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Molecular and Cellular Biology, August 2001, p. 4996-5007, Vol. 21, No. 15
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.15.4996-5007.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
NoBP, a Nuclear Fibroblast Growth Factor 3 Binding
Protein, Is Cell Cycle Regulated and Promotes Cell Growth
Kerstin
Reimers,1,
Marianne
Antoine,1
Marcus
Zapatka,1
Volker
Blecken,1
Clive
Dickson,2 and
Paul
Kiefer1,*
Institut für Hämostaseologie und
Transfusionsmedizin, Medizinische Fakultät,
Heinrich-Heine-Universität, D-40225 Düsseldorf,
Germany,1 and Imperial Cancer Research
Fund Laboratories, London WC2A 3PX, United
Kingdom2
Received 14 November 2000/Returned for modification 21 December
2000/Accepted 26 April 2001
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ABSTRACT |
Secreted and nuclear forms of fibroblast growth factor 3 (FGF3)
have opposing effects on cells. The secreted form stimulates cell
growth and transformation, while the nuclear form inhibits DNA
synthesis and cell proliferation. By using the yeast two-hybrid system
we have identified a nucleolar FGF3 binding protein (NoBP) which
coimmunoprecipitated and colocalized with FGF3 in transfected COS-1
cells. Characterization of the NoBP binding domain of FGF3 exactly
matched the sequence requirements of FGF3 for its translocation into
the nucleoli, suggesting that NoBP might be the nucleolar binding
partner of FGF3 essential for its nucleolus localization. Carboxyl-terminal domains of NoBP contain linear nuclear and nucleolar targeting motifs which are capable of directing a heterologous protein
-galactosidase to the nucleus and the nucleoli. While NoBP
expression was detected in all analyzed proliferating established cell
lines, NoBP transcription was rapidly downregulated in the promyelocytic leukemia cell line HL60 when induced to differentiate. Analysis on the expression pattern of NoBP mRNA throughout the cell
cycle in HeLa cells synchronized by lovastatin demonstrated a
substantial upregulation during the late G1/early S phase.
NoBP overexpression conferred a proliferating effect onto NIH 3T3 cells and can counteract the inhibitory effect of nuclear FGF3, suggesting a
role of NoBP in controlling proliferation in cells. We propose that
NoBP is the functional target of nuclear FGF3 action.
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INTRODUCTION |
In mammals, the fibroblast growth
factor (FGF) family is currently comprised of 20 genes encoding
structurally related proteins with molecular masses in the range of 20 to 40 kDa. In vitro, the FGFs demonstrate the ability to regulate cell
proliferation, differentiation, cell motility, extension of neurites,
and cell survival, depending on the context. In vivo, many members of
this family of intercellular signaling molecules have been shown to be
crucial for normal development, while their inappropriate activity has
been implicated in a wide range of pathological conditions, including
skeletal dysplasias, tumorigenesis, and metastasis (3, 4, 10, 23,
25, 28, 34).
FGFs have been shown to bind three different types of transmembrane
receptor. A cystein-rich receptor which binds FGFs and transforming
growth factor (TGF) with high affinity. This receptor resides in the secretory pathway as well as on the cell surface. Its
function is nuclear, although there is evidence to suggest that it
influences the intracellular trafficking of FGFs (7, 26, 30, 33,
39). Intercellular signaling by FGFs is mediated by high-affiniy
cell surface receptors (FGFR) with intrinsic tyrosine kinase activity
(12, 15). However, there is also a requirement for a
lower-affinity heparan sulfate-containing proteoglycan receptor which
forms part of the multimeric signaling complex (23). There are four different genes encoding high-affinity FGFRs, although receptor complexity is expanded by alternative splicing that gives rise
to receptor isoforms with different ligand binding specifities (29, 36, 37). However, there is good evidence that several FGFs, including FGF2 and FGF3, can signal by directly entering the
nucleus, thereby providing a cell with the potential to respond directly to intracrine signals, in addition to autocrine or paracrine signals, via cell surface receptors (9, 16, 18, 27).
FGF3 was identified as a proto-oncogene in virally induced mouse
mammary tumors. However, subsequent analyses revealed that it is not
normally expressed in the mammary gland but rather is primarily
restricted to prenatal mouse development. In situ hybridization revealed a dynamic pattern of expression from gastrulation to birth,
suggesting potential roles in mouse development (14, 32,
38). The biosynthesis of FGF3 is unusual in that a single CUG
initiation codon is the major translation start site which gives rise
to a protein that is directed in similar proportions to the cell
nucleus and the secretion pathway. The dual fate of FGF3 is achieved by
finely balanced opposing signals near the amino terminus: an internal
signal peptide for vectorial translation across the endoplasmic
reticulum and a bipartite nuclear localization signal (NLS). The import
of FGF3 into the nucleus is mediated by karyopherin 
1 (NPI-1), the
NLS binding subunit of a heterodimeric receptor of the nuclear import
machinery. The N-terminal targeting signals of FGF3 are weak signals
since substitution with stronger signals changes the balance between
the secretory pathway and nuclear uptake. These weak signals are
mechanistically important to allow competition between the
intracellular trafficking pathways. To overcome the disadvantage of a
weak bipartite NLS, an additional NLS is located in the body of the
protein, which also interacts with karyopherin 1 to enhance nuclear
uptake without disturbing the balance of the competing N-terminal
targeting motifs (2). A C-terminal motif was found to be
necessary for efficient nucleolar association but was dispensable for
the nuclear import of FGF3. Cells expressing low levels of an FGF3
mutant, lacks the signal peptide and therefore is exclusively nuclear,
proliferate very poorly. The growth-inhibitory effect depends on the
nucleolar localization of FGF3. Cells transfected with cDNAs in which
the encoded FGF3 lacked the C-terminal motif essential for nucleolar accumulation exhibited growth rates similar to those of the
nontransfected cells (2, 18, 20).
Nuclear localization of FGFs is not an exclusive property of FGF3,
since FGF1 and FGF2 have been shown to localize to the nucleus by two
apparently independent processes (34). Moreover, FGF2
shows an intracellular route to the nucleus, as well as an extracellular uptake and transport to the nucleolus. Extracellular uptake of FGF2 to the nucleolus occurs during late G1 phase
of the cell cycle in growing aortic endothelial cells and is correlated with increase rRNA transcription (6). Intracellular
nuclear transport occurs primarily with amino-terminally extended
isoforms of FGF2 that are initiated at CUG codons. In contrast to FGF3, the nuclear localization of FGF2 appears not to involve a classical NLS
but rather requires methylated glycine-arginine-rich sequences within
the amino-terminal extension (5, 24).
To gain some insight into the signaling pathway used by nuclear FGF3,
we used a yeast two-hybrid screen to identify genes encoding possible
FGF3 interacting proteins. We identified a human gene of unknown
function whose 305-amino-acid product interacts with FGF3 in vitro and
in vivo. The protein contains a nuclear and a nucleolar targeting
signal and accumulates in the nucleoli. We therefore named the protein
NoBP, for nucleolar binding protein. NoBP transcription is regulated in
a cell cycle-dependent fashion, and overexpression of NoBP in NIH 3T3
cells resulted in proliferation under serum-reduced conditions.
Significantly, overexpression of NoBP in nuclear FGF3-expressing mouse
mammary epithelial cells can abrogate the inhibitory effect of nuclear FGF3.
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MATERIALS AND METHODS |
Cell culture.
COS-1, HeLa, and NIH 3T3 cells were routinely
maintained in Dulbecco modified Eagle medium (DMEM) containing 10%
fetal calf serum (FCS). HC11 mouse mammary epithelial cells were
maintained in RPMI 1640 medium supplemented with 8% FCS, 10 ng of
epidermal growth factor (EGF) per ml, and 5 µg of insulin per ml as
described previously (20). HL60 cells were maintained in
RPMI 1640 medium supplemented with 10% FCS. To induce granulocyte
differentiation, HL60 cells were resuspended at a concentration of
2 × 105 cells/ml in the growth medium supplemented
with 1.2% dimethyl sulfoxide (DMSO), and for the induction of
monocyte-macrophage differentiation the growth medium was supplemented
with 3.3 × 10
8 M tetradecanoyl phorbol acetate
(TPA). Differentiation was monitored by examining the morphological
appearance and by the ability to reduce nitroblue tetrazolium. For
growth rate comparisons, equal numbers of each cell type were seeded in
DMEM with the indicated concentration of FCS. At the times indicated,
triplicate samples were harvested with trypsin, and four independent
dilutions were counted in a hemocytometer. For transient DNA
transfections, 20 µg of purified plasmid DNA was introduced into
5 × 105 COS-1 cells by electroporation (450 V/250
µF) using a Bio-Rad Gene-Pulser. At between 48 and 72 h after
transfection, the cells were harvested for immunoblot analysis or
processed for immunofluorescence. For stable DNA transfections,
purified plasmid DNAs were introduced by lipofection using Transfast
(Promega) as recommended by the manufacturer.
RNA isolation and Northern blot hybridization.
Total
cellular RNA was extracted from cultured cell lines and mouse tissues
by guanidium isothiocyanate and cesium trifluoroacetate gradient
purification. For Northern blot analysis, 20 µg of total RNA was
fractionated in denaturing Glyoxal gels, transferred to Hybond N
(Amersham), and hybridized with 32P-labeled probes under
stringent conditions (1).
Plasmid constructions.
pNoBP1.1 was constructed by inserting
the anti-RGS(His)6 epitope upstream and in frame of
the coding region of human NoBP cDNA. The modified NoBP cDNA was then
inserted into the expression vector pKC4 under control of the early
simian virus 40 (SV40) promoter. To obtain the plasmids pNoBP1.2,
pNoBP1.3, and pNoBP1.4, PCR was used to delete the carboxyl-terminal
44, 86, and 139 amino acids of NoBP, respectively. The vector pKC4.16,
which expresses a mutant FGF3 lacking the signal peptide, has been
described previously (18). pNoBP1.5 was produced by
deleting the 162 N-terminal amino acids and inserting 5' the sequence
encoding the anti-RGS(His)6 epitope. The -galactosidase-NoBP fusion
proteins were based on the expression plasmids pGAL1.0 and pGAL1.1,
which have been previously described. Using PCR, partial sequences of
NoBP, including the His-tag, were amplified with 3' primers that
introduced an XhoI site and 5' primers that introduced an
XbaI site. The resulting PCR fragments were inserted into
the single XhoI site and the XbaI site of
pGAL1.1, replacing the fgf3 sequences. The expression plasmid pDobs4.16 was described previously (20). A
retrovirus vector based on Moloney murine leukemia virus was used to
construct pBabe NoBP1.1 by inserting the NoBP cDNA from pKCNoBP1.1 as a blunted HindIII/EcoRI fragment into the
SnaBI and EcoRI sites of the pBabe neo vector.
Cell cycle analysis.
Medium was removed from growing HeLa
cells and replaced with fresh medium containing 60 µM lovastatin for
33 h. At time zero, cells were stimulated by replacing the medium
with fresh medium plus 6 mM mevalonic acid. At the indicated times, the
level of DNA synthesis was estimated by labeling the cells with 5 µCi
of 3H-radiolabeled thymidine per ml for 1 h at 37°C
in medium lacking thymidine and hypoxanthine (17). DNA
synthesis was then assayed as described previously (21).
Immunofluorescence.
COS-1 cells grown on glass coverslips
were transfected with the appropriate plasmids, and 48 h later
they were fixed in 4% paraformaldehyde in phosphate-buffered saline
(PBS) for 20 min. The cells were then permeabilized with 0.2% Triton
X-100 in PBS and processed as previously described (22).
Immunoblot analysis and in vitro translation.
The procedures
used for preparing cell lysates have been described in detail elsewhere
(18). Samples from equivalent numbers of cells were
fractionated by sodium dodecyl sulfate-polyacrylamide gel
electrophoresis (SDS-PAGE) in 12.5 or 15% polyacrylamide gels, transferred to nitrocellulose membranes (Schleicher & Schuell), and
then probed with rabbit polyclonal antibody to FGF3 or a mouse monoclonal antibody against the RGS-His tag (Qiagen). The
immunoreactive proteins were detected by enhanced chemiluminescence
using horseradish peroxidase-coupled anti-rabbit immunoglobulin
antibodies as described by the manufacturer (Amersham International).
Mouse FGF3 and NoBP cDNAs in pGem4Z were used in an in vitro
translation system (Promega) to generate 35S-labeled
products for use in binding assays as described in the text.
GST fusion proteins.
To obtain the glutathione
S-transferase (GST)-NoBP constructs, DNA sequences encoding
the appropriate amino acids were amplified by PCR using Pfu
polymerase (Stratagene) and oligonucleotides with SmaI and
EcoRI recognition sequences. The PCR products were cloned
into SmaI-EcoRI-digested pGEX (Pharmacia). All
expression constructs were verified by DNA sequence analysis and
transformed into Escherichia coli DH5 for the expression
of the fusion proteins.
GST-NoBP fusion protein affinity chromatography.
An
overnight 30-ml E. coli culture containing pGEX-NoBP or a
control GST plasmid was diluted 10-fold into Luria-Bertani or ampicillin medium and grown at 37°C to an optical density at 600 nm
of 1.0 before induction with 0.5 mM
isopropyl--D-thiogalactopyranoside (IPTG). Bacteria were
lysed by pulse sonication in lysis buffer (1% Triton X-100, 1.5%
N-laurylsarcosine, 25 mM triethanolamine, and 1 mM EDTA in
PBS). Then, 200 µl of a 50% slurry of glutathione (GSH)-agarose
beads (Molecular Probes) was added, and the mixture was incubated at
4°C overnight. After six washes in PBS-1% Triton X-100 (PBS-TX),
agarose beads containing bound proteins were analyzed by SDS-PAGE,
followed by Coomassie blue staining and immunoblot analysis.
Interactions between GST-NoBP and 35S-labeled FGF3 or
cell-associated proteins were analyzed using 0.5-ml aliquots of
fgf3-transfected COS-1 cells or 2 µl of
35S-labeled FGF3 to which 50 µl of the prepared GST- or
GST-NoBP-glutathione-agarose beads was added. The binding reactions
were incubated at 4°C overnight. The beads were washed, resuspended
in PBS-TX buffer, and poured into a column. The columns were
extensively washed with an excess of PBS-TX, and the retained proteins
were analyzed by SDS-PAGE. FGF3 was detected by immunoblotting or fluororadiography.
Immunoprecipitation of His-NoBP from transfected COS-1
cells.
COS-1 cells transfected with vectors containing His-NoBP
cDNA or pKC4.16 (18) were washed twice with PBS and lysed
in ice-cold lysis buffer (50 mM Tris, pH 8.0; 150 mM NaCl; 1% Nonidet
P-40; 0,5% sodium deoxycholate; 0.1% SDS; 0.02% sodium azide; 1 mM
phenylmethylsulfonyl fluoride; 10 µg of aprotinin per ml). The
lysates were incubated at 4°C overnight with anti-PentaHis (Quiagen)
preadsorbed onto 40 µl of protein G-Sepharose (Pharmacia). The
precipitates were washed four times with sodium phosphate wash buffer,
eluted in Laemmli loading buffer, and subjected to SDS-PAGE and Western blot analysis with anti-His monoclonal antibody or anti-FGF3 serum.
Yeast two-hybrid screening.
The bait contained fgf3
cDNA encoding the entire protein (4.12 [18]) fused
in frame to the DNA-binding domain of Gal4. The cDNA insert from
pKC4.12 was inserted at the NcoI/SalI restriction sites of vector pAS2 (Clontech). The bait was used to screen a human
B-cell lymphoma cDNA library (a generous gift of Steve Elledge [8]) cloned in pACT. After cotransfection of the
pAS2-construct and the pACT library into Y190 yeast cells, positive
clones were selected on triple-minus plates (Leu
Trp His) containing 25 mM 3-aminotriazol
and assayed for -galactosidase activity. Positive cDNA clones were
cycloheximide selected and tested by cotransfection and by mating with
control bait vectors and with the original pAS2 vector to confirm the
interaction. Mutations in the NoBP constructs were made by PCR, and the
sequence was confirmed by DNA sequencing before the mutations were
analyzed in the yeast two-hybrid assay. The N-terminal and C-terminal
deletion mutants of FGF3 were previously described (20),
and the inserts were transfered into the
NcoI/SalI restriction sites of the pAS2 vector.
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RESULTS |
Identification of an FGF3 NoBP.
A yeast two-hybrid screen was
used to search for FGF3 binding proteins. A cDNA library prepared from
human B-cell lymphoma cells and containing in-frame fusions with the
activator domain of GAL4 in the vector pACT was screened with a bait
containing a full-length FGF3 cDNA fused to the DNA binding domain of
GAL4 in the vector pAS2. From a total of 2.5 × 107
transformants, 29 clones were isolated. Inserts from 19 independent clones that gave strong signals with the FGF3 bait were isolated, sequenced, and compared to sequences in GenBank using the BLAST search
program. Four identical clones (F2, F3, F17, and F31) were found to be
very similar to a partial human cDNA designated p40, which was
submitted as a sequence encoding a nucleolear protein of unknown
function (D. Henning et al., GenBank NM_006824). The NoBP is 306 amino
acids long, with a calculated molecular weight of 39,000. The amino
acid derived sequence of the clone F2 was found to begin at amino acid
53 of the published cDNA sequence. Features of NoBP include a consensus
sequence for casein kinase II phosphorylation at the N terminus, two
overlapping basic domains which may function as NLSs, and a GR- and
GK-rich region at its C terminus. A search of the mouse EST database
revealed overlapping cDNA sequences which would encode a protein which
shares 82% amino acid sequence identity with the human NoBP protein
(Fig. 1), and a BLAST search of the
GenBank database with the entire NoBP coding cDNA sequence revealed
57% identity with a hypothetical Caenorhabditis elegans
protein of 40 kDa, and a 32% identity with a hypothetical protein of
49 kDa encoded by the open reading frame (ORF) YKL172W in
Saccharomyces cerevisiae. (EMB CAA82014.1). The predicted
human NoBP product aligned with the sequences of C. elegans
and S. cerevisiae proteins (Fig. 1b) demonstrates the
highest homology acids over the central region of 100 amino acids
(residues 103 to 203) with 62% identity and 55% similarity,
respectively, allowing for substitution of chemically similar amino
acids.
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FIG. 1.
(a) Amino acid sequence of human NoBP (Hm) and
comparison to mouse NoBP (Mm). Alignment of the deduced amino acid
sequence of human and mouse cDNAs using the DNAsis program. Identical
amino acids are indicated by gray boxes. Two amino acid differences
were found in the human NoBP compared to the sequence present in the
GenBank database (accession no. NM_006824) and are indicated as
superscripts. The basic amino acid-rich regions involved in targeting
are boxed. (b) Amino acid sequence alignment of the middle region of
human NoBP and the yeast ORF YKL172w. Identical and chemically similar
amino acid residues are boxed in gray.
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To determine whether the p49 from
S. cerevisiae could
interact with mouse FGF3, the hypothetical ORF encoding p49 (YKL172W)
was amplified by PCR and cloned into the pACT vector to create
an
in-frame fusion with the activator domain of GAL4. The generated
plasmid, pACTY49, was cotransformed into yeast with the FGF3 bait
vector. A good positive signal was obtained, indicating conservation
of
the FGF3 interacting region in the NoBP homologs (data not
shown).
NoBP associates with FGF3 in vitro and in vivo.
To investigate
the interaction between FGF3 and NoBP, we used recombinant NoBP
generated as a GST fusion protein immobilized on GSH-Sepharose beads to
bind to in vitro-translated 35S-FGF3. The result was a
strong retention of 35S-FGF3 by GST-NoBP, demonstrating
that the two proteins can interact and that posttranslational
modifications of the proteins are unlikely to be needed for the
interaction (Fig. 2a). Moreover, binding under conditions of increasing NaCl concentration demonstrated that the
complex can form in 1 M NaCl, which is indicative of a strong
interaction (Fig. 2b). Similarly, an extract of COS-1 cells expressing
a mutant of FGF3 (pKC4.16) that resides exclusively in the nucleus
and/or nucleolus, was mixed with GST-NoBP bound to GSH-Sepharose beads,
washed, subjected to SDS-PAGE, and immunoblotted for FGF3. The results
confirmed the ability of FGF3 to bind NoBP in vitro. To show that FGF3
and NoBP may form an intracellular association, COS-1 cells were
cotransfected with vectors expressing NoBP (pKCNoBP1.1) and FGF3
(pKC4.16), and cell extracts were immunoprecipitated with anti-Penta
His monoclonal antibody, which detects the histidine tag at the N
terminus of NoBP encoded by pKCNoBP1.1. After separation by SDS-PAGE,
FGF3-related proteins were detected by immunoblotting using a
polyclonal antibody against FGF3 (Fig. 2d, upper panel). To detect the
expression of NoBP, a monoclonal anti-RGS(His) antibody was used in
similar immunoblots (Fig. 2d, lower panel). The results demonstrate
that detection of FGF3 was dependent on the presence of NoBP.
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FIG. 2.
Interaction between NoBP and FGF3. (a) In
vitro-translated 35S-labeled FGF3 (FGF3 4.16) was incubated
with GST beads containing the NoBP fusion protein or GST beads as
indicated. After an extensive washing, the retained proteins were
analyzed as described in the text. (b) To assess the affinity of FGF3
binding to NoBP bound to GST beads, the beads were loaded with
35S-labeled FGF3 at increasing concentrations of NaCl as
indicated. (c) Cell extracts from Fgf-3-transfected COS-1
cells were affinity precipitated with GST-NoBP-loaded beads. Bound
proteins were eluted, subjected to SDS-12.5% PAGE, and examined for
the presence of FGF3 by immunoblotting with a rabbit anti-FGF3 peptide
antibody. (d) COS-1 cells were transfected with
RGS(His)6-tagged full-length NoBP cDNA (pKCNoBP1.0) or with
the control vector alone, together with pKC4.16. The cell lysates were
immunoprecipitated with the anti-PentaHis monoclonal antibody (Qiagen)
and immunoblotted with the anti-FGF3 peptide antibody or with an
anti-RGS(His) monoclonal antibody (Qiagen).
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Localization of the sequences necessary for the FGF3 and NoBP
association.
Previous mutation analyses have implicated different
basic domains in the carboxy-terminal region of FGF3 as important for nuclear uptake and nucleolar association (20). To
determine whether the nucleolar retention sequences are necessary for
NoBP binding, several deletion and point mutants of FGF3 previously described (Fig. 3a) were analyzed for
NoBP binding in a yeast two-hybrid screen. The results are summerized
in Fig. 3a and show a perfect correlation between nucleolar
localization in COS-1 cells and colony formation in the yeast screen.
Mutant FGF3 analysis and the results obtained with the FGF chimera
demonstrated that the sequences necessary for nucleolar localization
have to be presented in a certain structural context, suggesting a
nucleolar retention via binding to interacting proteins rather than a
linear nucleolar targeting motif (19). The FGF3 mutant
4.26 lacking the sequences encoded by the second exon which is highly
conserved in the FGF family and thought to be essential for their
structural integrity is no longer located in the nucleoli and no longer
interacted with NoBP in the yeast two-hybrid binding assay. The deleted
N-terminal FGF3 sequences could be functionally replaced by the
corresponding sequences of the exclusively secreted FGF family member
FGF4 (Hst1.2). The mutant 4.19, in which the FGF4 C terminus is
substituted for that of FGF3, was not detected in the nucleoli and did
not bind to NoBP. These findings support the idea that, in fact,
binding of FGF3 to NoBP is essential for its nucleolar accumulation.
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FIG. 3.
Deletion analysis of the FGF3 and NoBP binding domains
in the yeast two-hybrid system. (a) fgf3 cDNAs encoding
wild-type or mutant FGF3 proteins with previously characterized
subcellular localizations (18, 20) were cloned into the
pAS2 vector and examined for NoBP binding in the two-hybrid system.
Interactions between FGF3 and NoBP were scored based on growth on
His plates and -galactosidase (-gal) activity. The
fgf3 cDNA encodes a signal peptide (Sp), a bipartite NLS
(biNLS), a second NLS, and a C-terminal motif essential for nucleolar
accumulation (checkered pattern). The part of the FGF proteins encoded
by the second exon is marked by vertical stripes. The subcellular
localization of the mutants are summarized to the right of each
depicted cDNA as follows: N, nuclear; No, nucleolar; S, secreted; and
C, cytoplasmic. (b) Truncation mutations of NoBP were generated by
cleavage with appropriate restriction enzymes and then cloned into
pACT2. Interactions between the NoBP mutations and wild-type FGF3 were
scored as in panel a. (c) The binding of FGF3 to mutations of NoBP was
assessed by affinity precipitation. Deletion mutations of NoBP fused to
GST are indicated. The fusion proteins were expressed in E. coli, and extracts were bound to GSH-Sepharose beads as described
in the text. The washed beads were incubated with
35S-labeled FGF3, and the retained protein was analyzed as
described in Fig. 2b.
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To locate the domain in NoBP that interacts with FGF3, truncation
mutants were generated and assayed for FGF3 binding in the
yeast
two-hybrid screen (Fig.
3b). The results indicate that a
fragment
composed of amino acids 160 to 236 retained the ability
to bind FGF3.
This result was substantiated using a similarly
truncated NoBP as
GST-fusion protein in an in vitro binding assay
with
35S-labeled in vitro-translated FGF3 (Fig.
3c). The results
show
that the region of NoBP between amino acids 160 and 236 is
sufficient
for FGF3
binding.
Nuclear FGF3 and NoBP colocalize in cells.
The association
between FGF3 and NoBP was further investigated by immunofluorescence
microscopy. FGF3 and His-tagged NoBP protein were coexpressed by
transfecting COS-1 cells with pKC4.16 (FGF3) and pKCNoBP1.1 (NoBP)
(Fig. 4). The nuclear and nucleolar distribution of both proteins appears to be virtually identical. For
staining of the cotransfected cells, a rabbit polyclonal antibody against FGF3 and a monoclonal anti-His antibody was used with species-specific secondary antibodies conjugated to different fluorescence dyes (Texas red and fluorescein). Extensive colocalization of nuclear FGF3 and NoBP was observed. In experiments with
single-staining antibodies, no crossover was observed between the
channels for Texas red and fluorescein.
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FIG. 4.
Colocalization of nuclear FGF3 and NoBP in COS-1 cells
by immunofluorescence microscopy. COS-1 cells transiently transfected
with pKC4.16 encoding nuclear FGF3 (a) or with RGS(His)-tagged NoBP
(pKC-NoBP1.1) (b) or cotransfected with pKC4.16 and pKC-NoBP1.0 (c and
d) were grown on coverslips for 48 h, fixed in 4%
paraformaldehyde, and permeabilized with Triton X-100 as described in
the text. The coverslips were then stained with a rabbit polyclonal
peptide antibody against FGF3 or with anti-RGS(His) monoclonal antibody
(Qiagen) against the His epitope. The NoBP His-tagged protein complexes
were visualized with goat anti-mouse immunoglobulin tagged with
fluorescein and the anti-FGF3 immunocomplexes were detected with goat
anti-rabbit immunoglobulin tagged with Texas red.
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Localization of elements in NoBP necessary for nuclear uptake and
nucleolar association.
The NoBP sequence contains several clusters
of basic residues located in the C-terminal half of the protein as
depicted schematically in Fig. 5. To test
the importance of these motifs on nuclear uptake, a series of deletion
mutations were introduced into pKCNoBP1.1 which removed combinations of
these potential targeting motifs. Deletion of the C terminus from amino
acid 167, which encompasses all of the basic elements, leads to an even
distribution of the protein between the nucleus and cytoplasm, but
without nucleolar association. Deletion of the carboxyl terminus from
amino acid residue 220, which conserves a lysine-, arginine-, and
glutamine-rich domain resulted in exclusively a nuclear location of the
product, but with exclusion from the nucleoli. In contrast, deletion of the carboxy-terminal 45-amino-acid residues did not affect the nuclear
or nucleolar distribution. Moreover, deletion of the N-terminal half of NoBP (amino acids 1 to 166), did not change the
subcellular location of the truncated protein. These results indicate
that the domain between amino acids 167 and 220 contains sequences that
are important for nuclear localization, while the sequences between
amino acids 220 and 262 are necessary for nucleolar association (Fig.
5).
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FIG. 5.
Deletion mutations affecting nuclear and nucleolar
localization of NoBP. (a) Deletion mutations of pKC-NoBP1.1. Domains
rich in basic amino acids are depicted schematically by the various
stripped boxes (see Fig. 1). (b) Subcellular distribution of
NoBP-related products of the deletion mutations depicted in panel a
were analyzed by immunofluorescence using the anti-RGS(His) monoclonal
antibody. Examples of the staining patterns are shown and are
summarized alongside the depiction of each mutation shown in panel a.
N, nuclear; No, nucleolar; C, cytoplasmic.
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Motifs in the carboxyl terminus of NoBP can confer nuclear and
nucleolar localization to a heterologous protein.
A more stringent
test of nuclear and nucleolar targeting function is whether the
candidate C-terminal motifs are sufficient to direct a heterologous
cytoplasmic protein into the nucleus and associate it with the
nucleolus. Segments of the carboxy terminus of NoBP were fused with the
bacterial gene -galactosidase as depicted in Fig.
6. After transfection of the various
constructs into COS-1 cells, their intracellular localization was
determined by immunofluorescence by using antibodies to
-galactosidase. The parental vector, Gal1.0 was located in the cell
cytoplasm while, in contrast, constructs with segments of the carboxyl
terminus of NoBP fused at the N terminus of the -galacosidase
accumulated in the nucleus. The fusion protein containing NoBP
sequences between amino acids 162 and 262 and amino acids 220 and 262 both showed nuclear and nucleolar staining indistinguishable from that
of NoBP. However, the segments at 162 and 220 only showed a nuclear staining pattern with exclusion from the nucleoli, a result again consistent with the deletion analysis of NoBP (Fig. 5). Taken together,
the deletion analysis and signal transfer experiments suggest that
there is a nucleolar targeting motif contained in amino acids 220 to
262 which is necessary and sufficient to direct a heterologous
cytoplasmic protein into the nucleus and associate it with the
nucleoli.
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|
FIG. 6.
Localization of NoBP nuclear and nucleolar localization
signals. (a) Segments of the carboxy terminus of NoBP, encompassing
amino acids 162 to 262, were fused to the coding domain of
-galactosidase. The shading used to mark the different
basic domains in the C-terminal region of NoBP are the same as in Fig.
5. (b) The location of the NoBP--galactosidase fusion proteins was
determined by staining with a monoclonal antibody against
-galactosidase, followed by the addition of a secondary antibody
conjugated to fluorescein.
|
|
NoBP is widely expressed in mouse tissue and cell lines.
The
expression of NoBP in adult mouse tissues and several cell lines of
mouse and human origin was assessed by Northern blot analysis. A single
transcript of 1.5 kb was detected in all mouse tissues and cell lines
examined. The highest levels of expression were found in the lung,
heart, spleen, and kidney. The broad expression of NoBP in mouse
tissue, which does not express FGF3, suggests that NoBP has a
common function in all cells and presumably interacts with
partners other than FGF3 (Fig. 7).
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FIG. 7.
Expression of NoBP transcripts in human and mouse cell
lines and adult mouse tissues. Northern blots containing 10 µg of
total RNA from different established human cell lines (a) or mouse cell
lines (b) were hybridized with 32P-labeled human or mouse
NoBP cDNA probe. (c) Northern blot of 10 µg of total RNA from
different adult mouse tissues was done with a 32P-labeled
mouse NoBP cDNA probe. The size of the NoBP-specific transcripts are
indicated.
|
|
Modulation of NoBP transcripts in differentiating HL60 cells and
cell cycle synchronized HeLa cells.
To determine whether NoBP is
regulated during the cell cycle, we examined NoBP RNA expression in two
different systems: differentiating HL60 cells and HeLa cells reentering
the cell cycle from a lovastatin block. HL60 promyelocytic leukemia
cells can be induced to differentiate into monocytes by treatment with
a phorbol ester such as TPA or into granulocytes by treatment with DMSO
(19). Differentiation is preceded by a withdrawal from the
cell cycle. To examine expression of NoBP in differentiated cells,
total RNA was prepared from HL60 cells exposed to DMSO or TPA for 3 days and then analyzed by Northern blotting. No NoBP-specific
transcription was detectable in the differentiated HL60 cell
populations. To investigate the kinetics NoBP transcript disappearance,
HL60 cells were monitored for 3 days as they ceased to proliferate and
differentiate in response to TPA treatment. Under these conditions,
NoBP transcripts diminished in the absence of proliferation, but not as
rapidly as c-myc transcripts (Fig. 8a).
The kinetics of disappearance will be a function of transcriptional
repression and messenger half-life which were not separable in this
experiment; nevertheless, downregulation of NoBP appears to parallel
exit from the cell cycle.
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FIG. 8.
NoBP transcripts are downregulated in HL60 cells
following differentiation. (a) Northern blot analysis of RNA samples
were taken after 72 h of treatment of HL60 cells with TPA or DMSO.
As a control for RNA loading, the blot was reprobed for
glyceraldehyde-3-phosphate dehydrogenase (GAPDH). (b) Kinetics of NoBP
RNA (nobp) downregulation following treatment with TPA to
induce monocyte-macrophage differentiation. (c) Transcriptional
regulation of nobp expression in lovastatin-synchronized
HeLa cells. HeLa cells were cultured in 60 µM lovastatin for 33 h, at which time lovastatin was replaced with medium containing
mevalonate as described in the text. Cell samples were harvested at the
indicated times after lovastatin removal, and the extracted RNA was
analyzed by Northern blotting. The membranes were probed with
32P-labeled cDNA to nobp, p21, and GAPDH. RNA
loading was also monitored by ethidium bromide staining of the RNA gel.
The DNA synthesis rate was monitored by pulse labeling the DNA with
[3H]thymidine as described in the text.
|
|
To further investigate the association of NoBP transcription with the
cell cycle, lovastatin, an inhibitor of the cholesterol
biosynthetic
pathway, was used to synchronize HeLa cells in early
G
1
(
17). After 33 h in lovastatin, the cultures were
refed with
medium supplemented with mevalonate to stimulate their
reentry
into the cell cycle. After release from the lovastatin block,
there was a delay in DNA synthesis for several hours before an
increase
in incorporation of [
3H]thymidine was observed (Fig.
8c).
Immediately after release
there was a peak of p21 (CIP1/WAF1) RNA
expression (
11), followed
by a peak of NoBP transcription
in late G
1 and early S phases.
However, NoBP expression
decreased before the peak of DNA synthesis.
These results demonstrate a
strong correlation between proliferation
and the expression NoBP
mRNA.
NoBP expression confers a growth-stimulating effect on NIH 3T3
cells.
To determine whether the level of NoBP expression affected
the proliferation rate, we tested the effect of overexpressing NoBP.
NIH 3T3 cells were transfected with pBABE-NoBP1.1, and stably expressing clones were selected. Clones were selected on the basis of
high or moderate levels of NoBP protein expression and analyzed for
their proliferation potential (Fig. 9a).
Expression of NoBP in NIH 3T3 did not lead to a transformed morphology
and, with a full serum supply, a growth stimulatory effect was only
detected in the cell line expressing high levels of NoBP (Fig. 9b).
Still even in culture medium supplemented with 10% serum, NoBP is able to induce a twofold increase in the growth rate of NIH 3T3 cells. However, under serum-reduced conditions, the cell line expressing high
and moderate levels of NoBP grew significantly better than the parental
cells. The cell line with the low level of NoBP expression still grew
at a 10-fold-higher rate than the parental NIH 3T3 cell line and the
NoBP-overexpressing cell line (NIH-NoBP-A) induced a 100-fold-higher
growth rate compared to the control cells. These findings suggest that
higher expression levels of NoBP can confer a clear growth-promoting
effect on NIH 3T3 cells without changing the cell morphology (Fig. 9c).
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FIG. 9.
NoBP is growth stimulatory for NIH 3T3 cells. Two stable
clones of NIH 3T3 cells expressing human NoBP (designated
pBabeNoBP1.1-A and pBabeNoBP1.1H) were selected and tested for
growth in complete medium or in low-serum conditions. (a) Immunoblot
analysis of His-tagged NoBP expression in the two transfected NIH cell
lines are compared to control COS-1 cells transiently transfected with
pKCNoBP1.1. Protein samples corresponding to the same number of cells
were analyzed. Cells were seeded at 2.5 × 103 cells
per well in 24-well dishes and grown for 8 days in DMEM containing 10%
FCS (b) or 2% FCS (c) for 15 days. Cells were harvested and counted,
and the cell numbers were plotted as the means of triplicate
determinations, with bars indicating the standard error of the mean.
|
|
Expression of NoBP can antagonize the inhibitory effect of
nucleolar FGF3 on HC11 cells.
Expression of the nucleolar isoform
of FGF3 in mammary epithelial HC11 cells inhibits cell proliferation
(20). To determine whether overexpression of NoBP could
reverse the block, a cell line (HC4.16-16 [20])
expressing nucleolar FGF3 was cotransfected with an SV40-based vector
expressing the human NoBP cDNA and selected with a vector carrying the
puromycin-resistant gene. Transfected cells were selected by resistance
to puromycin, and several colonies were chosen and passaged in complete
medium supplemented with FCS, EGF, and insulin. A cell line expressing
a high level of NoBP mRNA was selected (Fig.
10, upper panel). The growth rate of
this cell line (HC4.16-16-K3) was compared with those of the parental
cell line HC4.16-16 under low-serum conditions. A cell line of HC11
cells transfected with the empty vector DNA was used as control (HC
Dobs-1). Cells were seeded at a low density in medium supplemented with
2.5% serum, EGF, and insulin. Under these conditions, there was a
significant correlation of high growth rate with high NoBP expression
(Fig. 10b). The HC11 cells transfected with the 4.16 cDNA which encodes
the nucleolus-associated form of FGF3 grew at a much lower growth rate
than the control cells. However, when these cells were transfected with
the NoBP cDNA and were expressing similar levels of NoBP transcripts as
the HeLa cells, the growth-inhibitory effect of FGF3 was antagonized and NoBP induced a 10-fold increase in the growth rate compared to the
parental cell line (HC4.16-16). These findings clearly demonstrate that
expression of NoBP can counter the inhibitory effect of nuclear FGF3
and suggest that the growth-inhibitory effect of nuclear FGF3 may be
due to an interaction of nucleolar FGF3 with NoBP, slowing entry into
the S phase of the cell division cycle.
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FIG. 10.
NoBP expression can reverse the inhibitory effect of
nuclear FGF3 in HC11 cells. (a) An HC11 cell line expressing the
nuclear form of FGF3 (HC4.16-16) was transfected with a vector encoding
human His-tagged NoBP protein and a high-expression cell clone was
selected (HC4.16-16-K3), followed by Northern blot analysis. (b) The
nuclear FGF3 expressing cell line HC4.16-16, a control vector
transfected cell clone (HC Dobs-1), and the NoBP and nuclear FGF3
expressing cell clone (HC4.16-16-K3) were seeded at 2.5 × 103 cells per well in 24-well dishes and grown for 9 days
in DMEM containing 2% FCS, EGF, and insulin. Cells were harvested and
counted, and the cell counts are plotted as the means of triplicate
determinations, with bars indicating the standard error of the mean.
|
|
| |
DISCUSSION |
Many FGF family members have important intercellular signaling
functions during mammalian development (34). For autocrine and paracrine signaling, the FGFs are secreted and activate receptors on the same or adjacent cells. However, several members of the FGF gene
family encode isoforms that have a nuclear location (4). These include FGF1, FGF2, and FGF3, as well as the more recently described FGF homology factors (FGF11 to FGF14) (31). The
latter encode proteins that do not contain signal sequences for
secretion and may primarily function as nuclear proteins. In contrast,
FGF3 encodes isoforms that are either exclusively secreted or have a
dual localization. Thus, the amino-terminally extended isoform either
enters the secretion pathway or is translocated to the nucleus or
nucleolus. This allows the same protein to potentially have two
signaling pathways: one autocrine or paracrine through secretion and
receptor activation and a second directly acting on some nuclear
targets. In an effort to establish possible components of a nuclear
FGF3 signaling pathway, we used a yeast two-hybrid assay to identify an
FGF3 binding protein that normally resides in the nucleolus. The
affinity of FGF3 for NoBP is sufficiently strong to account for its
nucleolar localization. Moreover, a mutation analysis of FGF3 shows a
correlation between nucleolar localization and binding to NoBP. A
search of the databases showed that NoBP was previously identified as a
nucleolar protein of no known function. Here we demonstrate that it not
only binds to FGF3 but is regulated in a cell cycle-dependent manner.
Unlike FGF3, NoBP is widely distributed in different tissues and cell lines, and there appear to be homologues in flys and yeast, suggesting that it may have a function common to most, if not all, eukaryotic cells.
A mutation analysis of NoBP shows that FGF3 binding and its ability to
translocate to the nucleus and associate with the nucleolus reside in
the carboxy-terminal region of the protein (Fig. 3 and 5). A
preliminary deletion analysis suggests that sequences between amino
acids 162 and 220 encode the nuclear localization motif. This region is
rich in basic amino acids (Fig. 1). Inclusion of amino acid sequences
that are more carboxy terminal confer nucleolar association. Moreover,
amino acid sequences between 220 and 262 are sufficient to confer
nuclear localization and nucleolar association on -galactosidase
that normally resides in the cytoplasm. Interestingly, amino acids 162 to 220 will translocate -galactosidase to the nucleus, indicating
some redundancy of NLSs. The carboxy-terminal domain of NoBP is quite
complex, encoding nuclear localization sequences, the nucleolar
association domain, as well as a region that binds FGF3. How proteins
which have no obvious RNA-binding domain elements accumulate in the
nucleoli is not well understood.
Expression of human NoBP in NIH 3T3 cells resulted in a reduced
requirement for serum and could keep them in a proliferating state
under conditions in which they would normally quiesce. Furthermore, expression of NoBP RNA is regulated during the cell cycle, peaking during the late G1 and early S phases, supporting the idea
that NoBP may be involved in controlling progress through the cell division cycle. The high degree of sequence homology between the mammalian NoBP and the putative S. cerevisiae gene product
p49 suggests that the function of these proteins may be conserved during evolution. Homozygous deletion of p49 is lethal, establishing an
essential function (data not shown). Recently, two groups demonstrated that the yeast homologue of NoBP is an essential nucleolar protein required for pre-rRNA processing (13, 35). The sequences
critical for the essential activity of the yeast homologue comprise the most conserved region between the yeast and human protein and two
putative NLSs (13). The FGF3 binding domain of human NoBP corresponds to the C-terminal part of the conserved region. Since the
synthesis of ribosomes is essential for growing cells, mechanisms involved in the control of ribosome synthesis are therefore expected to
determine the coordination between cell growth and cell division. Also,
candidate c-myc target genes implicated in cell growth control regulate
rRNA transcription and processing. In the light of these new findings,
it is interesting to notice that immunogold electron microscopy locates
FGF3 within the dense fibrillar components, which are regarded as the
site of active transcription of rRNA genes and processing of pre-rRNA
(20). Taken together, these findings suggest NoBP may be
essential for integrating growth-regulatory signals with gene
transcription and RNA processing.
Dual subcellular localization of FGF3 appears to reflect two opposing
biological effects. Hence, secreted FGF3 induces cell proliferation
through cell surface tyrosine kinase receptors, while in the same HC11
cells a nuclear-targeted FGF3 suppresses proliferation in the
G1 phase of the cell cycle. This dual arrangement of
signaling might hypothetically cause an FGF3-producing cell to send a
paracrine signal inducing a mitogenic response, while its nuclear form
blocks autocrine proliferation by an intracrine signal. We would
suggest that NoBP serves as a target for the inhibition of cell
proliferation by nuclear FGF3.
| |
ACKNOWLEDGMENTS |
We thank A. Eldredge for the kind gift of the human B-lymphoma
cDNA library.
This work was supported by a grant from the DFG to P.K.
K.R. and M.A. contributed equally to this work.
| |
FOOTNOTES |
*
Corresponding author. Mailing address:
Heinrich-Heine-Universität, Medizinische Fakultat, Institut
für Hämostaseologie und Transfusionsmedizin, Moorenstrasse
5, D-40225 Düsseldorf, Germany. Phone: 49-211-811-7344. Fax:
49-211-811-6649. E-mail: kiefer{at}med.uni-duesseldorf.de.
Present address: Ruhr-Universität Bochum, Institut für
Pharmakologie, D-44780 Bochum, Germany.
| |
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Molecular and Cellular Biology, August 2001, p. 4996-5007, Vol. 21, No. 15
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.15.4996-5007.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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Goldfarb, M.
(2001). Signaling By Fibroblast Growth Factors: The Inside Story. Sci Signal
2001: pe37-pe37
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Introduction
