Department of Biology, University of North Carolina, Chapel Hill, North Carolina 27599-3280
Activation of a facultative, dicentric chromosome provides a unique opportunity to introduce a double strand DNA break into a chromosome at mitosis. Time lapse video enhanced-differential interference contrast analysis of the cellular response upon dicentric activation reveals that the majority of cells initiates anaphase B, characterized by pole-pole separation, and pauses in mid-anaphase for 30-120 min with spindles spanning the neck of the bud before completing spindle elongation and cytokinesis. The length of the spindle at the delay point (3-4 µm) is not dependent on the physical distance between the two centromeres, indicating that the arrest represents surveillance of a dicentric induced aberration. No mid-anaphase delay is observed in the absence of the RAD9 checkpoint gene, which prevents cell cycle progression in the presence of damaged DNA. These observations reveal RAD9- dependent events well past the G2/M boundary and have considerable implications in understanding how chromosome integrity and the position and state of the mitotic spindle are monitored before cytokinesis.
Budding yeast has been one of the key genetic systems in defining the progression of cell cycle
events. One of the major paradigms is the accumulation and destruction of cyclin-cyclin-dependent kinase
complexes (Nasmyth, 1993 Relatively little information addresses cell cycle regulation and checkpoint pathways that may be critical for coordinating spindle position and disassembly with cytokinesis.
Our recent results from high-resolution video enhanced-
(VE)1 and digital enhanced- (DE) differential interference
contrast (DIC) microscopy of living cells reveal discrete kinetic and morphological transitions during anaphase progression (Yeh et al., 1995 Studies in populations of budding yeast, after activation
of a facultative, dicentric chromosome are also indicative
of a mid-anaphase cell cycle checkpoint which can delay
progression through mitosis (Neff and Burke, 1992 In the present study, we have used video enhanced and
digital enhanced-DIC microscopy to determine the kinetics of spindle elongation in individual cells harboring an
active dicentric chromosome. Having established a framework of morphological landmarks for anaphase spindle
progression in wild-type cells (Yeh et al., 1995 Media
Yeast rich medium, YPGal and YPD, contained 2% galactose and glucose, respectively, 2% peptone, and 1% yeast extract. Yeast minimal media (SD-URA) contained 0.67% yeast nitrogen base, 2% glucose or galactose supplemented with 0.5% casamino acids, and adenine (16.5 µg/ml).
Strains and Plasmids
All strains used in this study are isogenic derivatives of J178-1D (Mat a ade1
met14 ura3-52 leu2-3,112 his3). The 45-kb dicentric chromosome III strain
J178#24 (his4 Immunofluorescence
Immunofluorescent staining of yeast cells was performed essentially as described by Pringle et al. (1989) To visualize the nucleus, cells were fixed in 3.7% formaldehyde for 1 h
at 25°C. Fixed cells were washed once with water and resuspended in 1 µg/
ml DAPI for 5 min. The cells were washed once with water and mounted
in mounting medium.
Fluorescent In Situ Hybridization
J178#24 was grown to an A660 = 0.2 density in galactose-containing medium before switching to YPD for 1 h. Cells were fixed and stained with
DAPI (1 µg/ml for 5 min) or subjected to fluorescent in situ hybridization
(FISH) as described by Guacci et al. (1994) Real Time Analysis of Activated
Dicentric Chromosomes
Cultures were grown to early logarithmic growth phase and spotted directly from galactose medium to YPD/25% gelatin slabs. Cells were
filmed using high resolution VE-DIC and DE-DIC microscopy and analyzed as described in Yeh et al. (1995) The probability of double strand breakage in a dicentric
chromosome is influenced by the behavior of each of the
paired centromeres relative to the spindle poles. If the two
centromeres on one sister chromatid are oriented to opposite poles, a dicentric bridge is formed, followed by breakage, or chromosome loss. Conversely, if both centromeres
from one sister are attached to the same pole, the chromosome will separate without engendering a break. If each centromere behaves independently, we expect to observe
two populations of cells. Half of the cells will generate a
broken chromosome, and half of the cells may propagate
intact, dicentric molecules during cell division (Fig. 1;
Koshland et al., 1987
Real Time Analysis of Cells Harboring an Active
Dicentric Chromosome
VE-DIC microscopy of individual cells allowed us to visualize distinct cellular responses upon dicentric chromosome activation (Fig. 2). Cells containing the facultative
dicentric chromosome were grown to mid-logarithmic phase
in galactose (monocentric conditions) and switched to glucose (dicentric conditions) for VE-DIC analysis. Two distinct mitotic populations of cells were observed (Figs. 3
and 4) and confirm the expectations predicted from the independent behavior of the two centromeres. One population, 7/29 cells (Fig. 3), mimicked wild-type cells in their
kinetic progression through the cell cycle. The initial rapid
elongation was completed in 7 ± 2 min, the transition from
the sausage shape to bi-lobed nuclear morphology took
9 ± 2 min, and cytokinesis followed 35 ± 5 min later (Yeh
et al., 1995
Aberrant nuclear morphology and a considerable delay
between the fast and slow phases of anaphase were observed in 22/29 of the mitotic cells (Figs. 2 and 4). During
the initial phases of spindle elongation, a finger-like protrusion of the nucleus into the bud was seen, rather than
the typical formation of a sausage-shaped nucleus. This
protrusion seemingly snaked its way into the bud for ~5 ± 1 min (Fig. 4 A). As the spindle elongated to ~4 µm in length, the nucleus remained rounded in shape as it traversed the neck of the dividing cell (Fig. 2 C). The time
from nuclear protrusion to the formation of this rounded
sausage nucleus took 10 ± 6 min (Fig. 4 A). Interestingly,
the nucleus continued to maintain this round to sausageshaped morphology for 47 ± 18 min before further spindle
elongation and the transition to bi-lobed structures. This is
significantly longer than the 9 ± 2 min transition in wildtype cells, indicating a significant delay in both the kinetics
and morphological transitions that accompany anaphase B. Once the bulk of the nucleus formed a bi-lobed morphology and began the slow phase of spindle elongation,
the time to cytokinesis was 38 ± 10 min, similar to that observed in wild-type cells.
Coincidence of Nuclear and Spindle Position at the
Mid-anaphase Delay
Bending of the mitotic spindle in and out of the plane of
focus often precludes direct visualization of the spindle by
VE-DIC microscopy. To confirm that position of the nucleus during mid-anaphase corresponds to actual spindle
elongation through the neck, we compared the length of
the nucleus in fixed cells, as determined by DAPI staining,
to the length of the mitotic spindle, as visualized by indirect immunofluorescence. Cells containing the conditional dicentric chromosome were grown on galactose-containing medium and switched to glucose-containing medium
for 2 h to activate the dicentric chromosome. Cells were
fixed and stained for nuclear (DAPI) and spindle (anti-
Kinetic Analysis of Spindle Elongation
The kinetics of spindle elongation were determined using
a semi-automated tracking system to quantitate spindle
morphogenesis and elongation (Skibbens et al., 1993 Sister Chromatid Separation at the
Mid-anaphase Transition
The partially elongated spindles indicate a delay in anaphase B spindle pole separation. However, the degree of
chromosome separation was not apparent in the VE-DIC
images. We therefore used FISH to visualize sister chromatids in cells arrested in mid-anaphase. Asynchronous
populations of cells containing the conditional dicentric
chromosome were grown on galactose and switched to
glucose for 1-2 h, when ~16% of the cells were arrested as large budded cells with DNA spanning the neck (Table I).
Table I.
Quantification of Nuclear Morphology by DAPI
; Murray, 1995
a). By delaying
or advancing the timing of cyclin-cyclin-dependent kinase
activity, the cell is able to coordinate steps in cell cycle
progression, as well as respond to environmentally induced damage before downstream events. Cells can delay
the onset of DNA synthesis (S phase) or mitosis (M phase)
after exposure to x-rays,
irradiation, or ultraviolet light
(Hartwell and Weinert, 1989
; Weinert and Lydall, 1993
;
Murray, 1995
b). DNA lesions are recognized by proteins
engaged either in DNA processing (Rad9, 24, 17, and
Mec3) or signalling (Mec1 and Mec2/Rad53) (Siede et al.,
1993
; Allen et al., 1994
; Weinert et al., 1994
; Lydall and
Weinert, 1995
). Aberrant spindle assembly and alterations
in kinetochore structure and function are also subject to
surveillance mechanisms that act to delay anaphase onset
(Hoyt et al., 1991
; Li and Murray, 1991
; Spencer and Hieter, 1992
; Gorbsky and Ricketts, 1993
; Li and Nicklas, 1995
; Wang and Burke, 1995
). These lesions are monitored, at least in budding yeast, by the MAD1, 2, and 3 and
BUB1, 2, and 3 genes (Hoyt et al., 1991
; Li and Murray,
1991
; for review see Wells, 1996
).
). Most notable are the sequential
fast and slow phases of spindle elongation and the morphological transition from a sausage shape to a bi-lobed nucleus that accompany these rate changes. At anaphase onset, the 1.5-2 µm spindle spanning the preanaphase
nucleus elongates rapidly through the neck of the budded
cell (1.0 µm/min) until the spindle and nucleus achieve a
length of ~3-4 µm in a haploid cell. The rate of spindle
elongation decreases (0.3 µm/min), and the nucleus converts from a sausage-shaped structure to a bi-lobed configuration and elongates until the maximal length of 10-12 µm is reached. Similar rates and evidence for biphasic
spindle elongation have been obtained from observations
of spindle pole body movement in living cells, as well (Kahana et al., 1995
). Chromatin separation, as seen by staining with DAPI, appears to be completed in the bi-lobed
nucleus. Differential regulation of microtubule dynamics
and nuclear and cytoplasmic motor proteins are likely to
be involved in the regulation and translocation of the spindle during anaphase. Indeed, spindle elongation is confined primarily to the mother in cells lacking the microtubule-based motor protein dynein (DHC1), and spindle
disassembly and cytokinesis are delayed until the nucleus
traverses the neck of the budded cell (Eshel et al., 1993
; Li
et al., 1993
; Yeh et al., 1995
). The spatial consequence of
division by budding is that the plane of cleavage is established well before bi-polar spindle formation. This configuration requires spindle migration through the neck before successful cell division, and the dynein mutants reflect the cellular capacity to monitor spindle and/or nuclear position.
; Brock
and Bloom, 1994
). These dicentric chromosomes contain
two centromeres, one of which is conditionally regulated
by the GAL1 transcriptional promoter (Brock and Bloom,
1994
). Transcription is repressed on glucose, and the centromere is completely functional. Growth on galactose activates the promoter, which in turn, inactivates the centromere. The conditional dicentric chromosome is stably
maintained in a monocentric state by growth on galactose
and becomes dicentric on glucose. Cells harboring an active, dicentric chromosome are delayed in their cell cycle
transit. A third to one half of the cells in a population are
large budded, with nuclear DNA spanning the neck and a
short spindle bisecting the nucleus, after the switch to glucose as the sole carbon source for growth (Neff and Burke,
1992
; Brock and Bloom, 1994
). p34cdc28 kinase activity is
elevated in cells containing an active dicentric chromosome, compared to cells with monocentric chromosomes
grown on glucose for comparable times (Neff and Burke,
1992
; Brock and Bloom, 1994
). The inference from these
studies was that the delay preceded the decline of p34cdc28
kinase activity, and the cells were arrested prior to the exit from mitosis.
), we have
quantitated the kinetics of anaphase, spindle morphology, and spindle length, in individual cells containing active dicentric chromosomes from anaphase to cytokinesis. These
studies clearly demonstrate a mid-anaphase delay which is
dependent upon the RAD9 checkpoint gene. RAD9 has
been shown previously to prevent cell cycle progression in
the presence of DNA damage prior to anaphase onset
(Weinert and Hartwell, 1988
). Our results are indicative of
a regulated progression from early anaphase to late
anaphase during the later stages of mitosis.
Materials and Methods
::URA3 GALCEN3) was constructed by fragment-mediated transformation of the conditional centromere at the HIS4 locus (Hill
and Bloom, 1989
). The rad9
dicentric strain was constructed by fragment-mediated transformation into J178#7 (his4
::URA3 GALCEN3::
his4), as previously described by Brock and Bloom (1994)
. The 3-kb dicentric plasmid yC2 (Hill and Bloom, 1987
) was introduced into J178-1D
by standard transformation. All dicentric strains were grown in galactosecontaining medium to maintain chromosome III or the plasmid yC2 as
monocentric.
. Cells were grown to early to mid-logarithmic
phase growth in galactose-containing medium. Cells were pelleted, washed
once with sterile water, resuspended in glucose-containing medium, and
returned to 32°C for 1-2 h. Cells were fixed in 3.7% formaldehyde for 2 h
at 25°C before processing for immunofluorescence. Microtubules were visualized with the rat anti-
-tubulin antibody YOL1/34 (Accurate Chemical and Scientific Corp., Westbury, NY). Rhodamine-conjugated goat anti-
rat (Cappel Labs, Malvern, PA) was used as the secondary antibody. Cells
were incubated with DAPI (1 µg/ml) for 5 min before the addition of mounting medium. Images were acquired and stored for further analysis, as described for FISH. Fluorescent digital images were analyzed with distance measuring tools within Metamorph software (Salmon et al., 1994
).
. Images were visualized with a
microscope (Microphot FXA; Nikon) using a 60X/1.4NA PlanApo objective. Metamorph software (Universal Imaging Corp., West Chester, PA)
was used to control a Metaltek filter wheel (Salmon et al., 1994
). A shuttered mercury lamp was used for fluorescence excitation (490 nm). Images
were collected with a cooled CCD camera (C4880; Hamamatsu) and
stored on an optical drive (Pinnacle Micro, Irvine, CA). 100-200 nuclei
were counted.
.
Results
). The timing of decatenation of sister
chromatids will also affect the behavior of the dicentric
chromosome. This potential for different chromosome configurations on the spindle and hence, chromosome
breakage or maintenance, has limited previous studies on
populations of cells.
Fig. 1.
Dicentric chromosome breakage resulting from centromere movements during prometaphase or anaphase. A schematic diagram representing possible centromere attachments of
a dicentric chromosome to the mitotic spindle during prometaphase and anaphase. During prometaphase, the two centromeres
will independently form bipolar attachments to the mitotic spindle. A dicentric chromosome in which the two centromeres have
formed initial monopolar attachments to opposite spindle poles is
shown in the top figure. Centromere movements toward opposite
spindle poles, as indicated by the arrows, may result in chromosome breakage. During anaphase B, when the two centromeres
of a dicentric chromosome have successfully formed bipolar attachments, centromere movements at anaphase may result in
chromosome breakage. If the two centromeres of each chromosome are oriented toward the same spindle pole (top), chromosome segregation is normal. If the centromeres are oriented toward opposite spindle poles (bottom), anaphase bridges are
formed, and chromosome breakage can occur (Brock and Bloom,
1994).
[View Larger Version of this Image (25K GIF file)]
).
Fig. 2.
High resolution DE-DIC images of mitosis upon dicentric chromosome activation. A pair of arrows on each frame demarcates
the nucleus. The time of each frame is indicated in the upper right corner. Bottom cell: (A) Pre-anaphase B/metaphase spindle (1.62 µm) with the nucleus positioned at the neck; (B) spindle elongation into the bud (2.99 µm); (C-F) the nucleus persists in the neck at a
length ranging from 2.57-3.45 µm for 38 min; (G) spindle elongation ensues (5.76 µm spindle); (H-K) the nucleus continues to elongate
to the distal ends (7.85 µm) and septum formation occurs (J and K); (L) cytokinesis and new bud formation. Top cell: (I) Spindle elongation; (J-K) nucleus in the neck. (L) The appearance of septum formation through the nucleus.
[View Larger Version of this Image (163K GIF file)]
Fig. 3.
No mid-anaphase pause. (A) Kinetic analysis of
changes in nuclear morphology and spindle dynamics in dicentric
cells displaying wild-type kinetics. The time between spindle
elongation and cytokinesis, seen as cell separation, was determined from the time lapse videos. 7 out of 29 cells filmed displayed these kinetics. (B) Spindle movements relative to the bud
neck. The distance (µm) between the neck and the leading and
lagging edge of the nuclear envelope was measured and plotted
as a function of time (min). A schematic representation of the nuclear morphology and position at the different stages is shown
above the plot. The neck is designated as 0 µm. The length from
the leading edge to the neck (proximal to bud, diamonds) is designated with negative numbers. The length from the lagging edge
to the neck (proximal to mother, squares) is designated with positive numbers. Preanaphase spindle is at T = 0.
[View Larger Version of this Image (19K GIF file)]
Fig. 4.
Mid-anaphase pause. (A) Kinetic analysis of changes in
nuclear morphology and spindle dynamics in dicentric cells displaying mitotic delay. 22 out of 29 cells displayed these kinetics.
(B) Spindle movements relative to the bud neck were determined
as described in the legend to Fig. 3.
[View Larger Version of this Image (24K GIF file)]
tubulin immunofluorescence) analysis. In all budded cells
with DNA spanning the neck (36/36), the mitotic spindle
had elongated through the neck (compare Fig. 5, C and D;
E and F). Quantitation of the length of tubulin immunofluorescence and of DAPI staining along the mother bud
axis in G2 and mid-anaphase arrested cells shows an excellent correlation between the two measurements. In G2
cells (medium size bud, nucleus near the neck), the mean
spindle length was 1.25 ± 0.23 µm, and the mean nuclear length was 1.31 ± 0.19 µm (n = 13) (Fig. 5, A and B).
Early stages of anaphase in cells containing an active dicentric chromosome were often characterized by finger-like
protrusions of the nucleus into the bud (Fig. 2 B, VE-DIC;
Fig. 5 D, DAPI staining). Correspondingly, the spindle
spanned the distance from the end of the bulk of chromatin in the mother to the tip of the finger-like protrusion in
the bud (Fig. 5 C, 2.54 µm in length). In cells exhibiting a
mid-anaphase pause, the mean spindle length was 4.17 ± 0.92 µm and the mean nuclear length was 4.09 ± 0.91 µm
(Fig. 5, E and F, n = 31). Thus the fixed images corroborate
the progression, as well as the length measurements, in
early to mid-anaphase, as determined in the real time analysis, and indicate the close correspondence between nuclear and spindle elongation throughout anaphase.
Fig. 5.
Progression of anaphase in cells containing a dicentric
chromosome. Cells were fixed and processed for immunofluorescence after two hours of growth in glucose-containing medium.
The panels on the left are cells stained with anti-tubulin antibodies; the panels on the right are the same cells stained with DAPI.
The arrows mark the ends of the spindle or nucleus, respectively. (A and B) Cells in the G2 stage, medium budded with the DNA
near the neck. (C and D) Cells in the early stages of anaphase,
having a slightly elongated spindle with DNA just visible in the
bud. (E and F) Typical of cells paused in mid-anaphase with a 4 µm spindle and DNA through the neck of large budded cells.
Bar, 1 µm.
[View Larger Version of this Image (130K GIF file)]
). The
direction of spindle movement could be assessed by determining the position of the leading and lagging edge of the
nuclear envelope relative to the neck of the budded cell.
The neck provided an accurate frame of reference in standardizing data from individual cells and was set at 0 µm.
Movements of the spindle pole into the bud (leading edge)
were plotted as negative values and movement into the
mother (lagging edge) as positive values. The nucleus
abutted the neck immediately preceding spindle elongation, and elongation was directed into the bud. In an example of a dicentric cell that displayed wild-type kinetics,
both fast and slow phases of spindle elongation, from 2 to
8-10 µm, were complete in ~22 min (Fig. 3 B). Cells delayed in anaphase B progression (Fig. 4 B) displayed the
initial rapid elongation phase (2-4 µm), which was followed by a pause in spindle elongation in which the nucleus remained in the neck for a significant amount of time
(up to 60 min in Fig. 4 B). Only after this pause, was the
second phase of elongation able to proceed to the maximal
spindle length of 10-12 µm.
Using chromosomal markers proximal to CEN1 on
chromosome I (kindly provided by V. Guacci; Guacci et al.,
1994), we determined that 34% of cells containing an active dicentric chromosome contained two spots within the
nucleus (Fig. 6). In contrast, 8% of the cells were observed
to have two fluorescent spots within the nucleus in wildtype, asynchronous populations using the same DNA
probes (Fig. 6). The 8% of cells with separated sisters in
wild-type populations can be attributed to the time expected for centromeres to separate within one chromatin
mass (Yeh et al., 1995
). Anaphase spindle elongation (from
the fast phase to the bi-lobed structures) persists for ~9
min (Fig. 3 A). 9/90 min doubling time predicts that 10%
of the population will be caught in the mid-anaphase stage.
This value compares quite favorably to the 8% determined by FISH (Fig. 6 B; Guacci et al., 1994
). By the same
reasoning we can predict what fraction of cells harboring a
dicentric chromosome will be in mid-anaphase in a logarithmic growing population. The dicentric delay persists
for 57 min (Fig. 4). The doubling time of this population is
~150 min, resulting in ~38% of the cells at the midanaphase transition at any one time. However, only about a third of the cells in a population pause in response to activation of the dicentric chromosome (Neff and Burke, 1992
;
Brock and Bloom, 1994
). We therefore estimate 2/3(8%) + 1/3(38%) = 17.8% of cells to be in mid-anaphase. This
value compares quite favorably to the 16% of cells found
to be in mid-anaphase, as determined by DAPI staining
(Table I), but less than that determined by FISH (34%).
While the high FISH value is certainly indicative of sister chromatid separation in the population of mid-anaphase
cells, it may also reflect centromere separation in a fraction of large-budded cells with DNA at the neck (Table I)
as well as cells with separated nuclei (Table I, last column),
in which the spindles may have collapsed and given rise to
apparently undivided nuclei with two spots. In any case,
the centromere regions of sister chromatids have separated in nuclei of cells containing active dicentric chromosomes, indicating these cells traverse the metaphase/
anaphase boundary and become blocked following either
anaphase A or anaphase A and B, with partially elongated
spindles, i.e., mid-anaphase.
Checkpoint Versus Physical Constraints on Spindle Elongation
The mid-anaphase delay could reflect a physical constraint
on spindle elongation, with the DNA between the two
centromeres constraining the poles from further separation. Alternatively, a cellular response to the dicentric insult could prevent further elongation (Fig. 7). To distinguish between these possibilities we have analyzed the
kinetics and spindle length of the mid-anaphase transition
in cells containing variants of dicentric chromosome III, in
which the centromeres are 3 vs. 45 kb pairs apart. 45 kb of
DNA is ~15 µm in its linear form. Estimation of the packing ratio in chromatin (sevenfold around a nucleosome) or
the degree of condensation from FISH (80 fold; Guacci et al.,
1994) provide an approximate length of this region to be
anywhere from 0.2-2 µm in vivo. Similarly, dicentric chromosomes with their centromeres 3 kb apart would be expected to span ~0.02-0.2 µm in vivo. If the physical constraint model is correct, the length of the spindle at the
arrest point would reflect centromere-centromere distances, and activation of a dicentric chromosome with the
centromeres 3 kb apart might result in a 10-fold difference
in spindle length at the delay point. As shown in Fig. 8,
cells containing the 3-kb dicentric minichromosome exhibit similar kinetics and morphologies as those of a cell
containing the 45-kb dicentric chromosome. Thus the midanaphase pause is not a function of the length between the
two centromeres.
Checkpoint Genes in the Mid-anaphase Transition
Defects in chromosome alignment, kinetochore attachment, or DNA breakage have all been shown to be subject
to cell cycle surveillance. The distinguishing feature of defects monitored by these checkpoint pathways is that they
delay anaphase onset. Previous studies performed by
DAPI staining of fixed populations and FACS® analysis
have revealed RAD9 to be involved in mediating the dicentric response (Brock and Bloom, 1994). We have reexamined the role of RAD9 in the real time assay to determine whether the delay in mid-anaphase is also dependent
upon this checkpoint gene. A single cellular response was
observed upon dicentric chromosome activation in the
rad9 deletion strain (Fig. 9, 9/9 cells; Table II). The behavior of the spindle and the timing of nuclear transitions were indistinguishable from wild-type cells.
Table II. Anaphase B Dicentric Pause Is Dependent on RAD 9 |
Time lapse, VE- and DE-DIC analysis of cells containing
an active dicentric chromosome reveals a delay in their
progression through anaphase. By two criteria, spindle
elongation and sister chromatid separation, cells containing an active dicentric chromosome transiently pause in
mid-anaphase, before maximal spindle elongation and the
exit from mitosis. This mid-anaphase delay is dependent on the RAD9 DNA checkpoint gene, indicative of DNA
damage surveillance pathways operative during late stages
in the cell cycle (Fig. 10).
The mid-anaphase delay was distinguished by both kinetic and morphological criteria. Upon activation of the
dicentric chromosome, the bulk of the nucleus remained in
the mother cell as the spindle began to elongate (Fig. 2 B).
Even as the spindle doubled its length the nucleus remained rounded and only later became noticeably sausage
shaped (Fig. 2 C). In contrast, the nucleus in wild-type cells underwent a rounded to sausage-shaped transition as
it traversed the neck and elongated to 4 µm (Fig. 3; Yeh
et al., 1995). The morphological transitions characteristic
of dicentric chromosome activation were accompanied by
a 30-120-min temporal delay in the subsequent elongation
of the mid-anaphase spindle. This 4 µm stage of spindle
morphogenesis is likely to represent a critical juncture in
spindle function in wild-type cells as well. In an elegant
three-dimensional, serial section reconstruction of a yeast
spindle, populations of anaphase spindles sorted into two classes based on their lengths: 3.7 and 9.4 µm (Winey et al., 1995
). Both populations of spindles were shown to straddle the neck, and in either population, sister chromatids
had already migrated to the poles based upon the length of
the presumptive kinetochore microtubules. These data
corroborate our findings that sister chromatids have separated at the 4 µm mid-anaphase delay (Fig. 6). The preponderance of 3.7 µm spindles reported by Winey et al.
(1995)
also reflects the brief pause which often occurs in
wild-type cells between the fast and slow phases of anaphase spindle elongation (Yeh et al., 1995
). In addition,
the oscillatory motion observed in the 4 µm spindle in
wild-type cells (Yeh et al., 1995
) is indicative of a natural
transition in spindle progression. Thus, both serial reconstruction of fixed cells and VE-DIC microscopy of live
preparations indicate a clear transition from medial to
elongated nuclear structures in wild-type cells. The dicentric chromosome insult simply prolongs this natural transition in the development of the anaphase spindle.
There are several aspects of dicentric chromosome activation that may contribute to the delay. One is that tension generated by the chromosome bridge could restrain spindle elongation. The finger-like protrusions of the nucleus into the bud (Figs. 4 A and 5 D), appear to be futile attempts by the spindle/nucleus to initiate anaphase spindle pole separation. This period (5 min duration) has no correlate in the kinetic progression of a wild type cell. These protrusions, and the rounded morphology of the nucleus as it traversed the neck of the dividing cell (Fig. 2 C), probably reflect transient physical constraints on the spindle. The time lapse studies with centromeres at different distances (3 vs. 45 kb apart) indicate that the arrest in spindle elongation is not exclusively due to a DNA bridge constraining anaphase pole separation. Cells containing either dicentric chromosome display virtually identical spindle morphologies and lengths (4 µm) for similar durations (47-59 min on average; Table II). Thus the mid-anaphase delay likely represents surveillance mechanisms that effectively inactivate the microtubule assembly and motility mechanisms which normally produce further spindle elongation.
The dependency of the mid-anaphase delay on the
RAD9 gene reveals that the DNA damage checkpoint
continues to monitor chromosome integrity well after the
start of anaphase, as well as before anaphase onset (Fig. 10).
Thus RAD9-dependent DNA damage arrests the cell at
any stage (G1, S, G2, and now mid-anaphase). This notion
is similar to recent findings that checkpoint genes (RAD9, Siede et al., 1993; and the SAD1/RAD53 protein kinase,
Allen et al., 1994
) indeed control multiple checkpoints.
Whether the damage leads to the same or different signal
in each stage, or different signals in the same stage, is not
well understood, but several genes are clearly involved at
multiple stages of the cycle. Rad9p is constitutively expressed throughout the cell cycle (Schiestl et al., 1989
),
consistent with the proposal that this protein is involved in
DNA surveillance throughout G1/S, G2/M, and anaphase/ cytokinesis. It is also likely that DNA lesions, in addition
to a dicentric-induced aberration, are also subject to
RAD9 surveillance at mid-anaphase. However, due to the
rapidity of spindle elongation and the relatively extended
lengths of G1/S and G2/M, the mid-anaphase delay would
be difficult to identify in a population study. In this regard,
we have examined the effect of a dominant negative form
of topoisomerase I (top1-103), which also results in a
RAD9-dependent cell cycle arrest (Levin et al., 1993
). As
reported previously, a large fraction of cells exhibited the
large budded RAD9-dependent arrest morphology following 8 h of top1-103 induction. However, DAPI staining of
the cells revealed two classes of arrest morphologies. About two-thirds of the cells displayed a single nucleus at
the neck of large budded cells, while one-third exhibited
elongated nuclei (sausage-shaped) spanning the neck region between the mother and bud (Beach, D., and K. Bloom, unpublished results). This second class of cells is
identical in morphology to cells which arrest in midanaphase and indicates that a variety of DNA lesions can lead to delays in mid-anaphase.
The description of a mid to late-anaphase checkpoint
leads to the notion that the major cyclin-dependent kinase-cyclin complexes, other regulatory kinases, e.g., DBF2
and 20 (Toyn and Johnston, 1994), cyclin destruction, or
other anaphase-progression factors, are operative after
anaphase onset (Irniger et al., 1995
). In fact, H1 kinase
levels remain elevated for prolonged periods in yeast cell
populations following activation of the dicentric chromosome (Neff and Burke, 1992
; Brock and Bloom, 1994
). Cyclins and H1 kinase activity persist throughout anaphase in
budding yeast, Drosophila, and nontransformed mammalian cells (Surana et al., 1993
; Girard et al., 1995
; Sigrist et al.,
1995
). In budding yeast, fully activated cyclins or overexpression of nondegradable forms of cyclin prevent spindle
disassembly at telophase, rather than anaphase onset
(Stueland et al., 1993
; Surana et al., 1993
), and high levels
of cdc28/clb are found in cells arrested at telophase (cdc15;
Surana et al., 1993
; Irniger et al., 1995
). The persistence of
cyclin/clb complexes throughout anaphase raises the possibility that they may be involved in regulating the progression of anaphase directly, or by delaying anaphase progression in response to perturbation. The coexistence of
subpopulations of degraded and protected cyclins (Irniger
et al., 1995
) is also suggestive of a role for the cdc28/cyclin B complex in mediating the progression of anaphase, spindle disassembly, and cytokinesis. Thus the sequential degradation of different cyclins may drive the progression
from metaphase to telophase, or may be required to delay
anaphase progression in the event of damage.
The description of a mid-anaphase transition raises two
major questions. Upon sister chromatid separation, the
cells lose a major pathway for repair of DNA damage.
Therefore, why have a mid-anaphase checkpoint? Secondly, what perturbations are monitored by this checkpoint in the normal course of cell division? Several attributes of mitosis in budding yeast shed light on these
issues. Yeast chromosomes have not been observed to
align on a metaphase plate before anaphase onset. This
has been thought to reflect the absence of chromosome
condensation. However, Winey et al. (1995) demonstrated
that kinetochore microtubules shorten asynchronously, reflecting the asynchronous movement of chromosomes to
the poles. Mid-anaphase may therefore represent the last
time in the cell cycle where errors in attachment may be
rectified. Alternatively, the mid-anaphase transition could
represent the last stage for DNA repair between sister
chromatids. While FISH experiments (Guacci et al., 1994
)
and results from analysis of sister chromatids at the midanaphase delay (Fig. 6) indicate that sister centromeres have separated at this stage, the chromosome arms may
not be completely disjoined. The uniformity of DAPI staining in cells with 4 µm spindles spanning the neck indicates
that the bulk of the chromosomal DNA is evenly distributed within the nucleus. In contrast, the morphological
transition to a bi-lobed nucleus results in substantial separation of chromosomal DNA. This most likely represents
the final decatenation between sister chromatids and the
irreversible commitment to chromosome separation (Fig.
10). In this view, the mid-anaphase transition represents
the stage prior to the final commitment to complete DNA
separation. The temporal coordination between completion of sister chromatid decatenation and force generation
for spindle elongation necessary for preventing chromosome breakage may be the primary reason for the midanaphase pause, and one that may be important for all eukaryotic organisms. Loss of coordination of these events in
transformed cells lacking mid-anaphase checkpoints may
result in increased chromosome breakage, giving rise to
chromosomal rearrangements, loss of genomic integrity, and hence, the neoplastic state.
Received for publication 6 June 1996 and in revised form 15 November 1996.
Please address all correspondence to Kerry Bloom, Department of Biology, University of North Carolina, Chapel Hill, NC 27599-3280. Tel.: 919962-1182; Fax: 919-962-1625; E-mail: ksb.fordham{at}mhs.unc.eduWe thank Dr. Vinny Guacci (Carnegie Institute, Baltimore, MD) for his generous gifts of probes, protocol, and invaluable expertise for the FISH experiments. We thank Drs. Danny Lew (Duke University, Durham, NC) and Jim Allen (University of North Carolina, Chapel Hill, NC) for critical comments. Thank you also to Paul Maddox for assistance with microscopy and image processing.
This work was supported by research grants from the National Institutes of Health General Medical Sciences (K. Bloom and E.D. Salmon).
DE and VE, digital and video enhanced; DIC, differential interference contrast; FISH, fluorescent in situ hybridization.