First published online 3 October 2007
doi: 10.1242/dev.011361
Development 134, 3837-3848 (2007)
Published by The Company of Biologists 2007
Cortical granule exocytosis in C. elegans is regulated by cell cycle components including separase
Joshua N. Bembenek1,*,
Christopher T. Richie2,
Jayne M. Squirrell1,
Jay M. Campbell1,
Kevin W. Eliceiri1,
Dmitry Poteryaev3,
Anne Spang3,
Andy Golden2 and
John G. White1
1 University of Wisconsin-Madison, Laboratory of Molecular Biology, 1525 Linden
Drive, Madison, WI 53706, USA.
2 Laboratory of Biochemistry and Genetics, NIDDK, National Institutes of Health,
Building 8, Room 323, 8 Center Drive, Bethesda, MD 20892-0840, USA.
3 Growth and Development, Biozentrum, University of Basel, Klingelbergstrasse
50/70, CH-4056 Basel, Switzerland.
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Fig. 1. Identification of cortical granules. (A-C) Succynilated
WGA-labeled cortical granules in C. elegans oocytes (A), and
prometaphase I embryos (B), but not in embryos after meiosis I (C) (DNA in
blue). (D-F) WGA-labeled cortical granules (D) are associated with
SP12::GFP-labeled reticulate ER (E) at the cortex of a metaphase I embryo;
merge in F. (G-I) UGTP-1::GFP-labeled 1 µm vesicles were clustered
in prometaphase I (arrows, G) and redistributed across the cortex by metaphase
I (arrows, H). Smaller cytoplasmic puncta remain after loss of the 1 µm
vesicles (arrows, I). (J-L) WGA staining (J) co-localized with
UGTP-1::GFP (K) in cortical granules in the cortex of a metaphase I embryo;
merge in L. Scale bar: 10 µm.
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Fig. 2. TEM of cortical granules. (A) A mature C. elegans
oocyte contains cortical granules (arrows); inset shows higher magnification
of vesicles near the oocyte chromosomes (asterisks). (B) An embryo
within the spermatheca contains a cortical granule near the plasma membrane
(upper right arrow), and a cluster of heterogeneous vesicles (lower arrows).
(C) A metaphase I embryo contains cortical granules (arrows)
distributed across the cortex (asterisk denotes chromosome in spindle). The
cortical granules are found in close association with reticulate ER (A-C).
(D) Embryo at metaphase II (chromosome in spindle indicated by white
asterisk) lacks cortical granules, and the polar body (black asterisk) is
trapped between eggshell layers (arrows). Scale bar: 2 µm.
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Fig. 3. A wave of exocytosis during anaphase I. C. elegans embryos
expressing histone::GFP and labeled with the plasma membrane dye FM2-10 were
imaged using SFC every 200 milliseconds. After the chromosome separation
initiated (A), exocytic events (arrows) occurred near the spindle
(B) and spread across the cortex (C,D) before the
completion of anaphase I. Images in C and D are maximum projection summations
of several frames in which a vesicle fusion event occurs. A gap is formed
between the plasma membrane and the vitelline layer near the polar body
(E, bracket). (F) Images of the plasma membrane before and after
exocytosis, labeled with FM2-10 or a fluorescent dextran. Scale bar: 10
µm.
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Fig. 4. RNAi of OID genes affects cortical granules. (A) Organization
of the C. elegans gonad, showing approximate cell cycle stages based
upon the position of oocytes and embryos in wild-type animals. (B-D)
Cortical granules labeled with UGTP-1::GFP (indicated by arrows; insets show
higher magnification of vesicles). In wild-type animals, embryo +1 was
undergoing meiosis I and contains cortical granules, whereas embryo +2 was in
the first mitotic division and lacks cortical granules. (C)
chs-1(RNAi) oocytes and embryos showed the same UGTP-1::GFP pattern
as the wild type. (D) apc-2(RNAi) caused retention of clustered
UGTP-1::GFP-labeled cortical granules. (E) sep-1(RNAi) caused
retention of UGTP-1::GFP-labeled cortical granules in the first three embryos.
Scale bar: 10 µm.
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Fig. 5. TEM of APC/C mutant and sep-1(RNAi) embryos. (A) The
+2 embryo in a mat-1(ye121) C. elegans did not exit meiosis (asterisk
indicates chromosomes in meiotic spindle) and retained cortical granules
(arrows). (B) sep-1(RNAi) embryos were not arrested, but
retained cortical granules (arrows). (C,D) Comparison of
eggshell structures. In wild-type meiosis I embryos that contain cortical
granules, a single vitelline layer was present (C). In mitotic embryos,
cortical granules were lost and a three-layer eggshell (arrows) structure was
observed (D). The +2 embryo in APC/C mutant (E) and
sep-1(RNAi) (F) animals contained cortical granules and had a
single vitelline layer (arrows), similar to immature wild-type eggshells.
Scale bars: 3 µm in A,B; 0.5 µm in C-F.
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Fig. 6. The dynamics of the exocytic wave during anaphase I. C.
elegans embryos labeled with histone::GFP and FM2-10 were imaged every
333 milliseconds using MPLSM. (A) Total exocytic events observed in
wild-type, chs-1(RNAi) and cks-1(RNAi) embryos were nearly
twice that of sep-1(e2406) and sep-1(RNAi) embryos.
(B) Kinetic profiles of chromosome separation (plotted as a line) and
exocytic events (columns) from single embryo recordings representative of
average dynamics. Images from the movies are shown in C-K; brackets
indicate distance measured between chromosomes, arrows indicate quantitated
exocytic events. In wild type (green), degranulation initiated after
chromosomes separated by 1.5 µm, and completed before polar body extrusion.
In sep-1(RNAi) (red), chromosome separation was severely reduced, the
wave of exocytosis was reduced and took much longer. By contrast, in
sep-1(e2406) embryos (blue) chromosomes initially separated normally,
but still had a reduced level of exocytosis that began after chromosomes
separated by 2.5 µm. Scale bar: 10 µm.
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Fig. 7. Separase localizes to cortical granules in C.
elegans. (A) Before ovulation, cytoplasmic GFP::SEP-1
rapidly accumulated in the nucleus, on chromosomes (asterisks) and cortical
filaments (arrows). By metaphase I, GFP::SEP-1 was lost from filaments and
appeared on cortical granules (B,C, arrows). GFP::SEP-1
disappeared during the exocytic wave in anaphase I and accumulated on the
cortex near the polar body (D, arrow). (E,F) During
mitosis, SEP-1::GFP localized to centrosomes (arrows), chromosomes (asterisks)
and a diffuse cloud around the spindle. (G-I) Immunofluorescence with
 -SEP-1 (green) and DNA (blue). (G) Separase-labeled vesicles (arrows)
were absent from the vicinity of the spindle in an embryo that had partly
completed the exocytic wave during anaphase I (maximum projection image).
Separase localizes to six central spindle elements (arrowhead) between
homologous chromosomes and accumulates on the cortex near the polar body
(asterisk indicates sperm pronucleus). (H) During prometaphase I, separase
localized to filaments in the cortex (arrows) and in the spindle (asterisk).
(I) Separase appeared on centrosomes (arrow) and chromosomes (asterisk) during
mitosis. Scale bar: 10 µm.
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Fig. 8. Separase co-localization during meiosis I in C.
elegans. During prometaphase I, the outer kinetochore protein,
HIM-10 (A, red), co-localized in cortical filaments with separase
(B, green); merge in (C). During anaphase I, cortical granules
labeled with WGA (D, red) are also labeled with separase (E,
green); merge in F, maximum projection image of four cortical planes. A
sep-1(e2406) mutant embryo in anaphase I had cortical granules
labeled with WGA (G, red) that were not labeled with separase antibody
(H, green), although separase was still present but reduced on the
anaphase spindle (arrow); merge in I. Scale bar: 10 µm.
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Fig. 9. Regulation of cortical granule trafficking in C.
elegans. Depiction of several steps in cortical granule
trafficking and eggshell formation, along with the OID genes involved.
Separase localization is indicated. Immature oocytes form cortical granules
(red) as they grow while separase remains in the cytoplasm. Just before
ovulation, separase accumulates in the nucleus, on oocyte chromosomes (blue)
and cytoplasmic filaments. The vitelline layer (brown) separates from the
plasma membrane (green) around the time of fertilization (sperm pronucleus in
black), and cortical granules cluster near the cortex. Separase is lost from
filaments and accumulates on cortical granules as they redistribute in the
cortex. Separase is lost during the wave of cortical granule exocytosis in
anaphase I. Subsequently, the cargo of cortical granules assembles into the
chitin (pink) and lipid (red) layers, which are permeable until late meiosis
II.
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© The Company of Biologists Ltd 2007
