(Received for publication, December 11, 1996, and in revised form, February 21, 1997)
From Bristol-Myers Squibb Pharmaceutical Research
Institute, Seattle, Washington 98121 and the § Department
of Pharmacology, University of Wisconsin,
Madison, Wisconsin 53706-1532
Human cyclin G2 together with its closest homolog
cyclin G1 defines a novel family of cyclins (Horne, M. C., Goolsby, G. L., Donaldson, K. L., Tran, D., Neubauer, M., and Wahl, A. F. (1996) J. Biol. Chem. 271, 6050-6061). Cyclin G2 is highly
expressed in the immune system where immunologic tolerance subjects
self-reactive lymphocytes to negative selection and clonal deletion via
apoptosis. Here we investigated the effect of growth inhibitory signals
on cyclin G2 mRNA abundance in different maturation stage-specific murine B cell lines. Upon treatment of wild-type and p53 null B cell
lines with the negative growth factor, transforming growth factor 1,
or the growth inhibitory corticosteroid dexamethasone, cyclin G2
mRNA levels were increased in a time-dependent manner 5-14-fold over control cell levels. Unstimulated immature B cell lines
(WEHI-231 and CH31) and unstimulated or IgM B cell receptor (BCR)
-stimulated mature B cell lines (BAL-17 and CH12) rapidly proliferate
and express low levels of cyclin G2 mRNA. In contrast, BCR-stimulated immature B cell lines undergo growth arrest and coincidentally exhibit an ~10-fold increase in cyclin G2 transcripts and a decrease in cyclin D2 message. Costimulation of WEHI-231 and CH31
cells with calcium ionophores and protein kinase C agonists partially
mimics anti-IgM stimulation and elicits a strong up-regulation of
cyclin G2 mRNA and down-regulation of cyclin D2 mRNA. Signaling mutants of WEHI-231 that are deficient in the phosphoinositide signaling pathway and consequently resistant to the BCR
stimulus-induced growth arrest did not display a significant increase
in cyclin G2 or decrease in cyclin D2 mRNAs when challenged with
anti-IgM antibodies. The two polyclonal activators lipopolysaccharide
and soluble gp39, which inhibit the growth arrest response of immature B cells, suppressed cyclin G2 mRNA expression induced by BCR
stimulation. These results suggest that in murine B cells responding to
growth inhibitory stimuli cyclin G2 may be a key negative regulator of cell cycle progression.
Proliferation signals promote the coordinated progression of a
cell through the cell division cycle. In eukaryotes this process is
controlled by the sequential formation, activation, and inhibition of
cyclin-cyclin-dependent kinase
(CDK)1 complexes (1). Active cyclin-CDK
complexes phosphorylate specific targets such as the tumor suppressor
RB, various transcription factors, DNA polymerase , and cytoskeletal
proteins (2) and thus trigger progression through the cell cycle. The
levels of many cyclins oscillate during the cell cycle and act as
rate-limiting positive regulators of CDK activity. Mammalian cyclins
are classified into different types based on their structural
similarity, functional period in the cell division cycle, and regulated
expression (1, 3, 4). 12 different cyclins in mammalian cells (cyclins A-I, some with multiple subtypes) have been identified (1, 5-7)
either functionally or through an ~110-amino acid homologous region
essential for cyclin-CDK complex formation (8-10) referred to as the
cyclin box (3, 11). Cyclin-CDK activity is also subject to regulation
by CDK inhibitors (CDKIs) such as p15INK4 and p16INK4,
p21WAF1/CIP1, and p27KIP1 which, in response to
negative stimuli, bind cyclin-CDK complexes and block cell cycle
progression (5, 12). In addition to participation in cellular
proliferation, CDKs and cyclin-CDK pairs may participate in processes
not directly related to cell cycle regulation as evidenced by
Pho80-Pho85 cyclin-CDK participation in yeast phosphate metabolism (13,
14), the involvement of p35·CDK5 in promoting neurite outgrowth
(15-17), the association of the cyclin H/CDK7 pair in the TFIIH
transcription factor complex (18, 19), and the cyclin C/CDK8 and
SRB10/11 cyclin-CDK regulation of RNA polymerase II (20, 21).
We studied the effects of stimulatory and inhibitory signals on cell
cycle components expressed in B lymphocytes representative of two
different maturation stages of development. A robust immune system has
to deliver specific and effective immune responses to foreign antigens
and yet be immunologically tolerant of self-antigens. Such tolerance is
achieved because T and B cells pass through stages in their development
when ligation of their antigen receptors by self-antigens results in
negative regulatory signals that induce either unresponsiveness and
functional inactivation (clonal anergy) or their physical elimination
(clonal deletion) (22-24). During clonal deletion, activated
autoimmune cells are eliminated from the repertoire of potentially
reactive immune cells by the induction of growth arrest and apoptosis
(25, 26). This process is contextual and dependent on such factors as
the type of antigen, strength of the antigen-induced signal, the
ontogeny of the cell, the microenvironment of the immune cell, and the
presence of positive costimulatory signals (27-30). Bone marrow
immature IgM+IgD B cells are particularly
prone to undergo growth arrest and eventual PCD upon stimulation of
their antigen receptor (24, 31, 32), as are self-reactive B cells in
the germinal centers of the spleen (30, 33, 34). In contrast IgM
stimulation of non-self-reactive peripheral IgM+ mature B
cells in the presence of appropriate T cell help results in their entry
into an active cell cycle, cellular proliferation, and clonal expansion
(29, 30, 35, 36). Thus, a developmental switch in the differentiation
pathway of B cells coupled to a sensing of the microenvironment through
appropriate costimulatory signals has a profound effect on cell cycle
regulation in response to antigen receptor stimulation of B
lymphocytes.
Because the cyclin G gene was identified as a transcriptional target of
the tumor suppressor p53, a key cell cycle check point control protein
(37-39), and its expression is induced following DNA damage, cyclin G
is hypothesized to play a role in cell cycle check point control (40,
41). Although the function of cyclin G has not yet been determined,
cDNAs encoding a longer form of human and murine cyclin G, referred
to as cyclin G1, and a novel human homolog, cyclin G2, were recently
cloned and characterized (6). The mRNAs for human cyclins G1 and G2
are strongly expressed in tissues rich in terminally differentiated
cells (cardiac and skeletal muscle for cyclin G1 and cerebellum for
cyclin G2) and tissues populated with cells subjected to PCD (spleen
and thymus). Murine cyclin G1 mRNA is expressed independently of
p53 in a number of tissues of p53 null mice (e.g. brain,
heart muscle, and stomach) and can be up-regulated in a p53 null murine
B cell line by TGF- treatment (6). While cyclin G1 mRNA is
constitutively expressed and encodes a protein with no prototypic
"destruction box" involved in ubiquitin-dependent
degradation (42), or protein destabilizing PEST sequences (43), human
cyclin G2 mRNA oscillates through the cell cycle, peaks in S-phase,
and encodes a protein containing a carboxyl-terminal PEST sequence (6).
The closest homolog of this family, cyclin I, is also strongly
expressed in differentiated tissues and has been localized by in
situ hybridization to terminally differentiated neurons of the
hippocampus and cerebellum (7).
We cloned the cDNA encoding the murine form of cyclin G2 and investigated its expression pattern in rodent tissues and various murine cell lines. Our results indicate that cyclin G2 transcripts are present at high levels in murine B cells treated with agents causing growth inhibition or growth arrest but not in cells receiving a positive costimulus that promotes cell cycle progression. In contrast, we found that transcripts for cyclin D2, the D-type G1-phase cyclin associated with proliferation in B cells (44), are down-regulated during G1-phase growth arrest. The up-regulation of cyclin G2 mRNA during cell cycle arrest and its expression in terminally differentiated tissues suggest that this cyclin, and perhaps the related cyclins G1 and I, may function in specific contexts as negative coordinators of cell cycle progression.
Phorbol 12,13-dibutyrate (PdBu), ionomycin
(calcium salt), and propidium iodide were obtained from Calbiochem.
Lipopolysaccharide Escherichia coli serotype 0111:B4 (LPS),
porcine transforming growth factor 1 (TGF-
), dexamethasone and
5-bromo 2
-deoxyuridine (BrDu) were purchased from Sigma. Fluorescein
isothiocyanate-conjugated goat anti-BrDu antibodies were obtained from
Becton-Dickinson (Mountain View, CA.) and µ chain-specific F(ab
)2
goat anti-IgM antibodies were purchased from Jackson ImmunoResearch
(West Grove, PA). COS cell supernatants containing soluble gp39 was the
generous gift of Dr. Diane Hollenbaugh (Bristol-Myers Squibb) (45).
The murine B cell lines WEHI-231 (46) and BAL-17 (47), CH12, CH31 (48), and the WEHI-231 mutants W88.1, W305.1, and W306.1 (49) were kindly provided by Dr. A. DeFranco (University of California, San Francisco). Cells were grown in RPMI 1640 (Life Technologies, Inc.) supplemented with 10% heat-inactivated fetal bovine serum, 2 mM L-glutamine, 1 mM sodium pyruvate, and 50 µM 2-mercaptoethanol at 37 °C in 6% CO2. During experiments, the cultures were maintained in the exponential phase of growth (1-6 × 105/ml).
Isolation of Library cDNA ClonesCyclin G2 DNA probes
were synthesized by polymerase chain reaction using the GeniusTM
system digoxigenin-labeled dNTP mix from human G2 cDNA clones
(Boehringer Mannheim). The resulting polymerase chain reaction
fragments were purified by agarose gel electrophoresis using the
GeneClean II® DNA purification kit (Bio 101, La Jolla, CA) and used to
screen a Zap II murine thymus cDNA library (Stratagene, La
Jolla, CA). Cross-species screening of the murine cDNA library with
human cyclin G2 cDNA probes was done at low stringency with the
hybridization buffer containing 30% formamide and filters hybridized
and washed at 37 °C. Development of the filters with alkaline
phosphatase-conjugated anti-digoxigenin antibodies and the Lumi-PhosTM
530 reagent (Boehringer Mannheim) was done according to manufacturer's
protocol. The isolated phagemid DNA was amplified, extracted, and
purified for sequence analysis following the manufacturer's recommended methods and standard techniques (50).
DNA
sequences were determined using the SequenaseTM (version 2.0) system
following procedures recommended by the manufacturer (United States
Biochemical Corp.). cDNA fragments present in the Lambda Zap® II
phagemid (Stratagene) cloning vectors were sequenced from reactions
primed with either a vector-specific oligonucleotide or
oligonucleotides homologous to the cloned fragment's internal sequences. [33P]dATP or [
32P]dATP (at
800 Ci/mmol) was used to radioactively label the DNA fragments.
Nucleotide sequences were read from scanned gels with the aid of
BioImage® sequence analysis software. The computer-aided editing and
alignment of DNA sequences was accomplished using Genetics Computer
Group (GCG) (Madison, WI) sequence analysis software. Additional
nucleotide and cDNA-derived peptide sequence comparisons were
performed using the BLAST program. Final alignments were performed
using the GCG Pileup and Pretty programs.
Murine lymphocytes were separated into progressive stages of the cell cycle by centrifugal elutriation, and the cell cycle position of elutriated fractions was determined as described previously (6). Unelutriated cell populations stimulated with different reagents were examined using dual-parameter flow cytometric analysis of total DNA content and newly incorporated BrDu. Briefly, following a 20-30-min pulse of a culture with 10 µM BrDu, ~2.0 × 106 cells were sedimented by centrifugation, washed in phosphate-buffered saline and fixed with ice-cold 70% ethanol, and stored at 4 °C until staining and analysis could be performed. The permeabilization and staining with propidium iodide and fluorescein isothiocyanate-conjugated anti-BrDu antibodies were done following protocols supplied by Becton-Dickinson. Flow cytometry was performed utilizing either a FACScan and Lysis II software (Becton-Dickinson Instruments, San Jose, CA) or Coulter EPICS Profile II Analyzer with Multigraph and MultiCycle software (Coulter Electronics, Miami, FL).
Northern Blot AnalysisTotal RNA was isolated from murine
tissues and cells utilizing TRIzol® reagent (Life Technologies, Inc.).
The glyoxal denaturation of total RNA and electrophoresis in
glyoxal-agarose was done following a standard protocol (50). After
electrophoresis, the relative amount and quality of the RNA was
controlled by short wave UV fluorescent shadowing of the ribosomal RNAs
on a F-254 TLC plate. The fractionated RNAs were transferred and fixed
to MagnaGraph® nylon membranes (MSI, Westboro, MA) followed by removal
of residual glyoxal as described (50). Membranes were routinely stained with methylene blue to control for RNA transfer efficiency as described
(50). The [32P]dTTP and [
32P]dCTP
radioactive labeling of DNA fragments was done using polymerase chain
reaction generated and GeneClean II®-isolated DNA fragments as
templates and reagents obtained from the Life Technologies, Inc. random
priming kit. Hybridization of DNA probes to Northern blots was done
according to the methods described by the manufacturer of the nylon
membrane and standard protocols (50). PhosphorImaging (Molecular
Dynamics) of the washed Northern blot filters was routinely obtained
immediately before autoradiography. All Northern blot experiments were
performed at least twice with reproducible results.
Hybridization screening of a murine thymic
cDNA library with an internal cDNA fragment of the human cyclin
G2 ORF (6) at low stringency identified 15 independent overlapping
partial cDNA clones encompassing the full murine cyclin G2 ORF. One
clone comprised nearly the full ORF lacking only the first two
nucleotides of the translation initiation codon. In contrast to the
human cDNA fragments of cyclin G2 cloned from a Jurkat lambda ZapII
cDNA library (6), these murine cyclin G2 cDNA clones did not
contain intron-exon junctions and represented the mature spliced form of cyclin G2. Double-stranded nucleotide analysis verified that the
cDNA clones encompassed a 1035-base pair ORF with 85% nucleic acid
sequence identity to the human cyclin G2 ORF. It encodes a predicted
345-amino acid protein with a molecular mass of 41 kDa which has 94.5%
identity to the predicted human cyclin G2 protein (Fig.
1). Like the human homolog, murine cyclin G2 features a
PEST-rich sequence near the carboxyl terminus, a motif thought to
direct protein degradation (43). Murine and human cyclins G1 and G2
share a carboxyl-terminal sequence motif, previously identified in rat
cyclin G (51), which is homologous to the epidermal growth factor and
polyoma virus middle T antigen autophosphorylation sites (6, 51, 52).
The murine cyclin G2 and murine cyclin A proteins share 47% similarity
and 26% identity. Our analysis indicates that human cyclin I, a cyclin
of unknown function highly expressed in brain and skeletal muscle (7),
is more related to full-length human cyclins G1 and G2 (52% similarity
and 30% identity for both) than to cyclin A (46% similarity and 24%
identity).
Crystallography of cyclin A has defined a new structural motif
consisting of two tandem repeats of a five-helix bundle referred to as
the "cyclin fold" (10, 53, 54). The first repeat spans the cyclin
box (1-
5, see Fig. 1) immediately followed by the second
(
1
-
5
). The amino acid identity between the cyclin G family and
cyclin A is highest in the cyclin box region, yet it extends to the
amino- and carboxyl-terminal regions suggesting that the G family of
cyclins possess a cyclin fold structure similar to cyclin A (Fig. 1).
The amino-terminal region of cyclin A contributes important residues
for CDK binding and structural integrity of cyclin A and is likely to
have a similar function for cyclins G1, G2, and I. Cyclin A residues
Arg-211 and Asp-240 form a buried salt bridge connecting helix 1 with
helix 2 and are essential for cyclin A-CDK activity (9, 10, 53, 55).
The equivalent residues in the sequences of cyclins G1, G2, and I are
conserved, as they are among most cyclins (3). Amino acids at position 266 (lysine) and 295 (glutamate) in cyclin A are crucial CDK contact residues (10, 53) and are maintained in cyclins G1 and G2 and human
cyclin I, although the residues equivalent to the cyclin A 266 lysine
in murine and human cyclin G2 have been conservatively exchanged with
an arginine (Fig. 1). Alanines 235 and 264 are essential for the tight
packing at the interhelical crossing points of cyclin A (10, 53) and
are conserved in the amino-proximal
2 and
3 helices of the G
family cyclins. Additional residues determined to contribute to the
structure of cyclin A (10, 53) which are conserved in the cyclin G2
sequence are indicated by upward arrowheads in Fig. 1.
In contrast, there are nonconserved amino acid exchanges between the
cyclin G family and cyclin A that might modify their structure (10,
53). Alanines 333 and 363 in the carboxyl-proximal 2
and
3
helices of cyclin A, necessary for tight packing of the helices, have
been replaced by negatively charged residues in both human and mouse
cyclins G1, G2, and cyclin I. Extensions of the interhelical regions in
the carboxyl-terminal half of cyclins G1, G2, and I suggest a
distinction between the A and G family of cyclins that may allow for
novel interactions of the G family with other proteins. Furthermore,
crystallography of the cyclin A·CDK2·p27KIP1 complex has
demonstrated the importance of the conserved cyclin A
1 and
3
helix sequences (MRAILVDW and RGKLQ; bold type indicates residues critical for p27 contact) in the interaction of p27KIP1 with cyclin A
through the p27 LFG motif, a motif shared by the Kip/Cip family of
CDKIs (54). A lack of sequence conservation between cyclin A and
cyclins G1, G2, and cyclin I in this region (Fig. 1) suggests that the
latter three do not interact with these CDK inhibitors through the p27
LFG motif.
To determine the size and distribution of cyclin G2
mRNA in murine tissues and cell lines, Northern blot analyses were
performed. A single cyclin G2 mRNA band of ~2.8 kilobases was
differentially expressed in murine tissues compared with cyclin G1.
Abundant cyclin G2 transcripts were found in total brain, neocortex,
spleen, thymus, and intestine (Fig. 2A). In
contrast to cyclin G1, cyclin G2 mRNA was only weakly expressed in
skeletal muscle and heart. Notably cyclin G2 transcripts are most
abundant in tissues rich in either terminally differentiated cells or
cells subject to growth inhibitory signals and PCD. These results were
obtained twice in independent Northern blot analyses and are in
agreement with our observations for human cyclin G2 (6). Functional p53 expression positively correlated with increased cyclin G1 transcripts in proliferating murine B lymphocyte cell lines and in kidney but not
in other terminally differentiated tissue (such as skeletal muscle,
stomach, and brain) (6). The relationship of p53 to cyclin G2 mRNA
expression in cell lines or various developing or terminally
differentiated tissues was not known. Therefore, cyclin G2 mRNA
expression in various tissues from p53 null, heterozygous, and
wild-type p53 mice was compared. No positive correlation between wild-type p53 and cyclin G2 mRNA expression was seen in the tissues examined (Fig. 2B). Cyclin G1 mRNA levels are increased
in stomach and skeletal muscle and slightly in total brain tissue of
p53 null mice (6). Now we report a notable increase in cyclin G2 mRNA in brain tissue of p53-deficient mice (Fig. 2B). As
our previous investigation indicated cyclin G1 expression is inverse to
p53 expression in some stages of embryonic development (6), a
comparative Northern blot analysis of cyclin G2 was performed on murine
embryonic mRNAs. Unlike the on-off-on expression pattern seen for
cyclin G1 transcripts, cyclin G2 mRNA is very abundant throughout
all stages of development and does not parallel p53 transcript levels ((6) and data not shown). Taken together, cyclin G2 and cyclin G1
mRNA expression appear to be independently and differentially regulated during murine embryonic development and tissue
differentiation, and cyclin G2 mRNA levels do not correlate with
p53 expression.
As cyclin G2 is strongly expressed in both human (6) and murine immune system tissues, we examined cyclin G2 expression in several murine leukocyte cell lines. Cyclin G2 mRNA was present at moderate levels (when normalized to GAPDH) in the B cell lines A-20, BCL-1, and WEHI-231, the myeloid leukemia cell line C1498, and thymic epithelium TE-71 cells but was not well expressed in T lymphoid cells (EL-4 and L1210) (data not shown). To further investigate the relationship of p53 to cyclin G2 mRNA expression and examine the cell cycle position-dependent expression of murine cyclin G2, Northern blot analysis was performed on fractionated cells from the p53 wild-type, IgM+ immature B cell line WEHI-231, and the p53 null, IgM+ mature B cell line BAL-17 (Fig. 2C). Exponentially growing cultures of these two B cell lines were fractionated by centrifugal elutriation into populations at progressive stages of the cell cycle, and the position of each fraction was verified by flow cytometry. Northern blot analysis indicated that in WEHI-231 cyclin G2 mRNA was slightly more abundant in the S-phase fractions compared with G1-phase and, in contrast to cyclin G1 expression, decreased in subsequent stages of the cell cycle. In BAL-17 cells the cyclin G2 message was at levels similar to WEHI-231 expression, in contrast to cyclin G1, and moderately increased in S-phase fractions. Expression from the cyclin G1 gene in murine lymphocytes is constitutive (following initial up-regulation in early G1 phase) and partially dependent on transcriptional activation by wild-type p53 (6, 40). In contrast, cyclin G2 transcript levels moderately oscillate through the cell cycle and do not appear to be influenced by the expression of p53.
Modulation of Cyclin G2 Expression by the Growth Inhibitory Factors TGF-To determine if the level of cyclin G2
mRNA could be modulated by positive or negative growth stimuli we
tested the effect of several growth factors on cyclin G2 expression in
a variety of B cell lines. In the B cell compartment TGF- acts as a
negative immunomodulatory cytokine by inhibiting interleukin-7 growth
stimulation of pre-B cells,
light chain expression, and transition
of human and murine B cells from the G1- to S-phases of the
cell cycle (56-59). We have previously shown that cyclin G1 mRNA
is up-regulated by TGF-
in a time-dependent manner
independent of the p53 status of the B cell line (6). Here,
exponentially growing cultures of BAL-17 and WEHI-231 were treated with
TGF-
at 1 ng/ml over 30 h, and aliquots were periodically
sampled for RNA isolation. Northern blot analysis followed by
PhosphorImaging of Northern blots indicated an ~14-fold increase of
the cyclin G2 message in BAL-17 relative to untreated cells within
29 h of treatment (Fig. 3), a time point when the
TGF-
-mediated inhibition of DNA synthesis is ~20% (58). A similar
response was seen with TGF-
-treated WEHI-231 cells, the basal level
of cyclin G2 mRNA expression increasing ~10-fold in cells treated
for 16-29 h (Fig. 3). Glucocorticoid hormones also act as growth
inhibitory factors on lymphoid cells (58, 60-62). We examined the
effect of the glucocorticoid dexamethasone on the expression of cyclin
G2 mRNA. Dexamethasone inhibited the growth of a number of B cell
lines with kinetics similar to that observed with TGF-
; DNA
synthesis was ~83% of untreated control levels after 26 h of
treatment of both BAL-17 cultures with 1 µM dexamethasone
and CH12 cells with 10 µM dexamethasone. Longer periods
of treatment or increasing dexamethasone concentration to 10 µM resulted in a corresponding decrease in cellular
proliferation, with a 35% decrease in the S-phase population of BAL-17
cells after 31 h of culture with 10 µM
dexamethasone. Cyclin G2 mRNA was increased ~5-fold in
dexamethasone-treated cells as compared with untreated controls (Fig. 3
and data not shown). This effect was most obvious in the mature B cell
lines BAL-17 and CH12 (Fig. 3) but was also evident in similarly
stimulated WEHI-231 cells (data not shown). Reprobing all of these
Northern blots with p53 cDNA showed no differences in the p53
mRNA levels of stimulated cells relative to the respective
untreated control (data not shown). Thus cyclin G2 mRNA is
up-regulated, independent of p53, during the response of murine B cells
to two growth inhibitory agents.
Up-regulation of Cyclin G2 and Down-regulation of Cyclin D2 mRNAs Coincident with BCR-induced Growth Arrest and Apoptosis
We next investigated whether other growth inhibitory
signals also elicit an up-regulation of cyclin G2 mRNA in B
lymphocytes. IgM+ immature B cell lines and
IgM+ mature B cells exhibit differential responses to
surface IgM (BCR) ligation (27-29). WEHI-231 and CH31 are immature B
cell lines that undergo growth arrest and eventual apoptosis following
BCR cross-linking (63-65) analogous to self antigen-induced clonal abortion (24, 28) and are often used as in vitro models for B cell tolerance and the elucidation of BCR-mediated signal
transduction pathways (66-69). Logarithmically growing cultures of
WEHI-231 and CH31 cells were stimulated with goat anti-IgM antibodies. The viability and growth of treated and control cultures was monitored by microscopy and trypan blue exclusion. Northern blot analysis for
cyclin G2 and GAPDH mRNA indicated that BCR cross-linking of
immature B cells induces an ~5-10-fold amplification of cyclin G2
transcripts by 12 h of treatment in WEHI-231 and 14 h in
CH31, with the increased level maintained through 24 h of
stimulation (Fig. 4). Hybridization of the same Northern
blot with either cyclin G1 or p53 cDNA probes did not show a change
in their mRNA levels (data not shown). Flow cytometry DNA analysis
indicated that the increase in cyclin G2 transcripts paralleled
G1-phase growth arrest and, in the case of CH31, apoptosis
(tabulated in Fig. 4). Probing the same Northern blots with cyclin D2
cDNA revealed that cyclin D2 mRNA levels decreased relative to
untreated controls, coincident with the onset of growth arrest and the
accumulation of cyclin G2 transcripts (Fig. 4). In contrast, BCR
cross-linking of BAL-17 cells did not result in an increase of cyclin
G2 mRNA or decreased levels of cyclin D2 mRNA (Fig. 4) and
induces a proliferative response rather than growth arrest (Fig. 4).
Likewise, BCR stimulation of CH12 cells does not induce growth arrest
(70) and did not produce a significant elevation of cyclin G2 mRNA
at either 14 or 24 h of treatment (data not shown).
Anti-IgM-stimulated WEHI-231 cells arrest in the G1-phase
of the cell cycle (71, 72). Some have proposed that WEHI-231 late
G1- and S-phase cell populations are insensitive to the
negative signals elicited by BCR cross-linking (71), whereas others
have shown that the efficiency of G1-phase growth arrest is
dependent on the length of time between signal initiation and arrival
of the population at the G1-phase restriction point (72).
We wanted to determine whether there was a cell cycle position
dependence for cyclin G2 up-regulation and cyclin D2 down-regulation in
response to anti-IgM-mediated growth arrest. Purified populations of
early G1-, G1/S-, and early S-phase WEHI-231
cells were isolated by centrifugal elutriation and cultured in the
absence or presence of anti-IgM antibodies. Aliquots were obtained at
progressive times for Northern blot analysis and flow cytometry (Fig.
5). Significant G1-phase growth arrest was
achieved for each population by 25 h of treatment, and full arrest
was attained by 39 h. However, comparison of the early
G1-phase fraction to the S-phase fraction indicated that
the early G1 fraction accumulated a small but detectable population of cells that appeared to be arrested by 6 h of
treatment and a more significant population was observed by 15 h
(one cell cycle) of treatment. In contrast, only a very small arrested
population in the anti-IgM-treated S-phase (fraction 5) culture was
observed by 18 h. Thus there was an ~12-16-h delay in the
initial accumulation of G1 cells following BCR
cross-linking the S-phase population in comparison to the
G1-phase population. Similar results were seen with the
G1/S-phase population (fraction 3); a detectable accumulation in G1 cells was only seen after 18 h of
stimulation. Analogous studies examining the sensitivity and timing of
G1-phase arrest initiation of mid G1-, S-, and
G2-phase populations from 10 to 28 h of treatment with
anti-IgM had comparable results; the majority of cell cycle arrest
occurs following one full cell cycle as the population cycles for a
second time into G1 and reaches the G1 arrest
point (data not shown).
The down-regulation of cyclin D2 and up-regulation of cyclin G2, like the induced G1-phase arrest, is a gradual process. The decrease in cyclin D2 preceded the gradual increase in cyclin G2 message (Fig. 5). This decrease in cyclin D2 followed by a continuous decline was obvious by 3-21 h of anti-IgM stimulation of the early G1-phase fraction but was not clear until 6 h through at least 15 h of IgM cross-linking of either the G1/S- or early S-phase fractions. The increase in cyclin G2 mRNA, when normalized to GAPDH, was apparent by 6 h of signaling in the G1/S fraction and clearly detectable by 7 h in the early G1 population. There appeared to be an additional 2-3-h delay in the up-regulation of cyclin G2 mRNA in the S-phase-stimulated fraction. This occurred while the cells were proceeding through mitosis and entering G1-phase but had not yet entered the S-phase (Fig. 5). A similar experiment with an enriched S/G2 fraction yielded comparable results. Cyclin D2 down-regulation occurred through 7-35 h of stimulation, but the onset of detectable cyclin G2 expression was delayed until after 10-14 h of stimulation (data not shown). Although the length of stimulation necessary for cyclin G2 mRNA induction may be moderately influenced by the cell cycle stage where the signaling begins, the induction of cyclin G2 mRNA accumulation is mostly cell cycle position-independent and precedes a nearly complete G1-phase arrest by 10-15 h.
Increased Expression of Cyclin G2 mRNA Parallels Growth Arrest and Apoptosis of Immature B Cell Lines Stimulated with Phorbol Esters Plus Calcium IonophoresThe phosphoinositide-derived second
messengers diacylglycerol (DAG) and cytosolic calcium
(Ca2+i) play an important role in mediating the
effects of antigen receptor stimulation (73-75). Anti-IgM-induced
growth arrest of immature B cells can be partially mimicked by
treatment of B cells with a combination of phorbol esters and calcium
ionophores (72, 74); however, this pharmacological treatment does not result in growth inhibition of mature B cells (74). To examine if the
increased expression of cyclin G2 mRNA and decrease in cyclin D2
mRNA can be elicited through an increase in
Ca2+i and activation of a PKC-dependent
pathway, we treated logarithmically growing WEHI-231, CH31, BAL-17, and
CH12 cells with 7 nM PdBu in combination with 250 nM ionomycin for a period of 24-44 h. In the
pharmacologically stimulated immature B cell lines WEHI-231 and CH31,
cyclin G2 mRNA up-regulation paralleled the growth arrest response,
while a corresponding reduction in cyclin D2 mRNA was apparent in
WEHI-231 for the first 22 h of treatment (Fig. 6).
Unlike WEHI-231 and CH31, BAL-17 and CH12 cells grown in the presence
of PdBu plus ionomycin did not contain increased cyclin G2 mRNA nor
decreased cyclin D2 message and did not exhibit growth arrest, similar
to the response of these mature B cell lines to BCR stimulation (Fig.
6). Thus the enhanced expression of cyclin G2 transcripts correlates
with a growth arrest response induced by calcium influx and PKC
stimulation.
Anti-IgM-stimulated Mutants of WEHI-231 Deficient in the Phosphoinositide Signaling Pathway Do Not Alter Cyclin G2 or Cyclin D2 Transcript Levels
Cyclin G2 expression in immature B cells
appears to be modulated by signaling networks generating DAG and
Ca2+i. We therefore examined if WEHI-231 mutants
deficient in these pathways and correspondingly resistant to
anti-IgM-induced growth arrest (49) up-regulate cyclin G2 message upon
BCR cross-linking. Three independent WEHI-231 mutants were tested for
the induction of cyclin G2 by anti-IgM treatment. Mutant W306.1 elicits
a reduced level of phosphoinositol production due to a defect in the
activation of phospholipase C; W305.1 has a defect in an undefined
component farther downstream in the signaling cascade triggered by
increases in Ca2+i and DAG, perhaps PKC, and W88.1
is a receptor mutant with less surface IgM but an intact
phosphoinositide signaling cascade (49). Anti-IgM treatment did not
significantly increase cyclin G2 mRNA in W305.1 or W306.1, and
cyclin D2 mRNA was only slightly decreased (Fig. 7).
Only the mutant W88.1, which exhibited some growth inhibition,
displayed an elevation in cyclin G2 and decrease in cyclin D2 message
upon IgM receptor cross-linking, although these alterations are not
equivalent to the wild-type response (Fig. 7). Repeated BCR stimulation
time courses of theses mutants showed comparable results.
Lipopolysaccharide (LPS) and Soluble gp39 Inhibit the Growth Arrest Response and Cyclin G2 mRNA Amplification in Anti-IgM-activated WEHI-231
Polyclonal activators of B lymphocytes such as
bacterially derived mitogens, T cell-derived lymphokines, and helper T
cell membrane proteins are known to protect vulnerable B cells from anti-IgM-induced PCD. The bacterial cell wall component LPS, a potent
activator of both immature and mature lymphocytes, is a strong
inhibitor of the anti-IgM-mediated growth arrest response of WEHI-231
(44, 68, 76). Ligation of the CD40 receptor on immature B cells
in vivo and on WEHI-231 cells in vitro with the T
cell membrane ligand gp39 (CD40L) or anti-CD40 antibodies also
abrogates IgM-mediated PCD (77-79). We tested the protective effect of
these activators in combination with anti-IgM stimulation on cyclin G2
and cyclin D2 mRNA expression in WEHI-231 cells. Cells were
cultured in the presence or absence of anti-IgM antibodies with or
without 1 µg/ml LPS. When stimulated with LPS alone, an increase in
cyclin D2 message was found for the first 2-12 h of treatment followed
by a decline to basal levels between 12 and 14 h (Fig.
8A, right panel). In addition, the decrease
in basal cyclin D2 transcripts observed in anti-IgM growth-arrested
WEHI-231 was inhibited through at least 10 h of costimulation with
LPS, followed by a decline to basal or lower levels thereafter (Fig. 8A, left and right panel). Rather than
inhibiting cyclin D2 expression, costimulation of WEHI-231 with LPS and
anti-IgM antibodies strongly enhanced cyclin D2 transcript expression,
as an increase in cyclin D2 mRNA was observed after 2-10 h of
treatment.
The protective effect of LPS on anti-IgM-induced growth arrest also correlates with a suppression of cyclin G2 mRNA accumulation (Fig. 8A). The early rise in cyclin G2 transcripts at 6 and 10 h in anti-IgM-stimulated cells is strongly repressed by LPS and parallels the protection of WEHI-231 from BCR-induced G1 phase arrest (Fig. 8A, left panel). The rise in cyclin G2 and decline in cyclin D2 mRNA levels at 14 h coincided with loss of the protective effect of LPS (see next paragraph). WEHI-231 cultures stimulated with LPS plus BCR cross-linking antibodies do not, however, produce the same amount of cyclin G2 message as elicited by anti-IgM alone, even after 24 h of costimulation.
Following 12-14 h of stimulation B cell cultures adapt to LPS and no longer respond to its mitogenic signals (76). We tested if pretreatment of WEHI-231 with LPS for 14 h, followed by anti-IgM treatment, provides the same level of protection as obtained when LPS is applied simultaneously with anti-IgM. Cyclin G2 mRNA is increased when LPS had been added 14 h before anti-IgM for a total of 29 and 39 h as compared with simultaneous application of LPS and anti-IgM for 15 and 25 h (Fig. 8A, right panel, first 6 lanes). This increase parallels the increase in G1-phase arrested cells. Thus, due to adaptation, the protective effect of LPS against BCR-induced growth arrest of WEHI-231 is lost following 14 h of prestimulation, and this loss of protection correlates with a rise in cyclin G2 mRNA and a decline in cyclin D2 mRNA back to or below the pre-LPS stimulation basal levels.
A similar repression of cyclin G2 up-regulation was seen when the anti-µ-induced growth arrest is inhibited by a soluble form of gp39 (Fig. 8B), the murine CD40 ligand expressed on T helper cells (45, 80). In this case the reduction of cyclin G2 mRNA is more prominent at 12 h of treatment when the protective effect of soluble gp39 on growth inhibition is most pronounced. Similar to LPS, gp39 by itself strongly up-regulated cyclin D2 mRNA (Fig. 8B, left two lanes), and the inhibition of cyclin D2 mRNA down-regulation by the gp39 costimulation was more obvious earlier in the time course when the abrogation of the arrest response was most effective and fewer cells were in G1-phase arrest compared with controls (Fig. 8B). Taken together, inhibition of anti-IgM-mediated growth arrest and PCD by polyclonal activators of the B cell compartment such as LPS or gp39 correlates with the inhibition of cyclin G2 mRNA up-regulation and at least a modest up-regulation of cyclin D2 mRNA.
We present compounding evidence that expression of cyclin G2 is up-regulated in B cells during responses to negative signaling, and we present arguments for its possible role as a negative regulator of the cell cycle. The gene for cyclin G1, the closest homolog of cyclin G2 (6), is a transcriptional target of the cell cycle check point control protein p53 and may play a role in cell cycle arrest (40, 41). Our finding that cyclin G2 is expressed in both wild-type and p53-deficient murine tissues and cell lines suggests that there is no positive correlation between p53 status or proliferative state of the tissue and cyclin G2 mRNA levels. Cyclin G2 expression may be repressed by p53 as it is enhanced in the brain of p53 null mice. This increase is considerably more than we, and later others (6, 81), have observed for cyclin G1 mRNA in p53 nullizygous brain. Cyclin G1 and G2 mRNAs are abundant in terminally differentiated tissues, e.g. brain and muscle, and those rich in cells subject to PCD (e.g. spleen, thymus) (Fig. 2). We further examined cyclin G2 expression during responses to negative and positive signal transduction using immature and mature B cell lines as a model system.
TGF- B
cells as well as most other cell types have specific TGF- receptors
(57, 82). In many cell types TGF-
stimulation induces the expression
or translocation of CDKIs (e.g. p27KIP1,
p15INK4, and p21CIP1) that block cell cycle progression
(82-85). TGF-
not only induces G1-phase growth arrest
but also apoptosis in normal human and Burkitt B lymphoma cells and
potentiates anti-Ig-induced apoptosis of murine immature B cell lines
(57-59, 70, 86, 87). It is not known if a CDKI is involved in
TGF-
-mediated growth inhibition of WEHI-231, but TGF-
treatment
of WEHI-231 and CH31 results in the accumulation of a
hypophosphorylated form of the retinoblastoma tumor suppressor protein
RB (70).
TGF- growth inhibition in various B cell lines is a slow process,
with a ~20% decrease in cellular proliferation after 24 h of
culture, which for WEHI-231 increases to 40% by 72 h of treatment (58). In contrast to the early transient increase in cyclin G1 mRNA
for TGF-
-treated BAL-17 and WEHI-231 cells (6), cyclin G2 mRNA
steadily increased in similarly treated cultures of both cell lines,
reaching a 10-14-fold elevation at 29 h of culture. In the p53
null cell line BAL-17, up-regulation of cyclin G2 mRNA was
detectable after 15 min, typical for an early response, but in WEHI-231
this effect was not seen before 3-8 h of culture. In both cell lines
this increase did not accompany a change in p53 or, at least in the
case of BAL-17, cyclin D2 mRNA levels2
and preceded a more complete inhibition of cellular proliferation. Analogous to the induction of several CDKIs by TGF-
in other systems
(82, 85), TGF-
induces cyclin G2 mRNA accumulation in murine B
cells. Dexamethasone inhibits the proliferative response of B cells to
anti-Ig and interleukin-4 (58, 60, 61). It caused a strong increase in
cyclin G2 mRNA in CH12 and BAL-17 cells coinciding with a moderate
level of growth inhibition observed at 22-31 h (Fig. 3). This
treatment did not change p53 or cyclin D2 mRNA levels (data not
shown). Enhanced cyclin G2 mRNA expression is thus correlated with
a p53 independent growth inhibitory response of B cell lines to two
immunosuppressive agents known to have negative effects on cell cycle
progression. It is not known if cyclin G2 mRNA levels continue to
increase with extended treatment of murine B cells with either TGF-
or dexamethasone, but it is interesting that both agents enhance
anti-IgM-induced growth arrest of WEHI-231 and block the ability of LPS
to protect WEHI-231 from this growth arrest response (see below)
(58).
BCR stimulation of both immature and mature B cells
induces protein tyrosine phosphorylation, hydrolysis of
phosphoinositide, and activation of PKC (69). This stimulation strongly
up-regulated cyclin G2 mRNA in WEHI-231 and CH31 cells coincident
with the onset of growth arrest and apoptosis (Figs. 3, 6, and 8, and
data not shown) but not in proliferating populations of unstimulated controls or in the anti-IgM-treated mature B cell lines BAL-17 and
CH12. Cyclin G2 mRNA accumulates to detectable levels by 6 h
in unsynchronized anti-IgM-stimulated WEHI-231 and rises by 14 h
to near maximum levels that are maintained for at least 35 h (data
not shown). Simultaneous application of phorbol diesters and calcium
ionophores partially mimics the anti-IgM growth arrest response in
WEHI-231 and CH31 (72, 74) and up-regulates cyclin G2 mRNA. In
addition, the anti-IgM-resistant WEHI-231 mutants W305.1 and W306.1,
which are deficient in either the phosphoinositide signaling pathway or
in a downstream component responsive to Ca2+i
elevation and PKC activation (49), did not up-regulate cyclin G2
mRNA in response to BCR cross-linking. Thus BCR signaling pathways
involving a combination of Ca2+i elevation and PKC
activation are likely to be important for the up-regulation of cyclin
G2 mRNA. The transcription factors c-myc,
junB, c-fos, egr-1, nur77,
nup475, and pip92 are immediate early response
genes that are activated by BCR stimulation and PKC activation with
phorbol esters (69, 88). In addition the pre-existing transcription
factors NF-B, CREB, and Ets-1 are altered upon BCR stimulation, the
first two becoming activated through PKC signaling events, and the
latter inhibited by CaM kinase II phosphorylation (69, 89). While it is
not yet established if a burst of transcriptional activity or the
accumulation of a more stable transcript is responsible for rises in
cyclin G2 mRNA, any one of the above transcription factors could be
involved.
A striking decline in cyclin D2 mRNA preceded the rise in cyclin G2 mRNA during the BCR-evoked growth arrest response of WEHI-231 and CH31 cells (Fig. 4). No change in cyclin D2 mRNA was obvious in the mature B cell lines or WEHI-231 anti-IgM-resistant mutants (Figs. 4, 5, 6 and data not shown). Cyclin D2 is the major D-type cyclin promoting the progression of B cells and other hematopoietic cells through the G1 phase of the cell cycle (44, 90, 91). Mitogenic stimulation of murine primary B lymphocytes with anti-Ig antibodies induces proliferation, cyclin D2 and CDK4 synthesis, and the formation of cyclin D2/CDK4 holoenzymes capable of phosphorylating RB (44). In contrast, anti-IgM treatment of WEHI-231 considerably reduces CDK4 and CDK6 protein levels by 24 h of treatment (79), resulting in accumulation of a hypophosphorylated form of RB (70, 92). During cell cycle regulation, RB and the other related pocket proteins, p107 and p130, are dephosphorylated in early G1-phase, promoting their binding to the E2F family of transcription factors and thereby preventing the transcription of genes important for entry into S-phase, DNA synthesis, and subsequent cell cycle events (93, 94). Cyclin D/CDK4 and cyclin D/CDK6 holoenzymes are believed to be the resident early and mid-G1-phase active kinase complexes responsible for the hyperphosphorylation of RB and related proteins (4, 91). A decrease in cyclin D2 levels in WEHI-231 cells might result in decreased phosphorylation of RB, p107, and p130, a consequent continued binding of these pocket proteins to E2F transcription factors blockading cells at the G1-phase restriction point and inhibiting their entry into S-phase (93, 95). As D-type cyclin proteins are reported to be very unstable proteins (4, 96), it would not be expected that high levels of cyclin D2 protein in WEHI-231 and CH31 cells could persist in the absence of de novo synthesis from cyclin D2 transcripts.
Others have investigated cyclin A protein expression, an S/G2-phase cyclin, and the activity of cyclin A-CDK2 and G1/S-phase cyclin E·CDK2 complexes in growth arresting WEHI-231 (92, 97). After 24 h of BCR cross-linking, when 70-75% of a WEHI-231 cell population is expected to be arrested in G1, cyclin A-CDK2 and cyclin E-CDK2 associated in vitro kinase activity was decreased (97). 12-16 h after BCR cross-linking the expression of p27KIP1 is up-regulated, with increasing amounts of p27KIP1 forming complexes with cyclin A·CDK2 (97). The decrease in cyclin A-CDK2 and cyclin E-CDK2 kinase activity may be secondary to preceding G1-phase cell cycle arrest. While Eshevsky et al. (97) did not examine cyclin D2-CDK4 or cyclin D2-CDK6-associated kinase activity nor the expression of CDK6 protein, they did not find an obvious decrease in CDK4 protein levels or cyclin D2 levels in WEHI-231 cells, in disagreement with results presented here and by others (79). The reason for this discrepancy is not clear, but as these authors indicated it could be due to differences in WEHI-231 clones. We examined transcript abundance compared with both ribosomal RNA and GAPDH mRNA levels, thereby correcting for loading differences or changes in total mRNA under the various conditions. As discussed above we would not expect the unstable cyclin D2 proteins to persist.
How would the dramatic increase in cyclin G2 transcripts and drop in cyclin D2 transcripts during BCR-induced growth arrest ultimately affect the cell cycle? Our observations on the lack of cell cycle dependence of WEHI-231 cells to negative signaling are similar to earlier findings (72) and demonstrate that the anti-IgM growth arrest response is a slow process, the efficiency of arrest increasing with the duration of treatment preceding entry into the G1 phase restriction point. Several inhibitory regulators of the cell cycle may act at different targets to cause cell cycle arrest at the G1-phase restriction point. Synchronized WEHI-231 cells show a considerable drop in cyclin D2 mRNA levels in the early G1-phase fraction by 3 h of anti-IgM treatment and a rise of cyclin G2 levels starting by 6-7 h of treatment. If cyclin D2·CDK4 and cyclin D2·CDK6 complexes decrease when the cells are in G1-phase, RB and related proteins would remain underphosphorylated and associated with E2F transcription factors, thereby inhibiting subsequent transcription of genes important for passing the restriction point. Those cells that passed this restriction point would then complete the rest of the cell cycle until they re-enter the G1-phase and are challenged to cross the restriction point again. This may account in part for the passage of anti-IgM-stimulated late G1 and S-phase WEHI-231 cells through one round of cell cycle before arrest occurs in the following G1-phase, although a balance between the amount of residual D2 message and the onset of cyclin G2 expression may also be important.
As indicated by crystallographic analysis (10, 54) and our protein
sequence alignments, cyclin G2 possesses a cyclin box domain similar to
the cyclin A domain which mediates cyclin A-CDK2 interaction but lacks
the amino-terminal motif important for cyclin A-p27 interaction. While
it is possible that cyclin G2 binds one or more CDKs, it appears
unlikely that cyclin G2 interacts at its amino terminus with p27 or
related CDKIs. As cyclin G2 protein abundance increases, it may
displace other cyclins in cyclin-CDK complexes or may sequester CDKs
not bound to a CDKI and may itself act as a CDKI. Because cyclins G1,
G2, and I contain carboxyl-terminal regions different from other
cyclins, cyclin G2·CDK complexes could further inhibit CDK activity
through a possible interaction with other proteins at its carboxyl
terminus. It is intriguing that cyclin G1 has recently been reported to
interact with two isoforms of the B regulatory subunit of protein
phosphatase 2A (98). The concerted action of several inhibitory
components on the cell cycle, with cyclin G2 perhaps acting as an
anti-cyclin inhibiting the formation of active cyclin-CDK complexes not
yet bound by CDKIs, could cause an eventual G1-phase
arrest. Because rises in cyclin G2 expression are associated with a
G1-phase arrest, it might constrain components that promote
transition through the G1/S-phase restriction point.
LPS is a strong B cell mitogen that accelerates the maturation of immature B cells and protects the immature B cell lines WEHI-231 and CH31 from BCR-induced growth arrest (58, 63, 68, 76). LPS also induces both cyclin D2 synthesis and the formation of cyclin D2·CDK4 complexes in primary murine B lymphocytes (44). We showed that LPS costimulation significantly decreased the abundance of cyclin G2 transcripts and up-regulated cyclin D2 mRNA levels in anti-IgM-stimulated WEHI-231 cells. The degree of cyclin G2 repression and cyclin D2 augmentation correlated with the degree of cellular proliferation. We demonstrated that stimulation of WEHI-231 cultures with LPS alone significantly increased the level of cyclin D2 transcripts for ~12 h of treatment. After that period, it declined to a level observed in the untreated control. This increase in cyclin D2 paralleled an increase in the amount of S-phase cells. Thus, as observed by Tanguay and Chiles (44), high cyclin D2 expression may be a reflection of a highly proliferative B cell population.
A delay in the addition of LPS up to 6 h after the addition of anti-IgM does not result in a loss of protection, but longer delays decrease this protection so that by 14 h less than 20% of the maximal protection is achieved (76). In addition, WEHI-231 cells can adapt to LPS. After prestimulation for 12 h with LPS, WEHI-231 cells are no longer resistant to anti-IgM-induced effects (76). The kinetics of LPS protection of WEHI-231 from growth arrest parallels the kinetics of cyclin G2 mRNA induction. If WEHI-231 cells are stimulated simultaneously with LPS and anti-IgM, cyclin G2 mRNA expression is repressed until 14 h. Then cyclin G2 mRNA accumulation begins and parallels the decrease in the S-phase population seen thereafter. The rise in cyclin G2 levels in the presence of LPS can be augmented if BCR-stimulated WEHI-231 cultures are pretreated with LPS for 14 h prior to the addition of anti-IgM, and these prestimulated cultures contain fewer S-phase cells and more G1-phase-arrested cells than simultaneously costimulated cultures. Thus it appears that a balance between the amount of cyclin D2 and cyclin G2 mRNAs is an important indicator of the protection provided by LPS to immature B cells challenged by B cell receptor ligation. When the balance is tipped so that cyclin G2 transcripts accumulate to high levels and cyclin D2 declines to near or below the amount present in untreated cells, growth arrest ensues. This hypothesis is supported by the observation that inhibition of anti-IgM-mediated growth arrest through CD40 stimulation resulted in a similar decrease in cyclin G2 message and a slight enhancement in cyclin D2 message levels; the rise in cyclin D2 later declining and cyclin G2 rising as the protection afforded by CD40 ligation decreased.
Our investigation suggests that cyclin G2, and perhaps the related cyclins G1 and I, may play a role that is antagonistic to the function of proliferative cyclins. The cloning of murine cyclin G2 and characterization of its expression in various murine tissues provides the basis to further investigate the function of cyclin G2 expression during growth arrest and tissue differentiation by controlled over-expression in different rodent cell lines and the generation of transgenic mice. Production of antibodies specific for cyclin G2 for immunohistochemical studies of selected tissues as well as for the identification of proteins associated with cyclin G2 by immunoprecipitations should now be possible.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) U95826[GenBank].
We thank Drs. A. DeFranco and P. Mittelstadt, University of California, San Francisco, for providing murine wild-type cell lines and mutant B cell subclones and for providing some Northern blots for initial preliminary experiments; Dr. Diane Hollenbaugh for soluble murine gp39; and Becky Hoffman, Wisconsin State Laboratory of Hygiene, for exceptional assistance with DNA flow cytometry. We also thank Joe Cook, Trent Youngman, and Bill Bear for excellent DNA sequence analysis support and Brian Gavin for providing tissue samples from p53-deficient mice. We are grateful to Drs. A. DeFranco, P. Bertics, and W. Heideman for critical reading of the manuscript.