Cell Biology
Cell Biology
Cell Biology
cell biology courses. The primary text is generally on the left side of the vertical divider,
Cell Cycle : and printed in black. Details that are usually left to an advanced course are printed in
blue and found on the right side of the divider. Finally, additional biomedically relevant
information can be found in red print on either side of the divider.
DNA replication has already been covered in detail in chapter 7. In bacteria, the pro-
cess is initiated at the origin of replication by DnaA. However, in archaea, synchronous
initiation of replication at multiple sites on the chromosome as well as recognition
proteins homologous to eukaryotic ORC proteins suggests that there are similarities
between archaebacterial and eukaryotic DNA replication to be explored.
Once the DNA is replicated and moved to opposite sides of the cell, the midcell septum
forms to split the cell. At least 9 gene products are involved in this process including
FtsZ, the prokaryotic tubulin homologue that forms a circumferential ring, FtsI, a pepti-
doglycan synthetase involved in septum formation, FtsL, whose function is unclear but
is involved in ingrowth of the cell wall at the septum, and ZipA, which anchors the FtsZ
ring. The ring contracts, pulling the membrane in with it. Eventually the membrane is
pinched in enough to fuse and generate two completely separate cytoplasmic compart-
ments. Other septation enzymes make cell wall components that fill in as the septum
forms simultaneously with membrane/FtsZ contraction, and the cells separate.
Most eukaryotic cells undergo a reproductive cycle to generate either another copy of
themselves or to generate gametes (sex cells), and in doing so require a complex mecha-
nism to govern the safe and accurate replication of their much larger (than prokaryote)
genomes. Immediately following mitosis, the newly created cells are in the G1 phase.
This is largely a growth phase, during which there is a lot of biosynthesis of proteins,
lipids, and carbohydrates. However, there is no synthesis of new DNA at this time. G1
is the longest of the cell cycle phases in many cell types, and most of the physiological
activity of a cell happens during G1. Following G1, the next phase of the cell cycle is the S
phase, during which synthesis of new DNA occurs. In other words, the genome is being
replicated during this phase; thus at the end of S phase, the cell has twice the normal
amount of DNA. After S phase, the cell proceeds into G2, which provides an opportunity
for the cell to perform a self-assessment and make final preparations (such as more cell
growth, repairs of DNA) as necessary before it finally heads into mitosis. Mitosis, or M
phase, is primarily (1) the breakdown of the nucleus, (2) re-distribution of the DNA to
opposite sides of the cell, and (3) formation of two new nuclei around that DNA, and
cytokinesis, the final splitting of the cell itself.
G2 - M Checkpoint
-DNA fully replicated?
-Environment?
Metaphase Checkpoint
M Phase -Chromosomes attached to spindle?
Mitosis and Cytokinesis
G2 Phase
Further Cell Growth and Development
G1 Phase
Cell Growth and Development
S Phase
DNA Replication
G1 - S Checkpoint
-Environment?
Figure 1. The Eukaryotic Cell Cycle. -Cell large enough to divide?
-DNA quality?
There are three major checkpoints for cell cycle control (fig. 1). The first regulates the
transition from G1 to S phase. Recall that G1 can be a very long phase, even (in the case
of G0) as long as the lifespan of the cell. However, once the cell reaches S phase, it is
committed to going through S, G2, and M phases to reproduce. This is because once S
phase has begun, there is more than the normal diploid complement of DNA inside the
cell. Over time this would confuse the cell (e.g., by overexpression of duplicated genes)
as it tried to use the DNA to direct RNA and protein synthesis, and it could become
sick and die. The second major checkpoint regulates entry into mitosis. Once mitosis
begins, most of the metabolic activity of the cell is shut down, and the cell concen-
trates its resources on dividing the nuclear and cellular material equally to support the
life of both resulting daughter cells. If the cell needs more time to make final repairs
on the DNA or even to bulk up a little, this checkpoint can hold the cell in G2 a little
longer for those things to happen. Finally, the third major checkpoint occurs during
mitosis, and regulates the transition from metaphase into anaphase. Since the sister
chromatids are being split apart and moved to opposite poles to form the new nuclei,
it is important that all of them are perfectly lined up at metaphase and the proteins
holding them together have dropped off. If they do not split evenly, the daughter cells
will have abnormal numbers of chromosomes (aneuploidy) usually leading to deleteri-
ous consequences.
What is the molecular mechanism that regulates the progress of the cell cycle? While
many of the checkpoint sensing mechanisms are still unclear, they seem to converge
on two sets of proteins that act together to trigger cell cycle advancement. These pro-
teins are known as the cyclins and the cyclin-dependent kinases (cdk). As the names
suggest, the cyclins are proteins that regulate progression through the cell cycle, and
G2 - M Checkpoint
-DNA fully replicated?
-Environment?
Metaphase Checkpoint
M Phase -Chromosomes attached to spindle?
Mitosis and Cytokinesis
G2 Phase
Further Cell Growth and Development
Cyclin B
Cdk1
Cyclin D
Cyclin A Cdk4,6
Cdk2 Cyclin E
Cdk2
G1 Phase
Cell Growth and Development
S Phase
DNA Replication
G1 - S Checkpoint
-Environment?
-Cell large enough to divide?
-DNA quality?
The methodology of some of the early experiments is perfectly suited to explaining how
this works. The seminal paper in this field was a 1971 paper in J. Exp. Zool. by Masui
and Markert. In it, they examined frog (Xenopus laevis) eggs that were arrested at G2.
The oocytes arrest for about 8 months naturally in order to build up the mass needed
to start a new organism once it has been fertilized. The basic question being asked is
what is causing the eggs to come out of G2 and into M phase? It was already known
In later experiments, other investigators attempted to find the specific protein trigger,
and from there, presumably, the rest of the mechanism. Fractionating the M-phase
oocyte cytoplasm by column chromatography, a protein, named cyclin B, was found to
rise and fall in concentration in direct synchronization with MPF activity. Furthermore,
addition of cyclin B alone was sufficient to rescue MPF activity from M-phase cytoplas-
mic extract that had been depleted by RNase treatment (preventing synthesis of any
new proteins, including cyclin B, and abolishing MPF activity). This clearly places cyclin
B in the forefront of the maturation mechanism, but there was one major issue: cyclin
B had no enzymatic activity. How was it effecting the changes needed for progress
from G2 to M phase?
This problem was answered by experiments on a very different organism, the fission
yeast, Schizosaccharomyces pombe. Because they have a very short cycle time, a rela-
tively small genome, and they can be given random mutations en masse by irradiation
or chemical treatment, yeast are excellent model organisms for many types of biologi-
cal study. After random mutation of a population of yeast, they can be screened for
mutations of particular types, such as cell division cycle (cdc). When the mutations are
sequenced and identified, they are often named by the type of mutation and order of
discovery. Cdc2, it turns out, showed two interesting phenotypes when mutated in op-
posite directions. Mutations that knocked out function of cdc2 caused the formation of
extremely large yeast that do not undergo cell division, while mutations that made cdc2
overactive caused the formation of rapidly dividing very small cells. The interpretation
was that when cdc2 is missing or inactive, the cells cannot progress to mitosis, so they
stay in G2 accumulating bulk material in preparation for a cell split that never comes.
Conversely, when cdc2 is overactive, it drives the cell quickly into mitosis, even if it has
not been in G2 long enough to synthesize enough mass to form two normal-sized cells.
This ties cdc2 nicely to cell cycle regulation, and it even has an enzymatic activity: it is
a kinase. This made it a perfect candidate as a first-order coordinator of cellular events
because phosphorylation is fast, phosphorylation usually activates some other enzyme,
and kinases usually act on an array of targets, not just one. So we now have a cyclin
(identified as cdc13 in S. pombe) and a cyclin-dependent kinase that work together to
promote cell cycle progression into M phase.
As you will see in a later section of this chapter, MPF performs many functions, some
of which prevent progress of mitosis past anaphase. Therefore, there must be a way
to turn off MPF (and for that matter, any cyclin/cdk complex) quickly and completely
when the cell reaches the appropriate stage of the cell cycle. This is borne out by time-
course studies of MPF activity, which show a precipitous drop in activity in anaphase.
This coincides with a depletion of the cyclin B (cdc13 in S. pombe) due to a combina-
cyclin
MPF
e
se
An ase
se
se
se
An se
se
se
An ase
se
e
as
as
as
as
ha
ha
ha
ha
ha
ha
ha
ha
ha
ph
ph
ph
ph
op
ap
ap
rp
op
ap
ap
rp
op
ap
ap
lo
lo
lo
r
te
te
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et
et
et
Pr
Pr
Pr
Te
Te
Te
In
In
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M
M
Mitosis 1 Mitosis 2 Mitosis 3
Essentially, MPF ensures its own destruction: one of its phosphorylation targets is
cdc20. Upon phosphorylation, cdc20 is activated and then activates anaphase promot-
ing complex (APC). APC is a ubiquitin ligase (type E3) that polyubiquitinates the cyclin
of the MPF complex, making it a target for proteolytic degradation by a proteosome.
Note that only the cyclin is destroyed, while the kinase is left alone. Without the cyclin,
the kinase is inactive and must wait for cyclin levels to rise again before it can be re-
activated by a fresh round of phosphorylation and dephosphorylation.
Active MPF
Mitotic Cyclin
P
Activation CDK
Thr
P
Ub Ub
+ Polyubiquitination
P Ub Ub
Cdc20 Inactive Active
APC APC
Mitotic Cyclin
Ub Ub
Ub Ub CDK
P
Degradation by proteasome
The G1 phase is the state a cell is in immediately following cytokinesis. At that point,
the cells will be somewhat undersized, and need to take up materials and energy
sources, and convert them to cellular components in order to support the eventual cell
division. During this time, the cell goes about doing its “normal” business - an endo-
crine cell makes and secretes hormones, an intestinal epithelial cell absorbs nutrients
from the gut and passes them on to the bloodstream, a neuron conducts signals, etc.
Most types of cells spend the majority of their cycle in G1, although there are excep-
tions, such as the frog oocytes mentioned earlier. The length of G1 is generally constant
for a given cell type under normal conditions, but can vary greatly between different
cell types. Post-mitotic cells, which have left the cell cycle and will no longer divide,
are in G1 until they die, barring reactivation of the cell cycle by stress conditions. This
continuous G1-like state is referred to as G0.
For those cells preparing to move from G1 into S, cyclins D and E, and cdk 2, 4, and 6
predominate, with activation of cyclin D complexes preceding activation of cyclin E
complexes. Two major questions are asked by the cell: is the DNA undamaged and
complete, and is the extracellular environment favorable for cell division? The cellular
sensors for these conditions then link to cyclin complexes effect restriction points on
cell cycle progression. The extracellular environment questions can be a tricky one,
because this can include more than just assessment of nutrient availability or predatory
threats; it can also be a requirement for an external trigger such as a mitogenic hor-
mone or paracrine signal. In fact, nearly all normal animal cells require an extracellular
signal to progress through the G1/S checkpoint. The cyclin E/ cdk2 combination is the The active cyclin E/cdk2 complex phosphorylates the tumor sup-
principal regulator of entry into S phase and DNA replication. pressor protein Rb (retinoblastoma), which causes E2F to trans-
locate to the nucleus and turn on genes needed for entry into S
S phase phase.
Mitosis
Mitosis consists of prophase, metaphase, anaphase, and telophase, with distinct cellular
activities characterizing each phase. This completes the duplication of the nucleus, and
is followed by cytokinesis, in which the cell divides to produce two daughter cells.
Interphase (G2)
Inner CENP-E
Kinetochore
Layer
MCAK
GDP
GDP
GDP
GDP
GDP
GDP
GDP
GDP
GDP
Kinetochore Microtubule
Outer
Kinetochore
Layer Dynein
Fibrous Corona
Chromosomal DNA
Figure 8. The kinetochore assembles on the centromere of the chromosome. Spindle micro-
tubules attach to the fibrous corona of the kinetochore through kinesins and dyneins.
The kinetochores attaching to the centromere DNA are trilaminar protein structures
consisting of an inner layer, an outer layer, and a fibrous corona. The kinetochore
microtubules of the mitotic spindle are primarily attached to the fibrous corona. As
depicted in the figure, it is attached through CENP-E, a kinesin, and dynein motor pro-
teins that bind along the barrel of the microtubule. In fact, sometimes the first contact
between a chromosome (via the kinetochore) and a spindle microtubule is somewhere
until they are all lined up along the midline of the mi- crotubules are stained green, f-actin (+) (-)
(-) (-)
is stained red, and chromosomes, (-) (+)
totic spindle, which in most (but not all) cases is also with centromeres lined up along the
the midline of the cell. Once they are all lined up, the midline, are stained blue. Note the
surrounding cells, which are not in
cell is considered to have reached metaphase. Unlike mitosis, with their MT and MF cy-
the other phases, metaphase is a relatively static phase toskeletons more overlapped. This photo
released to public domain by the US goverment.
C
- it is a checkpoint for lining up the chromosomes.
(+)
(+)
(-) (-)
The chromosomes must be properly aligned to ensure that both daughter cells receive
(-) (-)
the proper complement of chromosomes. How does the cell know when the chro- (+)
mosomes have reached the center of the spindle? An elegantly simple experiment (+)
demonstrated that the general mechanism is a tension check - if the two microtubules
connecting to the pair of sister chromatids from each side are of the same length, they Figure 9. Molecular motors set up the mitotic spindle.
should be exerting equal tension on the chromosomes. If the microtubule-kinetochore
connection is severed at metaphase, the cell will be prevented from progressing (Nick-
las, R.B., et al, J. Cell Biol. 130: 929-39, 1995). However, if an equivalent tension is applied In fact, there appear to be two mechanisms at work: the bub1/
by tugging on the chromosome with a glass microneedle, progression of mitosis is bub2 system works in the tension sensing pathway, while another
restored! metaphase protein, mad2 appears to be important in suspending
mitosis upon disconnection of the kinetochore with the spindle
microtubule.
Barring pathological situations, if and only if the chromosomes all line up at the meta-
phase plate will the cell proceed to the next stage of mitosis: anaphase. The sister chro-
matids separate and are pulled toward opposite poles of the mitotic spindle. Somewhat
perversely, even as the chromosomes move towards the spindle poles, the poles them-
selves move outward slightly. Separation of the sister chromatids requires the dissocia-
tion of the molecular “glue” holding them together: the cohesin proteins. The cohesins A cohesin is a multimer of four subunits, Scc1, Scc3, Smc1, and
bind to both molecules of DNA and hold them together shortly after replication back Smc3 in yeast. An additional protein has also been observed in
in S phase. As anaphase approaches, the enzyme separase is activated, which then cuts Xenopus. The SCC1 protein is cleaved by separin in yeast, but in
the cohesin molecules. Once all of the cohesin molecules are cut, the sister chromatids metazoans, SCC1 may be removed from chromosomes by another
can finally be separated. The removal of the cohesins proceeds roughly inwards from method as well. It is phosphorylated, which decreases its affinity
the distal points of the chromosomes to the centromere, which is generally the last for DNA, and may expose a site for separase-catalyzed hydrolysis.
region of attachment.
Separase also promotes anaphase by activating Cdc14, a phos-
Anaphase can actually be divided into two stages, sometimes referred to as early and phatase needed to dephosphorylate the cdk substrates that had
late or A and B. At first, the kinetochore microtubules are shortening from both ends, been phosphorylated by the cyclin-cdk complexes of early mitosis.
and kinesin-family motors pull the microtubules back toward the spindle poles. As late In addition, Cdc14 is also required for cytokinesis in the yeast S.
anaphase starts, polar microtubules elongate, and an additional chromatid-separating cerevisiae and nematode C. elegans.
force is applied by kinesin-family motor proteins [kinesin-5] that push the polar mi-
crotubules against one another to increase the separation between the poles. Dynein-
family motors help to direct movement of the poles as well, through their attachment
to the aster microtubules and the cortical (peripheral) cytoskeleton.
When both sets of chromosomes arrive at their respective poles, telophase begins.
Technically, it was slowly building up since anaphase: when MPF was inactivated by
APC, its ability to phosphorylate nuclear lamins was ended. Protein phosphatases in the
cell remove the phosphate groups, allowing the lamins to once again interact with one
another, and by telophase they are reconstituting the nuclear lamina and the nuclear
envelope. Since the lamins and other nuclear membrane proteins also interact with
DNA, the nuclear membrane fragments dispersed back in late prophase now coalesce
around each set of DNA to form the new nuclear envelopes. The other fragmented
membranous organelles (ER, golgi) also start to re-form. By the end of telophase, the
product is a single large cell with two complete nuclei on opposite sides. The next and
A cell may die either intentionally (usually referred to as apoptosis or programmed cell
death, though also once known also as “cellular suicide”), or unintentionally (necrosis).
The microscopic observation of these two processes shows strikingly different mecha-
nisms at work. In apoptosis, the cell begins to shrink and lose shape as the cytoskel-
eton is degraded, then the organelles appear to pack together, except for the nucleus.
Inside the nucleus, the chromatin condenses and attaches to the nuclear envelope,
which then loses its integrity and starts to break apart. The cell membrane begins to
show irregularities, descriptively known as blebs, and eventually, the cell breaks apart
into vesicles that are neatly cleaned up by phagocytes drawn to the site by apoptotic
signals emitted by the dying cell. Necrosis, on the other hand, is quite literally a mess.
The cell appears to swell and the plasma membrane begins to lose its integrity. It is
soon catastrophically leaking cytoplasm, and leaves behind cell debris that can accumu-
late and trigger necrotic death of adjacent cells.
A B
Figure 13. (A) A cell underdying by necrosis is disorganized, generally bursts and leaks its
contents. (B) A cell undergoing apoptosis first subdivides itself, digesting itself in an orderly
fashion and compartmentalizing everything for scavenging by phagocytes.
When death receptors are activated, the subsequent caspase cascade does not involve
the mitochondria or APAF-1. The best studied case, FasR (Fas receptor) activates caspas-
es 2, 8, and 10 by clipping procaspases and by releasing caspases from inhibiting com-
plexes. These activate caspases 3, 6, and 7, which leads to the final stages of apoptosis.
In both internally and externally triggered apoptosis, the final steps are the same: some
of the final targets of the caspases are the nuclear lamins and ICAD (inhibitor of cas-
The other major function for apoptosis is to kill dangerous cells. In some cases, these
may be cells infected by a pathogen. In others, the cells have accumulated mutations
that do have affected the DNA error-correction system or cell-cycle checkpoints. When
the former occurs, each generation has an increased likelihood of even more mutations.
It is important to activate apoptosis in such cells before they have a chance to acquire
errors that removes all cell cycle checkpoints, allowing unchecked cell proliferation.
This could lead to tumor formation and potentially cancer (see next chapter). When
such cells need to be killed for the benefit of the organism, it may happen by the trig-
gering of an internal sensor such as mitochondrial damage, or by external means, such
as an immune system cell recognizing an infected cell.
In metazoa, there are two situations in which a cell gives rise to daughter cells. The
first, and by far most common, is mitosis. The second is meiosis. Meiosis is the process
by which gametes (sex cells) are generated. Animals and plants are generated by sexual
reproduction (if this is news to you, please consider majoring in something other than
biology). These organisms start life through the fusion of two cells: a sperm and an
egg. Both contribute genetic material to the new organism. In order to maintain the
proper number of chromosomes in each generation, the gametes each contribute one
set of chromosomes, so that the fertilized egg and all other cells in the organism have
two sets of chromosomes — one from each parent. The purpose of meiosis, and its pri-
mary difference with mitosis, is not generating daughter cells that are exact replicates,
but generating daughter cells that only have half the amount of genetic material as the
original cell.
Let us take a look at this situation selfishly: meiosis in human beings. Almost every cell Mature red blood cells contain no nucleus, and some muscle cells,
in your body has a nucleus containing 46 chromosomes, a set of 23 from your father, while multinucleated because they form from the fusion of sev-
and a set of 23 from your mother. The only exceptions are the gametes: the spermato- eral myoblasts, nevertheless have 46 chromosomes in each of the
cytes in men and the oocytes in women. The somatic cells are said to be 2n or diploid, nuclei.
that is having 2 sets of chromosomes, and the gametes are 1n or haploid, having only
one set of chromosomes. Sometimes, meiosis can be a little confusing to students Polyploidy, while uncommon in humans, is a normal state for
because it occurs in the same part of the cell cycle as mitosis, which is to say after G2. many organisms. The frog, Xenopus laevis, a common research
Because of this, the cell entering meiosis actually has 4 sets of chromosomes, since the animal, is tetraploid.
DNA has already undergone replication in S phase.
Meiosis consists of two consecutive meiotic divisions each of which has phases similar
to mitosis: prophase, metaphase, anaphase, telophase, and each of which finishes with
complete cytokinesis. Note that immediately following meiotic telophase I, the cell
divides, and both daughter cells are immediately in prophase II. There is no interven-
ing G1, S, or G2 phase.
4 Diplotene 5 Diakinesis
Recombination occurs when a piece of the paternal chromosome is swapped for the
homologous piece of DNA on the matching maternal chromosome (or vice versa). Note
that sister chromatids (i.e. exact copies) do not recombine - only homologous non-sister
chromatids can recombine. Obviously, this kind of a DNA swap must be done carefully
and with equivalence, so that the resultant DNA on each side contains all the genetic
information it is supposed to, and no more information than it is supposed to. In order
to ensure this precision in recombination, the non-sister homologous chromatids are
held together in a synaptonemal complex (SC). This ladder-like complex begins to form Lateral elements are composed several proteins, including con-
in the zygotene stage of prophase I and completes in pachytene. The complete SC con- densins and cohesins. The cohesins are meiosis-specific variants,
sists of proteinaceous lateral elements (aka axial elements) that run along the length of with substitutions for the Scc1 and Scc3. Likewise, condensin
the chromatids and a short central element composed of fibrous proteins forming the subunits also have meiosis-specific alleles. In addition to the
rungs of the ladder perpendicular to the two lateral elements. The central element is condensins and cohesins, which other than their meiotic-specific
formed of transverse filament dimers that interact with one another in offset fashion, variants, are common chromosomal proteins, there are SC-specif-
as well as with the lateral elements. These filament proteins (e.g. SCP1 (mouse), Zip1p ic proteins, including SCP2 and SCP3. Both are localized to con-
(yeast)) have central coiled-coil regions that function as protein interaction domains. densed chromosomes in early meiosis, and SCP3 has been show
Although SCP3 and therefore complete lateral element formation are unnecessary for by knockout analysis to be necessary for lateral element forma-
a functional synaptonemal complex, condensin and cohesin do appear to be necessary tion. However, it is not necessary for recombination.
for proper transverse filament attachment of the lateral elements.
5’ 3’
3’ 5’
3’ 5’
Double strand break in one duplex
5’ 3’
5’ 3’ 5’ 3’
3’ 5’ 3’ 5’
Gap is widened,
3’ 5’
5’ 3’ leaving two 3’ overlapping tails
5’ 3’ 5’ 3’
3’ 5’ 5’ One single-stranded 3’ tail invades
3’
5’
5’
3’
the other DNA duplex
5’ 3’ 5’ 3’
3’ 5’ 3’ 5’
3’ 5’
5’ 3’ 3’ 5’
DNA repair enzymes fill in gaps 5’ 3’
Single Holliday junction resolves by reversing invasion
5’ 3’ 5’ 3’
3’ 5’ 3’ 5’
3’ 5’ 3’ 5’
5’ 3’ 5’ 3’
2nd end capture forms DNA heteroduplex, branch migration, DNA repair enzymes fill in gaps
two Holliday junctions resolve
5’ 3’ 5’ 3’
3’ 5’ 3’ 5’
3’ 5’ 3’ 5’
5’ 3’ 5’ 3’
Crossover No Crossover
Recombination may occur with or without the formation of double-strand breaks, and
in fact, can occur without the formation of the synaptonemal complex, although the SC
probably enhances the efficiency of recombination. In S. pombe, meiosis occurs without
the formation of a synaptonemal complex, but there are small discontinuous structures
somewhat similar to parts of the SC. In the fruit fly, Drosophila melanogaster, females
undergo meiosis using a synaptonemal complex, but males do not undergo meiotic
recombination, and their chromosomes do not form synaptonemal complexes. In most
cases, recombination is preceded by the formation of recombination nodules, which are
protein complexes that form at potential points for recombination. The best studied
mechanism for meiotic recombination involves a double-stranded break of one of the
chromosomes initiated by the meiosis-specific endonuclease, Spo11. The 5’ ends (one in
each direction) of this cut are degraded slightly to form 3’ single-stranded overhangs.
This leads to the formation of Holliday junctions with a strand from one chromosome
acting as a template for a missing portion of the homologous cut chromosome. This
may be resolved one of two ways, with or without a crossover, as illustrated (fig. 17).
As the cell goes from meiotic prophase I to meiotic metaphase I, another difference
between mitosis and meiosis is revealed: the chromosomes line up at the metaphase
plate as tetrads rather than as pairs. Because of this, when they pull apart in anaphase,
sets of sister chromatids segregate to opposite poles. Of course, due to recombination,
the sister chromatids are unlikely to still be identical.
Metaphase I Anaphase II
Anaphase I Telophase II
Haploid
Telophase I
Daughter Cells
Figure 18. Meiosis generates 4 haploid daughter cells from one diploid precursor. To do so, it undergoes a
two rounds of meiotic nuclear and cell division,
After a conventional anaphase and telophase, the cell splits, and immediately the daugh-
ter cells begin the second meiotic division (fig. 18, right side). In some cell types, chro-
mosomes do not decondense in meiotic telophase I, but if they have, they re-condense
Egg cells, as genetic and bulk material donors, need to be large but sperm cells, as ge-
netic donors only, do not. The diagram below depicts the generation of the egg cells.
Only one oocyte is generated from a meiotic event; the other three daughter cells are
termed polar bodies, and contain so little cytoplasmic material that they are only viable
for a short time. The asymmetric distribution of cytoplasm in the first meiotic division
for oocytes is due to the position of the meiotic spindle in the periphery of the cell
rather than centered. Since the center of the spindle determines the position of the
contractile ring for cytokinesis, this leads to unevenly sized daughter cells.
Oogonium
Mitotic division
Primary oocytes
Meiotic division I
Meiotic division II
Type A1 spermatogonia
Type A2 spermatogonia
Type A3 spermatogonia
Mitotic divisions
Type A4 spermatogonia
Intermediate spermatogonia
Type B spermatogonia
Primary spermatocytes
Meiotic division I
Secondary spermatocytes
Meiotic division II
Spermatids
Spermatids
Differentiation
Residual bodies
and
Mature sperm
Not all organisms reproduce with the human-like egg and sperm mechanism, i.e. ga-
metic meiosis. As just described, in a gametic meiosis life cycle, meiosis generates hap-
loid gametes, which then fuse/fertilize to become a diploid zygote. The zygote becomes
a multicellular diploid organism, and once it reaches sexual maturity can make more
haploid gametes via meiosis. The only multicellular state is diploid, and the gametes
are haploid.
Gametes
mitosis
Gametes
(egg)
(sperm)
Spores
Zygote
Zygote
Sporophyte
Adult individual
Diploid (2n) Diploid (2n)
Figure 21. Gametic meiosis (left) and Sporic meiosis (right).
An example of this type of life-cycle and the role of meiosis is found in moss. What we
think of as the body of the moss is actually a gametophyte, made up of haploid cells
generated by mitotic division of a haploid spore. These gametophytes generate either
sperm or eggs in specialized structures in their distal tips, and under the right condi-
tions (e.g. rain) the sperm is carried to the eggs and fertilization occurs. The fertilized
(diploid) egg now develops by mitotic division and differentiation into a sporophyte. In
this case, the sporophyte is a specialized reproductive structure on the tip of the moss,
and is also diploid. On the tip of the sporophyte is the sporangium, which is where
meiosis takes place to generate haploid spores. The spores may then be dispersed (by
wind or rain) and begin the cycle again by dividing and forming a new gametophyte.