)-13; P(GrM)-1. The embryo in Fig. 5 was from a 4-h collection from females of the genotype y w P(GrM)-13; cn mei-S3327 px sp/Df(2R)X58-6 pr cn. Oregon-R embryos were used as a control for background autofluorescence.
|
Embryos were dechorionated in 50% bleach, and fixed for 30 min in
8% MeOH-free formaldehyde in cacodylate buffer (see above). After
washing in PBS, embryos were rolled out of their vitelline membranes between two glass slides (Theurkauf, 1994). To stain for DNA, two methods
were used. Embryos in Figs. 4 A, C, and D were treated with 1 mg/ml
RNase A for 30 min, stained with 1 µg/ml propidium iodide for 30 min,
and mounted in Vectashield with propidium iodide (Vector Labs Inc.).
The embryos shown in Figs. 4 B and E, and 5 were stained with DAPI at 1 µg/ml in PBS for 10 min, followed by two 15-min rinses in PBS before
mounting in 50% glycerol.
|
Microscopy
Two kinds of epifluorescence microscopy were used in our investigations. Conventional epifluorescence microscopy was performed using either a Nikon Optiphot-2 microscope or a Nikon Eclipse E800 equipped with a Nikon 60× oil objective (Garden City, NY). A Photometrics CE200A cooled CCD video camera was used to photograph images. The images were further processed with the CELLscan 2.0 system (Scanalytics) to create volume views from focal planes separated by 0.25 µm. 32 focal planes are shown for the oocyte images in Fig. 2, 45 focal planes for the rosette in Fig. 4 B, 20 focal planes for the mitotic interphase nucleus in Fig. 4 E, and 7 focal planes for the images in Fig. 5. Chromatin and MEI-S332-GFP in Figs. 1, A-G, 4 A, C, and D were visualized on a confocal laser scanning head (MRC 600; BioRad, Hercules, CA) equipped with a krypton/argon laser, mounted on a Zeiss Axioskop microscope (Oberkochen, Germany), with 20 and 40× oil Plan Neofluar objectives. In some cases, optical sections were taken and projected into a single plane. All images were further processed, colorized, and merged using Adobe Photoshop 3.0 on a Macintosh Power PC.
|
|
Western Blot Analysis
The rabbit anti-MEI-S332 antibodies (Covance, Research Products Inc.,
Denver, PA) were generated against a COOH-terminal MEI-S332 peptide conjugated to keyhole limpet hemacyanin. This 15-mer peptide (residues 386-400), (C)KNKLRNGSKGKAKAK, was chosen as the antigen because of the availability of the mei-S3327 allele, which lacks the COOH-terminal region of the protein due to a nonsense mutation at residue arg293
(Kerrebrock et al., 1995) and, hence, provides a negative control for the
antibodies. The anti-peptide antibodies were affinity purified from rabbit
serum using GST-MEI-S332 fusion protein bound to immobilon-P strips.
The antibodies were eluted from the strips by acid elution buffer (5 mM
glycine-HCl, pH 2.5, 150 mM NaCl) and immediately neutralized by 1 M
NaPO4 buffer, pH 8. The GST-MEI-S332 fusion protein was generated by
cloning a 1.35-kb BamHI-EcoRI mei-S332 cDNA fragment in frame with
GST in the pGEX-4T-3 expression vector (Pharmacia Biotechnology,
Inc., Piscataway, NJ). The resulting pGEX.MEI plasmid allowed for expression of the full-length MEI-S332 protein, fused to GST at the NH2 terminus, in BL21 (
DE3)pLysS cells.
Embryonic extracts were made by dechorionating Oregon-R embryos
in 50% Clorox bleach and homogenizing in urea sample buffer (USB: 8 M
urea, 2% SDS, 5% -mercaptoethanol, 100 mM Tris, pH 7.6, and 5% Ficoll) at 5:1 USB/embryo (vol/vol). Oocyte extracts were made from mature oocytes isolated as described in Page and Orr-Weaver (1997)
. Females were fattened for 3-5 d with yeast before blender isolation. Oocytes
were homogenized in one urea sample buffer at 3:1 USB/oocyte (vol/vol).
Ovary extracts were made by dissecting previtellogenic, immature ovaries,
or mature ovaries in PBS from newly eclosed females or females that were fattened on yeast for 3 d, respectively, and homogenizing pooled ovaries
in USB (~1 µl buffer/ovary). All protein extracts were cleared by centrifugation, frozen in liquid nitrogen, and stored at
80°C.
For the analysis of MEI-S332 levels in oocytes before and after activation, oocytes were isolated in IB, in either the presence or absence of 100 µg/ml cycloheximide (Fluka), from 300 y w females fattened on wet yeast
for 3 d, as described above. After isolation, half of the oocytes were fixed
by immersion in MeOH (unactivated) and the other half were activated in
AB and ZAB in either the presence or absence of 100 µg/ml cycloheximide, as described above. The total incubation time in AB + ZAB was 60 min. These activated eggs were then fixed by incubation in MeOH. After
several hours of fixation in MeOH at room temperature, oocytes and eggs
were rehydrated in PBS. Rehydrated samples were mixed with 1:1 EB/4 × Laemmli sample buffer (EB: 10 mM Tris 7.5, 80 mM Na -glycerophosphate, pH 7.5, 20 mM EGTA, 15 mM MgCl2, 2 mM Na3VO4, 1 mM benzamidine, 1 mM sodium metabisulfite, 0.2 mM PMSF) by crushing with the
melted tip of a glass pipette. The ratio of sample to buffer added was 1:4
(vol/vol). Samples were boiled for 15 min, cleared by centrifugation, and
frozen in a dry ice/MeOH bath. Control extracts for this experiment were
made by isolating and fixing unactivated oocytes from pr cn mei-S3327 bw
sp/cn mei-S3327 px sp and Oregon-R females as above. A cross-reacting
band on the Western blot, just below the MEI-S332 signal, is also present in the mei-S3327 negative control, and is perhaps an artifact of this sample
preparation.
Protein extracts were separated on 12% 150:1 (acrylamide/bis-acrylamide) gels and blotted onto immobilon-P membranes (Millipore Corp., Waters Chromatography, Milford, MA). About 200 µg of total protein was loaded per lane, and Ponceau S staining was used to verify equivalent protein loading before immunoblotting. Blots were blocked in 5% nonfat dry milk and 2% BSA in TBST (0.01 M Tris, pH 7.5, 0.9% NaCl, and 0.1% Tween 20) for 1 h at room temperature, and then incubated overnight at room temperature with affinity-purified anti-MEI-S332 peptide antibodies diluted at 1:40 in the block solution. Alkaline phosphatase-conjugated anti-rabbit secondary antibodies (Promega Corp., Madison, WI), diluted 1:7,500 in the block solution, were used to detect bound anti-peptide antibodies. The MEI-S332 protein was visualized using the BCIP/ NBT color development substrate (Promega). Although it is predicted to be 44 kD, the MEI-S332 protein migrates as a 55-kD band.
![]() |
Results |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
MEI-S332 Localizes to Centromeric Regions in Oocytes
Although the localization of MEI-S332 has been determined
in spermatocyte meiosis (Kerrebrock et al., 1995), the differences between male and female meiosis in D. melanogaster and the existence of mei-S332 alleles that affect the
two sexes with different severity led us to ask where MEI-S332 is localized in oocyte meiotic divisions. Specifically,
we asked whether it localizes to meiotic centromeres, and
if so, what is the fate of the protein when the sisters separate at anaphase II.
To visualize the MEI-S332 protein in oocytes, we used a
fusion of GFP to the NH2-terminal end of mei-S332 (mei-
S332+::GFP) that has been shown to complement fully the
mutant phenotype in both males and females (Kerrebrock
et al., 1995). In Drosophila, mature oocytes arrest at
metaphase I with a tapered spindle and an elongated nucleus. We examined fixed oocytes stained for DNA and
observed that MEI-S332-GFP was present in two caps at
opposite ends of the oocyte nucleus (Fig. 1 A). The orientation of the caps with respect to the morphology of the
oocyte nucleus suggested that these caps were facing the
poles of the metaphase I spindle, and tubulin staining later
confirmed this interpretation (see below). Because it has
been shown that the centromeric regions of chromosomes
are positioned on opposite sides of the chromatin mass
during the metaphase I arrest in Drosophila oocytes
(Dernburg et al., 1996
), it was likely that caps of MEI-S332-GFP represented centromeric localization.
We wanted to determine what happens to these caps of
MEI-S332 when the meiotic cell cycle resumes after the
oocyte arrest. In particular, we sought to observe the localization of the protein during anaphase I, when centromeric
localization would be most apparent, and observe what
happens to the protein at the metaphase II-anaphase II
transition when the sister chromatids separate. Historically, it has been difficult to observe any of the stages of female meiosis that follow the metaphase I arrest in Drosophila oocytes, but recent advances in egg activation in
vitro now allow all the stages of meiosis to be examined
(Page and Orr-Weaver, 1997). Accordingly, oocytes from
mothers carrying the mei-S332+::GFP transgene were activated in vitro to complete meiosis, and then fixed and
stained for DNA. Oocytes in anaphase I had eight pairs of
sister chromatids, four on each side, as is expected since
the haploid chromosome number in Drosophila is four.
Such oocytes also had eight dots of MEI-S332-GFP visible
at the leading edges of the separating chromosomes, one
per pair of sister chromatids (Fig. 1 B). The observation
that each pair of sister chromatids had MEI-S332 at their
leading edge argued strongly that MEI-S332 is localized at
the centromeric regions of chromosomes in female meiosis. MEI-S332-GFP was continually visible on the chromosomes between anaphase I and metaphase II (Fig. 1, B-E
and see below). When sister-chromatid cohesion was released at anaphase II, the sister chromatids separated, and
for the first time during the meiotic divisions, MEI-S332
was not observed on the chromosomes (Fig. 1 F). After the
meiotic divisions, the chromatin decondensed into four nuclei (three polar bodies and one pronucleus) in the postmeiotic interphase. MEI-S332-GFP was not detectably localized during the postmeiotic interphase (Fig. 1 G).
The cytology of nuclei between the meiotic divisions has
been difficult to observe in oocytes. Indeed, even with the
in vitro activation system, the lack of familiar cytological
landmarks between anaphase I and metaphase II has meant
that it was still unknown what happened to chromosome
morphology between the divisions. Although it is known
that in Drosophila male meiosis the telophase I nuclei decondense and then recondense for meiosis II (Cenci et al.,
1994), it was unclear whether such decondensation occurred in Drosophila females. In experiments activating hundreds
of mei-S332+::GFP transgenic oocytes, we never observed
oocytes with only two decondensed nuclei, in agreement
with our unpublished observations with oocytes from nontransgenic flies. Thus, it appears that Drosophila oocyte nuclei remain condensed throughout meiosis until telophase II.
Because it was clear from the early anaphase I figures that MEI-S332-GFP labels the centromeric regions of oocyte meiotic chromosomes (Fig. 1 B), we were able to use it as a tool in deducing the order of events in chromatin remodeling between anaphase I and metaphase II. We observed that late anaphase I chromosomes appear to become shorter and rounder as they approach the poles, but despite these morphological changes they could always be identified by the leading edge of MEI-S332-GFP at the centromere (Fig. 1 C). Between the divisions, the chromosomes rounded up and formed two clusters of three or four individual balls of chromatin (Fig. 1 D). Each ball was associated with a dot of MEI-S332-GFP, but the dots were no longer oriented at the leading (outside) edge of the chromosomes. We think it likely that each ball represents the sister chromatids of each of the three large chromosomes, with the small fourth chromosome only sometimes visible. Metaphase II was evident when the clusters of chromatin balls compacted to form metaphase plates, usually parallel to each other, with MEI-S332-GFP in the middle of the compacted chromatin (Fig. 1 E). Often, as in Fig. 1 E, the two nuclei were slightly out of synchrony. Even though there is no decondensation between the meiotic divisions, a series of interesting changes occurs in chromosome morphology between anaphase I and metaphase II.
When Does MEI-S332 Localize to Centromeres?
In spermatocytes, MEI-S332 protein is observed in the cytoplasm during prophase I, and it is localized to the chromosomes as they compact for prometaphase I (Kerrebrock et al., 1995). We examined when and how MEI-S332
is localized before metaphase I in oocytes, as there are
marked differences between spermatocytes and oocytes
during prophase I. The origin of the cytoplasm in oocytes
differs from that in spermatocytes, because much of it is
created in the nurse cells, and the volume of cytoplasm is much greater in oocytes than in spermatocytes. Another
important difference is that synaptonemal complex is seen
on oocyte chromosomes, but not on spermatocyte chromosomes. Sex-specific differences in the origin and amount
of cytoplasm or in the structure of the meiotic chromosomes suggested that the timing of MEI-S332 localization should be examined in oocytes to see if it differed from
spermatocytes.
To examine MEI-S332 localization in oocytes during early developmental stages, ovaries were dissected from females carrying the mei-S332+::GFP transgene, fixed, and stained for DNA (data not shown). MEI-S332-GFP was not observed in egg chambers during prophase I, corresponding to oocyte development through stage 12, either in the cytoplasm or on the condensed meiotic chromosomes in the karyosome. Multiple foci of MEI-S332-GFP were first observed on the meiotic chromatin after the chromatin compacted into the small round mass characteristic of prometaphase I. Using egg chamber morphology to judge developmental stage, we determined that these foci first appeared in stage 13. By stage 14, MEI-S332-GFP was observed in two caps on either side of the nucleus (Fig. 1 A and see below).
Because the meiotic spindle is organized shortly after
the chromatin compacts, we further characterized the localization of MEI-S332-GFP with respect to formation of
the spindle by isolating stage 13 and 14 oocytes, and labeling both the DNA and tubulin. After compaction of the
chromatin in stage 12, the nuclear envelope breaks down
and short microtubule fibers captured by the chromatin subsequently coalesce into a bipolar spindle during stage
13 (Theurkauf and Hawley, 1992). The earliest stage at
which MEI-S332-GFP was observable was coincident with
the beginning of spindle formation. A small number of
dots of MEI-S332-GFP were distributed throughout the
chromosomal mass (Fig. 2 A). When spindles appeared
more bipolar and elongated, typical of late stage 13 and
stage 14 oocytes, the MEI-S332-GFP foci were more
clearly combined into caps on the ends of the chromatin
mass that face the spindle poles (Fig. 2, B-C).
The Metaphase II-Anaphase II Transition
In both female and male meioses MEI-S332 was not visible on the sister chromatids after they separated at
anaphase II, consequently we investigated what happened
to the protein when sister-chromatid cohesion was released. In yeast and Xenopus mitosis, an inhibitor of sister-chromatid separation is degraded by the cyclin destruction machinery at the metaphase-anaphase transition (Holloway et al., 1993; Irniger et al., 1995
; Cohen-Fix et al., 1996
).
Because MEI-S332 is essential for sister-chromatid cohesion, it seemed plausible that it might be degraded at the
metaphase II-anaphase II transition.
To study protein levels directly, we generated polyclonal rabbit antibodies against a peptide corresponding to the COOH-terminal fragment of the MEI-S332 protein (Fig. 3 A). Affinity-purified antibodies recognized a band of ~55 kD on a Western blot of ovary and oocyte extracts (Fig. 3 B). This band was absent in extracts made from mei-S3327 oocytes and ovaries (Fig. 3 B, lanes 2 and 3). Extracts from mei-S3327 homozygotes and hemizygotes provided a critical negative control, as this mutation creates a nonsense codon that prematurely truncates the protein so that it lacks the epitope for the COOH-terminal peptide antibodies (Fig. 3 A). As additional evidence that the identified band is MEI-S332, we probed extracts from transgenic ovaries that had four extra copies of a genomic mei-S332+ fragment, in addition to the two endogenous copies, and we found that the band was significantly more intense (Fig. 3 B, lane 1). These data lead us to conclude that the peptide antibodies recognize the MEI-S332 protein as a 55-kD band on Western blots. This protein migrates during electrophoresis as a 55-kD band even though its predicted size is 44 kD.
To determine whether MEI-S332 is degraded at the
metaphase II-anaphase II transition, we analyzed in vitro
activated oocytes. 60 min after activation, eggs can be selected so that 95-99% have completed meiosis (Page and
Orr-Weaver, 1997). We compared MEI-S332 protein levels between extracts of unactivated oocytes, which have
MEI-S332 localized to the chromosomes (Fig. 1 A), and
extracts of eggs that have passed through the metaphase
II-anaphase II transition after activation for 60 min. On
Western blots, these protein levels remained essentially
unchanged (Fig. 3 C, lanes 3 and 4), a result that was repeated several times. This suggests that although the
protein dissociated from the chromosomes at anaphase II,
it was not degraded.
Although the total levels of MEI-S332 remained constant before and after meiosis was completed, we were
concerned that continuing translation of new MEI-S332
protein might mask protein degradation. To address this
concern, we activated oocytes in the presence of the translational inhibitor cycloheximide. Metabolic labeling experiments have demonstrated that oocytes activated in the
presence of cycloheximide have protein synthesis inhibited to about 5% of wild type levels, but that about 95% of
oocytes still complete meiosis under these conditions, arresting at the postmeiotic interphase (Page and Orr-Weaver, 1997). Western blotting of extracts from arrested,
unactivated oocytes incubated in cycloheximide, compared to extracts from oocytes activated in the presence of cycloheximide, further demonstrated that there was no detectable degradation of MEI-S332 during meiosis, suggesting
that it instead delocalized (Fig. 3 C, lanes 3-6).
MEI-S332 during Mitosis
The phenotype of mei-S332 mutants was previously shown
to be exclusively meiotic and not mitotic: no cytological
defect has been detected in proliferating tissues, mutants
are completely viable, and no increase in somatic clones
from mitotic errors is observed (Kerrebrock et al., 1992,
1995
). However, our finding that the protein was not degraded at anaphase II led us to ask whether the protein
persisted in the developing embryo. We examined extracts
from wild type oocytes and embryos by Western blotting, and we found significant amounts of MEI-S332 in a collection of embryos of ages 0-2 h (Fig. 3 B, lane 6). The protein level appeared to increase in populations of embryos
of ages 2-4 h (Fig. 3 B, lane 7), suggesting that MEI-S332
did not merely persist into embryogenesis, but could be
playing a role there. Additionally, we noted that there appeared to be different mobility forms of MEI-S332, an observation that is currently under investigation.
We used the mei-S332+::GFP transgene to determine
whether MEI-S332 could localize onto chromosomes in
the embryo, and we observed persistent localization of the
protein on polar body rosettes (Fig. 4, A and B). Chromosomes from the unused meiotic products are pulled into a
radial formation by a sphere of tubulin, after replicating
and condensing into a metaphase-like state. These are
found in the anterior dorsal quadrant of early embryos,
typically fused so that there exist only one or two rosettes
(Foe et al., 1993). MEI-S332-GFP localized to the condensed chromosomes facing the inside of the rosette,
where centromeres are expected to be located (Foe et al.,
1993
). Moreover, when all the unused meiotic chromosomes have fused into a single rosette formation, the number of chromosomes should be 12, or after replication 24, and we count ~24 foci of MEI-S332-GFP in a typical single rosette formation (Fig. 4 B). As in meiosis, MEI-S332
localized to the apparent centromeric regions of replicated
sister chromatids.
MEI-S332-GFP also localized to condensed chromosomes
in the early mitotic divisions. Drosophila embryos have 13 syncytial nuclear division cycles before gastrulation. On
condensed prometaphase and metaphase chromosomes of
these early cycles we observed MEI-S332-GFP in punctate
dots resembling those on meiotic chromosomes, consistent with centromeric localization (Fig. 4 C). These punctate dots were not observed in interphase nuclei (Fig. 4, D and E).
In addition to chromosome localization, diffuse clouds of
fluorescence were observed in the vicinity of each mitotic
nucleus (Fig. 4 C). Similar diffuse clouds of MEI-S332-
GFP fluorescence were evident near interphase nuclei (Fig.
4, D and E) and produced a signal brighter than the background autofluorescence in embryos lacking the transgene (data not shown). These clouds of fluorescence may correspond to energids, regions of yolk-free cytoplasm that
have been observed in the early cycles of Drosophila embryos (Foe et al., 1993). Immunofluorescence with anti-peptide antibodies confirmed the localization to polar
body chromosomes and condensed mitotic chromosomes (data not shown).
In later syncytial divisions, the nuclei migrate to the surface of the embryo, and mitosis proceeds in a wave across the embryo. We examined mitotic chromosomes in these easily visualized nuclei to analyze localization of MEI-S332 during the metaphase-anaphase transition in mitosis. To simulate the same mei-S332 gene dosage as that of wild type oocytes, embryos from mothers hemizygous for mei- S3327 and carrying two copies of the mei-S332+::GFP transgene were examined after fixation in formaldehyde and DNA staining. MEI-S332-GFP was observed in bright dots aligned on the metaphase plates with the chromatin (Fig. 5 A; see arrow for one example). Sometimes much dimmer dots of MEI-S332-GFP were observed on chromosomes in early anaphase (Fig. 5 B, arrowhead). The residual MEI-S332-GFP was found on the leading edge of chromosomes. By late anaphase and telophase, no MEI-S332-GFP was observed on any of the chromatin. Thus, the metaphase-anaphase transition begins a process of delocalization of MEI-S332. The alignment of the dots on the metaphase plate and the association of residual MEI-S332-GFP with the leading edges of chromosomes strongly suggests that MEI-S332 is localized to the centromeric regions of mitotic chromosomes. Thus, in mitosis as in meiosis, MEI-S332 is localized to the centromeric regions of chromosomes condensed for metaphase, and MEI-S332 begins to dissociate from the chromatin when cohesion is lost and the sister chromatids segregate.
![]() |
Discussion |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
In this study we examined the expression and localization
of MEI-S332 in Drosophila oocytes and embryos. We
found that in oocytes, MEI-S332 localizes to the centromeric region of condensed meiotic chromosomes from
prometaphase I until the metaphase II-anaphase II transition, when sister chromatids separate. This is essentially the same localization pattern as has been observed in spermatocyte meiosis (Kerrebrock et al., 1992). It is striking
that although no mitotic phenotype has been observed in
mei-S332 mutants (Kerrebrock et al., 1995
), MEI-S332
protein has a similar localization pattern in the early mitotic divisions in the embryo, where it appears bound to
condensed chromosomes until the sister chromatids separate at anaphase. On the chromosomes of polar bodies,
which are constitutively condensed in a configuration analogous to metaphase, MEI-S332 is consistently observed at
the expected centromeric regions. Thus MEI-S332 appears
localized to centromeres of metaphase chromosomes in
each of these three different cell cycles, and it is dispersed each time sister chromatids separate.
MEI-S332 and the Metaphase-Anaphase Transition
Precisely what happens to MEI-S332 when sister chromatids separate at anaphase is a question of great interest. One possibility is that the protein is degraded at the metaphase-anaphase transition. To test this idea, we examined the levels of MEI-S332 in oocytes before and after the completion of meiosis. We found that even in the presence of cycloheximide to prevent new protein synthesis, the levels of MEI-S332 appeared unchanged before and after the metaphase II-anaphase II transition. This result demonstrates that on a global level MEI-S332 is not degraded at anaphase II. Although we have not directly examined the question of degradation in mitosis, the observation that MEI-S332 protein is visible in clouds around interphase nuclei strongly supports the idea that it is not degraded on a global level in the developing embryo during the syncytial divisions. Still, we cannot exclude the possibility that centromere-localized protein is locally degraded at either the metaphase II-anaphase II transition in oocytes or at the mitotic metaphase-anaphase transition. If a subpopulation of MEI-S332 was degraded at anaphase II, however, the amount degraded would have to be insignificant compared to the persisting fraction, as we do not observe any decrease in protein levels by Western blotting.
A second possibility is that dissociation of MEI-S332
from the centromeric regions triggers sister-chromatid
separation. An analogous mechanism may occur in the
yeast S. cerevisiae, because the Mcd1p/Scc1p cohesion protein localized on the chromosomes is not degraded until
after anaphase. Instead it is removed from the chromosomes beginning at anaphase (Guacci et al., 1997; Michaelis et al., 1997
). Noting that MEI-S332 appears to run as a
doublet on Western blots, we speculate that dissociation of
MEI-S332 may be regulated at some level by phosphorylation. Consistent with this speculation, the MEI-S332 protein has 30 possible phosphorylation sites recognized by
protein kinase C, casein kinase II, cAMP-dependent protein kinase, and tyrosine protein kinase.
There is a third possibility, however, that MEI-S332 may
first be inactivated to permit anaphase movement and subsequently dissociate from the chromosomes. This model is
supported by our detection of MEI-S332 on the centromeres of chromosomes in early anaphase, although the
levels are reduced compared to metaphase. Similarly,
some Mcd1p/Scc1p remains localized to the chromosomes in anaphase (Guacci et al., 1997; Michaelis et al., 1997
).
We cannot distinguish between these two latter models at
this point, because it is possible that sufficient amounts of
MEI-S332 or Mcd1p/Scc1p dissociate at the metaphase-
anaphase transition to permit sister-chromatid separation.
Residual levels may then be removed subsequently.
Establishment Versus Maintenance of Sister-Chromatid Cohesion
In spermatocytes, oocytes, and early embryos, MEI-S332
is not detectable on the chromosomes until prometaphase.
It is possible that sister-chromatid cohesion is not fully established until this point and that the localization of MEI-S332 marks the establishment of cohesion. It may be the
case, however, that cohesion is established immediately after DNA replication. In FISH studies done in yeast, separate signals from the two sister chromatids were not observed until anaphase, indicating that sister chromatids are
tightly associated from the time of their replication (Guacci
et al., 1993, 1994
). This suggests that cohesion is established
during S phase. If this is true, then MEI-S332 may be required to maintain or augment cohesion when spindle forces
come into play, rather than to establish cohesion. For example, it may serve to protect and preserve proteins directly
attaching the sister chromatids until anaphase.
A Mitotic Role for MEI-S332?
We were surprised to find that MEI-S332 localizes to mitotic chromosomes in much the same way it localizes to
meiotic chromosomes in spermatocytes and oocytes because no function has been ascribed to MEI-S332 in mitosis. The presence of MEI-S332 on mitotic chromosomes is
not unique to the early embryonic cycles. MEI-S332 protein is present in dividing larval tissues and can localize to
the chromosomes during mitosis (LeBlanc, H., T.T. Tang,
and T.L. Orr-Weaver, unpublished results). We and our
colleagues have undertaken careful phenotypic analyses of
mei-S332 mutants in order to determine whether the protein is required for mitosis. Viability studies have demonstrated that mei-S332 homozygotes and their heterozygous siblings survive equally (Kerrebrock et al., 1992), even
when the maternal mei-S332 contribution is eliminated
(LeBlanc, H., and T.L. Orr-Weaver, unpublished data).
Examinations of large numbers of larval brains, a mitotically active tissue that when squashed flat gives excellent
mitotic cytology, demonstrated no significant difference in
mitotic index or premature sister-chromatid separation
between mei-S332 hemizygous (mei-S332/Df) and wild type larval brains (Kerrebrock et al., 1995
). Furthermore,
experiments testing the frequency of chromosome missegregation in the developing wing demonstrated no significant difference between mei-S332 hemizygotes and their
heterozygous siblings (Kerrebrock et al., 1995
).
If MEI-S332 is localized to mitotic centromeres, why do
we not see a phenotype in mei-S332 mutants? One possibility is that in mitosis there is redundancy in the mechanisms that hold sister chromatids together. The simplest
model for redundancy is that both MEI-S332 and another
protein act independently to bind sister chromatids together at the centromeric regions in mitosis, and therefore
no phenotype is observed when mei-S332 is mutated. Currently there are no candidates for such a protein. Although
mutations have been characterized in three genes that encode Drosophila centromere-binding proteins, none appear to promote sister-chromatid cohesion. The HP1 and
PROD proteins affect centromere condensation and presumably kinetochore function (Kellum and Alberts, 1995; Torok et al., 1997
), whereas ZW10 may monitor spindle
attachment to the kinetochore (Williams et al., 1996
). Another version of this redundancy model is that whereas
MEI-S332 acts at mitotic centromeres to attach sister
chromatids, other proteins act along the lengths of the
chromatid arms to ensure cohesion and proper orientation
with respect to the mitotic spindle. The loss of MEI-S332 would result in the loss of centromeric cohesion, but this
would not have phenotypic consequences in mitosis because arm cohesion would be sufficient to hold the chromatids together. This redundancy is not provided solely by
ORD, a Drosophila protein required for arm cohesion in
meiosis, because flies lacking both mei-S332 and ord have
demonstrated no abnormalities in somatic mitoses (Bickel, S.E., D.P. Moore, C. Lai, and T.L. Orr-Weaver, manuscript submitted for publication).
Alternatively, it is possible that MEI-S332 does play a nonredundant role in mitosis, but it is required only in response to perturbations of the cell cycle. For example, if it were necessary for a cell to delay the onset of anaphase, persistence of MEI-S332 at the centromeric regions could, in principle, restrain the sister chromatids from separating. The discovery of a mitotic phenotype, under any conditions, would greatly enhance our understanding of the mitotic function of MEI-S332.
Meiotic Cytology
Because MEI-S332 localizes to centromeres throughout
meiosis until anaphase II, we were able to use it as a tool
to examine meiotic chromosome morphology. In metaphase
I arrested oocytes, the two caps of MEI-S332-GFP demonstrate that the centromeric regions of homologues are
closest to the spindle poles during metaphase I, as would
be anticipated if homologues are connected by chiasmata
on the chromosome arms. Again using MEI-S332 to identify centromeres and chromosome orientation, we were
able to infer an order of events after anaphase I. We found
that in Drosophila, as in Xenopus and other organisms,
oocyte chromosomes do not decondense between the two
meiotic divisions (Murray and Hunt, 1993), in contrast to
spermatocyte chromosomes that do decondense between the divisions (Cenci et al., 1994
).
Conclusions
Our finding that MEI-S332 is present on both meiotic and mitotic chromosomes reinforces the idea that meiosis and mitosis are highly conserved processes, even at the molecular level. In both types of divisions, it is localized to the centromeric regions of sister chromatids aligned on a bipolar spindle, and it is no longer present on the sister chromatids when they segregate from one another in anaphase. The function of MEI-S332 is essential during meiosis and not mitosis probably because of the meiosis-specific requirement that sister chromatids remain attached in the centromeric region during the first meiotic cell division. It is ironic that MEI-S332 is now implicated in mitosis, because if it had a strong mitotic phenotype, lethality would have hindered the genetic and cytological analyses that defined its role in sister-chromatid cohesion. Our findings indicate that the analysis of meiosis will lead to a deeper understanding of chromosome segregation mechanisms in general.
![]() |
Footnotes |
---|
Received for publication 31 October 1997 and in revised form 5 January 1998.
A.W. Page and T.T. Tang were supported by predoctoral fellowships from the National Science Foundation. This research was funded by a grant from the National Science Foundation (MCB-9604135).We thank Sharon Bickel for advice on DNA stains and antibody affinity purification, Lisa Elfring for help with Western blots, and Ya-Huei Tu for assistance with microscopy (all from Whitehead Institute for Biomedical Research, Cambridge, MA). We are grateful to Abby Dernburg (Stanford University, Palo Alto, CA), Doug Koshland (Carnegie Institute of Washington, Baltimore, MD), and Kim Nasymth (Institute for Molecular Pathology, Vienna, Austria) for communicating results before publication, and to Sharon Bickel and Heidi LeBlanc (Whitehead) for permission to cite unpublished results. Angelika Amon (Whitehead), Dean Dawson (Tufts University, Boston, MA), Lisa Elfring, Heidi LeBlanc, and Jacqueline Lopez (Whitehead) provided critical comments on the manuscript. We thank an anonymous reviewer for insightful comments and suggestions.
![]() |
References |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
1. | Bickel, S.E., and T.L. Orr-Weaver. 1996. Holding chromatids together to ensure they go their separate ways. Bioessays. 18: 293-300 |
2. |
Cenci, G.,
S. Bonaccorsi,
C. Pisano,
F. Verni, and
M. Gatti.
1994.
Chromatin and microtubule organization during premeiotic, meiotic, and early postmeiotic stages of Drosophila melanogaster spermatogenesis.
J. Cell Sci.
107:
3521-3534
|
3. | Cohen-Fix, O., J.-M. Peters, M.W. Kirschner, and D. Koshland. 1996. Anaphase initiation in Saccharomyces cerevisiae is controlled by the APC-dependent degradation of the anaphase inhibitor Pds1p. Genes and Dev. 10: 3081-3093 [Abstract]. |
4. | Davis, B.. 1971. Genetic analysis of a meiotic mutant resulting in precocious sister-centromere separation in Drosophila melanogaster. Mol. Gen. Genet. 113: 251-272 |
5. | Dernburg, A.F., J.W. Sedat, and R.S. Hawley. 1996. Direct evidence of a role for heterochromatin in meiotic chromosome segregation. Cell. 86: 135-146 |
6. | Foe, V.E., G.M. Odell, and B.A. Edgar. 1993. Mitosis and morphogenesis in the Drosophila embryo: point and counterpoint. In The development of Drosophila melanogaster. M. Bate and A. Martinez Arias, editors. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY. 149-300. |
7. | Funabiki, H., H. Yamano, K. Kumada, K. Nagao, T. Hunt, and M. Yanagida. 1996. Cut2 proteolysis required for sister-chromatid separation in fission yeast. Nature. 381: 438-441 |
8. | Goldstein, L.S.B.. 1980. Mechanisms of chromosome orientation revealed by two meiotic mutants in Drosophila melanogaster. Chromosoma (Berl.). 78: 79-111 |
9. | Guacci, V., A. Yamamoto, A. Strunnikov, J. Kingsbury, E. Hogan, P. Meluh, and D. Koshland. 1993. Structure and function of chromosomes in mitosis of budding yeast. Cold Spring Harbor Symp. Quant. Biol. 58: 677-685 |
10. | Guacci, V., E. Hogan, and D. Koshland. 1994. Chromosome condensation and sister chromatid pairing in budding yeast. J. Cell Biol. 125: 517-530 [Abstract]. |
11. | Guacci, V., D. Koshland, and A. Strunnikov. 1997. A direct link between sister chromatid cohesion and chromosome condensation revealed through the analysis of MCD1 in S. cerevisiae. Cell. 91: 47-57 |
12. | Holloway, S.L., M. Glotzer, R.W. King, and A.W. Murray. 1993. Anaphase is initiated by proteolysis rather than by the inactivation of maturation-promoting factor. Cell. 73: 1393-1402 |
13. | Irniger, S., S. Piatti, C. Michaelis, and K. Nasmyth. 1995. Genes involved in sister chromatid separation are needed for B-type cyclin proteolysis in budding yeast. Cell. 81: 269-277 |
14. |
Kellum, R., and
B.M. Alberts.
1995.
Heterochromatin protein 1 is required for
correct chromosome segregation in Drosophila embryos.
J. Cell Sci.
108:
1419-1431
|
15. |
Kerrebrock, A.W.,
W.Y. Miyazaki,
D. Birnby, and
T.L. Orr-Weaver.
1992.
The Drosophila mei-S332 gene promotes sister-chromatid cohesion in meiosis
following kinetochore differentiation.
Genetics.
130:
827-841
|
16. | Kerrebrock, A.W., D.P. Moore, J.S. Wu, and T.L. Orr-Weaver. 1995. MEI-S332, a Drosophila protein required for sister-chromatid cohesion, can localize to meiotic centromere regions. Cell. 83: 247-256 |
17. | Lamb, N., S.B. Freeman, A. Savage-Austin, D. Pettay, L. Taft, J. Hersey, Y. Gu, J. Shen, D. Saker, K.M. May, et al . 1996. Susceptible chiasmate configurations of chromosome 21 predispose to non-disjunction in both maternal meiosis I and meiosis II. Nat. Genet. 14: 400-405 |
18. | Lengauer, C., K.W. Kinzler, and B. Vogelstein. 1997. Genetic instability in colorectal cancers. Nature. 386: 623-627 |
19. | Maguire, M.P.. 1974. The need for a chiasma binder. J. Theor. Biol. 48: 485-487 |
20. | Maguire, M. P.. 1993. Sister chromatid association at meiosis. Maydica. 38: 93-106 . |
21. | McKee, B.D.. 1996. The license to pair: identification of meiotic pairing sites in Drosophila. Chromosoma. 105: 135-141 |
22. | Michaelis, C., R. Ciosk, and K. Nasmyth. 1997. Condensins and cohesins: proteins that hold sister chromatids together. Cell. 91: 35-45 |
23. | Moore, D.P., and T.L. Orr-Weaver. 1998. Chromosome segregation during meiosis: building an unambivalent bivalent. In Meiosis and Gametogenesis. M.A. Handel, editor. Academic Press, San Diego, CA. 263-299. |
24. | Murray, A., and T. Hunt. 1993. The Cell Cycle: An Introduction. Freeman, New York. 251 pp. |
25. | Orr-Weaver, T.L.. 1995. Meiosis in Drosophila: seeing is believing. Proc. Natl. Acad. Sci. USA. 92: 10443-10449 [Abstract]. |
26. | Orr-Weaver, T.L.. 1996. Meiotic nondisjunction does the two-step. Nat. Genet. 14: 374-376 |
27. | Page, A.W., and T.L. Orr-Weaver. 1997. Activation of the meiotic divisions in Drosophila oocytes. Dev. Biol. 183: 195-207 |
28. | Theurkauf, W.E. 1994. Immunofluorescence analysis of the cytoskeleton during oogenesis and early embryogenesis. In Methods in Cell Biology. Vol 44. L.S.B. Goldstein, and E.A. Fyrberg, editors. Academic Press, New York. 489-505. |
29. | Theurkauf, W.E., and R.S. Hawley. 1992. Meiotic spindle assembly in Drosophila females: Behavior of nonexchange chromosomes and the effects of mutations in the nod kinesin-like protein. J. Cell Biol. 116: 1167-1180 [Abstract]. |
30. | Torok, T., P.D. Harvie, M. Buratovich, and P.J. Bryant. 1997. The product of proliferation disrupter is concentrated at centromeres and required for mitotic chromosome condensation and cell proliferation in Drosophila. Genes and Dev. 11: 213-225 [Abstract]. |
31. | Williams, B.C., M. Gatti, and M.L. Goldberg. 1996. Bipolar spindle attachments affect redistribution of ZW10, a Drosophila centromere/kinetochore component required for accurate chromosome segregation. J. Cell Biol. 134: 1127-1140 [Abstract]. |
32. | Yamamoto, A., V. Guacci, and D. Koshland. 1996. Pds1p is required for faithful execution of anaphase in the yeast, Saccharomyces cerevisiae. J. Cell Biol. 133: 85-97 [Abstract]. |
33. | Yamamoto, A., V. Guacci, and D. Koshland. 1996. Pds1p, an inhibitor of anaphase in budding yeast, plays a critical role in the APC and checkpoint pathway(s). J. Cell Biol. 133: 99-110 [Abstract]. |