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Vol. 14, Issue 5, 1818-1834, May 2003
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* Institut Curie, Section Recherche, Unité Mixte Recherche 144 du Centre
National de la Recherche Scientifique, 75248 Paris, France;
Institut National de la Santé et de la Recherche Médicale U106,
Bat. Pédiatrie, Hopital Salpêtrière, 75651 Paris,
France
Submitted November 5, 2002;
Revised December 13, 2002;
Accepted January 23, 2003
Monitoring Editor: Tim Stearns
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ABSTRACT |
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 TOP ABSTRACT INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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INTRODUCTION |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). The centrosome
is typically composed of a pair of centrioles, each associated with a cloud of
pericentriolar material. The precise duplication of this organelle once during
each cell cycle is essential for the establishment of the mitotic spindle and
successful cell division. Although numerous microscopic studies have shown
that centrosome reproduction is mainly characterized by the semiconservative
centriole duplication (Kuriyama and
Borisy, 1981; Vorobjev and
Chentsov Yu, 1982; Kochanski
and Borisy, 1990), the molecular machinery that governs centrosome
duplication during the cell cycle is still unknown. It is one of the most
fascinating cell biology questions because it has long been proposed that
abnormal centrosome duplication could be at the origin of chromosome
instability and progression to a cancerous phenotype. This hypothesis has been
recently emphasized by the discovery of supernumerary abnormal centrosomes in
different human tumor cells (Lingle et
al., 1998; Pihan et
al., 1998; Brinkley,
2001).
Beside the templated semiconservative duplication of centrioles during the
cell cycle, centrioles can also self-assemble in absence of preexisting
centrioles. In particular, during the differentiation of ciliated cells from
various epithelia, hundreds of centrioles/basal bodies are assembled before
migrating and anchoring to the apical plasma membrane where they trigger cilia
formation (for review, see Dirksen,
1991). The molecular mechanisms that govern centriologenesis in
these cells also remain unknown.
Some progresses in our understanding of centrosome duplication mechanisms
came from genetic studies performed in unicellular organisms. In
Saccharomyces cerevisiae, the CDC31 and KAR1 gene
products were shown to be necessary for the initiation of the spindle pole
body (SPB, the functional homolog of the animal centrosome) duplication,
because cdc31 and kar1 mutants are both characterized by a
large bud, a G2 DNA content, and a single unduplicated SPB
(Baum et al., 1986;
Rose and Fink, 1987). Both
proteins are specifically localized to the half-bridge of the SPB on which the
satellite (the precursor of the new SPB) assembles (Spang et al.,
1993,
1995). A direct interaction
between Kar1p and Cdc31p has been described and Kar1p seems to be required for
the correct localization of Cdc31p, which could then interact with a
downstream uncharacterized effector and initiate SPB duplication
(Biggins and Rose, 1994;
Vallen et al., 1994;
Spang et al.,
1995).
Genetic approaches in the green algae Chlamydomonas reinhardtii
allowed to identify several mutants in the centriole/basal body duplication
cycle. In particular, the variable flagella number mutant
vfl2 is partially defective in templated centriole assembly and in
their subsequent segregation during the cell cycle
(Taillon et al.,
1992; Marshall et
al., 2001). Interestingly, the VFL2 gene encodes a
small protein called centrin (Crcentrin), which is a homolog to Cdc31p, both
proteins belonging to the EF-hand superfamily of calcium-binding proteins
(Taillon et al.,
1992).
Three centrin proteins (centrin1p, 2p, and 3p) have been identified so far
in mammals (Lee and Huang,
1993; Errabolu et
al., 1994; Middendorp
et al., 1997). Sequence comparison revealed that
centrin3p is close to ScCdc31p, whereas centrin1p and 2p are closer to
Crcentrin (Middendorp et al.,
1997). In contrast to centrin1p, which is mostly expressed in male
germ cells, centrin2p and 3p were shown to be ubiquitously expressed, and both
proteins are localized in the distal lumen of centrioles and in the
procentriole bud (Paoletti et
al., 1996; Hart et
al., 1999). Their potential implication in the centrosome
duplication process during the cell cycle was investigated in different
cellular systems. Ectopic expression of both human recombinant proteins in
Xenopus laevis embryos induced undercleavage of injected blastomeres
and overexpression of Hscentrin3p was shown to impair centrosome duplication
in this system (Paoletti et al.,
1996; Middendorp et
al., 2000). Moreover, it was recently shown that inactivation
of centrin2p expression in HeLa cells by RNA interference results in the
inhibition of centriole duplication and subsequent defects in the cell cycle
progression (Salisbury et al.,
2002). Together, these results obtained in different species, from
yeasts to mammals, suggest a key role for centrin proteins in the centrosome
duplication process.
In the present work, we report the identification and characterization of a novel, tissue-specific mammalian centrin that we called centrin4p.
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MATERIALS AND METHODS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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Reverse Transcriptase-Polymerase Chain Reaction (RT-PCR)
For RT-PCR analysis of centrin2 or centrin4 mRNA expression, first-strand
cDNA synthesis was performed with 1 µg of the different RNA samples by
using 10 pmol of an oligo(dT)-adaptor primer (Invitrogen). Amplification
reactions were performed using specific primers for centrin2 or centrin4
(Table 1). PCR conditions were
as follows: one cycle (94°C, 2 min); 37 cycles (94°C, 30 s; 55°C,
45 s; 72°C, 1 min), and one cycle (72°C, 5 min). Final products
obtained from kidney RNA sample were cloned and sequenced to confirm the
specificity of the PCR amplifications.
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3' and 5' Rapid Amplification of cDNA Ends (RACE)
For 3' RACE of centrin4 mRNA, first-strand cDNA synthesis was
performed with 1 µg of brain (hemisphere) total RNA by using 10 pmol of an
oligo(dT)-adaptor primer (Invitrogen). As a control for subsequent
amplifications, the same reaction was also performed in absence of the reverse
transcriptase. Two rounds of amplification were done with 10 pmol of each
primer (Table 1). The final
amplification product, which corresponds to the 3'-untranslated region
(3'-UTR) of centrin4 mRNA, was cloned in a Bluescript SK+ vector,
sequenced, and used to prepare the cRNA probe for in situ hybridization.
5' RACE was carried out essentially as 3' RACE, except that the first-strand cDNA synthesis was performed using 10 pmol of a specific primer for centrin4 (Table 1). After oligo(dC) tailing of the cDNA according to manufacturer's recommendations (Invitrogen), two successive rounds of amplification were performed using primers listed in Table 1.
PCR Amplification of Genomic DNA
Centrin4 gene (CETN4) cloning was carried out by a PCR
amplification approach on genomic DNA prepared from C57B16/DBA2 mouse tail
(Miller et al.,
1988). The first amplification was performed with 100 ng of
genomic DNA and 10 pmol of primers listed in
Table 1. The PCR conditions
were as follows: one cycle (94°C, 2 min); 35 cycles (94°C, 30 s;
55°C, 45 s; 72°C, 2 min), and one cycle (72°C, 5 min). The second
round of amplification was performed using 0.1% of the first PCR amplification
products under the following conditions: one cycle (94°C, 2 min); 35
cycles (94°C, 30 s; 62°C, 45 s; 72°C, 2 min) and one cycle
(72°C, 5 min). The final amplification product was cloned in a Bluescript
SK+ vector and sequenced.
Northern Blot Analysis
To analyze the expression profile of centrin4 mRNA, 20 µg of total RNA
from different tissues were separated on a denaturing agarose gel containing
formaldehyde (Sambrook et al.,
1989). Samples were transferred overnight to a Hybond
N+ nylon membrane (Amersham Pharmacia Biotech) using 50 mM NaPi, pH
7.2 as a transfer buffer, and visualized by methylene blue coloration.
Prehybridization was performed in 1 M NaPi pH 7.2, 7% SDS, 1 mM EDTA at
68°C for one hour. A cDNA fragment corresponding to 3' UTR of
centrin4 mRNA (see above) was 32P-labeled using the rediprime II
kit (Amersham Pharmacia Biotech) and purified using a Probe-Quant G-50 column
(Amersham Biosciences UK, Little Chalfont, Buckinghamshire, UK). The purified
probe (106 cpm/ml) was added to fresh hybridization buffer and
incubation was performed overnight at 65°C. After three washes in 40 mM
NaPi buffer containing 1% SDS, membranes were subjected to an autoradiography
analysis.
In Situ Hybridization
Adult mouse brains were collected and immediately frozen in isopentane.
Coronal sections (15 µm in thickness) were performed on a cryostat,
collected on SuperFrost Plus glass slides, and stored at —80°C
before use. Brain sections were postfixed for 15 min with 4% (wt/vol)
paraformaldehyde in phosphate-buffered saline (PBS), rinsed three times in
PBS, and then acetylated with 0.25% acetic anhydride/0.1 M triethanolamine for
10 min. After three washes in PBS, sections were dehydrated in ethanol and
air-dried.
One microgram of a Bluescript plasmid containing the 3'-UTR of
centrin4 mRNA was linearized with BamHI or EcoRI to generate
sense or antisense cRNA probes. In vitro transcription was performed using the
Promega kit and T7 or T3 RNA polymerase in the presence of 35S-UTP
(<1000 Ci/mmol; Amersham Biosciences UK). Hybridization was performed in a
humid chamber overnight at 48°C by using 106 cpm/slide of
35S-labeled RNA probe in 20 mM Tris-HCl pH 7.4, 5 mM EDTA, 0.3 M
NaCl, 10 mM phosphate buffer, 10 mM dithiothreitol (DTT), 50% formamide, 10%
dextran sulfate, 1x Denhardt's solution, and 0.5 mg/ml yeast total RNA
(Sigma Chemical, Poole, Dorset, United Kingdom). Sections were washed in
5x SSC, 1.6 mg/ml DTT at 42°C for 30 min, 2x SSC, 50%
formamide, 12.5 mg/ml DTT at 60°C for 20 min and treated with 20 µg/ml
RNAse A (Roche Diagnostics, Mannheim, Germany) for 30 min at 37°C. After
two washes in 2x SSC and 0.1x SSC, 15 min each at 37°C,
sections were dehydrated in ethanol and air-dried. Sections were first apposed
to hyperfilms (
-max; Amersham Biosciences UK) for 5 d and then dipped in
photographic emulsion (NTB-2; Kodak, Tokyo, Japan) and exposed for 2 to 3
weeks. After development, sections were counterstained with cresyl violet.
DNA Constructs and Cell Transfection
The different Hscentrin2p and Mmcentrin4p constructs were generated by a
PCR approach and subcloned in the mammalian expression vector pcDNA3
(Invitrogen) in fusion with an NH2-terminal myc epitope tag or in
the pGFP-C1 vector (BD Biosciences Clontech, Palo Alto, CA). The Nter4, Cter4,
and III-4 domains of centrin4p correspond to amino acids 1–100,
89–168, and 1–138, respectively. The Nter2 and Cter2 domains of
Hscentrin2p correspond to amino acids 1–104 and 93–172. The
sequence corresponding to amino acids 232–272 of Kar1p
(Spang et al., 1995)
was inserted in pGFP-N1 vector (BD Biosciences Clontech) downstream of an
initiating methionine.
Mouse L929 or human HeLa cells were grown as monolayers in DMEM containing
10% (vol/vol) inactivated fetal calf serum (Invitrogen) at 37°C in 5%
CO2. For transient expression experiments, 5 x 106
cells were transfected by electroporation with 50 µg of plasmid DNA at 300
V and 960 µF by using a gene pulser (Bio-Rad, Hercules, CA). HeLa cell
synchronization by a double thymidine block was performed as described by
Stein et al.
(1994).
Antibodies
Rabbit anti-centrin4p antiserum was generated against the following
synthetic peptide conjugated to KLH: K-A-A-K-V-E-L-N-D-T-Q-K-Q-E-C. GT335 is a
monoclonal antibody (mAb) directed against glutamylated tubulin, which stain
axonemes of ciliated cells (Wolff et
al., 1992; Tournier
et al., 1998). CC310 is a mAb raised against ciliary
cortices of quail oviduct epithelium, which stain striated rootlets in
ciliated epithelia (Klotz et al.,
1986; Peraldi-Roux et
al., 1991). Rabbit anti-
-tubulin antiserum has been
described previously (Moudjou et
al., 1996). Commercial monoclonal antibodies were anti-myc
(9E10; Santa Cruz Biotechnology, Tebu, France) and anti-green fluorescent
protein (GFP) (clones 7.1 and 13.1; Roche Diagnostics).
Immunofluorescence
Transfected cells growing on coverslips were briefly extracted with 0.5%
NP-40 in PHEM buffer (45 mM PIPES, 45 mM HEPES, pH 6.9, 10 mM EGTA, 5 mM
MgCl2) for 20 s and fixed in PBS containing 2% paraformaldehyde for
10 min at room temperature. Cells were subsequently permeabilized with 0.2%
Triton X-100 in PBS for 10 min and incubated with 100 mM glycine in PBS for 15
min. Coverslips were then preincubated with 3% bovine serum albumin in PBS
containing 0.1% Tween 20 for 30 min and incubated 1 h with primary antibodies
in the same blocking buffer. After three washes with 0.1% Tween 20 in PBS,
coverslips were incubated 1 h with rhodamine-conjugated secondary antibodies
(Jackson Immunore-search Laboratories, West Grove, PA). After three new
washes, coverslips were finally mounted with AF1 antifadent mountant solution
(Citifluor; City University, London, England).
Frozen brain sections (15 µm in thickness) were air-dried for 5 min at room temperature and fixed in methanol at —20°C for 6 min. Brain sections were then blocked with 3% bovine serum albumin in PBS containing 0.1% Tween 20 for 2 h and incubated overnight at room temperature with primary antibodies. After three washes with 0.1% Tween 20 in PBS, sections were incubated 1 h with secondary antibodies. Nuclei were stained using Hoechst 33528 at 5 µg/ml for 5 min. After three new washes, brain sections were finally mounted with AF1 antifadent mountant solution.
Quantification
The relative quantification of the accumulation of the different
GFP-centrin constructs to centrioles was performed as follows. HeLa cells were
transfected with the different GFP-centrin constructs in the same conditions
and 24 h later were briefly extracted with 0.5% NP-40 in PHEM buffer for 20 s
before fixation with 2% paraformaldehyde in PBS for 10 min at room
temperature. Then 10 sequential Z-axis 12-bit images were collected in
0.2-µm steps by using a DMIRBE microscope (Leica, Wetzlar, Germany)
equipped with a piezoelectric device, which allowed to cover the entire
centriolar signal in each transfected cell. For each Z-series, the maximal
intensity signal to centriole was determined using MetaMorph software
(Universal Imaging, Downingtown, PA) and the immediately surrounding
background was subtracted. We checked that preextraction and paraformaldehyde
fixation did not affect the GFP signal to centriole. Data are presented as the
mean values obtained in 30 transfected cells in each condition for one given
experiment. Results are representative of three independent experiments.
Coimmunoprecipitations
HeLa cells (5 x 106 cells) were cotransfected with 10
µg of an NH2-terminal myc epitope-tagged Mmcentrin4p or
Hscentrin2p construct and 40 µg of a Kar1p peptide-GFP plasmid. Twenty-four
hours later, cells were lysed in one-dimensional (1-D) buffer (50 mM Tris-HCl
pH 8, 150 mM NaCl, 1 mM DTT, 0.5% NP-40) containing 2 mM CaCl2 or 2
mM EGTA. Cellular debris were removed by a centrifugation at 10,000 x
g for 10 min at 4°C, and supernatants were then incubated with 5
µg of anti-GFP monoclonal antibodies coupled to protein G-Sepharose 4 Fast
Flow beads (Amersham Biosciences UK) for 1 h at 4°C. After four washes in
1-D buffer containing 2 mM CaCl2 or 2 mM EGTA, immunoprecipitates
were solubilized in SDS-PAGE sample buffer and processed for immunoblot
analysis.
Calcium Binding and Electrophoretic Shifts
HeLa cells (5 x 106 cells) transfected with the different
GFP-centrin constructs were lysed in three-dimensional buffer (0.5% NP-40,
0.5% deoxycholate, 0.05% SDS) for 10 min at 4°C and centrifuged at 10,000
x g for 10 min at 4°C. Supernatants were incubated with 5
µg of anti-GFP monoclonal antibodies coupled to protein G-Sepharose 4 Fast
Flow beads (Amersham Biosciences UK) for 1 h at 4°C under mild agitation.
After four washes in 1-D buffer, immunoprecipitates were solubilized in
SDS-PAGE sample buffer. One-dimensional SDS-PAGE (12% acrylamide) and protein
transfer on a nitrocellulose membrane were performed using standard protocols
(Sambrook et al.,
1989). After transfer, the membrane was washed in 10 mM
imidazole-HCl pH 6.8, 60 mM KCl, 5 mM MgCl2 for 90 min and then
incubated in the same buffer containing 20 µCi of 45Ca for 20
min (Maruyama et al.,
1984). After three washes in distilled water for 2 min each, the
membrane was processed for an autoradiography analysis.
For electrophoretic shifts analyses, transfected cells were lysed in 1-D buffer containing 2 mM CaCl2 or 2 mM EGTA. After a centrifugation at 10,000 x g for 10 min, supernatants were processed for immunoblot analyses with 2 mM CaCl2 or 2 mM EGTA in gels and 0.1 mM CaCl2 or 2 mM EGTA in running buffers.
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RESULTS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). The
single-length 5'-UTR of 87 nucleotides has a high C + G (73.6%) content
and the 3'-UTR of 464 nucleotides in length contains a perfectly
conserved polyadenylation signal (AATAAA) 13 bases upstream of the poly(A)
addition site (Figure 1A). The
open reading frame encodes a novel 168 amino acid protein with a calculated
molecular mass of 19,200 Da, that we propose to name centrin4p. Like other
centrin proteins, centrin4p has an acidic isoelectric point (pI = 4.74) and
contains four potential EF-hand calcium-binding domains, which consist of a
central calcium-binding loop flanked on both sides by a 
-helix
(Figure 2A). Comparison of the
four calcium-binding loop sequences with the consensus sequence predicted that
only the fourth EF-hand calcium-binding domain of centrin4p could be
functional (Figure 2B; see
below) (Marsden et al.,
1990).
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Amino acid sequence comparison with other centrin proteins revealed that
centrin4p is closer to the subgroup of centrin2p/centrin1p and Crcentrin than
the subgroup containing centrin3p and yeast centrins
(Figure 2C). In particular,
Mmcentrin4p and Mmcentrin2p that are closely related share 74% identity and
87% similarity and differ mostly in two short amino acid domains (underlined
in Figure 2A). The first domain
corresponds to the amino terminal region of Mmcentrin4p that is the most
divergent region between all known centrins and in part differentiates centrin
proteins from the related EF-hand calcium-binding protein calmodulin
(Figure 2A). The second
specific amino acid domain of Mmcentrin4p is located between the second and
third EF-hand calcium-binding domains, a region corresponding to the central
helix of calmodulin (Figure
2A). Structural studies of calmodulin have revealed that the first
two and the last two EF-hands form two globular functional units separated by
a flexible central helix (for review, see
Nelson and Chazin, 1998). The
ability of calmodulin to recognize different target proteins is a consequence
of the flexibility of this central helix, which is able to bend at the amino
acid Ser81, thereby allowing the two globular domains to wrap around target
peptides (O'Neil and DeGrado,
1990). This amino acid was also shown to be a substrate of casein
kinase II in vitro (consensus phosphorylation site, S/T-X-X-E)
(Quadroni et al.,
1994). We noticed that the subgroup of centrin2p/centrin1p and
Crcentrin have a serine or a threonine at the equivalent position (and share a
potential casein kinase II phosphorylation site), whereas the subgroup of
centrin3p and yeast centrins have a proline residue
(Figure 2A, arrowhead).
Interestingly, centrin4p contains a negatively charged amino acid at the
equivalent position, which could confer conformational specificities
(Figure 2A, arrowhead).
We next used the sequence of the two specific domains of centrin4p to
search for homologs in other species. We identified numerous EST in some
mammalian species (rat, cow, pig, and human) that allowed to obtain the full
open reading frame of rat (accession no. BG662613
[GenBank]
) and cow centrin4p
(accession nos. AV591122
[GenBank]
and BE667637
[GenBank]
) (our unpublished data). On the other
hand, we were unable to identify EST for centrin4p in nonmammalian species.
Finally, we identified in databases a genomic clone containing the full
sequence of the mouse centrin4 gene (CETN4, accession no. AL645982
[GenBank]
).
We used mouse tail genomic DNA to amplify a part of the gene encompassing the
coding exons (see MATERIALS AND METHODS). Sequencing revealed two nucleotide
differences with the cDNA in the coding region but no differences at the amino
acid level (our unpublished data). The centrin4 gene, located on chromosome 3,
contains five exons and four introns with a large intron positioned just after
the initiating methionine-coding triplet
(Figure 1B). Comparison with
the other murine centrin genes showed that in contrast to CETN3,
CETN4, and CETN2 genes share exactly the same intron/exon
junctions (centrin1 gene is intronless and was proposed to arise from a
retrotransposition of centrin2 mRNA, (Hart
et al., 1999) (Figure
1C). This observation confirms the phylogenetic relationship
between centrin4p and centrin2p and suggests that the respective genes arise
from a duplication of a common ancestor. Because they are closely related, we
compared the properties of centrin4p and centrin2p.
Tissue-specific Expression of Centrin4 mRNA
Given the relationship between CETN4 and CETN2 genes, we
first wanted to determine whether centrin4 mRNA is also ubiquitously
expressed. Northern blot analysis of total RNA from various adult mouse
tissues with a specific 32P-labeled 3'-UTR probe revealed
that centrin4 mRNA possesses a tissue-specific expression profile. Centrin4
mRNA is highly expressed in the brain (cerebellum and cerebral hemispheres),
lung, kidney, and ovary (Figure
3A). A very low signal was also detected in spleen, whereas
centrin4 mRNA was undetectable in other tissues (testis, colon, stomach,
thymus, skeletal muscle, heart, intestine, and liver). This result was further
confirmed by a RT-PCR analysis, which gave qualitatively the same expression
profile (Figure 3B).
Surprisingly, using primers designed to amplify the full coding sequence of
centrin4p, we obtained one major band at the expected size and one or two
lower bands in the same tissues (Figure 3B,
arrows in A and B). The different bands were then subcloned and
sequenced. As expected, the major band corresponds to the full coding sequence
of centrin4p, indicating that the PCR amplification was specific. Sequence
analysis revealed that bands A and B correspond to the same coding sequence
with an internal deletion of different sizes (our unpublished data). More
importantly, these internal deletions correspond exactly to a deletion of the
sequence of exon IV (band A) or to a deletion of the sequence of exons III and
IV (band B) (Figure 3C). The
two corresponding mRNAs are thus most probably transcribed from the same gene
but correspond to differential splicing variants of centrin4 mRNA. The
corresponding proteins possess a deletion of the third EF-hand or of the
second and third EF-hands and were called Mmsplice4A and Mmsplice4B,
respectively (Figure 3C). Finally, using primers designed to amplify the full coding sequence of
centrin2p and centrin3p, only one band was detected at the expected size in
all tissues tested (Figure 3B;
our unpublished data). Sequence analysis confirmed that the PCR products
correspond to the centrin2p or centrin3p coding sequence (our unpublished
data).
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Together, our results show that in contrast to centrin2 and centrin3, centrin4 mRNA has a tissue-specific expression profile and possesses at least two splice variants.
Ectopically Expressed Centrin4p Localizes to Centrioles
Previous work showed that mammalian centrin2p and centrin3p are present in
the distal lumen of centrioles and in the procentriole bud
(Paoletti et al.,
1996; Middendorp et
al., 1997). In a first step to examine its subcellular
localization, centrin4p was ectopically expressed as a green fluorescent
protein (GFP) fusion protein. As the same results were obtained in different
cell lines, we illustrate the localization of centrin4p in HeLa cells. In
asynchronous fixed HeLa cells, one or two pairs of dots located near the
nucleus were observed (Figure
4A). Double immunostaining with anti--tubulin antibodies
confirmed that these dots correspond to centrioles
(Figure 4A, G1). However, in a
given pair, the two dots frequently differed in their intensity
(Figure 4A, insets). To follow
the modification of the dot staining during the centrosome duplication cycle,
cells were synchronized at the G1/S transition by a double thymidine block and
then allowed to progress in S, G2, and M phases. During the progression in the
cell cycle, the intensity of the two dots in a given pair became progressively
comparable, whereas the distance separating the two dots increased (compare
Figure 4A, G1/S and G2). These
observations strongly suggest that ectopically expressed centrin4p accumulates
to procentrioles during their elongation and is most probably located at their
distal part, as previously demonstrated for centrin2p
(Paoletti et al.,
1996). However, comparison of the localization of GFP-centrin2p
and GFP-centrin4p in living cells gave a striking difference
(Figure 4B). Both proteins were
in a large part diffusely located in the cytoplasm but, in contrast to
GFP-centrin2p, the accumulation of GFP-centrin4p to centrioles was more hardly
detected (Figure 4B, arrow).
This difference does not depend upon their respective stability because we
checked that both proteins were expressed to a very similar level (our
unpublished data). Relative quantification (see MATERIALS AND METHODS)
revealed that the accumulation of GFP-centrin4p to centrioles is in average 2
or 3 times lower than GFP-centrin2p (or GFP-centrin3p)
(Figure 4C).
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To further investigate the centriolar targeting of centrin4p, we next
examined the intracellular localization of its two splice variants. In
contrast to centrin4p, splice4A and splice4B were never detected at the
centrioles, as identified by a -tubulin staining
(Figure 5A). This suggests that
the third EF-hand of centrin4p is at least necessary for its centriolar
targeting. In an attempt to define a minimal amino acid domain necessary for
its centriolar localization, we generated different constructs of centrin4p
containing either the two first or the two last EF-hand calcium-binding
domains (Nter4 and Cter4 domains, respectively) or lacking only the last
EF-hand calcium-binding domain (III-4 domain)
(Figure 6B). Transient
expression in HeLa cells showed that all of these truncated forms were unable
to accumulate to centrioles, suggesting that the four EF-hand calcium-binding
domains of centrin4p are essential for its proper localization
(Figure 5B; our unpublished
data). Surprisingly, using equivalent constructs of Hscentrin2p, we observed
that the COOH-terminal domain (Cter2) of centrin2p accumulates to centrioles,
whereas the NH2-terminal domain (Nter2) was diffusely located in
the cytoplasm (Figure 5B). The
same result was also obtained with the two truncated forms Cter3 and Nter3 of
Hscentrin3p (our unpublished data). Moreover, relative quantification showed
that the COOH-terminal domain Cter2 (or Cter3) accumulates to centrioles to a
similar level as the full-length protein, suggesting that this domain is
necessary and sufficient for the proper localization of centrin2p (or
centrin3p) (Figure 4C).
Together, these results show that ectopically expressed centrin4p, but not its
two splice variants, is able to accumulate to centrioles and procentrioles.
However, the centriolar anchoring mechanism seems to differ between centrin4p
and centrin2p (or centrin3p) because the four EF-hand calcium-binding domains
of centrin4p are essential for its centriolar localization, whereas only the
two last EF-hand domains of centrin2p (or centrin3p) are needed for its proper
localization. One possibility to explain the different behavior between
centrin4p and centrin2p (or centrin3p) could be that they did not recognize
the same centriolar partners (see below).
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Centrin4p Does Not Bind to Kar1p Peptide
Despite numerous investigations, the centriolar partners of mammalian
centrins are still unknown. In contrast, in S. cerevisiae, the
centrin protein Cdc31p anchors to the SPB through its interaction with Kar1p
(see INTRODUCTION). The Cdc31p-binding peptide in Kar1p was previously
characterized and was shown to be recognized by Hscentrin2p in vitro in a
calcium-regulated manner (Spang et
al., 1995; Geier et
al., 1996). To investigate whether Kar1p peptide is a target
of centrin4p, NH2-terminal myc epitope-tagged Mmcentrin4p or
Hscentrin2p were cotransfected in HeLa cells with Kar1p peptide in fusion with
GFP (Figure 6A). The
interactions were tested by examining whether centrin proteins were
coimmunoprecipitated with Kar1p peptide in presence
(Ca2+) or absence of calcium (EGTA). We observed that
centrin2p effectively binds to Kar1p peptide and that this interaction is
calcium dependent (Figure 6A, bottom). In contrast, no interaction between centrin4p and Kar1p peptide could
be detected independently of the presence of calcium. As centrin proteins were
expressed to a similar level (Figure
6A, top), this suggests that they do not recognize the same target
peptide and that they could have different centriolar partners.
Centrin4p Is a Ca2+-binding Protein
As the four potential EF-hand calcium-binding domains of centrin4p seem to
be essential for its proper localization to centrioles, we wanted to determine
which domain(s) can bind a calcium ion. GFP-tagged centrin4p, its two splice
variants, and the different truncated forms were ectopically expressed in HeLa
cells and immunoprecipitated using anti-GFP monoclonal antibodies. Proteins
were then separated by gel electrophoresis, transferred on a nitrocellulose
membrane, and either revealed with anti-GFP antibodies or incubated with
45Ca (Figure 6B).
Autoradiography revealed that the full-length centrin4p binds calcium
(Figure 6B, lane 2). A
radioactive signal was also obtained with the COOH-terminal domain (Cter4) and
the two splice variants (Splice4A and 4B) of centrin4p that share only the
fourth EF-hand calcium-binding domain. However, the signals obtained were
weaker than with centrin4p and could reflect that deletions of calcium-binding
domains modify the conformational stability of these truncated forms. In
contrast, no signal was obtained with the NH2-terminal domain
(Nter4) or with the truncated form (III-4 domain) lacking only the last
EF-hand calcium-binding domain. Together, these results strongly suggest that
only the fourth EF-hand calciumbinding domain of centrin4p is functional, in
agreement with sequence analyses (Figure
2B). We further investigated electrophoretic mobility of centrin4p
(our unpublished data) and of its COOH- and NH2-terminal domains
(Cter4 and Nter4) in presence or absence of calcium, because it is well known
that calmodulin shows a Ca2+-dependent migration
behavior in SDS-PAGE (Figure
6C). We observed that centrin4p (our unpublished data) and its
COOH-terminal domain migrate with a lower apparent molecular weight in
presence (Ca2+) than in absence of calcium (EGTA),
suggesting that the Ca2+-bound form could adopt a more
compact conformation (Figure
6C). In contrast, the migration behavior of the
NH2-terminal domain was unaffected in both conditions
(Figure 6C). These results are
in good agreement with our observation that centrin4p binds calcium only
through its fourth EF-hand calcium-binding domain.
In the Adult Mouse Brain, Centrin4 mRNA Is Specifically Expressed in
Ciliated Cells
Centrin2p and centrin3p that seem to be involved in the regulation of
centriole duplication in proliferating cells are both ubiquitously expressed
in adult mouse tissues (see INTRODUCTION). In contrast, we showed by Northern
blot analyses that centrin4 mRNA has a restricted expression profile with an
unexpected high expression in the adult brain (cerebellum and hemispheres), a
tissue containing mostly quiescent cells. To better understand the potential
function(s) of centrin4p, we examined its distribution in this particular
tissue by in situ hybridization with a specific 35S-labeled cRNA
probe corresponding to the 3'-UTR of centrin4 mRNA. A strong expression
of centrin4 mRNA was detected in cells lining the different ventricular
cavities (i.e., lateral ventricles, third and fourth ventricles)
(Figure 7, A–F). Centrin4
mRNA was also detected in the choroid plexus epithelium inside the lateral and
fourth ventricles (Figure 7, B and
F, arrowheads) and to a weaker level in the hippocampus (Ammon's
horn and dentate gyrus) (Figure 7, C and
D). Finally, no signal was detected in other brain areas. This
restricted expression profile was very informative because it is known that
ependymal cells lining the ventricles as well as cells from the plexus choroid
have numerous cilia on their surface, which drive the transport of
cerebrospinal fluid (Roth et al.,
1985). Moreover, the presence of a primary nonmotile cilium in
some neuronal cells, in particular hippocampal cells, has been described
previously (Popov and Tsyganova,
1996; Handel et al.,
1999). Together, these results suggest that centrin4 mRNA is
specifically expressed, at least in the brain, in cells bearing motile cilia
and to a lower extent in some cells with a primary nonmotile cilium.
|
Centrin4p Is Localized to Basal Bodies in Ciliated Cells
To confirm the expression of centrin4p in ciliated cells, we generated a
rabbit polyclonal antiserum directed against a specific amino-terminal peptide
(see MATERIALS AND METHODS). We first examined its specificity by an
immunoblot analysis. Mouse L929 cells were transiently transfected with
GFP-tagged centrin2p, centrin3p, or centrin4p and processed for immunoblotting
with anti-centrin4p or anti-GFP antibodies
(Figure 8A). We observed that
the anti-centrin4p antiserum recognized one polypeptide corresponding to
GFP-centrin4p but did not cross-react with GFP-centrin2p or GFP-centrin3p.
Moreover, no other protein was detected in cell mouse extracts
(Figure 8A). We next tested the
specificity of this antiserum by immunofluorescence on mouse brain slices. The
anti-centrin4p antiserum yielded a strong signal in cells lining the
ventricles (see below) that was totally abolished by a preincubation with the
corresponding peptide (Figure
8B). Finally, we were unable to detect endogenous centrin4p by a
Western blot analysis on mouse brain extracts probably due to the fact that
this protein is expressed in a very small fraction of cells. Together, these
results show that our antiserum specifically recognizes centrin4p.
|
Using this antiserum, centrin4p was exclusively detected in the brain in
cells lining the different ventricles and in the choroid plexus, in good
agreement with our in situ hybridization results
(Figure 8C, left). However, we
were unable to detect centrin4p in hippocampal cells, possibly as a
consequence of a lower expression level in these cells, which possess only a
monocilium. To unambiguously identify cells expressing centrin4p, we performed
a double-immunostaining with a mAb (CC310) that specifically recognizes
ciliary rootlets in ependymal and choroidal cells
(Peraldi-Roux et al.,
1991). This experiment confirmed that centrin4p is exclusively
expressed in ciliated cells (Figure
8C). Closer examination revealed a punctuate staining of centrin4p
that is less abundant in choroidal than in ependymal cells
(Figure 8D, top, insets
correspond to choroidal cells). This dot staining does not colocalize with the
ciliary rootlet staining in ependymal and choroidal cells
(Figure 8D, top). Moreover, on
a lateral view of choroidal cells, centrin4p staining is clearly localized in
a more apical position than the ciliary rootlet staining (arrowheads).
Together, these observations strongly suggest that centrin4p is localized to
basal bodies, in agreement with our observations that centrin4p accumulates to
centrioles when ectopically expressed in different cell lines. Finally, we
performed a double-immunostaining using GT335, a mAb directed against
glutamylated tubulins, which stain axonemes of ciliated cells
(Wolff et al., 1992;
Tournier et al.,
1998). Centrin4p staining was restricted at the base of cilia and
no colocalization was detected in cilia axonemes
(Figure 8D, bottom). Together,
our results show that centrin4p is specifically expressed in ciliated cells in
the brain and strongly suggest that it is concentrated to basal bodies at the
origin of cilia axonemes.
|
DISCUSSION |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). In contrast to centrin4p, its two splice variants were
never found associated with centrioles. We do not investigate at the present
time the regulation of the splicing of centrin4 mRNA, but our observations
raise the possibility that centrin4p activity could be regulated by a
posttranscriptional regulation mechanism.
Examination of the subcellular localization of centrin4p expressed in
different cell lines showed that this protein shares with other mammalian
centrins the ability to accumulate to centrioles but with different
properties. In fact, centrin4p accumulates to centrioles at a lower level than
centrin2p or centrin3p. Moreover, we demonstrated that the COOH-terminal
domain (constituted of the two last EF-hand calcium-binding domains) of
centrin2p and centrin3p is necessary and sufficient for their localization to
centrioles, whereas both NH2 and COOH-terminal domains of centrin4p
are required for its proper localization. Based on the relationship between
centrin proteins and calmodulin, centrin4p could have a target interaction
mechanism more similar to calmodulin than other centrins, in spite of the fact
that only its fourth EF-hand calcium-binding domain seems to be functional. In
fact, in vitro structural studies have shown that calmodulin binds both ends
of its target peptides through their interaction with its NH2 and
COOH-terminal domains (for review, see
Zhang and Yuan, 1998). On the
other hand, the observation that only half of centrin2p or centrin3p is
sufficient for their anchoring to centrioles was totally unexpected. However,
it could be related to mutational studies of the yeast centrin, suggesting
that the COOH-terminal domain of Cdc31p mediates its interaction with Kar1p
and possibly its correct localization to the SPB
(Ivanovska and Rose, 2001).
Moreover, recent structural analyses of C. reinhardtii centrin showed
that its interaction with Kar1p peptide in vitro is primarily mediated by its
COOH-terminal domain (Veeraraghavan et
al., 2002). Thus, the target interaction mechanism of
centrin2p and centrin3p could be different from that of calmodulin and
centrin4p and involve mostly their COOH-terminal domain. Interestingly, one
centrin-related protein was recently discovered in Dictyostelium
discoideum, which possesses only two EF-hands in its COOH-terminal
domain, suggesting that this protein could share the same target interaction
mechanism with centrins 2p/3p (Daunderer
et al., 2001).
In contrast to centrin2 and centrin3 mRNA, which are ubiquitously
expressed, we observed that centrin4 mRNA is highly expressed in the brain,
lung, kidney, and ovary and is expressed to a very low level in the spleen.
Interestingly, this expression profile is very similar to that of Polaris, the
product of the Tg737 gene, which is expressed in brain, kidney, lung,
and in the reproductive tracts (oviduct and testis)
(Taulman et al.,
2001). Moreover, in brain, Polaris shares the same cellular
distribution with centrin4p and is specifically expressed in multiciliated
ependymal and choroidal cells where it is localized to basal bodies and cilia
axonemes (Taulman et al.,
2001). In the other tissues, Polaris was detected in the ciliated
lung epithelium, in sperm, and in kidney cells harboring a monocilium where it
is also localized to basal bodies and cilia or flagella axonemes. Thus,
similar tissue expression profiles as well as similar cellular and subcellular
localizations in the brain raise the possibility that centrin4p could be
expressed in other ciliated epithelia bearing motile cilia (possibly ciliated
epithelia from lung and oviduct). Centrin4p could be also expressed in
different cells harboring a primary immotile cilium. Interestingly, presence
of cells harboring a monocilium in kidney, spleen, and ovary has been
described previously (Abdel-Bari and
Sorenson, 1965; Motta et
al., 1971). Further experiments will be performed to
investigate this hypothesis. We also noticed similarities in the expression
pattern of centrin4 and that of HFH-4 mRNA, which encodes a forkhead
transcription factor involved in the ciliogenesis process of lung, oviduct,
choroid plexus, and ependyma epithelia
(Blatt et al., 1999;
Brody et al., 2000).
The target genes regulated by this transcription factor are still unknown, but
a DNA consensus sequence specifically recognized by HFH-4 was identified
(Lim et al., 1997).
Interestingly, we found in the CETN4 gene sequence a putative HFH-4
binding site localized upstream of the transcription initiation site (our
unpublished data). Thus, it will be of interest to investigate whether
CETN4 gene expression is under control of this transcription
factor.
We observed that centrin4p is specifically expressed in ciliated cells in
the adult mouse brain where it is localized to basal bodies at the origin of
cilia axonemes, in agreement with its ability to accumulate to centrioles when
ectopically expressed in different cell lines. Examination of the expression
profiles of centrin2p and centrin3p in the brain showed that both proteins are
also expressed in ciliated cells lining the different ventricles where they
are localized to basal bodies (Gavet et al., unpublished data).
However, both proteins are broadly expressed in the brain and are found
associated to the centrosome in neuronal and glial cells (Gavet et
al., unpublished data). Thus, the more restricted expression profile of
centrin4p versus centrins 2p/3p in the brain is a first indication that
centrin4p could be more specifically involved in the differentiation process
of some ciliated cells. In agreement with this hypothesis, we observed that
centrin4p expression correlates with the apparition of CC310 immunoreactivity
in ependymal cells during brain development (Gavet et al.,
unpublished data). The ciliogenesis process in multiciliated cells of
vertebrate tissues has been morphologically described (for review, see
Dirksen, 1991). The first
cytoplasmic structures involved in centriologenesis are fibrogranular
aggregates that consist of clouds of filamentous material associated with
electron-dense granules. Immature centrioles occur around these electron-dense
granules and then mature and migrate to the apical membrane where they trigger
axonemal microtubule polymerization and cilia formation. Interestingly, during
the differentiation of nasal epithelial ciliated cells in culture, centrin2p
and centrin3p were found associated with fibrogranular aggregates and
elongating procentrioles, suggesting a role of these proteins in an early step
of centriologenesis (Laoukili et
al., 2000). Because centrin2p and centrin3p were detected in
ependymal and choroidal ciliated cells and as we observed that centrin4p
expression in these cells correlated with their differentiation, one could
imagine that centrins 2p/3p could be involved in an early step of
centriologenesis, whereas centrin4p could be involved later in basal body
maturation or in cilia formation and associated functions. In agreement with
this hypothesis, it was shown that the incubation of permeabilized nasal
epithelial ciliated cells with an anti-centrin antibody that recognizes both
centrin1p and 2p inhibits ciliary beating, suggesting that some centrin
proteins, possibly centrin4p, could be involved in cilia associated functions
(Laoukili et al.,
2000). However, at the present time, we cannot exclude that
centrin4p could be also involved in an early step of de novo centriole
assembly.
It will be difficult to investigate centrin4p function(s) in primary
cultures of ciliated cells. In fact, the differentiation process of ciliated
cells in vitro takes many weeks and limits the utilization of classical
approaches like the overexpression of dominant negative forms or the
inhibition of expression by RNA interference. Thus, the best way to
investigate whether centrin4p is effectively involved in the differentiation
process of ciliated cells and in which step of ciliogenesis it could be
required will be to generate CETN4 null mice. Interestingly,
inactivation of the HFH-4 gene as well as partial loss of Polaris
functions in Tg737orpk (hypomorphic allele) mutant mice
leads to a hydrocephalus phenotype as a consequence of the absence or reduced
number of cilia in ependymal cells (Brody
et al., 2000; Taulman
et al., 2001). Detailed analyses of the morphology of
ciliated cells in these mutant mice allowed to identify in which step of
ciliogenesis the corresponding proteins are required. Thus, Polaris seems to
be involved in ciliary assembly, whereas HFH-4 seems to control the expression
of proteins required for centriole migration and/or docking to the apical
membrane (Brody et al.,
2000; Pazour et al.,
2000).
To date, vertebrate organisms seem to express two ubiquitous centrins
(centrin2p and centrin3p) and two more specific "ciliary" centrins
(centrin1p and centrin4p). Due to the absence of analyses of centrin1 mRNA
expression by in situ hybridization and the lack of anti-centrin antibodies
that fully discriminate between centrin1p and centrin2p, the expression
profile of centrin1p and its relation with that of centrin4p is still unclear.
Centrin1 mRNA was clearly detected in testis by a Northern blot analysis, in
contrast to centrin4 mRNA (Hart et
al., 1999; this work). Centrin1 expression was also detected
by RT-PCR in retina photoreceptor cells, which possess a very specialized
primary nonmotile cilium, the connecting cilium
(Wolfrum and Salisbury, 1998).
Interestingly, in these cells, centrin1p was shown to interact with the
heterotrimeric G protein transducin of the visual transduction cascade
(Pulvermuller et al.,
2002). However, the expression profile of centrin1 mRNA in the
epithelial cells of respiratory tracts seems to be more confusing. In fact,
centrin1 mRNA was not detected in lung by a Northern blot analysis, in
contrast to centrin4 mRNA (Hart et
al., 1999; this work). On the other hand, centrin1 expression
was detected by RT-PCR in human nasal epithelial ciliated cells but not in
human tracheal epithelial ciliated cells
(LeDizet et al.,
1998; Laoukili et
al., 2000). Thus, it will be interesting to examine whether
ciliated cells of the different epithelia of respiratory tracts, which harbor
multiple motile cilia, can express both centrin1p and centrin4p or whether the
expression patterns of these proteins are mutually exclusive.
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ACKNOWLEDGMENTS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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Footnotes |
|---|
Present address: Laboratoire de Biologie Cellulaire du
Développement, Unité Mixte Recherche 7622, Centre National de la
Recherche Scientifique, Université Pierre et Marie Curie, 9 quai
Saint-Bernard, 72252 Paris Cedex 05, France. 
Corresponding author. E-mail address:
mbornens{at}curie.fr.
|
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