(Received for publication, August 30, 1996)
From the Human Retrovirus Section, ABL-Basic Research Program, NCI-FCRDC, Frederick, Maryland 21702-1201
Human immunodeficiency virus type 1 (HIV-1) mRNAs encoding structural proteins contain multiple inhibitory/instability elements (INS), which decrease the efficiency of viral protein expression. We have previously identified a strong INS element (INS-1) within the p17gag coding region. Here we show that poly(A)-binding protein 1 (PABP1) binds preferentially to INS-1 within the p17gag mRNA, but not to a mutated mRNA in which INS-1 function is eliminated. Competition experiments performed in the presence of different nucleic acids and homoribopolymers demonstrated preferential binding of PABP1 to the INS-1-containing RNA. In contrast to HeLa cells and several lymphoid cell lines, certain human glioma cell lines exhibit high levels of gag expression in the absence of Rev upon transient transfection with wild type gag expression vectors. We analyzed extracts of different cell lines and found that the binding of PABP1 to INS-1 RNA is significantly diminished in glial cell extracts. The expression levels of gag correlate with the absence of binding of PABP1 to the INS-1 RNA in cellular extracts. These results suggest a role for PABP1 in the inhibition of gag expression mediated through INS-1.
The post-transcriptional regulation of human immunodeficiency virus type 1 (HIV-1)1 is mediated through the Rev protein. Rev functions by facilitating the transport, stability, and translation of partially spliced and unspliced HIV-1 mRNAs that contain a Rev-specific RNA-binding region (RRE) (1-5). The mechanism of Rev function has been the subject of intense study. It has been shown that Rev increases the half-life of RRE-containing HIV-1 mRNAs (2) and promotes their transport to the cytoplasm (2-4, 6) and efficient translation (5, 7-9). Rev-dependent mRNAs are defective in expression, due to specific RNA regions scattered throughout the gag, pol, and env regions of HIV-1. These regions were named inhibitory sequences (INS/CRS/IN) and were shown to prevent efficient expression (10-15).2
We have previously reported the identification of a strong inhibitory RNA element (INS-1) within the coding region of the p17gag matrix protein of HIV-1 (11). This element acts in cis and its inhibitory effect can be overcome by Rev-RRE. Inactivation of INS-1 was achieved by introducing multiple point mutations distributed primarily in the regions of high AU content without altering the amino acid sequence of the encoded p17gag protein. This mutant displayed a Rev-independent, constitutively high level of expression of gag mRNA and protein, indicating that INS-1 had been inactivated.
Here we further characterize the mechanism of function of the inhibitory sequences. We studied the cellular factors interacting with INS-1 using UV-cross-linking of in vitro transcribed RNA to cellular extracts. We show that poly(A)-binding protein (PABP1) binds specifically to INS-1 within the p17gag mRNA, but not to mutated RNA (p17M1234). Moreover, the ability of PABP1 to bind p17gag RNA in vitro appears to be cell type-specific and correlates with inhibitory effects of INS-1 in vivo. We propose that binding of PABP1 to INS-1 within the gag mRNAs may contribute to the mechanisms regulating HIV-1 expression.
The human T cell line HPB-ALL (17), HLtat cells (18), and human astrocytoma cell line 85HG66 (19-21) have been previously described. The astrocytoma cell line U87-MG was obtained from the American Type Culture Collection (Rockville, MD). Nuclear and cytoplasmic extracts were prepared by the method of Moore and Fishel (17) with modifications. Briefly, cells were harvested by low speed centrifugation, washed three times with ice-cold phosphate-buffered saline, resuspended in hypotonic lysis buffer (10 mM Tris HCl, pH 7.8, 1 mM MgCl2, 4 mM KCl, 1 mM dithiothreitol, 1% Triton X-100, 2 mM Pefablock (Boehringer Mannheim)), and incubated on ice for 12 min. Released nuclei were centrifuged for 5 min at low speed. The supernatant was used in the cross-linking reactions (cytoplasmic extract). The nuclei were washed twice with the same buffer and resuspended in the lysis buffer containing 400 mM of KCl. After nuclear lysis, the nuclear extract was cleared by centrifugation at 14,000 × g for 15 min. The protein concentration of cytoplasmic and nuclear extracts was determined by the Bio-Rad DC protein assay (Bio-Rad).
TransfectionsHLtat cells, 85HG66, and U87-MG cells were transfected by the calcium coprecipitation technique (2, 22), with 5 µg of gag-expression plasmids (p17, p17R, and p17M1234) in the absence or presence of 1 µg of the Rev-expressing plasmid pBsrev (7). One microgram of tat-expressing plasmid, pL3tat, was added to the transfection mixtures for glial cells. Cotransfection with pL3luc, which contains the firefly luciferase gene linked to the HIV-1 long terminal repeat was used as an internal control for transfection efficiency. Luciferase activity was determined as described previously (23, 24). The total amount of DNA in the transfection mixtures was adjusted to 17 µg/0.5 ml of precipitate/60-mm plate by using pBluescript (Stratagene). Transfected cells were harvested in 0.5 × radioimmune precipitation buffer 24 h post-transfection. gag protein production was analyzed by Western blotting using HIV-1 patient serum as described previously (11).
In Vitro RNA SynthesispKS17 containing the p17gag
coding sequences (nucleotides 172-257 + 329-731 of the HXB2 HIV-1
sequence) was polymerase chain reaction amplified from pMcgag and
cloned into the Bluescript KS() vector (10). pKS17M1234 containing
p17M1234gag was isogenic to pKS17 except it contained 28 point
mutations introduced into gag sequence (11). pKS17 and
pKS17M1234 were linearized by EcoRI digestion and used as
templates for in vitro synthesis of KS17 RNA and
KS17MRNA by standard protocols (Promega). The in vitro
transcribed RNAs (535 nucleotides) were used in cross-linking reactions
after analysis in 6% polyacrylamide with 8 M urea
denaturing gels. [
-32P]UTP was included for synthesis
of radiolabeled RNAs.
RNA binding reaction mixtures contained approximately 0.1 pmol of 32P-labeled RNA probe and 1-10 µl of cytoplasmic extracts in a final volume of 30 µl, containing 20 mM Tris HCl, pH 7.5, 150 mM NaCl, 1 mM dithiothreitol, 20 units of RNasin (Promega), and 0.5 mg/ml yeast tRNA (Boehringer Mannheim). The reaction mixtures were incubated at room temperature for 15 min and then irradiated by UV light (254 nm, Stratalinker 2400, Stratagene) while on ice. After digestion with RNase A (1 mg/ml) at 37 °C for 20 min, the samples were heated at 65 °C for 5 min in SDS sample buffer and electrophoresed on 10% polyacrylamide-SDS gels (Novex). Dried gels were exposed to Kodak XAR film.
Immunoprecipitation of Cross-linked ProteinsAntiserum 61925 against PABP1 was obtained from Dr. R. Moon, University of Washington, Seattle (25). Polyclonal antisera were made in rabbits after immunizations with synthetic peptides CEAAQKAVNSATGVPTV (antiserum 39472) or CIPQTQNRAAYYPPSQVAQLRPS (antiserum 39473), derived from human PABP1 (26). For immunoprecipitations, three reaction mixtures were combined after UV irradiation, treated with RNase A, brought to a final concentration of 0.5 × radioimmune precipitation buffer using 5 × radioimmune precipitation buffer stock buffer, and incubated with rabbit antiserum against PABP1 or rabbit serum (5-10 µl) for 12-15 h at 4 °C, followed by addition of a 50% slurry of protein A-Sepharose. The samples were incubated for 3 h at 4 °C with rocking. The immunoprecipitate was prepared by low speed centrifugation and three washes with 0.5 × radioimmune precipitation buffer. Samples for SDS-polyacrylamide electrophoresis were prepared as described above.
Quantitative AnalysesDetermination of PABP1 by immunoblotting was done as described above for gag. Binding assays with PABP1 and poly(A) were performed using cytoplasmic extracts from HLtat, 85HG66, and U87-MG cells and poly(A)-Sepharose. Twenty microliters of a 50% slurry of poly(A)-Sepharose was incubated with 200 µl of cytoplasmic extract (corresponding to 5 × 105 cells) for 2 h at 4 °C in phosphate-buffered saline. Poly(A)-Sepharose beads were washed twice with phosphate-buffered saline containing 1 M NaCl, and the presence of bound PABP1 was analyzed by SDS-polyacrylamide electrophoresis and immunoblotting. Immunoblots were quantitated for bound 125I-labeled protein A on a PhosphorImager (Molecular Dynamics, Sunnyvale, CA).
We prepared
in vitro transcribed p17gag RNA containing the
region of INS-1 (KS17 RNA), and a mutant RNA transcribed from
pKS17M1234 (11), which has inactivated INS-1 (KS17M RNA). We used UV
cross-linking experiments to determine whether INS-1 in KS17 RNA
interacts with cellular proteins. We hypothesized that elimination of
inhibitory sequences in KS17M RNA alter RNA-protein interactions
important for inhibition. To test this hypothesis, we compared the
patterns of proteins interacting with these RNAs.
32P-Labeled KS17 RNA and KS17M RNA were incubated with
nuclear and cytoplasmic extracts from HPB-ALL cells. Binding reactions
were performed in the presence of excess unlabeled yeast tRNA to
eliminate nonspecific binding. After incubation, all reactions were
irradiated by UV light followed by RNase A treatment. As shown in Fig.
1, a strong band corresponding to a cytoplasmic protein
with an apparent molecular weight of approximately 70,000 (p70) was
detected with KS17 RNA (lane 1). The complex appeared to be
specific for KS17 RNA under the assay conditions used, since p70 was
not present after incubations with KS17M RNA (lane 2) or RRE
RNA (lane 3). Analysis of RNA-protein complexes obtained
from nuclear extracts did not reveal any differences between KS17 RNA
or KS17M RNA (compare Fig. 1B, lanes 1 and
2), but these complexes were distinct from those obtained
with RRE RNA (Fig. 1B, lane 3).
To examine the specificity of complex formation between p70 and KS17
RNA, we included an excess of various unlabeled nucleic acids in the
binding reaction and examined their ability to affect p70·KS17 RNA
complex formation (Figs. 2 and 3).
Presence of up to 100-fold molar excess of competitor DNA did not
affect binding of p70 to KS17 RNA (Fig. 2, compare lanes 1 and 2). On the contrary, inclusion of a 4-fold molar excess
of unlabeled KS17 RNA decreased complex formation with the labeled
probe (lane 3), whereas the presence of a 40-fold excess
completely abolished the interaction of p70 with labeled p17 RNA
(lane 4). The presence of rRNA (lanes 9 and
10) or unlabeled KS17M RNA (lanes 6-8) did not
prevent binding of p70 to the wild type KS17 RNA. Hence, formation of
the p70·KS17 RNA complex appears to be specific and parallels the
stability of p17gag mRNA.
We further analyzed the sequence specificity of p70·KS17 RNA complex formation by testing each of four homoribopolymers for the ability to compete with KS17 RNA (Fig. 3). The binding experiments were performed in the presence of increasing concentrations of poly(A), poly(C), poly(G), or poly(U). Only poly(A) was able to selectively inhibit p70·KS17 RNA complex formation. A 55% inhibition was achieved in the presence of 1 ng of poly(A) (Fig. 3, filled circles). The presence of poly(C) had no effect on the complex formation even in the presence of 4 µg of poly(C) (open circles). The sensitivity of complex formation to poly(G) was comparable to that of poly(C), while the presence of poly(U) increased the ability of KS17 RNA to interact with p70, probably due to elimination of unstable nonspecific interactions of KS17 RNA with other RNA-binding proteins present in the cytoplasmic extract (filled squares). The amount of unlabeled KS17 RNA necessary to inhibit complex formation of p70·KS17 RNA by 50% was 77 ng (filled triangles). These data suggest that the protein within the complex has strong preference for poly(A).
Antibodies against PABP1 Recognize Cross-linked p70The
observation that p70 has a high affinity for poly(A) and a similar
molecular weight led to the hypothesis that p70 is the previously
identified PABP1. To confirm this hypothesis, we tested polyclonal
antibodies raised against PABP1 for their ability to react with labeled
p70. UV cross-linking experiments were performed in the presence of
KS17 RNA (Fig. 4, lane 1) followed by
immunoprecipitation either with antibodies against PABP1 or with
preimmune rabbit serum. As it shown in Fig. 4, antibodies against PABP1
(lane 2) recognized p70. We could not detect any reaction of
preimmune rabbit serum with the complex (lane 3). This
experiment was repeated with all three available types of antibodies
against PABP1 (see "Materials and Methods"). Taken together, the
strong competition of poly(A) for p70 binding to KS17 RNA and the
ability of PABP1 antibodies to recognize labeled p70 support the
conclusion that p70 is PABP1.
Binding of PABP1 to KS17 RNA Correlates with Inhibitory Effect of INS-1 in Different Cell Lines
We next examined whether the level of inhibition of gag expression by INS-1 after transfection in different cell lines correlates with the ability of PABP1 to bind KS17 RNA in vitro. To measure the effects of INS-1 in different cell lines, we transfected gag-expressing plasmids into three different cell lines, HeLa tat, and human astrocytoma cell lines U87-MG and 85HG66. The plasmids used, p17, p17R, and p17M1234 have been previously described (27). p17 and p17R contain the wild type INS-1, p17R also contains a functional RRE, and p17M1234 contained inactivated INS-1.
gag expression by p17 was almost 10 times higher in U87-MG
cells compared with HLtat cells. The levels of gag produced
in the presence of Rev were similar to those produced by p17M1234 (Fig.
5A). Expression of the luciferase reporter
gene after cotransfections in these cell lines were comparable (average
values varied from 3 × 105 to 9 × 104 luciferase units). Examination of the second glial cell
line, 85HG66, revealed that the overall level of protein expression upon transient transfection was lower because of less efficient transfection. Expression of luciferase was also lower (4-6 × 103 units). To compare these different cell lines, we
expressed gag production in the absence of Rev as a
percentage of gag production obtained from p17M1234 (Fig.
5B). Expression of gag protein by p17 in the
absence of Rev was 48% of that obtained with p17M1234 for 85HG66 and
67.2% for U87-MG. This level is much higher than in HeLa cells (3.75%
of the levels produced with p17M1234). These results suggest that
inhibitory cellular factors are less functional in the astrocytoma cell
lines compared with HeLa cells.
To examine whether the ability of PABP1 to bind KS17 RNA in
vitro is different in extracts of different cell lines, we
compared cytoplasmic extracts derived from a human T cell line
(HPB-ALL), HeLa cells, and human astrocytoma cell lines U87-MG and
85HG66 by UV cross-linking. We performed UV cross-linking experiments using partially fractionated extracts from these cell lines (Fig. 6). We determined the total protein concentration in the
extracts, and performed UV cross-linking experiments with different
amounts of extracts. We found most of the specific binding in the
20-50% ammonium sulfate fraction of HPB-ALL and HeLa cell cytoplasmic extracts (lanes 1-3), whereas we could not detect
significant binding in any fractions of U87-MG or 85HG66 cells
(lanes 4-8). It is noteworthy that, although the amount of
total proteins used in lanes 1, 3, 5,
and 7 is comparable (approximately 7-12 µg), complex
formation is significantly reduced in U87-MG and 85HG66. Therefore,
binding of PABP1 to INS-1 RNA in cytoplasmic extracts correlates with
the inhibition of expression of these mRNAs in vivo.
By quantitative immunoblotting we also examined the levels of
expression of PABP1 in glial or HeLa cells and the ability of PABP1 to
bind poly(A) in vitro. The results showed that glial cells
produced 3-5 times less PABP1 as measured by Western blots. PABP1
levels correlated with the binding of poly(A) to cytoplasmic extracts
of the different cell lines as well as with the levels of UV
cross-linking (Fig. 7), suggesting that differences in
INS-1 binding might reflect different expression levels of PABP1.
PABP1 is the major cytoplasmic poly(A)-binding protein and is
highly conserved among eukaryotic organisms (26, 28-30). Deletion of
the PABP1 gene in yeast (Saccharomyces cerevisiae) is
lethal, indicating that PABP1 is an essential protein (31). The role of
PABP1 and poly(A) in mRNA metabolism remains unclear. PABP1 might
be a key factor in mediating regulation of mRNA turnover through
the inhibition of mRNA decapping by the poly(A) tail or by
influencing the rate of deadenylation (32-35). Additionally, several
lines of evidence argue that PABP1 plays a role in stimulating translation initiation (36, 37), suggesting that the interaction of
this protein with the 3 poly(A) sequence can influence events at the
5
end of an mRNA. PABP has at least two distinct and separable activities: specific poly(A) binding activity was found only in two
amino-terminal RNA binding domains, which could function in binding of
PABP1 to the poly(A) tail, whereas two other RNA binding domains do not
have preference for poly(A) binding and could function through binding
either to a different part of the same RNA or to other RNAs (38).
The results presented here suggest an interaction of PABP1 with the INS-1 region within p17gag mRNA. The p17gag coding sequence has four regions with a high content of A and U nucleotides. Point mutations resulting in elimination of the inhibitory effect of INS-1 were introduced to interrupt mostly A-rich stretches in these regions. INS-1 contains a maximum of 6 uninterrupted A nucleotides surrounded by AU-rich regions. The ability of PABP1 to bind wild type p17gag mRNA and not the mutant mRNA suggests that it binds to A-rich sequences other than poly(A). Our results confirm previous findings (16, 38) that PABP1 is a multifunctional RNA-binding protein and is able to interact with other sequences.
The observation that PABP1 binds less efficiently to INS-1 regions in cytoplasmic extracts from astrocytoma cell lines, coupled with the increased expression of p17gag in these cell lines, indicates a correlation between binding of PABP1 to INS-1-containing mRNA and expression of this mRNA in vivo. Therefore, binding of PABP1 to p17gag mRNA might play a role in the inhibition of gag expression mediated by INS-1.
We propose that the interaction of PABP1 with INS-1 within
p17gag mRNA might prevent its efficient expression.
Mutimerization of PABP1 on the 3 poly(A) tail of mRNA could lead
to the formation of a ribonucleoprotein particle capable of interacting
with the 5
end of the mRNA. This interaction may be necessary for
efficient initiation of translation. The presence of additional sites
for PABP1 binding within the INS-1 on the mRNA could result in the creation of cis-acting competitor sequences. Binding of
PABP1 to these sites might alter or inhibit functionally important
contacts on the 5
end of the mRNA with the 3
poly(A)-PABP1
ribonucleoprotein particle. Instead, nonfunctional complexes of 5
end
mRNA and PABP1 occupying INS-1 sites might form, resulting in
inefficient translation and/or higher degradation rate. In glial cells,
lower levels of expression of PABP1 are sufficient for interaction with poly(A) tails, but there is no excess of unbound protein for
interaction with additional targets such as INS-1; therefore,
inhibition by INS-1 is significantly reduced. This model is consistent
with our previous results that in the absence of Rev most HIV-1
mRNA is not efficiently translated and is associated with 40S
ribosomal subunits, but not with polysomes (7). Rev might direct
RRE-containing RNA through a different transport and utilization
pathway, preventing binding of PABP1 and possibly of other inhibitory
factors to INS-1, thus leading to efficient translation.
We thank B. K. Felber for encouragement, helpful discussions, and critical reading of the manuscript. We are grateful to S. Gulnik for support and help with experiments, to A. Gragerov, A. Zolotukhin, and R. Schnider for suggestions and discussions, to P. Carney and J. Harrison for technical assistance, R. Moon and T. Copeland for rabbit anti-PABP1 polyclonal antisera, and A. Arthur for editing.