From the Biotechnology Centre of Oslo, University of Oslo, Gaustadalleen 21, N0349 Oslo, Norway
Received for publication, January 27, 2003
, and in revised form, March 18, 2003.
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ABSTRACT |
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INTRODUCTION |
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MDDX28 was recently shown to contain an RNA-dependent ATP-hydrolyzing activity (1). Endogenous MDDX28 is localized in the mitochondria and the nucleus, where it is also found in the nucleolus. MDDX28-EGFP1 fusion protein has the same localization as the endogenous protein. In addition, and probably like the endogenous MDDX28, it shuttles between the nucleus and the cytoplasm (1). The double localization of MDDX28 is novel among RNA helicases and raises questions about the role of the protein.
All cellular proteins except for 13 mitochondrial proteins are encoded in the nucleus. The nuclear transcripts are transported to the cytoplasm where they are translated into proteins that are transported to their intracellular destinations. Much of the intracellular transport goes through large protein complexes in the intracellular membranes, e.g. of the nucleus and mitochondria, and is largely an active process. The transport involves a localization signal(s) present on the protein itself or on an associated factor and various types of transporter proteins or transporter complexes. Research on localization signals has revealed that there is no simple consensus signal for any of the intracellular compartments, suggesting that different transporter and control mechanisms apply. Several proteins localize to more than one compartment of the cell and, therefore, need to carry multiple transport signals. Proteins that localize to mitochondria and nucleus regulate the localization through formation of different isoforms by alternative splicing or by alternative transcription or translation initiation (6, 7, 8, 9, 10). The Mddx28 gene contains no introns and no internal ATG sites. Therefore, no isoforms can be made of the protein, and its intracellular localization has to be otherwise determined. The aim of the present study was to identify the targeting determinants of MDDX28 as a step toward understanding the function of the protein as well as the control mechanisms for the intracellular localization.
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EXPERIMENTAL PROCEDURES |
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Two in-frame deletions were made by cleaving the wild type plasmid with
XmnI and BclI (to make 149274) or with
BclI and AgeI (to make
276540). The fragments
were treated with Klenow and ligated. Five deletions were made by PCR.
44540 contained BamHI-digested fragment amplified with
forward primer, 5'-GG TGG ATC CTG TAG AGC CAC TGG GAT GC-3', and
the wild type reverse primer
(1).
220
contained BamHI/EcoRI-digested fragment amplified with
forward primer, 5'-GGA ATT CAG CCA CCA TGC GAC GGG GCC-3', and the
wild type reverse primer.
2139 contained
BamHI/EcoRI-digested fragment amplified with forward primer,
5'-GGA ATT CAG CCA CCA TGG CAC TAC AGG AGG CTG C-3', and the wild
type reverse primer.
520540 contained BamHI-digested
fragment amplified with the wild type forward primer and the reverse primer,
5'-GGT GGA TCC CGA GCC GCC AGC TCA ATC TT-3'.
2274
contained BamHI/EcoRI-digested fragment amplified with
forward primer, 5'-GGA ATT CAG CCA CCA TGA TCA GTC TGG AGC AAC
TC-3', and the wild type reverse primer. Double deletions were made by
combination of the methods described above.
1 was made by
amplification of the wild type plasmid with
2139 forward primer
and
520540 reverse primer.
2 was made by
amplification of the
149274 plasmid with wild type forward
primer and
520540 reverse primer.
4 was made with
in-frame deletion of
2139 as described above for
276540.
7 was made with
BamHI/EcoRI fragment amplified with
2274
forward primer and
520540 reverse primer.
Point-mutated constructs were made by site-directed mutagenesis following a
protocol from Stratagene using the wild type MDDX28-EGFP-N1 plasmid as
template. The 330GAT AAA mutation was made with
amplification using the primers 5'-CAG TTA GTG CTG GTA GCA
GCC GCA TTT CCC GAA GGT GTA GG-3' and 5'-CC TAC ACC TTC
GGG AAA TGC GGC TGC TAC CAG CAC TAA CTG-3' (mutated bases are underlined
in the forward primer). The 481YIHR
YIQQ mutation was made
by amplifying the wild type construct using the primers 5'-G CTG CAA GAT
TAC ATC CAG CAA GCA GGG AGA GTG GGC-3' and 5'-GCC CAC
TCT CCC TGC TTG CTG GAT GTA ATC TTG CAG C-3', and the 286DEAD
DQAD mutation was made with amplification of wild type construct using
the primers 5'-G GTG TTG GAT CAG GCA GAC ACA CTG C-3'
and 5'-G CAG TGT GTC TGC CTG ATC CAA CAC C-3'. A double mutant
(DM1) was made by mutating the 286DEAD
DQAD construct with
the YIHR
YIQQ primers. The suspected nuclear export signal (NES)
sequence was mutated in two steps. Initially three leucines were mutated by
amplification from the wild type MDDX28-EGFP-N1 using the primers 5'-CC
CTC GTG ACT CGG GCG GCC GCG GCG CCG CGA CGG
GGC-3' and 5'-GCC CCG TCG CGG CGC CGC GGC CGC CCG AGT CAC GAG
GG-3'. This was further mutated to 9AFSAVTRAAA (NES-5) with
primers 5'-G CGG CCG GTG CGG GCC TTT TCC GCC GTG
ACT CGG GC-3' and 5'-GCC CGA GTC ACG GCG GAA AAG GCC CGC ACC GGC
CGC-3'. Three basic regions corresponding to amino acids 4958,
98104, and 244247 containing putative nuclear localization
signals were mutated using the wild type or
520540 constructs as
templates and the following primers: NLS-1, 5'-CAG CGG CAG AGC
GCG GCG GCG AAC CTC CCG AGG-3' and
5'-CCT CGG GAG GTT CGC CGC CGC GCT CTG CCG CTG-3'; NLS-2,
5'-GGC TGG AAG AGT GCA GCC GCG GCT CGG
GAC CAC TTC-3' and 5'-GAA GTG GTC CCG AGC CGC GGC TGC ACT CTT CCA
GCC-3'; and NLS-3, 5'-GGC CAC GGC ATG GCT
GCG ATC GCC CTG CAG CTG TCC-3' and 5'-GGA
CAG CTG CAG GGC GAT CGC AGC CAT GCC GTG GCC-3'. The various mutations
were combined to give 14 different mutated constructs
(Table I).
NLS
constructs contain BamHI/EcoRI-digested fragments amplified
with forward primer, 5'-GGAATTCAGCCACCATGCGGCAGTTGGAACAG-3', and
reverse primer, 5'-GGTGGATCCGCGATGGAGAAGTGGTC-3', using wild type,
NLS-1, NLS-2, or NLS-1/2 as templates.
The twenty N-terminal amino acids from MDDX28 were inserted into TCF11 (11) to give the constructs TCF/NES-R (right orientation of insert) and TCF/NES-W (wrong orientation of insert). The PshAI/EcoRV fragment of TCF11 was transferred to an EcoRV/PshAI-cleaved pUC19 vector (New England Biolabs). Two 63-bp oligonucleotides identical to the 5' end of the MDDX28 gene were synthesized on an Applied Biosystems model 394 DNA/RNA synthesizer. The oligonucleotides were complementary over 59 bp, with 4-bp 3' overhangs identical to the cohesive ends of an NcoI restriction site. The oligonucleotides were annealed, treated with T4 polynucleotide kinase (New England Biolabs), and ligated to an NcoI-cleaved pUC19-TCF11 construct in both directions. These constructs were then transferred to pcDNA3 by cleaving vector and insert with EcoRI and XbaI.
Cell Culture and ImmunofluorescenceCOS-1 cells were grown on coverslips in Dulbecco's modified Eagle's medium (BioWhittaker) supplemented with 10% newborn calf serum (BioWhittaker) and 2 mM L-glutamine (Invitrogen). At appropriate times, the coverslips were washed briefly in PBS and fixed in 4% paraformaldehyde (Ferak) for 15 min (except for anti-PSP-1, 7 min). The cells were permeabilized in 0.5% Triton X-100 in PBS and blocked for 30 min in 3% bovine serum albumin (Sigma) in PBS. The samples were incubated with the primary antibody in 1% blocking solution at 4 °C overnight, washed 3 times in PBS with 0.1% Triton X-100, and incubated for 1h at room temperature with fluorescence-conjugated secondary antibody. When appropriate, the cells were counterstained with Hoechst 33258 (Sigma) before mounting. The samples were viewed with a Nikon Eclipse E400 microscope. The pictures were taken at 100x primary magnification with a SPOT digital camera and combined with SPOT32 software (Diagnostic Instruments). Alternatively, confocal laser-scanning microscopy images were recorded on a TCS SP scanner mounted on a DM IRBE microscope (Leica Microsystems Heidelberg GmbH). The objective was a Plan Apo 63X/1.32 oil immersion lens. Laser (dual) excitation was done at 488 (or 476) and 546 nm; the main beam splitter was a dual band pass filter DD488/568. The fluorescence detection bands in the scanner head were set to optimize detection and minimize bleed-through. The pinhole was set to 1.00 absorbance units. The photodetectors were class R6357/R6358 photomultiplier tubes (Hamamatsu Photonics KK). Data acquisition and data analysis were controlled by means of the LCS software version 2.770 (Leica Microsystems Heidelberg GmbH). A series of 40 sections at an axial distance of 4.9 µm and with a strong zoom factor (7.5) was used as raw data for three-dimensional image reconstruction. A simulated fluorescence process shadow projection series (61 images at 3° rotational progression) was created from median-filtered raw data (kernel size 5 x 5 x 3) with the LCS software. The series was saved as an avi-file and compressed from 48 to 5.9 kilobytes with the AVIedit software.
Transfections into COS-1 cells were performed using the FuGENE 6 transfection reagent in 4:1 FuGENE/plasmid ratio according to the Roche Applied Science protocol. Heterokaryon assays were performed as described earlier (1), except that treatment with cycloheximide was shortened in the assay of the TCF/NES constructs because the TCF11 protein has a half-life of less than 3 h.2
For RNase and DNase treatment of transfected cells, a method of Chiodi
et al. (12) was
followed. Briefly, 220-transfected cells that had been treated
with actinomycin D for 2 h were washed with cold PBS and incubated for 10 min
in Buffer A (100 mM NaCl, 300 mM sucrose, 10
mM Pipes, pH 6.8, 3 mM MgCl2, and 0.1% Triton
X-100) containing protease inhibitors (PIC, 10 µg/ml aprotinin, 10 µg/ml
leupeptin, 10 µg/ml antipain, 10 µg/ml chymostatin, 10 µg/ml
phosphoramidon, 1 mM phenylmethylsulfonyl fluoride). Cells were
incubated for 10 min in the same buffer made to 250 mM in ammonium
sulfate and washed twice in Buffer A before treatment for 20 min at 37 °C
with 36 µg/ml of RNase A (Sigma) in Buffer A. Cells were then washed in PBS
and fixed in ice-cold methanol.
Antibodies used were anti-SC35 (a generous gift of Dr. Kallan, University of Bergen), anti-p80 coilin (a generous gift of Dr. Lamond, University of Dundee), anti-paraspeckle protein-1 (PSP-1, a generous gift of Dr. Fox, University of Dundee), and Hsp60 (Stressgen Biotechnologies). For anti-promyelocytic leukemia bodies (PML), the monoclonal antibody 5E10 (13) was used. TCF/NES was detected with anti-nrf1 antibody (Santa Cruz Biotechnology). TRITC-, fluorescein isothiocyanate-, and Texas Red-conjugated secondary antibodies were used (DAKO, The Jackson Laboratories). All immunofluorescence studies were repeated at least twice, and all readings and quantifications were done blindly. Nucleolar, mitochondrial, and cytoplasmic localization were scored as present or not present, whereas nuclear localization was scored according to intensity of the localization as compared with the wild type.
Transcription InhibitionTransiently transfected cells were grown for 2024 h on coverslips before treatment with 10 µg/ml actinomycin D (Sigma). After 2 h (unless otherwise stated) the cells were fixed as described above and viewed immediately in the fluorescence microscope.
ImmunoprecipitationTransfected COS-1 cells were cultured in 10-cm tissue culture dishes. The constructs were tested for equal transfection efficiency with direct immunofluorescence. One day post-transfection, 40 µl of [14C]uridine (50 µCi/ml) was added to the cultures, and incubation was continued overnight. The cells were washed in PBS and incubated on ice in radioimmune precipitation assay buffer (1% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS) containing PIC. The cells were scraped off, homogenized, and centrifuged briefly at full speed in a bench-top centrifuge to remove debris. The extracts were precleared with 20 µl of M280 Dynabeads coated with sheep-anti-rabbit IgG (Dynal) for 1 h at 4 °C. Dynabeads were conjugated with 1.5 µg of GFP antibody (Santa Cruz Biotechnology) and incubated for 2 h at 4 °C. Conjugated beads were then added to precleared extracts and incubated at room temperature for 2 h. The beads were washed 3 times in PBS, suspended in 50 µl of PBS and mixed with Pico Aqua liquid scintillation mixture (Packard). The samples were counted in a Packard 1600TR liquid scintillation analyzer. The counting was adjusted for total protein of each sample as measured with the Bio-Rad assay. Background (EGFP-N1 vector only) was subtracted. The experiment was repeated three times.
StatisticsThe distribution of the number of punctate
structures containing SC35 and MDDX28 was compared in 100 cells with a
two-tailed independent sample t test using the SPSS software
package.
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RESULTS |
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Right orientation insertion of the 20 N-terminal amino acids of MDDX28 into the transcription factor TCF11 (TCF/NES-R, Fig. 1) was sufficient for mitochondrial localization of the otherwise nuclear-localized protein (Fig. 2A). The mitochondrial localization of this fusion protein is less visible in Fig. 2B, b, possibly due to the treatment with protein synthesis inhibitor. Wrong orientation of the insert (TCF/NES-W) did not result in mitochondrial localization (Fig. 2A). This shows that not only the sequence but also its correct orientation is necessary for mitochondrial transport.
NESWe have previously shown that when MDDX28-transfected
cells are treated with actinomycin D the protein is effectively exported from
the nucleus (1). The protein
does not reappear in the nucleus during transcription inhibition, suggesting
that its re-entry into the nucleus is blocked, e.g. by masking of the
nuclear localization signal (NLSs) by binding proteins or by phosphorylation.
To search for NES in MDDX28, the nuclear localization of proteins encoded by
several single deletion constructs (Fig.
1) was assessed after 824 h of actinomycin D treatment.
Whereas 149274,
276540, and
520540
as well as the wild type protein were successfully exported from the nucleus,
the
220 and
2139 mutants remained in the nucleus
of all cells even after 24 h of treatment
(Fig 2C, graph
a). We also noticed that, unlike the wild type protein, which localized
to the nucleus in about half of the transfected cells, the
220
and
2139 proteins as well as the
520540 protein
localized to the nucleus in all transfected cells.
To test whether amino acids 120 were sufficient to enable nuclear export, they were inserted in both directions into the N-terminal end of the short version of the nuclear-localized transcription factor TCF11 (TCF/NES-R and -W, Fig. 1). The nuclear export ability of the two constructs was examined in an interspecies heterokaryon assay. Untransfected NIH/3T3 mouse cells were fused to COS-1 cells that had been transfected with the TCF/NES constructs. The cells were treated with 50 µg/ml cycloheximide for 1 h before and for 1 h after the fusion before fixation with paraformaldehyde. Therefore, all fusion protein present in the nucleus of NIH/3T3 cells would have originated in the transfected COS-1 cells. To distinguish the nuclei derived from mouse and monkey cells, the cells were counterstained with Hoechst 33258 after fixation. The TCF/NES-R protein was seen in the nucleus of NIH/3T3 cells (Fig. 2B, ac) in numerous heterokaryons on every coverslip examined, indicating that the inserted sequence was active as an export signal. Six coverslips were scanned in the heterokaryon assay for TCF/NES-W, and only one NIH/3T3 nucleus containing TCF11 was found (data not shown). Thus, TCF/NES-W was largely incapable of nucleocytoplasmic shuttling, indicating that NES in the wrong orientation was not active as an export signal.
A leucine-rich sequence is located at amino acids 918. To test
whether the leucine residues were necessary for the nuclear export, all five
were mutated to alanine (9LFSLVTRLLL AFSAVTRAAA, NES-5).
After 24 h of actinomycin D treatment of cells transfected with NES-5, the
protein was seen in the nucleus of 70% of cells transfected with the NES-5
construct compared with 1020% for the wild type. Thus, although
mutation of the five leucine residues impaired the nuclear export ability of
the protein, it had not been completely inhibited. The export of the NES-5
mutant was further established using a heterokaryon assay
(Fig. 2B,
df). Together these results suggested that the leucine
residues were important but not absolutely essential for nuclear export and
that other residues among the 20 N-terminal amino acids are involved in the
export. The mitochondrial localization of protein encoded by the NES-5
construct was also greatly decreased (Fig.
2A), indicating that residues that play a role in the
nuclear export are also necessary for the mitochondrial import of MDDX28.
NLSWe had predicted earlier that the NLS might be the basic
stretch of amino acids at positions 520523 (RRRR), but deletion of
these (520540) failed to impair the nuclear import of the fusion
protein (Fig. 2C). To
search for the NLS, three deletion constructs were made, together spanning the
whole protein (
2139,
149274, and
276540). The resulting proteins all localized to the nucleus
(Fig. 2C), suggesting
that the nuclear localization signal is a composite, where no single sequence
is essential. At this stage, the possibility could not be ruled out that
MDDX28 enters the nucleus through a piggyback mechanism. Such a mechanism has
been suggested, e.g. for protein X of hepatitis B virus that is
imported into the nucleus by binding to the NLS-carrying I
B
(14).
To distinguish between active nuclear import and a piggyback mechanism, we
looked for candidate NLS in MDDX28. The most common type of NLS is made of
one, two, or more mono- or bipartite stretches of basic amino acids
(15). MDDX28 contains three
basic stretches (BS 13), at amino acids 4958, 98104, and
244247 in addition to the previously identified basic stretch at
position 520523 (BS-4). To test whether one or more of the basic
regions were important for the nuclear import, 14 different combinations of
mutated basic regions were made (Table
I). No decrease in the number of cells with nuclear localization
of the fusion protein or in the intensity of the localization was detected in
cells transfected with NLS-3, 520540, or a combination of the
two (Fig. 2,
CD, and data not shown). However, mutation of BS-1
and 2 (NLS-1 and -2 constructs, respectively) significantly decreased the
nuclear import of the corresponding protein, both seen as a decrease in the
number of cells with nuclear localization
(Fig. 2C, graph
b) and in decreased intensity of immunofluorescence in the nucleus
(Fig. 2D). Mutations
of both BS-1 and -2 (NLS-1/2) decreased the nuclear localization further, to
about 7% of transfected cells, indicating that the nuclear import was greatly
impaired (Fig. 2C,
graph b). Because the import was not completely inhibited by mutating
the two basic regions, other NLS with very limited activity may be present in
MDDX28. Alternatively, the mutations introduced into BS-1 and -2 may only
partially impair the NLSs, leaving a small part of the signal intact. Deletion
of the region around the two basic clusters (
2139) did not
exclude the resulting protein from the nucleus
(Fig. 2C), indicating
the presence of additional NLSs in the protein.
To test if additional amino acids surrounding BS-3 and -4 were important
for the nuclear localization, we analyzed five deletion constructs, each
covering at least two of the basic stretches (1,
2,
4,
7, and
2274).
Only when all four basic stretches and the surrounding amino acids had been
deleted (
7) was the protein completely excluded from the nucleus
(Fig. 2C). The absence
of the
7-encoded protein from the nucleus was further
established with confocal microscopy. Seven single cells (or their nuclei)
were examined. These revealed that no fluorescent particles matching GFP
spectral properties were located inside the nucleus (an animation of the
three-dimensional projection is available as Supplemental Material). This
indicated that residues between 139 and 274 and C-terminal residues could also
contribute to the nuclear localization.
To address the question of whether BS-1 and -2 were sufficient for nuclear
localization, four constructs were made with amino acids 44109 of
MDDX28 (containing both clusters) fused to EGFP
(Fig. 1). When the basic
clusters were in the wild type form (NLS) the fusion protein was
primarily seen in the nucleus of the transfected cells
(Fig. 2C). Mutation of
either of the basic clusters (
NLS-1 and
NLS-2) resulted in
protein that was localized to nucleus and cytoplasm, where the intensity of
nuclear-localized protein was much higher than that of the cytoplasmic protein
(Fig. 2C). The
intracellular localization of a fusion protein where both clusters had been
mutated (
NLS-1/2) could not be distinguished from the localization
pattern of EGFP alone (Fig.
2C). This indicated that
NLS-1/2 had lost all
localization information. Taken together, these results show that BS-1 and -2
are sufficient for nuclear localization and that mutation of either signal
sequence reduced the efficiency of the NLS.
It has been proposed that actinomycin D "inactivates" NLS, thereby shifting the localization of nuclear-shuttling proteins to the cytoplasm (16). We tested whether the NLSs of MDDX28 were differently affected by inhibition of transcription. After 824 h of treatment, NLS-1- and NLS-2-transfected cells showed a greatly reduced presence of MDDX28 in the nucleus. This reduction was not significantly different from that observed for the wild type protein (data not shown). This indicated that actinomycin D could inactivate the two major NLSs of MDDX28.
Nucleolar Localization Signal (NoLS)The wild type MDDX28
localized to the nucleolus in up to 20% of transfected cells, depending on
time after transfection (1). To
look for the NoLS, the nucleolar localization of three deletion constructs
(2139,
149274, and
276540) spanning
the whole protein was studied. All the constructs resulted in proteins that
lacked nucleolar localization (Fig.
2C). Because the deletions of the constructs do not
overlap, we suggest that the NoLS is composed of two or more sequences, which
are all essential. Alternatively, the nucleolar localization depends on the
enzymatic activity of the protein. Large parts of the conserved enzymatic
domain had been deleted from the two constructs, the encoded fusion proteins
of which no longer localized to the nucleolus.
We first addressed the question whether function of MDDX28 was important
for the localization of the protein. Drawing on the experience with the eIF4A
protein (17,
18), we mutated MDDX28 in
three of the conserved motifs, 330GAT AAA (SAT in eIF4A),
286DEAD
DQAD, and 481YIHR
YIQQ. The
corresponding residues in the eIF4A protein affected the helicase function,
the ATP hydrolysis, and the RNA binding, respectively. Cells transfected with
the DEAD and GAT mutants retained the nucleolar localization of the protein
(Fig. 2D).
Interestingly, the mutation of the DEAD-box resulted also in cytoplasmic but
not mitochondrial localization (Fig
2D). Mutation of the YIHR motif completely inhibited the
nucleolar localization of the fusion protein
(Fig. 2D), suggesting
its dependence on the RNA binding ability of the protein. Double-mutated
MDDX28 (DM1, 286DEAD
DQAD; 481YIHR
YIQQ)
had the same localization as 286DEAD
DQAD, except that it
did not localize to the nucleolus (Fig.
2D). To test whether the 481YIHR
YIQQ
mutation affected the RNA binding of MDDX28, the hybrid protein was
immunoprecipitated from transiently transfected COS-1 cells that had been
cultured overnight in the presence of [14C]uridine. The results
were normalized to the total amount of protein in each precipitate, and the
background (activity pulled down with EGFP-only) was subtracted. The
481YIHR
YIQQ-mutated protein had significantly reduced RNA
binding ability compared with the wild type protein or protein containing the
330GAT
AAA mutation (Fig.
3A). The importance of interaction with RNA for the
nucleolar localization of MDDX28 was further established by treating
transfected, transcription-inhibited cells with RNase A for 20 min before
fixation in methanol. This resulted in removal of nucleolar-localized MDDX28
protein in 50% of the cells, whereas treatment with Triton X-100 and ammonium
sulfate, designed to remove nuclear proteins not interacting stably with
either chromatin or the nuclear matrix, did not significantly affect the
nucleolar localization (Fig.
3B). The localization pattern of MDDX28 in cells
retaining nucleolar localization after RNase A-treated cells was also
different from that of untreated cells
(Fig. 3C). Only protein
localized in the fibrillar center (FC) remained after the RNase A treatment
(Fig. 3C, a),
whereas protein localized to the dense fibrillar component and the granular
component were removed by the treatment. This agrees with the findings that
dense fibrillar component and granular component contain the ribonucleoprotein
complexes, whereas the FCs are depots of rDNA genes (for a review, see Ref.
19).
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Thus, we have shown that the nucleolar localization of MDDX28 depends on
the RNA binding of the YIHR motif at amino acids 481484. However,
because proteins encoded by the 2139 and
149274
constructs did not localize to the nucleolus although these deletions leave
the YIHR box intact, other parts of the protein must also contribute to its
nucleolar localization. Because the most common NoLS identified to date
consists of a cluster of basic amino acids
(20,
21) we tested whether
mutations of basic regions BS 14 could affect the nucleolar
localization. Protein encoded by the NLS-1, NLS-2, and NLS-3 constructs were
all excluded from the nucleolus in transiently transfected cells
(Fig. 2D), suggesting
that in addition to the RNA binding ability, the basic regions of the protein
are necessary for its nucleolar localization.
Transcription Inhibition-dependent Nuclear Localization We
have reported earlier that the nuclear localization of MDDX28 depends on
ongoing polymerase II transcription
(1). When testing the effect of
RNA polymerase II inhibition on the nuclear localization of protein encoded by
the MDDX28 constructs we also noticed marked changes in the nuclear phenotype
of cells transfected with the 220,
520540, or the
wild type construct as well as of the endogenous MDDX28. Shortly after the
addition of actinomycin D, these proteins were seen in punctate structures in
the nucleoplasm and in caps at the nucleolar periphery
(Fig. 4A, a,
d, and g; data not shown for
520540, the wild type
construct or endogenous protein). The same effect was obtained with other
polymerase II inhibitors (
-amanitin and
5,6-dichloro-1-
-D-ribofuranosylbenzimidazole; data not
shown). This suggests that the protein accumulates in subcompartments of the
nucleus during transcription inhibition. The protein disappeared from the
punctate structures after 4 h of actinomycin D treatment in cells transfected
with the wild type and
520540 constructs as a result of the
protein being exported from the nucleus (data not shown). Therefore, this
phenomenon was not observed in the previous study where the shortest time
studied was 4 h post-initiation of actinomycin D treatment
(1). The
220
protein has lost the NES and is, therefore, not exported from the nucleus.
Accordingly, it was still localized in the punctate structures after 24 h of
actinomycin D treatment. Interestingly, localization to the punctate
structures during transcription inhibition was not observed in cells
transfected with constructs not encoding protein localized to the nucleolus,
including the YIHR mutant and the NLS-1, NLS-2, and NLS-3 mutants (data not
shown).
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We have studied whether MDDX28 in punctate nuclear structures colocalizes
with other known nuclear bodies (PML bodies, splicing speckles, Cajal bodies
(coiled bodies), and paraspeckles) by staining actinomycin D-treated cells
with antibodies against PML (Fig.
4A, b), SC35
(Fig. 4A, e),
p80-coilin (Fig. 4A,
h), and PSP-1 (Fig.
4A, k). Only the results for 220
are shown, because its localization to the punctate structures is not affected
by nuclear export, and therefore, the intensity of the structures remains
stronger. The same results were obtained for the wild type protein (data not
shown). The punctate nucleoplasmic structures did not co-localize with PML,
p80-coilin, or PSP-1; however, they were found to be adjacent to (but did not
colocalize with) the SC35 protein detected in conventional immunofluorescence
studies (Fig. 4A,
f). This was further confirmed with confocal microscopy
(Fig. 4B,
ae). SC35 speckles are bigger than the punctate structures
containing MDDX28. However, the number of these two structures in
transcription-arrested cells did not show significantly different distribution
(p > 0.422, Fig.
5).
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MDDX28 also formed caps at the nucleolar periphery in cells treated with actinomycin D. These were found to partially co-localize with PSP-1 (Fig. 4A, l) and to be adjacent to p80-coilin (Fig. 4A, i), as observed with conventional immunofluorescence microscopy. The adjacent colocalization with p80-coilin was further confirmed with confocal microscopy (Fig. 4B, fj).
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DISCUSSION |
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Most mitochondrial proteins are encoded in the nucleus, synthesized in the cytoplasm, and transported into the mitochondria either post- or co-translationally (for a review, see Ref. 22). No consensus sequence has been found for mitochondrial localization; however, sequences with shared characteristics have been described (23). The first 20 amino acids of MDDX28 have such MTS characteristics, and these were found to be both necessary and sufficient for mitochondrial localization of the protein in deletion and domain-swapping experiments. The EGFP protein and the transcription factor TCF11 gained mitochondrial localization when fused to the MTS sequence of MDDX28, whereas full-length MDDX28 lacking only the MTS did not localize to the mitochondria. The orientation of the sequence was found to be important, because only MTS inserted in the right orientation resulted in mitochondrial localization of the otherwise nuclear-localized TCF11. Furthermore, the five leucine residues of the sequence were essential for the mitochondrial localization.
A mutation of the conserved DEAD-box (286DEAD DQAD)
resulted in protein localized to the nucleus and to the cytoplasm but not to
the mitochondria. Due to the cytoplasmic localization of the
286DEAD-mutated protein it was not possible to test the shuttling
ability of the protein in a heterokaryon assay. The DEAD-box is a Walker B
motif involved in ATP hydrolysis and is highly conserved among RNA helicases.
The 286DEAD
DQAD mutation has been shown to affect the ATP
hydrolysis and not ATP binding to RNA helicases
(17,
24). Furthermore, it has been
shown that ATP hydrolysis causes conformational changes of the eIF4A helicase
and decreases its affinity for single-stranded RNA 40-fold
(25). Based on the similarity
of the core domain of eIF4A and MDDX28 and the finding that a double-mutated
MDDX28 (DM1, 286DEAD
DQAD; 481YIHR
YIQQ)
has the same localization as 286DEAD
DQAD, we propose that
in addition to the MTS, the conformational change caused by ATP hydrolysis is
necessary for successful mitochondrial localization of MDDX28. This change of
conformation may not be needed for
44540, where nearly the whole
MDDX28 is deleted. Transport of another RNA helicase, An3, is significantly
affected by mutation of the DEAD motif (An3 E389Q; Ref.
26), indicating that similar
mechanism may apply to the transport of both proteins.
In addition to functioning as a MTS, the first 20 amino acids of MDDX28 were found to be necessary and sufficient for nuclear export of the protein in deletion- and domain-swapping experiments. Transcription factor TCF11 was exported from the nucleus when fused to the NES sequence of MDDX28, whereas full-length MDDX28 lacking only the NES sequence was not exported from the nucleus. NES in the right orientation was much more efficient for nuclear export than NES in the wrong orientation.
Leucine-rich NES is the best-studied type of nuclear export signal (for a review, see Ref. 27). Proteins with leucine-rich NES as well as with NES rich in other hydrophobic amino acids are exported via the CRM1 pathway, which is sensitive to leptomycin B (27, 28, 29, 30). We have shown earlier that leptomycin B does not significantly alter the nuclear localization of MDDX28 (1), suggesting that the protein does not contain a classical leucine-rich NES. The 20 N-terminal amino acids of MDDX28 include 5 leucine residues. Although mutation of the leucine residues to alanine decreased the nuclear export of the resulting protein, it was not completely inhibited. This suggests that residues other than the N-terminal leucines of MDDX28 are also important for the nuclear export. Furthermore, the result presented here shows that the MTS and NES depend at least in part on the same amino acids within the sequence. Co-localization of these two signals has to our knowledge not been described before.
Most nuclear-localized proteins have been shown to rely on signal-mediated import (31). Therefore, we expect MDDX28 to contain a NLS for active nuclear import. This is further supported by the findings that MDDX28 is localized to the nucleus in about 50% of the cells, whereas it would be expected to localize to the nucleus of all cells if its nuclear import was passive. This further suggests that the protein is only temporarily needed in the nucleus or as a nucleo-cytoplasmic shuttling protein and that there is a mechanism for controlling its nuclear localization.
The most common NLS sequence is a small cluster of basic amino acids. Other types of NLS include the M9 sequence (38 amino acids long), which also mediates nuclear export, and the bipartite NLS, made of two small clusters of basic amino acids separated by 912 residues, (31) or NLS made of two or more mono- or bipartite basic domains separated by up to hundreds of amino acids (15, 32). We found that two clusters of basic amino acids, separated by 44 residues were necessary and sufficient for full nuclear localization of the protein in mutation and domain-swapping experiments. Additional unidentified NLS was also shown to contribute to the nuclear localization. Partial nuclear import was obtained with a series of deletion constructs where one or more basic clusters had been deleted or mutated. This is in concordance with the findings for proteins with two independent NLS, where both signals need to be deleted to fully inhibit the nuclear import (15, 33, 34).
Surprisingly, whereas protein encoded by 7 is cytoplasmic,
NLS-1/2-encoded protein is diffusely localized in nucleus and
cytoplasm. Both constructs contain EGFP fused to parts of MDDX28 lacking
functional NLSs. This discrepancy can only be explained with the size
difference between the two constructs. Together with EGFP, the size of the
protein encoded by
7 is
54 kDa, whereas the size of the
NLS-1/2 protein is 35 kDa, apparently allowing passive nuclear import
of the protein in the absence of intracellular targeting signal.
Little is known about the signal(s) that directs proteins to the nucleolus, although several proteins have been described with NoLS consisting of clusters of basic amino acids (20, 21). Even less is known about the mechanisms by which proteins are routed to the nucleolus, and no nucleolar transport proteins have yet been identified. It has been suggested that domains that are necessary and sufficient for nucleolar localization act as retention signals rather than targeting signals (35). MDDX28 was not identified as a nucleolar protein in a recent proteomic analysis of the nucleolus (36). We have shown, however, that the protein localizes to the nucleolus in a part of the cells, suggesting that the protein cycles between the nucleolus and other parts of the nucleus (1). We now show that the ability of MDDX28 to bind RNA is essential for the nucleolar localization of the protein, because mutation of the conserved YIHR motif completely inhibited the nucleolar localization as well as impaired the RNA binding ability of the protein. Furthermore, RNase A treatment of transfected cells significantly decreased the nucleolar localized protein.
In addition to the RNA binding ability, the three clusters of basic residues that are found in the N-terminal half of MDDX28 (BS 13) were shown to be independently necessary for the nucleolar localization. Two of these domains also confer nuclear localization of the protein, indicating that they are responsible not only for bringing the protein into the nucleus but also to the sites of RNA binding. The basic regions are hydrophilic and likely to be on the surface of the protein. They are, thus, possible sites of interaction of MDDX28 with other proteins or protein complexes, suggesting that both RNA and protein binding are needed for nucleolar targeting or retention of the protein in the nucleolus. Identification of proteins or protein-RNA complexes interacting with the basic regions of MDDX8 may reveal the function of the protein.
The nuclear localization of wild type MDDX28 is diffuse in untreated cells. When transcription inhibitors are added for 2 h, the protein relocates to punctate nucleoplasmic structures and to caps at the nucleolar periphery. We have found that only those MDDX28 constructs whose protein can localize to the nucleolus have the capability to form these structures, suggesting that the processes depend on the same mechanisms. This may be a combination of RNA and protein interactions. MDDX28 in punctate nucleoplasmic structures were adjacent to the splicing factor SC35, which upon transcription inhibition relocates to interchromatin granule clusters (37), normally associated with transcription of highly active genes (for a review, see Ref. 38). The organization of the nucleolus itself changes upon transcription inhibition; the compartments of the nucleolus disperse, and a necklace of tandemly organized rDNA and transcription of rRNA forms at the nucleolar periphery (39). After transcription, inhibition MDDX28 localized to the parts of the nucleolus that correspond to the necklace. There it partially co-localized with PSP-1 and was adjacent to p80-coilin, both of which have earlier been shown to relocate to nucleolar caps upon inhibition of transcription (40). The function of these proteins in the nucleolar caps is not yet known, and it remains to be resolved whether they are functionally related. At present the co-localization study serves only to identify the subnuclear compartments in which MDDX28 is trapped upon transcription inhibition. We have not studied whether MDDX28 interacts directly with the proteins with which it was shown to colocalize, and no other MDDX28-interacting proteins have yet been identified.
In conclusion, we have mapped the intracellular targeting signals of the MDDX28 protein. The conservation of signals for dual or triple purposes is interesting in terms of evolution as well as in understanding the control and function of MDDX28.
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FOOTNOTES |
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The on-line version of this article (available at
http://www.jbc.org)
contains a video.
A Research Fellow of the Norwegian Cancer Society.
To whom correspondence should be addressed. Tel.: 47-22840532; Fax:
47-22840501; E-mail:
hans.prydz{at}biotek.uio.no.
1 The abbreviations used are: EGFP, enhanced green fluorescence protein; BS,
basic stretch; FC, fibrillar centre; MTS, mitochondrial targeting signal; NES,
nuclear export signal; NLS, nuclear localization signal; NoLS, nucleolar
localization signal; PML bodies, promyelocytic leukaemia bodies; PIC, protease
inhibitor cocktail; PBS, phosphate buffered saline; PSP-1, paraspeckle
protein-1; TRITC, tetramethylrhodamine isothiocyanate; Pipes,
1,4-piperazinediethanesulfonic acid.
2 C. Husberg, personal communication.
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ACKNOWLEDGMENTS |
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