Originally published In Press as doi:10.1074/jbc.M000330200 on June 26, 2000
J. Biol. Chem., Vol. 275, Issue 38, 29660-29671, September 22, 2000
Novel Alternative Splicing and Nuclear Localization of Human
RGS12 Gene Products*
Tapan K.
Chatterjee and
Rory A.
Fisher
From the Department of Pharmacology, University of Iowa College of
Medicine, Iowa City, Iowa 52242
Received for publication, January 14, 2000, and in revised form, May 30, 2000
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ABSTRACT |
RGS proteins are GTPase-activating proteins for
certain G
subunits, accelerating the shutoff mechanism of G
protein signaling, and also may interact with
receptors and effectors to modulate G protein signaling. Here, we
report identification of 12 distinct transcripts of human RGS12 that
arise by unusually complex splicing of the RGS12 gene,
which spans 70 kilobase pairs of genomic DNA and contains 16 exons.
These transcripts arise by both cis- and trans-splicing mechanisms, are expressed in a
tissue-specific manner, and encode proteins ranging in size from 356 to
1447 amino acids. Both 5'- and 3'-splicing of two primary RGS12
transcripts occur to generate RGS12 mRNAs encoding proteins with
four distinct N-terminal domains, three distinct C-terminal domains,
and a common internal region where the semiconserved RGS domain is
located. Confocal microscopy and subcellular fractionation of COS-7
cells expressing RGS12 proteins with three different N termini (brain (B), peripheral (P), and trans-spliced (TS)) and a shared
short (S) C-terminal domain demonstrated exclusive nuclear localization of these proteins and an influence of the N-terminal region on the
pattern of intranuclear distribution. Both native RGS12TS-S in HEK-293T
cells and ectopically expressed RGS12TS-S localized to discrete nuclear
foci (dots), a characteristic of various tumor suppressor proteins.
Subnuclear localization of RGS12TS-S into nuclear dots was cell
cycle-dependent. Native RGS12TS-S associated with the
metaphase chromosome during mitosis, and ectopically expressed
RGS12TS-S induced formation of abnormally shaped and multiple nuclei in
COS-7 cells. Expression of RGS12 proteins with long and intermediate
C-terminal domains was not observed in COS-7 cells, suggesting that
3'-splicing of RGS12 transcripts may influence the expression or
stability of the encoded proteins. These results document extraordinary
structural complexity in the RGS12 family and the role of alternative
splicing and cell cycle-dependent mechanisms in expression
and subnuclear targeting of RGS12 proteins.
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INTRODUCTION |
Heterotrimeric G proteins are components of many major signaling
systems used by cells to transduce a variety of signals
(neurotransmitters, hormones, light, and olfactory and taste signals)
from specific cell-surface receptors to effector proteins (see Refs. 1
and 2 for review). These receptors activate G proteins by stimulating exchange of GTP for GDP on the subunit (G) of the inactive G
protein heterotrimer (G
) to promote dissociation into G-GTP and G subunits. Both of these G protein subunits function as signal-transducing molecules by regulating activities of various effector proteins including enzymes and ion channels. The intensity and
duration of signaling by G proteins are highly regulated. The key
element that controls the lifetime of active G and G is the
intrinsic GTPase activity of the G subunits, producing G-GDP and
its reassembly with G.
RGS (regulators of G protein
signaling) proteins constitute a family of proteins
originally defined by the presence of a semiconserved region of ~120
amino acids called the RGS domain (3). These proteins appear to
function as negative regulators of G protein signaling in organisms
ranging from yeast to man (4, 5). The discovery that RGS proteins, or
their isolated RGS domains, function as GTPase-activating proteins for
certain G subunits in vitro (6, 7) provided the first
insight into how these proteins may exert regulatory influences on G
protein signaling. The crystal structure of RGS4 bound to
Gi1 demonstrated interaction of the RGS domain with the
G protein switch regions and suggested that the mechanism of GTPase
activation by RGS proteins may be due to a reduction in the free energy
of the transition state (8). Coleman and Sprang (9) recently suggested
that RGS proteins may both stabilize the transition state and release
G subunits from an autoinhibited ground state to enhance their
GTPase activity. Additional studies have raised the possibility that some RGS proteins may interact with effectors or receptors to attenuate
G protein signaling. These studies showed that recombinant RGS proteins
can block phosphoinositide-dependent phospholipase C
activation by active Gq in vitro and produce
receptor-selective attenuation of Gq signaling when added
to permeabilized cells (10, 11). Although Koelle and Horvitz (3) first
predicted the existence of at least 15 mammalian RGS family members,
this number has grown to exceed that of the number of identified G subunits; yet the GTPase-activating protein activity of RGS proteins appears to be limited to proteins in the Gi and
Gq family (4), raising an interesting dilemma regarding the
physiological significance of such a large family of RGS proteins.
We undertook studies to clone members of the human RGS protein family
to further our understanding of the structural diversity within this
family. This knowledge is crucial to understanding the structural
determinants that might be involved in regulating the specificity and
function(s) of RGS proteins. Here we report the identification of 12 distinct transcripts of human RGS12 and define their molecular basis of
origin. These transcripts arise by extraordinarily complex splicing of
the RGS12 gene, providing the first documentation of
alternative splicing of an RGS protein gene. Transcripts encoding the
different N-terminal forms of RGS12 were expressed in a tissue-specific
fashion, and the expression and intracellular pattern of distribution
of RGS12 proteins were affected by splicing at the 5'- and 3'-ends of
their corresponding mRNAs. Our results demonstrate the exclusive
nuclear localization of three distinct N-terminal forms of RGS12 in
COS-7 cells, with one form (RGS12TS-S) localizing to discrete foci
(nuclear dots), a characteristic of various tumor suppressor proteins.
We developed an antibody to RGS12TS proteins and identified the
endogenous expression of RGS12TS-S in HEK-293T cells. Localization of
native RGS12TS-S in nuclear dots was cell cycle-dependent
and independent of changes in the level of RGS12TS-S protein. Native
RGS12TS-S associated with the metaphase chromosome in mitotic cells and ectopically expressed RGS12TS-S induced formation of abnormally shaped
and multiple nuclei in COS-7 cells.
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EXPERIMENTAL PROCEDURES |
Materials--
5'-RACE1-Ready
cDNA, Marathon-Ready cDNA, a Quick-Screen cDNA library
panel, and the pEGFP vector were purchased from
CLONTECH. pCR2.1 and pCR3.1 were from Invitrogen.
Elongase was from Life Technologies, Inc. Antibodies to lamin A/C,
c-Myc (9E10), and 14-3-3 were purchased from Santa Cruz
Biotechnology, and an antibody to Na+/K+-ATPase
was from Upstate Biotechnology, Inc. Cell culture medium and serum were
provided by the University of Iowa Diabetes and Endocrinology Research
Center. Oligonucleotide primers and other molecular biological reagents
were obtained from the University of Iowa DNA Core Facility. Polyclonal
anti-RGS12TS antibodies were generated with a synthetic peptide
immunogen corresponding to residues 1-15 of RGS12TS by Biosynthesis
Inc. (Lewisville, TX).
PCR Amplification of RGS12 cDNAs--
Full-length cDNAs
encoding various forms of RGS12 were amplified using a PCR-based
strategy we described previously (12). We utilized a 489-bp expressed
sequence tag identified as RGS12 (GenBankTM/EBI Data Bank
accession number T57943) to design two "RGS12" forward primers
(5'-CTTCATGAGATTGAAGATCTGCAGCTGCTG and
5'-GCTAGCTGGGCCTGGCTGTCGATGTTGACCG) and two RGS12 reverse
primers (5'-ACATGTTCAAGGAGCAGCAGCTGCAGATC and
5'-GATAGCTACACTCGCTTTCTGAAGTCCCC) for use in 5'- and 3'-RACE to
amplify overlapping segments of RGS12 cDNAs essentially as we
described previously (13). Semi-nested 5'-RACE was performed using
5'-RACE-Ready human brain cDNA (anchor sequence at 5'-cDNA end)
as template with a forward primer to the 5'-anchor sequence and nested
RGS12 reverse primers. The same template was used for semi-nested
3'-RACE using nested RGS12 forward primers and an oligo(dT) reverse
primer. Marathon-Ready human lung and placenta cDNAs (adapter
sequences on both cDNA ends) were also used as templates for 5'-
and 3'-RACE using adapter-specific forward or reverse primers in
combination with appropriate nested RGS12 forward or reverse primers.
Resulting PCR products were cloned into pCR2.1, and sequence analysis
of multiple clones revealed successful amplification of overlapping 5'-
and 3'-cDNA fragments of RGS12 from brain, lung, and placenta
cDNAs. Sequence analysis of these clones revealed the existence of
12 different splice variant forms of RGS12. Full-length cDNAs
encoding these splice variant forms of RGS12 were amplified using
forward and reverse primers encompassing the translational start and
stop sites, respectively, specific for each splice variant form.
Resulting full-length cDNAs were cloned into pCR3.1, and double-stranded sequencing was performed by automated fluorescent dideoxynucleotide sequencing by the University of Iowa DNA Core Facility.
PCR Analysis of Tissue Distribution of Transcripts Encoding RGS12
Splice Variants--
Human tissue cDNAs from the Quick- Screen
human cDNA library panel were used as templates in PCR for
amplification of the three 5'-splice variant forms of RGS12 that we
identified by 5'-RACE and cloning. PCR was performed using a forward
primer specific for each 5'-splice variant form of RGS12 (p1, p2, or
p3) and a reverse primer (p4) to regions common to all RGS12 splice
variants. The resulting products were diluted 1:100 and subjected to
PCR using the same forward primer and a nested reverse primer (p5), again to a region shared by all RGS12 splice forms. Amplified products
were separated by agarose gel electrophoresis. The identity of the
amplified products was confirmed by dideoxynucleotide sequencing (University of Iowa DNA Core Facility) following their cloning into
pCR2.1.
Preparation of EGFP Constructs of RGS12--
Various RGS12
protein cDNAs were PCR-amplified using gene-specific primers
incorporating restriction sites to facilitate their cloning into the
EGFP vector. First, amplified RGS12 protein cDNAs were
cloned in the T/A cloning vector pCR2.1 (Invitrogen). Then, restriction
enzyme digestion and agarose gel purification of the cloned RGS12
protein cDNAs were performed. RGS12 protein cDNAs were ligated
to the EGFP vector in frame with its C-terminal EGFP sequence.
Double-stranded sequencing of all cloned RGS12 protein cDNAs was
performed by automated fluorescent dideoxynucleotide sequencing by the
University of Iowa DNA Core Facility.
cDNA encoding the 310-amino acid C-terminal domain of long splice
forms of RGS12 was generated by PCR. A Kozak consensus sequence and an
ATG start codon were included for proper translation of the truncated
protein. Double-stranded sequencing of the cDNA construct was
performed by automated fluorescent dideoxynucleotide sequencing by the
University of Iowa DNA Core Facility.
Cell Culture and Transfection--
COS-7, HEK-293, and HEK-293T
cells were grown in DMEM supplemented with 10% fetal bovine serum and
gentamycin (50 µg/ml) (complete DMEM) in a 5% CO2
humidified atmosphere at 37 °C.
COS-7 cells were transiently transfected with vectors containing
various RGS12 protein cDNAs by electroporation using a Bio-Rad Gene-Pulser. Typically, COS-7 cells (107/ml) were
transfected with 40 µg of plasmid DNA at settings of 0.22 kV and
950 microfarads. Cells were diluted in complete DMEM and plated on
two-chambered slides (Nunc) at a density of ~106
cells/well. For use in immunoblotting, cells were plated at an equivalent density on 10-cm culture plates. Transfected cells were used
in experiments 40 h following transfection.
HEK-293 cells stably transfected with the pVgRXR vector were purchased
from Invitrogen. These cells were transfected with C-terminal
GFP-tagged RGS12TS-S (RGS12TS-S-GFP) in the pIND vector by
electroporation, and stable transfectants were isolated and propagated
in complete DMEM supplemented with G418 (800 µg/ml) and
Zeocin (200 µg/ml; Invitrogen). These cells, designated
EcR293-12TS-S-GFP, express RGS12TS-S-GFP within 12 h following
ponasterone A (5 µM) induction.
Immunofluorescence--
Cells were rinsed three times with DPBS
before fixation for immunofluorescence. For visualization of GFP-tagged
RGS12 proteins in COS-7 cells, cells were fixed by treatment with 4%
paraformaldehyde for 20 min at room temperature, followed by
permeabilization with DPBS containing 0.1% Triton X-100 and 0.1%
Nonidet P-40 for 10 min at room temperature. After permeabilization,
cells were treated with DPBS containing 100 µg/ml RNase A (Roche
Molecular Biochemicals) for 20 min at room temperature prior to
staining with propidium iodide. Cells were stained with propidium
iodide in DPBS for 20 min at room temperature, followed by three washes
with DPBS. Cells were air-dried and then mounted using VectaShield
mounting solution. For visualization of endogenous RGS12TS in HEK-293T
cells, cells were fixed with 70% ethanol at 
20 °C for 1 h,
followed by treatment with 4 N HCl for 30 min at room
temperature. Cells were then incubated with anti-RGS12TS antibody in
phosphate-buffered saline containing 2% bovine serum albumin and 0.2%
Tween 20, followed by washing and incubation with fluorescein
isothiocyanate-conjugated goat anti-rabbit secondary antibody (Sigma).
RNase A treatment and propidium iodide staining were performed as
described for COS-7 cells.
Confocal microscopy was performed with a Bio-Rad MRC 1024 confocal
microscope equipped with a krypton/argon laser at the University of
Iowa Central Microscopy Research Facility. EGFP fluorescence was
examined under a fluorescein isothiocyanate filter, and propidium iodide fluorescence was examined under a Texas Red filter using 60×
oil lenses. Images were captured after Kalman averaging. Images shown
are representative of a minimum of 1600 cells derived from four or more
separate transfections.
Subcellular Fractionation and Immunoblotting--
Subcellular
fractionation of COS-7 cells expressing Myc-tagged RGS12 proteins and
HEK-293T cells expressing native RGS12TS-S was performed as we
described previously (14). Polyclonal anti-RGS12TS antibodies were used
at 1:10,000 dilution. Immunoblotting for specific organelle markers
using lamin A/C as a nuclear marker, Na+/K+-ATPase as a plasma membrane marker, and
14-3-3 as a cytosolic marker in COS-7 cells confirmed the identity
of these fractions. Immunoblotting was performed essentially as we
described previously (13, 14).
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RESULTS |
Identification of Splice Variant Human RGS12 cDNAs--
We
employed a PCR-based strategy to amplify and identify 12 splice variant
forms of human RGS12 using sequence information from a 489-bp expressed
sequence tag (GenBankTM/EBI Data Bank accession number
T57943). Koelle and Horvitz (3) first identified this expressed
sequence tag as a potential RGS protein and named it RGS12. Based upon
this sequence, we designed two forward and two reverse primers for use
in 5'- and 3'-RACE to generate overlapping cDNA fragments of RGS12.
5'-RACE-Ready human brain cDNA and Marathon-Ready human lung and
placenta cDNAs were used as templates in these reactions. Sequence
information obtained from the resulting RACE products was used to
design additional primers for amplification of full-length RGS12
cDNAs. Sequence analysis identified two forms of RGS12 amplified
from human brain that differed at their 5'-ends. Similarly, the 5'-ends
of RGS12 cDNAs amplified from lung and placenta were unique from
each other and distinct from the brain-specific RGS12 cDNAs. In
addition to tissue-specific diversity at the 5'-ends of mRNAs
encoding RGS12, sequence analysis revealed that the 3'-ends of all of
the different RGS12 cDNA forms existed in three different forms.
The coding sequences of the 12 different RGS12 cDNAs ranged from
1068 to 4341 nucleotides, encoding proteins ranging from 356 to 1447 amino acids.
The four different types of 5'-ends of RGS12 cDNAs found in brain,
placenta, and lung encode four different N-terminal sequences for the
RGS12 proteins. We designated the proteins encoded by the two different
RGS12 cDNAs amplified from brain as RGS12B
(GenBankTM/EBI Data Bank accession number AF030109) and
RGS12TS (accession number AF030111) for trans-spliced (see
below). The proteins encoded by RGS12 cDNAs amplified from placenta
and lung were accordingly designated RGS12P (accession number AF030110)
and RGS12L (accession number AF030112), respectively. The three
different types of 3'-ends of the RGS12 cDNAs encoding these four
types of RGS12 proteins encode three different C-terminal sequences
that differed in both sequence and length. These three types of
sequences were designated L for long, S for short, and I for
intermediate to distinguish also the predicted RGS12 proteins on the
basis of their C-terminal sequences. Thus, the long C-terminal tail
form of RGS12B was designated RGS12B-L.
With the exception of the RGS12L isoforms, all RGS12 proteins share a
common internal region of 471 amino acids flanked by unique N- and
C-terminal sequences (Fig. 1). RGS12L
proteins share only 336 amino acids of this common internal domain.
This is a result of N-terminal truncation of the RGS12L proteins due to the presence of a stop codon in the 5'-end of their cDNAs that is
in frame with the RGS domain. Fig. 1 shows that the RGS domain (underlined) is located in the common internal region. The
RGS domain is N-terminally truncated in RGS12L proteins and comprises the N terminus of these RGS12 isoforms. RGS12TS, RGS12B, and RGS12P have unique N-terminal domains of 666, 18, and 8 amino acids, respectively. The region C-terminal to the common internal domain of
RGS12 proteins exists as a short (20 amino acids), intermediate (239 amino acids), or long (310 amino acids) form. The intermediate and long
C-terminal forms share a 235-amino acid sequence.
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Fig. 1.
Organization of the amino acid sequences
encoded by 12 RGS12 transcripts into variable N-terminal, common
internal, and variable C-terminal cassettes. The unique N-terminal
sequences of RGS12TS, RGS12B, and RGS12P are shown. The common internal
region is encoded by all splice variants of RGS12, although
N-terminally truncated for RGS12L (the methionine start codon of RGS12L
is shown in boldface). The unique C-terminal sequences of
short, long, and intermediate forms of RGS12 are shown. The
intermediate and long C-terminal forms of RGS12 share the first 235 amino acids with the C-terminal TSRF sequence of intermediate
forms replaced with a unique 75-amino acid sequence in long forms. The
12 forms of RGS12 encoded by RGS12 mRNAs are produced by assembling
different combinations of these domains.
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Structure of the Human RGS12 Gene--
The observation that the 12 RGS12 isoforms could be constructed from different combinations of N-
and C-terminal cassettes with a common internal domain suggested that
these forms might arise by alternative splicing of a single gene. A
BLAST nucleotide sequence similarity search of the human gene data
banks with the cloned human RGS12 cDNAs revealed that the
RGS12 gene is located within the Huntington disease region
of chromosome 4p16.3. RGS12B-L showed complete homology to interrupted
segments of human genomic DNA sequences from cosmid HS361H4B, HS361H4C,
HSL60G9A, and HSL60G9B. This enabled us to determine the complete
structure of the RGS12 gene. The coding region of the
RGS12 gene spans 69333 bp of DNA and is interrupted by 15 introns. The intron-exon organization of the RGS12 gene in
relation to the RGS12B-L mRNA is shown in Fig.
2. The RGS12 gene contains 16 exons within its coding region that range in size from 22 to 549 bp.
Table I shows the sizes of introns and
the intron-exon splice junction sequences in the coding region of the
RGS12 gene. As shown, the introns vary in size from 295 to
27.6 kilobases, and all of the splice acceptor and donor
sequences agree with the GT/AG consensus sequence (15). The
RGS12 gene intron phasing is type 0 (the intron occurs
between codons) for introns 1, 3-6, 8, 9, 11, and 13; type 1 (the
intron interrupts the first and second bases of the codon) for introns 2, 7, 12, 14, and 15; and type 2 (the intron interrupts the second and
third bases of the codon) for intron 10.
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Fig. 2.
Intron-exon organization of the human
RGS12 gene in relation to the coding sequence of
human RGS12B-L mRNA. The position of exons (filled)
and introns (empty) of the human RGS12 gene are
shown at the top. The structure of the human RGS12B-L mRNA
is shown at the bottom with the locations of introns (vertical
lines) indicated by the mRNA nucleotide number, with base 1 corresponding to the A of the AUG start codon. Sequences encoding the
RGS domain of human RGS12B-L are indicated with hatching.
kb, kilobases.
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Splicing of Human RGS12 Transcripts--
We examined the
relationship between exon and intron locations of the RGS12
gene to the structure of the 12 RGS12 variants we isolated to gain
insight into how the unique N- and C-terminal forms of RGS12 proteins
arise. RGS12B-L results from splicing of exons 1-16 (Fig.
3). Exon 1 encodes both the
5'-untranslated region and the unique N-terminal domain of RGS12B,
whereas the shared common internal domain found in all RGS12 proteins
is encoded by exons 2-13. The short and intermediate C-terminal forms
of RGS12B and all other RGS12 proteins arise by skipping of exon 14 and
retention of intron 15, respectively (Fig. 3). Although the transcript
encoding the intermediate C-terminal forms of RGS12 proteins is longer
than that encoding the long forms, the presence of a stop codon
produces a shorter protein. Thus, the RGS12 gene can be
alternatively spliced near its 3'-end to generate the three types of
C-terminal sequences present on the four N-terminal forms of
RGS12L.
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Fig. 3.
Representation of the splicing events
occurring in the human RGS12 gene to generate 12 splice variant RGS12 mRNAs. Exons are shown as filled
boxes, introns as empty boxes, and noncoding sequences
as hatched boxes. Two primary transcripts encode the four
5'-splice forms of RGS12; one is processed to RGS12B and RGS12TS, and
one is processed to RGS12P and RGS12L. The primary transcript encoding
RGS12B and RGS12TS mRNAs includes exon 1 of the human
RGS12 gene, and that encoding RGS12P and RGS12L mRNAs
uses an alternate transcriptional start site within intron 1 of the
human RGS12 gene. The middle of the figure shows
how 3'-splicing generates the long, short, and intermediate transcripts
of RGS12B as well as the 3'-splice forms of RGS12TS, RGS12P, and RGS12L
mRNAs. trans-Splicing of a transcript encoded by three
exons of an unknown gene (X gene) generates RGS12TS. RGS12L arises by
retention of intron 3 of the human RGS12 gene.
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Unlike RGS12B proteins, the unique N-terminal domains of RGS12P,
RGS12L, and RGS12TS proteins are not encoded by sequences from exon 1 of the RGS12 gene. Comparison of the sequence encoding the
N-terminal domain of RGS12P with that of the RGS12 gene
revealed that the unique N-terminal domain of RGS12P proteins is
encoded by sequences from intron 1 of the RGS12 gene. The
5'-end of transcripts encoding RGS12P proteins retains 1384 bp of the
3'-end of intron 1, presumably a result of an alternate transcriptional
start site at this location. An alternate translational start site in
frame with the RGS domain sequence is located 1360 bp from the 5'-end of the RGS12P transcript. Thus, this translational start site is
encoded by sequences located 24 bp from the 3'-end of intron 1 (Fig.
3). A similar analysis showed that the 5'-end of transcripts encoding
RGS12L retains both the 1384-bp intron 1 sequence as well as all of
intron 3 (Fig. 3). The N-terminal truncation of RGS12L within the
common internal region of RGS12 proteins results from a stop codon
present in the retained intron 3 sequences. The only start codon that
could produce a translational product in frame with the RGS domain in
RGS12TS transcripts is present in exon 5 and corresponds to
Met136 of the common internal region (Fig. 1). As a result,
the C-terminal half of the RGS domain encodes the N-terminal domain of
RGS12L proteins. Thus, the 5'-ends of transcripts of both RGS12P and RGS12L are located within sequences spliced out of transcripts encoding RGS12B.
The sequence encoding the unique N-terminal region of RGS12TS proteins
is not present within or upstream of the RGS12 gene. A BLAST
search of the human gene data banks with the sequence from the 5'-end
of RGS12TS transcripts showed complete homology to interrupted segments
from cosmids HSL185E6A and HSL21F12B. These cosmids map to a site on
chromosome 4p16.3 located 170 kilobases from the 3'-end of the
RGS12 gene from the DNA ()-strand. The 5'-ends of RGS12TS
transcripts are derived from nucleotides 15808-15924 of the
()-strand of HSL21F12B and nucleotides 12599-14580 and 15701-16502
of the ()-strand of HSL185E6A. Thus, the unique N-terminal domain and
the 5'-untranslated region of RGS12TS appear to be encoded by a
transcript arising from three exons of an unknown gene ("X" gene)
that splices onto exon 2 of the RGS12 gene to form the
full-length RGS12TS transcript. This phenomenon of splicing of two
independent transcripts, known as "trans-splicing" (16), is much less common than the cis-splicing used to generate
alternatively spliced variants from within a single gene. Accordingly,
the proteins encoded by RGS12 transcripts with this unique 5'-end were
designated RGS12TS.
Tissue Distribution of Human RGS12 Transcripts--
The divergence
in sequence of cDNAs encoding different N-terminal forms of RGS12
proteins enabled us to design primers to examine expression of their
transcripts in tissues by PCR. For these experiments, we used the
Quik-Screen library panel of cDNAs and primers specific for
sequences encoding the unique 5'-ends of RGS12 transcripts. Semi-nested
PCR was performed with a single specific forward primer and two nested
reverse primers to a region common to all RGS12 transcripts derived
from exon 7 of the RGS12 gene. Sequencing of resulting PCR
products confirmed their identities as the expected amplification
products. Fig. 4A shows that
PCR with a forward primer spanning the translational start site of RGS12B (exon 1 of the RGS12 gene) amplified the expected
product from brain cDNA, but not from other tissue cDNAs. Fig.
4B shows the results of PCR amplification using a forward
primer designed to the sequence derived from intron 1 of the
RGS12 gene that serves as the 5'-end of both RGS12P and
RGS12L. As shown, products of the expected size were amplified from
kidney, placenta, and lung, i.e. the lung product is larger
due to the retention of sequences derived from intron 3. Sequencing of
the smaller faint band amplified from lung showed that it was identical
to the products amplified from placenta and kidney that correspond to
the 5'-end of RGS12P cDNAs. Thus, the major amplification product
in lung corresponds to RGS12L, although a product corresponding to
RGS12P can also be detected. Fig. 4C shows the results of
PCR amplification using a forward primer designed to a sequence present
in the N terminus of RGS12TS that is derived from the second exon of
the X gene. The expected PCR products were amplified from kidney, lung,
and placenta, but not brain. These results show that transcripts
encoding different N-terminal forms of RGS12 proteins have both common and unique tissue expression patterns.
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Fig. 4.
PCR analysis of tissue-specific expression of
RGS12 transcripts with unique 5'-ends. Semi-nested PCR was
performed utilizing primers (p1, p2, and p3) specific for sequences
encoding the unique 5'-ends of RGS12 transcripts and the Quick-Screen
human cDNA library panel as templates. Two nested reverse primers
(p4 and p5) utilized in these PCRs were from a region common to all
RGS12 transcripts derived from exon 7 of the RGS12 gene.
Each panel shows a diagram of the RGS12 cDNA with locations of the
forward and semi-nested reverse primers used in PCR and the agarose
electrophoresis analysis of the amplified products. A, PCR
amplification with a forward primer spanning the translational start
site of RGS12B; B, PCR amplification with a forward primer
designed to the sequence derived from intron 1 of the RGS12
gene that represents the 5'-end of both RGS12P and RGS12L;
C, PCR amplification with a forward primer designed to a
sequence present in the N terminus of RGS12TS that is derived from the
second exon of the X gene. Molecular sizes of amplified products were
determined from 1-kilobase pair and 100-bp DNA ladders (Life
Technologies, Inc.) run in parallel. Sk., skeletal.
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Subcellular Localization of Human RGS12 Proteins--
The
different forms of RGS12 were tagged at their C termini with either GFP
or c-Myc to examine their expression by confocal microscopy and
immunoblotting, respectively. We focused our experimental attention on
the RGS12 proteins possessing a complete common internal region so that
any differences in expression or intracellular distribution of these
proteins could be correlated to splicing events leading to different N-
or C-terminal forms of the proteins. Fig.
5 shows confocal microscope images of
COS-7 cells expressing the GFP-tagged short forms of RGS12B, RGS12P,
and RGS12TS. The green color represents the GFP
fluorescence from expressed RGS12 proteins, and the red
color represents fluorescence from propidium iodide staining of
nuclei in these cells. To confirm any apparent nuclear localization of
expressed RGS12 proteins by visualization of GFP fluorescence alone, an
overlay image of the GFP and propidium iodide fluorescence is also
shown. As shown, all three RGS12 proteins were localized exclusively in
the nucleus of COS-7 cell transfectants. Although RGS12B-S and RGS12P-S
exhibited a homogeneous pattern of distribution throughout the nucleus,
RGS12TS-S exhibited a unique pattern of dotted distribution within the
nucleus. No evidence was obtained for accumulation of any of these
proteins in the cytoplasm or plasma membrane. The nuclear localization
of RGS12 proteins is quite distinct from the predominantly cytoplasmic localization of RGS4 that is observed in COS-7 cells (Fig.
6). As an alternate approach to examine
the intracellular distribution patterns of RGS12 proteins, we performed
immunoblotting of subcellular fractions of COS-7 cells expressing
Myc-tagged forms of these proteins. Fig.
7 shows that these three RGS12 proteins
were localized nearly exclusively in the nuclear fraction of COS-7
cells, in agreement with the confocal microscopic evidence for their
nuclear patterns of distribution in COS-7 cells.
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Fig. 5.
Confocal microscope images of COS-7 cells
expressing short forms of RGS12B, RGS12P, and RGS12TS tagged at their C
termini with GFP. Green represents GFP fluorescence
from expressed RGS12 proteins; red represents propidium
iodide (PI)-stained cell nuclei; and yellow (in
the overlay image) represents overlapping green and
red fluorescence. Transfection of COS-7 cells and
immunofluorescence measurements were performed as
described under "Experimental
Procedures."
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Fig. 6.
Confocal microscope images of COS-7 cells
expressing human RGS4 protein tagged with GFP at its C terminus.
Green represents GFP fluorescence from expressed RGS4;
red represents propidium iodide (PI)-stained cell
nuclei; and yellow (in the overlay image) represents
overlapping green and red fluorescence.
Transfection of COS-7 cells and immunofluorescence measurements were
performed as described under "Experimental Procedures."
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Fig. 7.
Immunoblots of subcellular fractions of COS-7
cells expressing C-terminal c-Myc-tagged forms of RGS12TS-S
(A), RGS12B-S (B), and RGS12P-S
(C). COS-7 cell transfectants were lysed
(Lys) and subfractionated into nuclear (Nuc),
cytosolic (Cyto), and membrane (Mem) fractions as
described under "Experimental Procedures." c-Myc immunoblotting was
performed on the resulting cell lysates and an equivalent amount of
each fraction as described under "Experimental Procedures."
Locations of molecular mass markers (in kilodaltons) are shown
to the left of the autoradiograms.
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In contrast to the reproducible nuclear expression of the short splice
forms of RGS12 proteins in COS-7 cells, we were unable to detect
expression of the long splice forms of these proteins. No GFP
fluorescence was detected in COS-7 cells transfected with the
GFP-tagged long splice form of RGS12B, RGS12P, or RGS12TS. Immunoblotting of lysates of cells transfected with c-Myc-tagged forms
of these proteins similarly showed no detectable expression of the
proteins. Treatment of transfectants with inhibitors of proteasome (10 µM MG-132)- or calpain (25 µM
N-acetyl-leucyl-leucyl-norleucinal)-dependent proteolytic pathways did not promote expression of the long splice forms of RGS12, suggesting that these pathways likely do not contribute to the lack of expression of the long splice forms of RGS12. We prepared a GFP-tagged construct of the intermediate splice form of
RGS12B and similarly were unable to detect its expression. These
results suggested that lack of expression of the long and intermediate
splice forms of RGS12 was due to sequences in the mRNA or protein
that encode or comprise, respectively, their unique C-terminal domains.
Therefore, we examined whether the unique 310-amino acid C-terminal
domain of the long splice forms of RGS12 could be expressed as a GFP
fusion protein. Fig. 8 shows that this
domain was expressed in both the nucleus and cytoplasm of COS-7 cells.
Thus, if this domain contributes to the inability to express the long
splice forms of RGS12, it must do so within the context of a
holoprotein or corresponding mRNA. Alternatively, we reasoned that
the lack of expression of long splice forms of RGS12 could result from
an inability of the cells expressing these proteins to survive. To
consider this possibility, we cotransfected cells with untagged
RGS12TS-L (in pCR3.1) and the GFP vector alone to determine whether
expression of GFP would be diminished in cells cotransfected with
RGS12TS-L compared with those cotransfected with the GFP and pCR3.1
vectors. Both transfectants exhibited comparable and robust expression
of GFP (data not shown).
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Fig. 8.
Confocal microscope images of COS-7 cells
expressing the 310- amino acid C-terminal domain of long splice forms
of RGS12 proteins tagged with GFP at their C termini.
Green represents GFP fluorescence from expressed RGS4;
red represents propidium iodide (PI)-stained cell
nuclei; and yellow (in the overlay image) represents
overlapping green and red fluorescence.
Transfection of COS-7 cells and immunofluorescence measurements were
performed as described under "Experimental Procedures."
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Subcellular Localization of Native RGS12TS-S--
We raised an
antibody to one of the N-terminal forms of RGS12 for use in determining
whether native RGS12 proteins show a pattern of nuclear localization as
observed in COS-7 cells expressing recombinant forms of these proteins.
This antibody was raised to a synthetic peptide corresponding to
residues 1-15 of RGS12TS proteins. This polyclonal anti-RGS12TS
antibody recognized ectopically expressed RGS12TS-S following
immunoblotting or immunocytochemistry (see below). We used the
anti-RGS12TS antibody to screen various human cell lines for endogenous
RGS12TS immunoreactivity and found that HEK-293T cells express
appreciable levels of RGS12TS. Fig. 9
shows that RGS12TS immunoreactivity in HEK-293T cells migrated with the
same molecular size as RGS12TS-S-Myc transiently expressed in COS-7
cells, suggesting that HEK-293T cells endogenously express the RGS12TS
protein variant we designated RGS12TS-S. Interestingly, although
SV40-transformed HEK-293T cells express RGS12TS-S, HEK-293 cells do
not. We developed stable transfectants of HEK-293 cells expressing
C-terminal GFP-tagged RGS12TS-S under the control of an
ecdysone-inducible promoter and named this stable cell line EcR293-12TS-S-GFP. As shown in Fig. 9, RGS12TS immunoreactivity was
present in lysates of these cells following ponasterone (5 µM) treatment to induce expression of RGS12TS-S-GFP, but
not in lysates from vehicle-treated cells. The RGS12TS immunoreactivity migrated as a doublet with the higher molecular mass band corresponding to the size expected for RGS12TS-S-GFP. Both RGS12TS-immunoreactive bands in ponasterone-induced EcR293-12TS-S-GFP lysates were detected also by immunoblotting with anti-GFP antibodies (data not shown). The
nature of heterogeneity in size of induced RGS12TS-S-GFP is unclear,
but may reflect post-translational changes or proteolysis of the
protein. Together, these results illustrate that the anti-RGS12TS antibody detects both native and ectopically expressed RGS12TS-S.
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Fig. 9.
RGS12TS-S is expressed endogenously in
HEK-293T cells. RGS12TS-S immunoblotting was performed on lysates
derived from HEK-293T cells, COS-7 cells transiently transfected with
c-Myc-tagged RGS12TS-S, and EcR293-12TS-S-GFP cells before and
after 5 µM ponasterone induction for 12 h.
Immunoblotting was performed as described under "Experimental
Procedures." Locations of molecular mass markers (in kilodaltons) are
shown to the left.
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We next examined the subcellular localization of native RGS12TS-S in
HEK-293T cells by subcellular fractionation and confocal microscopy.
Fig. 10A shows that
RGS12TS-S is found exclusively in the nuclear fraction of HEK-293T
cells. In agreement with these findings, confocal microscopy of
HEK-293T cells showed that RGS12TS immunoreactivity in HEK-293T
cells exhibits a dotted pattern of nuclear distribution (Fig.
10B). Thus, the pattern of expression of endogenously
expressed RGS12TS-S in HEK-293T cells is very similar, if not the same,
as that observed in COS-7 cells overexpressing RGS12TS-S-GFP (Fig.
5).
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Fig. 10.
Subcellular localization of native
RGS12TS-S. A, immunoblot of subcellular fractions of
HEK-293T cells endogenously expressing RGS12TS-S. HEK-293T cells were
lysed and subfractionated into nuclear, cytosolic, and membrane
fractions as described under "Experimental Procedures."
Immunoblotting with RGS12TS-specific antibody was performed on the
resulting lysate and an equivalent amount of each fraction as described
under "Experimental Procedures." Locations of molecular mass
markers (in kilodaltons) are shown to the left. B, confocal
microscope images of HEK-293T cells endogenously expressing RGS12TS-S.
Green represents fluorescein isothiocyanate
(FITC) fluorescence from RGS12TS immunoreactivity;
red represents propidium iodide (PI)-stained cell
nuclei; and yellow (in the overlay image) represents
overlapping green and red fluorescence.
Immunofluorescence measurements of endogenously expressed RGS12TS were
performed as described under "Experimental Procedures."
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Cell Cycle Regulation of RGS12TS-S Nuclear Dots--
The dotted
intranuclear distribution of RGS12TS-S is strikingly similar to that of
promyelocytic leukemia protein PML, leukemia-associated protein ALL-1,
and breast cancer-associated proteins BRCA1 and BARD1 (17-20). At
present, the precise functional significance of the distribution of
these proteins in nuclear dots is not understood. However, PML protein
promotes transcriptional silencing/enhancing and exhibits tumor
suppressor activities, and its dotted nuclear distribution de-localizes
during acute promyelocytic leukemia and certain viral infections
(21-26). BRCA1 functions as a tumor suppressor protein and localizes
to nuclear dots during the S phase of the cell cycle (19).
Hydroxyurea-mediated DNA synthesis arrest induces loss of BRCA1 nuclear
foci, a response accompanied by hyperphosphorylation of BRCA1. Thus,
BRCA1 S phase nuclear dots are dynamic elements, responsive to DNA
damage, and involved in replication checkpoint responses (19).
Therefore, we examined whether RGS12TS-S nuclear dots are cell
cycle-regulated by determining the nuclear immunolocalization pattern
of RGS12TS-S in HEK-293T cells blocked at different stages of the cell
cycle (Fig. 11). A pattern of evenly
distributed RGS12TS-S nuclear dots was present in asynchronously
growing HEK-293T cells. RGS12TS nuclear dots were unevenly distributed
and somewhat clumped together in cells blocked at the G1/S
cell cycle boundary by treatment with hydroxyurea, aphidicolin, or
thymidine. However, nocodazole-mediated blockade of HEK-293T cells at
the G2/M cell cycle boundary produced loss of RGS12TS-S
nuclear dots and a diffuse distribution of RGS12TS in the nucleoplasm.
A similar loss of RGS12TS-S nuclear dots occurred in quiescent cells
(G0) that exited the cell cycle by serum deprivation. The
loss of RGS12TS-S nuclear foci in HEK-293T cells at G0 and the G2/M cell cycle boundaries prompted us to examine the
localization of RGS12TS-S in cells undergoing mitosis. Fig.
11B shows that RGS12TS-S overlapped with the metaphase
chromosome and evenly distributed to dividing chromosomes. The amount
of RGS12TS-S protein in HEK-293T cells arrested at various phases of
the cell cycle did not differ significantly (Fig. 11C).
These findings suggest that RGS12TS-S localizes to nuclear dots during
the G1/S phase of the cell cycle. The localization of
RGS12TS-S to discrete nuclear foci in HEK-293T cells and the loss of
this localization during the G2/M and G0 phases
of the cell cycle appear to be independent of changes in the
steady-state level of RGS12TS-S protein.
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Fig. 11.
Cell cycle regulation of RGS12TS-S nuclear
dots. A, confocal microscope overlay images of
endogenously expressed RGS12TS-S in HEK-293T cells growing
asynchronously (panel a) or blocked at various phases of the
cell cycle by treatment for 24 h with hydroxyurea (panel
b), thymidine (panel c), aphidicolin (panel
d), and nocodazole (panel e). HEK-293T cells were also
deprived of serum (panel f) by culturing for 32 h in
serum-free DMEM. Endogenously expressed RGS12TS-S (green) is
seen against the propidium iodide-stained cell nucleus
(red). B, confocal microscope images of RGS12TS-S
localization within mitotic HEK-293T cells. Green
fluorescence represents RGS12TS-S immunoreactivity, and red
fluorescence represents propidium iodide (PI)-stained cell
nuclei. C, immunoblot of RGS12TS-S in lysates of HEK-293T
cells blocked at various phases of the cell cycle. Immunoblotting of
-tubulin is shown as a control for protein loading.
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Aberrant Nuclear Morphology and Multiple Nuclei in COS-7 Cells
Overexpressing RGS12TS-S--
Approximately 10% of COS-7 cells
transiently expressing RGS12TS-S-GFP exhibited aberrant nuclear
morphologies. Fig. 12A
illustrates an example of a dumbbell-shaped nucleus that also has
nuclear buds or blebs. In addition, a significant number of
RGS12TS-S-GFP-expressing COS-7 cells exhibited multiple nuclei (Fig.
12B). Both of these nuclear anomalies were not observed with
other GFP-tagged RGS proteins including RGS2, RGS4, RGS10, RGS16,
RGS12B-S, and RGS12P-S or in cells transfected with GFP vector alone
(data not shown). These nuclear abnormalities also were not observed in
EcR293-TS-S-GFP cells following induced expression of RGS12TS-S-GFP.
These results suggest that ectopic expression of RGS12TS-S dysregulates
nuclear division and/or cytokinesis in a subpopulation of COS-7 cells and that this response is cell type-dependent.
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Fig. 12.
RGS12TS-S induces formation of abnormally
shaped and multiple nuclei in COS-7 cells. A, confocal
microscope images depicting nuclear anomalies in COS-7 cells
ectopically expressing RGS12TS-S-GFP. Green represents GFP
fluorescence from expressed RGS12TS-S, and red
fluorescence represents propidium iodide (PI)-stained
cell nucleus. B, confocal microscope images showing
formation of multiple nuclei in transfected COS-7 cells ectopically
expressing RGS12TS-S-GFP. Immunostaining of -tubulin was performed
for visualization of the cell cytoplasm. Green
represents GFP fluorescence from expressed RGS12TS-S,
and red fluorescence represents endogenous -tubulin
immunoreactivity.
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DISCUSSION |
This study has elucidated a remarkable complexity in processing of
the RGS12 gene to produce 12 distinct forms of RGS12
differing in both N- and C-terminal sequences. These results are the
first to document alternative splicing of an RGS protein gene. Thus, both genes for RGS proteins and their presumed regulatory targets, G
subunits, may be spliced differentially to produce proteins with
distinct structural features. Our results show that transcripts encoding the different N-terminal forms of RGS12 are expressed in a
tissue-specific fashion and that the expression and intracellular pattern of distribution of RGS12 proteins are affected by splicing at
the 5'- and 3'-ends of their corresponding mRNAs. Our demonstration that the short forms of RGS12 proteins are nuclear proteins suggests that the functional role of these proteins might be very different from
that proposed for many members of the RGS protein family. Indeed, we
demonstrate here that native RGS12TS-S exhibits a pattern of subnuclear
targeting to nuclear dots (characteristic of various tumor suppressor
proteins) that is cell cycle-dependent and associates with
the metaphase chromosome during mitosis. Ectopic expression of
RGS12TS-S in COS-7 cells induced nuclear abnormalities and multinucleated cells that were not observed in cells expressing other
RGS proteins.
The complexity and mechanism of splicing of the RGS12 gene
are extraordinary. First, there appears to be two distinct primary transcripts arising from the RGS12 gene, one that includes
exon 1 and one that does not. The latter apparently arises from an alternate transcriptional start site resulting in retention of sequences from intron 1 and an in-frame translational start site located 24 bp 5' to exon 2. Second, the primary transcript lacking exon
1 can be spliced to remove or retain intron 3, producing the RGS12P and
RGS12L transcripts, respectively. Third, the primary transcript
retaining exon 1 undergoes cis- or trans-splicing
to generate RGS12B and RGS12TS, respectively. Finally, the 3'-ends of
the RGS12 transcripts are spliced to retain exons 14-16, to skip exon
14, or to retain intron 15 to produce the long, short, and intermediate
3'-splice forms of RGS12. This splicing appears to occur in each of the
four different 5'-splice forms of RGS12. Reverse transcription-PCR
analysis showed that the RGS12 transcripts encoding the four N-terminal
forms of RGS12 are expressed in a tissue-specific fashion,
i.e. with transcripts encoding RGS12B present only in brain,
those encoding RGS12L present only in lung, and those encoding RGS12P
and RGS12TS present in several tissues. Thus, these unique transcripts
appear to originate in an orderly and tissue-specific fashion.
RGS12TS is unique in being the only RGS12 protein encoded by splicing
of transcripts from discontinuous gene segments, a particularly novel
trans-splicing mechanism that has been described previously in only a limited number of genes. Such intermolecular splicing has
been implicated in the generation of mRNA species in protozoa, plants, and mammals (16). In mammals, rat androgen-binding protein/sex hormone-binding globulin gene transcripts, located on chromosome 10, are fused in mature mRNA transcripts to histidine decarboxylase gene transcripts, originating from chromosome 3 (27). Similar trans-splicing of coding sequences from different
chromosomes generates c-Myb mRNA in human thymic cells (28).
trans-Splicing also generates multi-isotype immunoglobulin
transcripts from a single B lymphocyte and multiple types of chimeric
germ-line immunoglobulin heavy chain transcripts in human B cells (29,
30). We considered the possibility that RGS12TS could arise from a
recombinant gene, arising in a somatic cell from chromosomal breakage
and gene rearrangement. However, no evidence indicates the occurrence
of such widespread gene rearrangements in a subpopulation of cells in
healthy individuals (i.e. CLONTECH
cDNAs), and the existing gene data bases show that the sequence
encoding the 5'-end of RGS12TS is located 170 kilobases downstream from the RGS12 gene on the opposite DNA strand.
It seems likely that the complex pattern of splicing of RGS12 mRNAs
is reflective of cellular mechanisms for orchestrating a diversity of
functions for the encoded RGS12 proteins. Our results suggest that
splicing at the 3'-end of RGS12 transcripts affects expression/stability of the protein, whereas RGS12 transcripts encoding
three different N-terminal forms of RGS12 showed equivalent levels of
expression in the nucleus. However, splicing at the 5'-end of the
primary RGS12 transcript can produce RGS12 proteins that are targeted
to discrete intranuclear sites as observed for RGS12TS-S. On the other
hand, retention of RGS12 mRNA sequences encoding the 491-amino acid
C-terminal region of all short forms of RGS12 may reflect the
importance of this region for RGS12 activity. Although this region
includes the conserved RGS domain, it shares no homology with any other
protein except RGS14, whose function is not yet known.
Both ectopically expressed short forms of RGS12 proteins and native
RGS12TS-S in HEK-293T cells are localized to the nucleus, suggesting
that these proteins are constitutively nuclear proteins; yet we cannot
discount the possibility that RGS12 proteins might translocate out of
the nucleus in response to some type of cellular stimulus. The presence
of RGS proteins in the nucleus suggests a dramatic separation in space
from their presumed regulatory targets, i.e. G proteins.
We are unaware of evidence for nuclear localization of G subunits,
although Park et al. (31) recently showed that
G5 complexes localize to the nucleus in NIH 3T3-L1 cells and attenuate the transcriptional repression activity of adipocyte enhancer-binding
protein (AEBP1). If G subunits do not localize to
and exert regulatory effects in the nucleus, it seems possible that RGS
proteins could have other functions in the nucleus. This seems
particularly likely for RGS12 proteins in view of their apparent
exclusive localization within the nucleus and the considerable
contribution of non-RGS domain sequences to the primary structure of
these proteins. However, RGS12 proteins are not unique among RGS
proteins in their nuclear localization. We recently showed that RGS4
and RGS16, although predominantly cytoplasmic proteins, shuttle in and
out of the nucleus via a leptomycin B-sensitive pathway, whereas RGS2
and RGS10 are predominantly nuclear proteins (14).
However, RGS12TS-S is unique among RGS proteins in its subnuclear
organization into nuclear dots, a feature shared by various tumor
suppressor proteins. Our results suggest that RGS12TS-S localizes to
nuclear dots during the G1/S phase of the cell cycle and
that this occurs independent of changes in the steady-state concentration of the protein. BRCA1 and BARD1 also localize to nuclear
dots during progression to S phase and disperse thereafter (19, 20).
Although BRCA1 localization into these structures is accompanied by
increases in both its steady-state level and phosphorylation state,
localization of BARD1 in these nuclear dots occurs independent of
changes in its content (20). Whether the mechanism underlying formation
of RGS12TS-S nuclear dots involves its phosphorylation or other
modification and/or its interaction with other proteins as part of a
multiprotein complex is not known at present. However, RGS12TS-S is
rich in consensus sites for phosphorylation by various protein kinases
and possesses various protein-binding modules including a PDZ domain
(amino acids 30-99), a phosphotyrosine-binding domain (amino acids
225-374), a phosphotyrosine-interacting domain (amino acids 928-939),
two Ras-like Raf-binding domains (amino acids 962-1032 and
1034-1104), and a guanylyl nucleotide exchange factor domain (amino
acids 1187-1209) in addition to its RGS domain (amino acids 715-832).
Although the precise function of BRCA1 is unknown, the sensitivity of S
phase BRCA1 nuclear dots to DNA damage (19), the inability of
BRCA1-deficient stem cells to carry out transcription-coupled DNA
repair (32), and the presence of germ-line mutations in BRCA1 in
approximately half the heritable forms of breast and ovarian cancers
(33) suggest an important role in genome surveillance.
Thus, it is interesting to note that RGS12TS-S is unique among various
RGS proteins we examined in its ability to produce abnormal nuclear
morphology and multinucleated cells when ectopically expressed in COS-7
cells. The mechanism by which RGS12TS-S influences nuclear morphology
is not clear; however, it appears that ectopic expression of RGS12TS-S
dysregulates cytokinesis and/or nuclear division in COS-7 cells. The
precise biochemical events involved in regulation of nuclear and cell
division processes are not fully understood. Among various proteins
implicated in cytokinesis and DNA replication checkpoint control are
aurora and Ipl1-like
midbody-associated protein (AIM-1) and ataxia
telangiectasia mutated- and Rad3-related protein (ATR) (34, 35). Ectopic expression of AIM-1 or its kinase-inactive mutant induces abnormally shaped and multiple nuclei in
cells (34), as we observed here for RGS12TS-S. Obviously, further
studies are needed to define the precise biological role of RGS12TS-S
and the mechanisms underlying its localization/delocalization in
nuclear dots and its ability to induce nuclear anomalies upon its
overexpression. The observed cell cycle-dependent
localization of RGS12TS-S in nuclear dots and its ability to induce
nuclear aberrations may indicate the involvement of RGS12TS-S in
nuclear processes that are cell cycle-regulated.
It is important to consider the present results in relation to previous
studies of RGS12. Koelle and Horvitz (3) first identified and named a
partial expressed sequence tag as RGS12 based upon its homology to the
RGS domains of Egl-10, RGS1, and RGS2. Although the identity of this
transcript is unknown because it includes only 51 amino acids of the
RGS domain, we utilized this sequence to amplify the RGS12 transcripts
described here. Snow et al. (36) first isolated, by
hybridization screening, a rat homolog of the cDNA named RGS12TS-I
in the present study. We then reported sequences encoding the long
forms of the four N-terminal forms of RGS12 in the
GenBankTM/EBI Data Bank. Snow et al. (37) used a
probe to the unique 3'-end of one of the sequences we reported to show
that RGS12TS transcripts also exist with this unique 3'-end
(i.e. corresponding to the long forms described here). In
this same report, these workers identified a cDNA encoding a rat
homolog of RGS12B and showed that a recombinant fusion protein of the
RGS domain of rat RGS12 acted as a GTPase-activating protein in
vitro for recombinant Gi and Go, but
not Gs or Gq. However, we failed to
detect Gi immunoreactivity in RGS12TS-S nuclear dots or
changes in plasma membrane-associated Gi
immunoreactivity in EcR293-12TS-GFP cells following inducible
expression of RGS12TS-S (data not shown). Mao et al. (38)
recently showed that transfection of NIH 3T3 cells with rat RGS12TS-I
attenuated serum response factor activation mediated by
GTPase-deficient forms of G12 and G13 as well
as by receptors acting through both
Gq/11-dependent and -independent pathways.
These results raise interesting questions concerning how this effect of
RGS12TS-I is mediated, in part due to the lack of GTPase-activating
protein activity of the isolated RGS domain of this protein toward
Gq (37). Moreover, the ability of rat RGS12 to inhibit
responses mediated by GTPase-deficient forms of G12/13
suggests this effect is not likely a result of GTPase activation.
Although we cannot discount the sequence differences between the rat
RGS12TS used in the study by Mao et al. (38) or their use of
NIH 3T3 cells, our results show that this form of RGS12TS is not
measurably expressed in COS-7 cells. In view of our evidence for
nuclear expression of RGS12, its interesting to consider a possible
direct nuclear role of RGS12 in inhibition of serum response
factor-mediated gene transcription, particularly that mediated by
GTPase-deficient forms of G12/13.
It is still unclear why such a large family of genes encoding RGS
proteins exists in man and other species. Here, we have complicated
this issue by demonstrating that a single gene in this family can be
processed to 12 distinct RGS protein transcripts. Perhaps the observed
differential expression of these forms in a heterologous system and
their nuclear patterns of expression reflect attributes fundamentally
important to the cellular activities of these proteins. Despite the
presence of an RGS domain, the apparent constitutive nuclear
localization of RGS12 proteins implicates them in activities distinct
from regulation of cell-surface G protein-coupled receptor signaling.
Hopefully, these results will facilitate studies to define the
biological functions of RGS proteins in the nucleus.
| |
FOOTNOTES |
*
This work was supported by National Institutes of Health
Grants HL-41071 (to R. A. F.) and DK-25295 (to the University of Iowa
Diabetes and Endocrinology Research Center).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) AF030109, AF030110, AF030111, and AF030112.
To whom correspondence should be addressed. Tel.: 319-335-8330;
Fax: 319-335-8930; E-mail: rory-fisher@uiowa.edu.
Published, JBC Papers in Press, June 26, 2000, DOI 10.1074/jbc.M000330200
| |
ABBREVIATIONS |
The abbreviations used are:
RACE, rapid
amplification of cDNA ends;
PCR, polymerase chain reaction;
bp, base pair(s);
GFP, green fluorescent protein;
EGFP, enhanced GFP;
DMEM, Dulbecco's modified Eagle's medium;
DPBS, Dulbecco's
phosphate-buffered saline.
| |
REFERENCES |
| 1.
|
Hamm, H. E.
(1998)
J. Biol. Chem.
273,
669-672
|
| 2.
|
Gilman, A. G.
(1987)
Annu. Rev. Biochem.
56,
615-649
|
| 3.
|
Koelle, M. R.,
and Horvitz, H. R.
(1996)
Cell
84,
115-125
|
| 4.
|
Berman, D. M.,
and Gilman, A. G.
(1998)
J. Biol. Chem.
273,
1269-1272
|
| 5.
|
Dohlman, H. G.,
and Thorner, J.
(1997)
J. Biol. Chem.
272,
3871-3874
|
| 6.
|
Berman, D. M.,
Wilkie, T. M.,
and Gilman, A. G.
(1996)
Cell
86,
445-452
|
| 7.
|
Berman, D. M.,
Kozasa, T.,
and Gilman, A. G.
(1996)
J. Biol. Chem.
271,
27209-27212
|
| 8.
|
Tesmer, J. J. G.,
Berman, D. M.,
Gilman, A. G.,
and Sprang, S. R.
(1997)
Cell
89,
251-261
|
| 9.
|
Coleman, D. E.,
and Sprang, S. R.
(1999)
J. Biol. Chem.
274,
16669-16672
|
| 10.
|
Hepler, J. R.,
Berman, D. M.,
Gilman, A. G.,
and Kozasa, T.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
428-432
|
| 11.
|
Zeng, W.,
Xu, X.,
Popov, S.,
Mukhopadhyay, S.,
Chidiac, P.,
Swistok, J.,
Danho, W.,
Yagaloff, K. A.,
Fisher, S. L.,
Ross, E. M.,
Muallem, S.,
and Wilkie, T. M.
(1998)
J. Biol. Chem.
273,
34687-34690
|
| 12.
|
Chatterjee, T. K.,
Liu, X.,
Davisson, R. L.,
and Fisher, R. A.
(1997)
J. Biol. Chem.
272,
12122-12131
|
| 13.
|
Chatterjee, T. K.,
Eapen, A. K.,
and Fisher, R. A.
(1997)
J. Biol. Chem.
272,
15481-15487
|
| 14.
|
Chatterjee, T. K.,
and Fisher, R. A.
(2000)
J. Biol. Chem.
275,
24013-24021
|
| 15.
|
Padgett, R. A.,
Grabowski, P. J.,
Konarska, M. M.,
Seiler, S.,
and Sharp, P. A.
(1986)
Annu. Rev. Biochem.
55,
1119-1150
|
| 16.
|
Bonen, L.
(1993)
FASEB J.
7,
40-46
|
| 17.
|
Koken, M. H. M.,
Reid, A.,
Quignon, F.,
Chelbi-Alix, M. K.,
Davies, J. M.,
Kabarowski, J. H. S.,
Zhu, J.,
Dong, S.,
Chen, S.-J.,
Chen, Z.,
Tan, C. C.,
Licht, J.,
Waxman, S.,
De The, H.,
and Zelent, A.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
10255-10269
|
| 18.
|
Yano, T.,
Nakamura, T.,
Blechman, J.,
Sorio, C.,
Dang, C. V.,
Geiger, B.,
and Canaani, E.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
7286-7291
|
| 19.
|
Scully, R.,
Chen, J.,
Ochs, R. L.,
Keegan, K.,
Hoekstra, M.,
Feunteun, J.,
and Livingston, D. M.
(1997)
Cell
90,
425-435
|
| 20.
|
Jin, Y.,
Xu, X. L.,
Yang, M.-C. W.,
Wei, F.,
Ayi, T.-C.,
Bowcock, A. M.,
and Baer, R.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
12075-12080
|
| 21.
|
Mu, Z. M.,
Chin, K. V.,
Liu, J. H.,
Lozano, G.,
and Chang, K. S.
(1994)
Mol. Cell. Biol.
14,
6858-6867
|
| 22.
|
Guiochon-Mantel, A.,
Savouret, J.,
Quignon, F.,
Delabre, K.,
Milgrom, E.,
and De The, H.
(1995)
Mol. Endocrinol.
9,
1791-1803
|
| 23.
|
Dyck, J. A.,
Maul, G. G.,
Miller, W. H.,
Chen, J. D.,
Kakizuka, A.,
and Evans, R. M.
(1994)
Cell
76,
333-343
|
| 24.
|
Weis, K.,
Rmabaud, S.,
Lavau, C.,
Jansen, J.,
Carvalho, T.,
Carmo-Fonseca, M.,
Lamond, A.,
and Dejean, A.
(1994)
Cell
76,
345-356
|
| 25.
|
Carvalho, T.,
Seeler, J.-S.,
Ohman, K.,
Jordan, P.,
Pettersson, U.,
Akusjarvi, G.,
Carmo-Fonseca, M.,
and Dejean, A.
(1995)
J. Cell Biol.
131,
45-56
|
| 26.
|
Doucas, V.,
Ishov, A.,
Romo, A.,
Juguilon, H.,
Weitzman, M.,
Evans, R.,
and Maul, G.
(1996)
Genes Dev.
10,
196-207
|
| 27.
|
Sullivan, P. M.,
Petrusz, P.,
Szpirer, C.,
and Joseph, D. R.
(1991)
J. Biol. Chem.
266,
143-154
|
| 28.
|
Vellard, M.,
Sureau, A.,
Soret, J.,
Martinerie, C.,
and Perbal, B.
(1992)
Proc. Natl. Acad. Sci. U. S. A.
89,
2511-2515
|
| 29.
|
Shimizu, A.,
and Honjo, T.
(1993)
FASEB J.
7,
149-154
|
| 30.
|
Fujieda, S.,
Lin, Y. Q.,
Saxon, A.,
and Zhabg, K.
(1996)
J. Immunol.
157,
3450-3459
|
| 31.
|
Park, J.-G,
Muise, A.,
He, G.-P.,
Kim, S.-W.,
and Ro, H.-S.
(1999)
EMBO J.
18,
4004-4012
|
| 32.
|
Gowen, L. C.,
Avrutskaya, A. V.,
Latour, A. M.,
Koller, B. H.,
and Leadon, S. A.
(1998)
Science
281,
1009-1012
|
| 33.
|
Easton, D. F.,
Bishop, D. T.,
Ford, D.,
and Crockford, G. P.
(1993)
Am. J. Hum. Genet.
52,
678-701
|
| 34.
|
Terada, Y.,
Tatsuka, M.,
Suzuki, F.,
Yasuda, Y.,
Fujita, S.,
and Otsu, M.
(1998)
EMBO J.
17,
667-676
|
| 35.
|
Cliby, W. A.,
Roberts, C. J.,
Cimprich, K. A.,
Stringer, C. M.,
Lamb, J. R.,
Schreiber, S. L.,
and Friend, S. H.
(1998)
EMBO J.
17,
159-169
|
| 36.
|
Snow, B. E.,
Antonio, L.,
Suggs, S.,
Gutstein, H. B.,
and Siderovski, D. P.
(1997)
Biochem. Biophys. Res. Commun.
233,
770-777
|
| 37.
|
Snow, B. E.,
Hall, R. A.,
Krumins, A. M.,
Brothers, G. M.,
Bouchard, D.,
Brothers, C. A.,
Chung, S.,
Mangion, J.,
Gilman, A. G.,
Lefkowitz, R. J.,
and Siderovski, D. P.
(1998)
J. Biol. Chem.
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ABSTRACT
INTRODUCTION
