* Department of Clinical Molecular Biology, Department of Urology, Faculty of Medicine, Kyoto University, Kyoto 606, Japan
In response to low ambient temperature, mammalian cells as well as microorganisms change various physiological functions, but the molecular mechanisms underlying these adaptations are just beginning to be understood. We report here the isolation of a mouse cold-inducible RNA-binding protein (cirp) cDNA and investigation of its role in cold-stress response of mammalian cells. The cirp cDNA encoded an 18-kD protein consisting of an amino-terminal RNAbinding domain and a carboxyl-terminal glycine-rich domain and exhibited structural similarity to a class of stress-induced RNA-binding proteins found in plants. Immunofluorescence microscopy showed that CIRP was localized in the nucleoplasm of BALB/3T3 mouse fibroblasts. When the culture temperature was lowered from 37 to 32°C, expression of CIRP was induced and growth of BALB/3T3 cells was impaired as compared with that at 37°C. By suppressing the induction of CIRP with antisense oligodeoxynucleotides, this impairment was alleviated, while overexpression of CIRP resulted in impaired growth at 37°C with prolongation of G1 phase of the cell cycle. These results indicate that CIRP plays an essential role in cold-induced growth suppression of mouse fibroblasts. Identification of CIRP may provide a clue to the regulatory mechanisms of cold responses in mammalian cells.
To adapt themselves to environmental temperature
shifts, organisms have developed sophisticated strategies. To survive in the winter, some animals have
developed a capacity for adaptive hypothermia (hibernation), in which they lower their body temperatures to a few
degrees above the ambient (Willis, 1987 The cold-shock responses of microorganisms have been
extensively investigated (Jones et al., 1987 CS-RBD, also referred to as ribonucleoprotein (RNP)
motif, RNP consensus sequence, or RNA recognition motif, is one of the major RNA-binding motifs and is the most
widely found and best characterized (Kenan et al., 1991 In the present study, we have screened for RNA-binding
proteins expressed in mouse testis with a PCR-based cloning method and isolated a cDNA encoding a novel GRP.
This protein was induced in response to cold stress and
designated as cold-inducible RNA-binding protein (CIRP).
Furthermore, we demonstrated that CIRP is involved in
temperature-dependent regulation of cell growth.
Cells and Culture Conditions
BALB/3T3 cells were cultured in D-MEM (Gibco Laboratories, Grand Island, NY) supplemented with 10% calf serum (Dainippon Pharmaceutical Co., Osaka, Japan) and 100 IU/ml penicillin at 37°C in a humidified atmosphere of 5% CO2 in air. BMA1, TAMA26, and COS-7 cells were cultured in D-MEM (Gibco Laboratories) supplemented with 10% FCS (Dainippon Pharmaceutical Co.) and 100 IU/ml penicillin at 37°C in a humidified atmosphere of 5% CO2 in air.
For temperature-shift experiments, BALB/3T3 cells (5 × 103 cells/cm2)
were grown for 24 h at 37°C and then shifted to 15, 25, 32, 37, 39, or 42°C
in a humidified atmosphere of 5% CO2 in air. After 6 h or other indicated
times, the cells were scraped and frozen in liquid nitrogen. Extraction of
total RNA, Northern blot analysis, and Western blot analysis were carried
out as described (Furutani et al., 1995 To assess the effects of antisense oligodeoxynucleotide (ODN), sense
ODN (0.5 µM), antisense ODN (0.5 µM), or vehicle alone was added to
the BALB/3T3 cells in exponential phase of growth, and the temperature
was shifted from 37 to 32°C. After 12 h of incubation, the expression of
p18cirp was analyzed by Western blotting. To assess the effects on growth, 5 × 103 BALB/3T3 cells were plated into each well of a 24-well plate. 16 h
later, 0.1, 0.5, or 1.0 µM of antisense ODN, sense ODN, or vehicle alone
was added to each well and the culture was continued. 2 d later, the numbers of cells were determined under a microscope. The experiments were
repeated three times, and each assay was performed in triplicate. Statistical differences between sample means were calculated by analysis of variance, followed by unpaired Student's t test. The results are expressed as
the mean ± SEM, and P < 0.02 was considered significant.
ODNs
Antisense and sense ODNs containing phosphorothioates were purchased
from Cruachem (Kyoto, Japan). The sequence of the sense ODN was
(5 Cloning of cirp cDNA
The first-strand cDNA was prepared from the total cellular RNA of
mouse testis (4-mo-old) by using a First-strand cDNA Synthesis Kit
(Pharmacia LKB Biotechnology, Piscataway, NJ) with random primers,
according to the manufacturer's instructions. For the PCR, we used a set of
degenerate primers, (5 RNA Extraction and Northern Blot Hybridization
Cells were dissolved in TRIzol reagent (Life Technologies, Grand Island,
NY), and RNA was extracted by following the manufacturer's instructions. 20 µg of total RNA of each sample was separated in 1.0% agarose/
formaldehyde gels by electrophoresis and was blotted onto nylon filters
(Hybond-N+; Amersham International, Buckinghamshire, UK). The filters were hybridized with [ Southern Blot Analysis
ZOO-BLOT was purchased from Clontech Laboratories, Inc. (Palo Alto,
CA). The ZOO-BLOT contained EcoRI-digested genomic DNAs from
nine eukaryotic species: human, monkey, rat, mouse (BALB/c), dog, cow,
rabbit, chicken, and yeast (Saccharomyces cerevisiae). For Southern blot
analysis of mouse genomic DNA, DNA was extracted from the mouse
liver of 4-mo-old ddy/std and C57BL/6 mice as previously described
(Kaneko et al., 1995). The extracted DNA was thoroughly digested with
one of the restriction enzymes, EcoRI, PvuII, or KpnI. 20 µg of the digested DNA was electrophoresed in 0.8% agarose gel and transferred
onto a nylon filter (Hybond-N+; Amersham International). Filters were
hybridized with an [ Protein Analysis
The anti-CIRP polyclonal antibody was produced by immunizing rabbits
with a carboxyl-terminal oligopeptide (DSYDSYATHNE). For Western
blot analysis, 10 µg of proteins were separated by 14% SDS-PAGE, blotted onto polyvinyl difluoride membranes (Millipore, Tokyo, Japan), and
treated with the antiserum (1:20,000 diluted). Bound antibody was detected using a goat anti-rabbit IgG conjugated with horseradish peroxidase (BioRad Labs, Hercules, CA) and the enhanced chemiluminescence
system (Amersham International). Protein concentrations were determined using the Bradford reagent (BioRad Labs).
Fluorescence Microscopy
Immunofluorescence microscopy was performed on BALB/3T3 cells as
previously described by Osborn (1994) Green fluorescence protein (GFP)/Thr65 was purchased from Clontech
Laboratories Inc., and was ligated into MluI and NotI sites of pMkit-neo
vector (pGFP). Cirp cDNA encoding amino acids 1-162 was ligated inframe into PstI site of GFP/Thr65 (pGFP-CIRP). To assess the intracellular localization of GFP-CIRP fusion protein and GFP, we transfected
pGFP-CIRP or pGFP DNA into COS-7 cells. After 3 d of culture at 37°C,
the medium was removed and replaced with PBS. Then the cells were examined by using a fluorescence microscope (Olympus, Tokyo, Japan)
equipped with the FITC filter set.
Northwestern Analysis
A glutathione-S-transferase (GST)-fusion protein was prepared by cloning a 519-bp PCR fragment (positions 83-601) of cirp cDNA into the
SmaI site of the expression vector pGEX-4T1 (Pharmacia LKB Biotechnology). Transformed DH5 Flow Cytometry
To analyze the effect of CIRP on cell cycle, we cloned the cirp cDNA into
the expression vector pH Isolation of Mouse cirp cDNA
By screening adult mouse testis cDNAs for RNA-binding
proteins with a PCR-based cloning method, we obtained
one fragment that was similar to plant GRPs. After
screening a mouse testis cDNA library with this fragment,
a clone with a 1.3-kb insert (RNP78) was obtained. In
Northern blot analysis, RNP78 hybridized to RNA bands
of ~1.3 and 2.9 kb in size derived from mouse testis (data not shown).
RNP78 (cirp) contained a 1,264-bp insert with an open
reading frame potentially encoding 172 amino acids (Fig.
1). The sequence around the first ATG codon at nucleotide position 81 provided a favorable context for translation initiation (Kozak, 1991
High Conservation of cirp Gene beyond Species
The predicted amino acid sequence of cirp was compared
to known sequences in GenBank using the Genetics Computer Group software package. The overall amino acid sequence of CIRP was similar to human RBM3 (Derry et al.,
1995 To assess the evolutionary conservation of the cirp gene,
Southern blot analysis of genomic DNAs from nine eukaryotic species, human, monkey, rat, mouse, dog, cow,
rabbit, chicken, and yeast, was carried out using the coding
region of cirp cDNA as a probe. As shown in Fig. 3 a, signals were detected in all samples under high-stringent conditions, suggesting that the cirp gene family is well conserved beyond species. When the genomic DNA samples from two different strains of mice were digested with one
of three restriction enzymes
RNA-binding Activity of CIRP
We expressed and purified CIRP as a GST-fusion protein
(Fig. 4 a) and analyzed its RNA-binding activity by Northwestern blot assay (Matunis et al., 1992
Accumulation of CIRP in Response to Cold Stress
To investigate the effect of temperature shifts on cirp expression, we exposed BALB/3T3 mouse fibroblasts to heat
or cold treatment. As shown in Fig. 5 a, Northern blot
analysis indicated that the levels of cirp mRNA increased
markedly in response to mild cold treatment (32-25°C)
but not to severe cold treatment (15°C). In contrast, heat
treatment (39 and 42°C) decreased the levels of expression. Similar results were obtained in two other mouse cell
lines, BMA1 bone marrow stromal cells (Fujita et al., 1983
Localization of CIRP in the Nucleoplasm
Immunofluorescence microscopy using the anti-CIRP
polyclonal antibody showed that signals were detected in
the nucleoplasm of almost all BALB/3T3 cells cultured at
32°C (Fig. 8, a and b), while no signals were detected using
preimmune serum (Fig. 8, c and d). To confirm this result,
we fused cirp and Aequorea GFP cDNAs in an expression
vector. GFP has been used as a molecular reporter to
monitor patterns of protein localization, gene expression, and intracellular protein trafficking in living cells (Ogawa
et al., 1995
Involvement of CIRP in Cold-induced Suppression of
Cell Growth
After a temperature shift from 37 to 32°C, the growth of
BALB/3T3 fibroblasts was impaired (Table I). To assess
whether the induction of the cirp expression is related to
the observed impairment of growth, we examined the effects of ODN antisense to cirp mRNA. The presence of
antisense ODN partially inhibited the induction of p18cirp
by temperature downshift (Fig. 9). Concomitantly, the
growth impairment at 32°C was partially alleviated (Fig.
10), suggesting that the induction of p18cirp is necessary for
growth suppression by cold stress.
Table I.
Effects of p18cirp Expression on the Cell Cycle of BALB/3T3 Cells
Prolongation of G1 Phase by Overexpression of CIRP
To further elucidate the role that p18cirp plays in the regulation of cell growth, a full-length cirp cDNA in an expression vector was stably transfected into BALB/3T3 cells.
Five clones overexpressing p18cirp and seven control clones
transfected with the vector DNA alone were analyzed. Expressions of p18cirp in a representative clone BAC-Sn3 and
a control clone BAC-C1 are illustrated in Fig. 11. The
p18cirp level in BAC-Sn3 cells maintained at 37°C was almost equal to that induced in BALB/3T3 cells upon cold
stress. When these p18cirp-overexpressing clones and control clones were cultured at 37°C, the doubling time of the
former was significantly longer than that of the latter (23.5 vs. 17.6 h, Table I). The cell cycle analysis revealed that
the percentage of cells in G1 phase was 45.4% for control
transfectants and 53.6% for CIRP transfectants. The percentage of cells in S phase was 40.5% for control transfectants and 32.4% for CIRP transfectants. Therefore, the
duration of G1 phase was 6.6 h for control transfectants
and 10.5 h for CIRP transfectants, suggesting that the
lower growth rate of CIRP transfectants was due to the
prolongation of G1 phase. Similar prolongation of G1
phase was observed when BALB/3T3 cells were transferred from 37 to 32°C (6.1 vs. 12.7 h). In addition to prolongation of G1 phase, the duration of S + G2 + M phase
was prolonged in BALB/3T3 cells cultured at 32°C, but
not in CIRP transfectants cultured at 37°C (Table I).
These results indicate that CIRP plays a role in regulation
of growth in response to temperature downshifts, but
other factors also contribute to the cold-induced growth
impairment.
In this paper, we identified a novel RNA-binding protein,
CIRP, the expression of which was induced in mouse fibroblasts in response to the lowered culture temperature.
Growth of mammalian cells is known to be regulated by
various environmental factors, including temperature.
Downshift of temperature from 37 to 31-33°C prolongs
the total generation time of cultured mammalian cells (Rao and Engelberg, 1965 CIRP consists of CS-RBD and a glycine-rich domain.
Binding experiments with ribohomopolymers and various
RNAs have established that most of the CS-RBD-containing proteins have distinct RNA-binding characteristics
(Burd and Dreyfuss, 1994 Recent studies on cold-shock response of E. coli have
shown that CsdA, one of the major cold-shock proteins associated with ribosome, has a helix-destabilizing activity,
and the csdA deletion impairs cell growth and the synthesis of a number of proteins at low temperature (Jones et
al., 1996; Aloia and Raison, 1989
). Although nonhibernating mammals maintain
high uniform body temperatures and have a poor tolerance for hypothermia, their cells may have a capacity for a
far wider cold tolerance (Michl et al., 1966
; Holecková et
al., 1968
). In mammals as well as other organisms, cold
stress changes the lipid composition of cellular membranes
and suppresses the rate of protein synthesis and cell
growth (Rao and Engelberg, 1965
; Sisken et al., 1965
; Watanabe and Okada, 1967
; Nelson et al., 1971
; Nishimune
and Komatsu, 1972
; Burdon, 1987
; Aloia and Raison,
1989
). In clinics, hypothermia is now employed in heart
and brain surgeries and in the preservation of donor organs (Fuller, 1987
). However, the molecular mechanisms regulating the response to cold stress in mammalian cells
are just beginning to be understood (Glofcheski et al.,
1993
; Matz et al., 1995
).
; Goldstein et al.,
1990
; Jones and Inouye, 1994
). Cold stress induces the synthesis of several cold-shock proteins, which are involved in
various cellular processes such as transcription, translation, and DNA recombination (Jones and Inouye, 1994
).
Recently, a family of proteins consisting of one amino-terminal consensus sequence RNA-binding domain (CSRBD)1 and one carboxyl-terminal glycine-rich domain has
been isolated from cyanobacterium (Sato, 1994
, 1995
),
plant cells (Gómez et al., 1988
; Bergeron et al., 1993
; Hirose et al., 1993
; Carpenter et al., 1994
; Heintzen et al.,
1994
), and human (Derry et al., 1995
). This protein family
is referred to as a glycine-rich RNA-binding protein
(GRP) family and some of them have been demonstrated
to be induced by cold stress (Bergeron et al., 1993
; Carpenter et al., 1994
; Heintzen et al., 1994
).
;
Burd and Dreyfuss, 1994
). It is composed of ~90 amino
acids, including two highly conserved sequences, an octamer designated RNP1 and a hexamer designated RNP2,
and a number of other, mostly hydrophobic conserved amino acids interspersed throughout the motif. A number of proteins with CS-RBD have been found in organisms ranging
from Escherichia coli to human (Fukami-Kobayashi et al.,
1993
). They contain one to four CS-RBDs and auxiliary domains that are characterized by an abundance of specific residues in their amino acid sequences (Bandziulis et al., 1989
).
Proteins with CS-RBD are involved in the posttranscriptional regulation of gene expression (Burd and Dreyfuss,
1994
). For example, poly(A)-binding proteins have one CS-RBD and a proline-rich domain and regulate mRNA
stability and translation. SF2/ASF, B52, X16, and PR264/
SC35, whose CS-RBDs make a cluster in the phylogenetic
tree, have a serine-arginine-rich domain and are splicing
factors. Some hnRNPs, such as hnRNP A1, have two CSRBDs and a glycine-rich domain and play important roles in mRNA biogenesis, such as splicing and RNA export.
Although GRPs, hnRNPs, and nucleolin have domains
rich in glycine in common, they belong to phylogenetically
distinct families, and no definite roles played by GRP have
been clarified (Bergeron et al., 1993
; Fukami-Kobayashi et
al., 1993
; Carpenter et al., 1994
; Heintzen et al., 1994
).
Materials and Methods
).
-AGCGGCTGCCATGGCATCAG-3
) spanning the translation initiation site of cirp mRNA, and that of antisense ODN was complementary to this sequence.
-TCGAATTCIAT[C]A[G]AAIC[G]CA[G]AAICC-3
[I; inosine]) encoding the amino acid sequence GFG/AFV/I and
(5
TCAAGCTTTTC[T]A[G]TIGGIGGIC[T]T-3
) encoding the amino
acid sequence F/YV/IGGL. The PCR reaction was repeated for 40 cycles
at 94, 37, and 72°C for periods of 1 min. The PCR products were cloned
into the EcoRV site of TA vector and then sequenced. Using the cloned
PCR fragment as a probe, clone RNP78 was isolated from a mouse testis
cDNA library constructed in
-Zap phage vectors (Stratagene, La Jolla,
CA). The nucleotide sequence of RNP78 insert (cirp) was compared to
known sequences in GenBank using the Genetics Computer Group software package.
-32P]dCTP-labeled random-primed cDNA
fragments, then washed under stringent conditions (65°C for 30 min in a
washing buffer composed of 0.1 × SSC and 0.1% SDS), and detected by
autoradiography. A 650-bp SacI-EcoRI fragment of cirp cDNA was used
as a probe. The filters were stripped and rehybridized with a cDNA probe
for the S26 ribosomal protein as an internal control.
-32P]dCTP-labeled probe at 65°C and washed under
high-stringent conditions (two times in 0.1 × SSC and 0.1% SDS at 65°C).
The coding region of cirp cDNA, positions 82-600, was used as a probe.
. The anti-CIRP polyclonal antibody was used at a dilution of 1:10,000. Detection was with FITC-conjugated goat anti-rabbit IgG (DAKO) diluted 1:1,000. As a control, preimmune serum was used at the same dilution.
E. coli cells were grown at 30°C and GST-
CIRP fusion protein was purified with Bulk GST Purification Modules
(Pharmacia LKB Biotechnology) following the manufacturer's instructions. 2 µg of GST or 1 µg of GST-fusion protein per lane was electrophoresed on 12% SDS-PAGE gels, one of which was stained with Coomassie blue. Others were blotted onto PVDF membrane (Millipore) and
denatured and renatured with guanidine-HCl methods, and Northwestern
analysis was carried out as described by Schumacher et al. (1995)
. Each
RNA homopolymer probe (Pharmacia LKB Biotechnology) was labeled
with [
-32P]ATP and incubated with the blot. To examine the strength of RNA binding, the blots were subsequently washed in the binding buffer
containing increasing concentrations of NaCl up to 2.0 M.
Apr-1 (Gunning et al., 1987
) in the forward orientation relative to the
-actin promoter (pH
Apr-1-CIRP). BALB/3T3
cells were transfected with the pH
Apr-1-CIRP DNA or the pH
Apr-1
DNA. Stable clones were selected in G418 and by limiting dilutions. Five
p18cirp-overexpressors and seven vector-transfected controls were analyzed. Doubling times were determined from the growth curves. For cell cycle analysis, trypsinized cell suspensions were adjusted to a concentration of 1 × 106 cells/ml in prechilled 70% ethanol. Samples stored at 4°C
overnight were stained with propidium iodide and analyzed by Epics Elite flow cytometer (Coulter Corp., Hialeah, FL). A minimum of 10,000 events
were collected, and cell cycle distribution was obtained using a computer
modeling program (Multicycle AV; Phoenix Flow Systems, San Diego,
CA). Experiments were repeated three times. Length of G1 phase was
calculated from the percent of cells in G1 phase according to the equation
Td × {1
log [2
F(G1)]/log 2}, in which Td is the doubling time and
F(G1) is the fraction of cells in G1 phase (Koyasu et al., 1989
).
Results
), and the 5
untranslated region contained an in-frame stop codon at position 10. The
predicted amino acid sequence displayed two main features: the presence of an amino-terminal CS-RBD and a carboxyl-terminal glycine-rich domain. The CS-RBD of
cirp contained consensus sequences of RNP1, RNP2, and
a number of other, mostly hydrophobic conserved amino
acids interspersed throughout the motif (Fig. 2 a). The carboxyl-terminal part was rich in glycine, serine, arginine,
and tyrosine (38.8, 16.4, 19.4, and 10.4%, respectively).
Fig. 1.
Cloning of cirp cDNA. Nucleotide and deduced amino
acid sequences of the clone RNP78 containing cirp cDNA.
Amino acid sequence is shown in single-letter code below the nucleotide sequence. The putative RNP motifs are underlined.
GYGGG and GGYGG, well conserved among GRPs, are doubly
underlined. Terminal codon is indicated by an asterisk. These sequence data are available from GenBank/EMBL/DDBJ under
accession number D78135.
[View Larger Version of this Image (68K GIF file)]
Fig. 2.
(a) Comparison of amino acid sequences in the RNA-binding domains of mouse CIRP, human RBM3 (Derry et al., 1995), B. napus BnGRP10 (Bergeron et al., 1993
), A. thaliana Ccr1 and Ccr2 (Carpenter et al., 1994
), and human hnRNP G (Soulard et al., 1993
).
The consensus sequence for the RNA-binding domain, as determined by Burd and Dreyfuss (1994)
, is also shown. Dots indicate amino
acids identical to the CIRP sequence. The sequences, RNP1, RNP2, DRET, and MNGKXXDG, are boxed. (b) Structural comparison of
CIRP with its related proteins. The length of each bar reflects the actual length of the sequences. The numbers in the black boxes indicate percent identity of amino acid sequence to CIRP in the CS-RBD (RNP motif). Note that the glycine-rich domain of cyanobacterium Anabaena variabilis RbpA1 (Sato, 1995
) is smaller than that of CIRP.
[View Larger Version of this Image (30K GIF file)]
) and plant GRPs such as Brassica napus BnGRP10
(Bergeron et al., 1993
) and Arabidopsis thaliana Ccr1
(AtGRP7) and Ccr2 (AtGRP8) (van Nocker and Vierstra,
1993; Carpenter et al., 1994
). In particular, CIRP was 60-
80% identical in the CS-RBD to these proteins and also
contained the sequences DRET and MNGKXXDG,
highly conserved in plant GRPs and human hnRNP G
(Soulard et al., 1993
) (Fig. 2 a). In addition, the putative CIRP protein is almost the same size as RBM3 (Derry et
al., 1995
) and plant GRPs (Bergeron et al., 1993
; Carpenter et al., 1994
) (Fig. 2 b). These structural similarities suggest that CIRP and plant GRPs are members of the same
family. Cirp is not a mouse counterpart of human RBM3
because we have recently isolated a human cDNA highly
homologous to cirp (95.7% identical in predicted amino
acids) and distinct from RBM3 (Nishiyama, H., and J. Fujita, unpublished data).
EcoRI, PvuII, or KpnI
and analyzed, a single band was detected in each DNA
sample (Fig. 3 b). Thus, the cirp gene is probably a singlecopy gene in mice.
Fig. 3.
(a) Southern blot analysis of EcoRI-digested DNA
from nine eukaryotic species (zoo blot analysis). DNAs were
from human (lane 1), monkey (lane 2), rat (lane 3), mouse (lane
4), dog (lane 5), cow (lane 6), rabbit (lane 7), chicken (lane 8),
and yeast (lane 9). The coding region of cirp cDNA was 32P-labeled
and used as a probe. Autoradiography was done overnight (lanes
1-7) or for 3 d (lanes 8-9) at 80°C. Mobilities of molecular size
markers, HindIII-digested
phage DNA, are indicated on the left. (b) Southern blot analysis of mouse genomic DNA. 20 µg of liver DNAs extracted from either ddy/std mouse (lanes 1, 3, and 5) or C57BL/6 mouse (lanes 2, 4, and 6) were digested with one of
the three restriction enzymes, EcoRI (lanes 1 and 2), PvuII (lanes
3 and 4), and KpnI (lanes 5 and 6), electrophoresed in 0.8% agarose gel, and transferred to a nylon membrane. The coding region
of cirp cDNA was 32P-labeled and used as a probe. Autoradiography was done overnight.
[View Larger Version of this Image (52K GIF file)]
; Schumacher et al.,
1995
). The GST-CIRP protein bound to all RNA homopolymers to a varying extent at low NaCl concentrations, while control GST did not (Fig. 4 b). At high NaCl
concentrations, GST-CIRP bound only to poly(U), suggesting that CIRP protein possessed a specific RNA-binding activity.
Fig. 4.
RNA-binding property of CIRP. (a) Bacterially
expressed GST protein and
GST-CIRP fusion protein
demonstrated by Coomassie blue staining. (b) Northwestern blots showing binding of
GST and GST-CIRP proteins
to radiolabeled ribonucleotide homopolymers, poly(A),
poly(C), poly(G), and poly(U),
at different salt concentrations as indicated.
[View Larger Version of this Image (44K GIF file)]
) and TAMA26 Sertoli cells (Kaneko et al., 1997
)
(Fig. 5 b and data not shown). To examine the expression
at the protein level, we raised a polyclonal antibody against
the predicted carboxyl-terminal peptide of CIRP. The antibody specifically recognized an 18-kD protein as expected
from the amino acid sequence in the lysates of BALB/3T3
cells (Fig. 6). In agreement with the results of Northern blot analysis, the protein level was found to be increased
24 h after a temperature shift from 37 to 32°C. Subsequent
Western blot analysis demonstrated that the level of
p18cirp increased within 6 h after the temperature shift and
peaked at 12 h, and the elevated level persisted for more
than 24 h (Fig. 7).
Fig. 5.
Temperature-dependent expression of cirp
mRNA. Northern blot analysis of total RNAs from
mouse cell lines, BALB/3T3
(a) and BMA1 and TAMA26
(b), harvested 24 h after the
indicated temperature shift.
The positions of 18S and 28S
ribosomal RNAs are indicated on the left. As a control
for the amount of RNA
loaded, the filter was rehybridized with a mouse S26 ribosomal protein cDNA probe (lower).
[View Larger Version of this Image (24K GIF file)]
Fig. 6.
Western blot analysis of BALB/3T3 cell lysates using
an anti-CIRP polyclonal antibody. BALB/3T3 cells were harvested 24 h after the indicated temperature shift. 10 µg of samples was separated by 14% SDS-PAGE. Note specific recognition of an 18-kD protein by the anti-CIRP antibody. Mobilities of
coelectrophoresed molecular size markers are indicated on the left.
[View Larger Version of this Image (31K GIF file)]
Fig. 7.
Kinetics of p18cirp induction in response to cold stress.
BALB/3T3 cells were harvested at indicated times (hour) after a
temperature shift from 37 to 32°C. Mobilities of coelectrophoresed
molecular size markers are indicated on the left.
[View Larger Version of this Image (24K GIF file)]
). When GFP-CIRP expression vector DNA
was transfected into COS-7 cells, fluorescence was found
only in the nucleoplasm (Fig. 8, e and f). On the other
hand, when GFP expression vector DNA was transfected,
fluorescence was detected in cytoplasm and nucleus (Fig.
8, g and h). These results suggest that CIRP is localized in
the nucleoplasm.
Fig. 8.
Localization of
CIRP. Immunofluorescence
microscopy of BALB/3T3
cells cultured at 32°C and
stained with an anti-CIRP
polyclonal antibody (a) or
preimmune serum (c). The
bound antibody was detected by an FITC-conjugated second antibody. Fluorescence
microscopy of COS-7 cells
expressing GFP-CIRP fusion protein (e) or GFP (g). Light (b, d, and f) or phasecontrast (h) microscopic images of the field of view identical to a, c, e, and g, respectively. Bars, 20 µm.
[View Larger Version of this Image (68K GIF file)]
Fig. 9.
Effects of antisense (As) ODN on the cold-induction of
p18cirp. BALB/3T3 cells were incubated at the indicated temperatures for 12 h in the presence of vehicle alone, As, or sense (Sn)
ODNs (0.5 µM). Note partial suppression of the cold-induced
p18cirp expression in the presence of antisense ODN.
[View Larger Version of this Image (40K GIF file)]
Fig. 10.
Effects of antisense (As) ODN on the cold-induced
suppression of cell growth. Cell numbers were determined after 2 d
of culture at the indicated temperature in the presence or absence of indicated concentrations of ODN. The results are expressed as the mean ± SEM. *Statistically different from controls
by unpaired Student's t test (P < 0.02).
[View Larger Version of this Image (34K GIF file)]
Fig. 11.
Expression of p18cirp in representative transfectants.
BALB/3T3 cells, cloned BALB/3T3 cells transfected with cirpexpression vector DNA (BAC-Sn3), or vector DNA (BAC-C1)
were cultured for 12 h at the indicated temperature and analyzed
by Western blotting.
[View Larger Version of this Image (42K GIF file)]
Discussion
; Watanabe and Okada, 1967
).
In mouse leukemic cells (L5178Y) and human amnion
cells, the G1 phase was the most severely affected of the
four phases of cell cycle, although other phases were also
affected to varying degrees (Sisken et al., 1965
; Watanabe
and Okada, 1967
). Our findings in mouse fibroblasts (BALB/3T3) were consistent with these previous observations. Furthermore, we demonstrated that overexpression
of CIRP resulted in reduced growth rate and prolongation
of the G1 phase. It remains to be determined how CIRP
interacts with the known regulators of the G1 progression
(Sherr and Roberts, 1995
) and how it affects duration of
the G1 phase. Interestingly, CIRP and plant GRPs seem
to belong to the same RNA-binding protein family, and
some plant GRPs, such as Sinapis alba SaGRP and Zea
mays ZMGRP, are expressed predominantly in meristematic and growing tissues (Gómez et al., 1988
; Heintzen et
al., 1994
). These plant GRPs are probably involved in regulation of growth rate and/or response to external stimuli
as demonstrated for CIRP in this study.
). The Northwestern assay indicated that CIRP preferentially bound to poly(U). Similar
nucleic acid-binding properties are known for hnRNP C,
hnRNP A1, RGP-1b, and RGP-2 (Swanson and Dreyfuss,
1988a
; Hirose et al., 1993
, 1994
). CIRP was localized to the
nucleoplasm as known for hnRNP C and hnRNP A1
(Dreyfuss et al., 1984
; Pin
l et al., 1989
). The hnRNP C
binds preferentially to U-rich polypyrimidine tracts found
at the 3
-ends of introns and in 3
untranslated regions of
mRNAs and is suggested to be important for 3
-end cleavage and polyadenylation (Swanson and Dreyfuss, 1988b
;
Wilusz et al., 1988
). The hnRNP A1 is suggested to be involved in the 5
-splice site selection in an alternative splicing and mRNA transport (Mayeda and Krainer, 1992
;
Pin
l and Dreyfuss, 1992
). In a similar fashion, CIRP may control the specific or general gene expression independently or by competing with hnRNP C and/or hnRNP A1
for the target binding sequences.
). The secondary structures in mRNAs that inhibit
translation initiation are considered to become more stable at low temperature and are deleterious for growth of
E. coli (Jones and Inouye, 1994
). By unwinding stable secondary structures in mRNAs as an RNA chaperone and
thus facilitating ribosomal functions, CsdA is supposed to
play an essential role in mRNA translation at low temperature (Jones et al., 1996
). The secondary structures and/or
RNA-RNA annealing of pre-mRNA/mRNA are also proposed to play a critical role in processing of pre-mRNA into mRNA (Steitz, 1992
, 1993
; Lamm and Lamond, 1993
).
Therefore, the cold-inducible helix-destabilizing proteins
are probably involved in processing of pre-mRNA at low
temperature as well. Interestingly, hnRNP A1, hnRNP C,
and its CS-RBD possess the ability to destabilize the helix
and/or promote annealing of complementary nucleic acids (Görlach et al., 1992
; Portman and Dreyfuss, 1994
). It remains to be determined whether CIRP has such an RNA
chaperone activity and how reduction of CIRP levels, contrary to the case with CsdA in E. coli, reverse growth inhibitory effects of low temperature in mammalian cells.
Received for publication 15 October 1996 and in revised form 27 February 1997.
This work was partly supported by Grants-in-Aid from the Ministry of Education, Science, Sports, and Culture of Japan.We thank S. Utsumi (Research Institute for Food Science, Kyoto University, Japan) for helpful suggestions. We would like to thank Ms. S. Takatori for skillful technical assistance.
CIRP, cold-inducible RNA-binding protein; CS-RBD, consensus sequence RNA-binding domain; GFP, green fluorescence protein; GRP, glycine-rich RNA-binding protein; GST, glutathione-S-transferase; ODN, oligodeoxynucleotide; RNP, ribonucleoprotein.