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Splicing Regulation

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In the A complex, SF1 is replaced by U2 snRNP at the branchpoint. ... Then, U2AF65 recruits U2 to the branch site sequence (BS) ... – PowerPoint PPT presentation

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Title: Splicing Regulation


1
Splicing Regulation
  • The role of SR proteins in spliceosome assembly

2
Spliceosome assembly The spliceosome assembles
onto the pre-mRNA in a stepwise manner. The E
complex contains U1 snRNP bound to the 5 splice
site, SF1 bound to the branchpoint, and U2AF65
and U2AF35 bound to the pyrimidine tract and 3
splice site AG, respectively. In the A complex,
SF1 is replaced by U2 snRNP at the branchpoint.
The U4/U6U5 tri-snRNP then enters to form the B
complex. A rearrangement occurs to form the
catalytically active C complex, in which U2 and
U6 interact, and U6 replaces U1 at the 5 splice
site.
3
Spliceosome assembly pathway. In the first step
of spliceosome assembly, U1 snRNP binds to the 5
splice site and U2 auxiliary factor (U2AF) binds
to the pyrimidine tract and 3 splice site YAG.
This complex commits the pre-mRNA to the splicing
pathway and is called the E, or early, complex.
Next, E complex is converted to A complex when
the U2 snRNP binds to the branchpoint.
Subsequently, B complex is formed when the U4,
U5, and U6 snRNPs enter the spliceosome as a
tri-snRNP particle. Finally, a massive
rearrangement occurs in which U6 replaces U1 at
the 5splice site, U6 and U2 interact, U5 bridges
the splice sites, and U1 and U4 become
destabilized. This rearranged spliceosome is
called the C complex and is catalytically active.
4
SR proteins act as molecular bridges in
spliceosome assembly
SR
SR
Branch site
Exon Enhancers
UNCURAC
5' splice site
3' splice site
A
  • CAG GUAAGU
  • A G

(U/C)nN AG G
Intron
Exon 2
Exon 1
Polypyrimidine Tract
5
Serine-Arginine-rich Splicing Proteins
  • SR proteins are essential splicing factors that
    contain an RNA-binding domain (N-terminus) and an
    arginine/serine-rich domain (C-terminus)
  • SR proteins play important roles in spliceosome
    assembly
  • SR proteins also play important roles in defining
    the 5 and 3 splice sites
  • SR proteins play important roles in alternative
    splicing in defining exons and weak splice sites

6
(No Transcript)
7
SR Proteins
  • SR proteins contain an RNA-binding domain and an
    arginine/serine-rich domain that functions to
    promote assembly of the spliceosome.

8
  • Human SR Proteins

SRp20
SC35
SRp46
SRp54
9G8
Z
SRp30c
SF2/ASF
SRp40
RRM
SRp55
RRM-2
RS
SRp75
9
SR Proteins RS Domains
  • SR proteins interact with each other and other
    splicing proteins by protein-protein interactions
    through the RS domains
  • The phosphorylation state of the RS domains is
    critical to these interactions

10
  • Human SR Proteins

SRp20
SC35
SRp46
SRp54
9G8
Z
SRp30c
SF2/ASF
SRp40
RRM
SRp55
RRM-2
RS
SRp75
11
SR Splicing Proteins
  • SR proteins play important roles in spliceosome
    assembly through protein-protein interactions to
    bridge components of the spliceosome
  • SR proteins also play important roles in defining
    the 5 and 3 splice sites by binding to specific
    sites in the pre-mRNA through the RNA-binding
    domain
  • SR proteins play important roles in alternative
    splicing in defining exons and weak splice sites
    by binding specific sites, termed Exonic Splicing
    Enhancers (ESE) through the RNA-binding domains.

12
Schematic diagram of human SR proteins and SR
related proteins
13
RS domain-dependent activities of SR proteins
  • Activity of SR proteins in spliceosome assembly

14
Recruitment of U1 snRNP to a 5 splice site An
SR protein bound to the upstream exon interacts
with U1-70K and recruits U1 snRNP to the 5
splice site
15
U2AF recruitment model An exonic enhancer-bound
SR protein interacts with the RS domain of
U2AF35, thereby recruiting U2AF65 to the pre-mRNA
16
SR proteins have been shown to participate in the
recruitment of the U4/U6U5 tri-snRNP, although
the mechanism by which they do so has not been
elucidated. Presumably this activity is mediated
by an interaction between an SR protein present
in the partially assembled spliceosome and a
component of the tri-snRNP. Two candidate
interaction targets of SR proteins are the
U5-100K and U4/U6U5-27K protein.
17
Model of spliceosome assembly using different SR
proteins
18
Model for Cross-Bridging The RS domain of
SF2/ASF may interact with the RS domains of
U1-70K and U2AF35 to facilitate cross-intron
bridging.
19
SR Proteins RS Domains
  • SR proteins interact with each other and other
    splicing proteins by protein-protein interactions
    through the RS domains
  • The phosphorylation state of the RS domains is
    critical to these interactions

20
SR Protein Specific Kinases
  • SR Protein Kinase I- SRPK1
  • Clk/Sty Kinase

21
SRPK1 and Clk/Sty Protein Kinases Show Distinct
Substrate Specificities for Serine/Arginine-rich
Splicing Factors
22
SRPK1 and Clk/Sty Protein Kinases Show Distinct
Substrate Specificities for Serine/Arginine-rich
Splicing Factors K.Colwill, L.L. Fengi, J.M.
Yeakley, G.D. Gish, J.F. Caceres, T. Pawson, and
X.-D. Fu J. BIOLOGICAL CHEMISTRY 271, 1996
23
SRPK1-mediated phosphorylation differentially
modulates the affinity of RS domain interactions
in vitro. In a GST pull-down assay,
mock-phosphorylated (-ATP) or SRPK1- treated
GST-ASF/SF2 (ATP) were bound to 35S-labeled-in
vitro translated U1-70k followed by analysis on
SDS-PAGE. Coomassie-stained bands are shown in
the top panel to illustrate the mobility shift
due to phosphorylation, and the lower panel shows
an autoradiograph of the same gel.
24
The Protein Kinase Clk/Sty Directly Modulates SR
Protein ActivityBoth Hyper- and
Hypophosphorylation Inhibit Splicing JAYENDRA
PRASAD,1 KAREN COLWILL, TONY PAWSON, AND JAMES L.
MANLEY MOLECULAR AND CELLULAR BIOLOGY,1999,
1969917000
25
The Protein Kinase Clk/Sty Directly Modulates SR
Protein Activity Both Hyper- and
Hypophosphorylation Inhibit Splicing
  • The splicing of mammalian mRNA precursors
    requires both protein phosphorylation and
    dephosphorylation, involving modification of
    members of the SR protein family of splicing
    factors.
  • Several kinases have been identified that can
    phosphorylate SR proteins in vitro, and
    transfection assays have provided evidence that
    at least one of these, Clk/Sty, can modulate
    splicing in vivo.
  • By using purified recombinant Clk/Sty, a
    catalytically inactive mutant, and individual SR
    proteins, it was shown that Clk/Sty directly
    affects the activity of SR proteins, but not
    other essential splicing factors, in
    reconstituted splicing assays.
  • Evidence is also provided that that both hyper-
    and hypophosphorylation inhibit SR protein
    splicing activity, repressing constitutive
    splicing.
  • These findings indicate that Clk/Sty directly and
    specifically influences the activity of SR
    protein splicing factors and, importantly, show
    that both under- and over-phosphorylation of SR
    proteins can modulate splicing.

26
SR Proteins must be appropriately phosphorylated
to activate splicing
P
-P
27
Hyperphosphorylation of SR proteins results in
Splicing Inhibition
Clk recombinant Clk/Sty kinase ClkRcatalytically
inactive mutant Clk/Sty kinase
28
Hypophosphorylation Inhibits Splicing
Unphosphorylated GST-ASF/SF2 inhibits pre-mRNA
splicing in HeLa nuclear extracts
Unphosphorylated GST-ASF/SF2 inhibits spliceosome
assembly in HeLa nuclear extracts
29
SR Protein Localization
  • Phosphorylation of SR proteins is required for
    their import into the nucleus, where they are
    stored in interchromatin granules (ICG) or
    speckles until they are required
  • Phosphorylation of SR proteins in the ICG moves
    SR proteins to sites of active transcription, and
    they participate in spliceosome assembly and
    splice site definition
  • Dephosphorylation by SR-specific phosphatases
    moves the SR back to the ICG

30
SR Protein Phosphorylation
  • Both Hypo- and Hyper-Phosphorylation of SR
    proteins renders them inactive in splicesome
    assembly
  • Inappropriately phosphorylated SR proteins remain
    in speckles (hypo-) or a diffuse distribution
    (hyper-) and do not move to sites of RNAP II
    transcription and splicing

31
(No Transcript)
32
SR protein SC35 redistributes to a diffuse
nuclear localization upon expression of Clk/STY.
A-431 cells transiently transfected with
GFP-Clk/STY wild-type (A) show diffuse
localization of SC35 (B) in contrast to
untransfected cells, or cells transfected with
catalytically inactive mutant GFP-Clk/STY K190R
(C) in which SC35 is localized in nuclear
speckles.
33
  • Mass Spectrometric and Kinetic Analysis of
    ASF/SF2 Phosphorylation by SRPK1 and Clk/Sty
  • Adolfo Velazquez-Dones, Jonathan C. Hagopian,
    Chen-Ting Ma, Xiang-Yang Zhong, Huilin Zhou,
    Gourisankar Ghosh, Xiang-Dong Fu, and Joseph A.
    Adams
  • JOURNAL OF BIOLOGICAL CHEMISTRY VOL. 280, pp.
    4176141768, 2006.

34
  • Assembly of the spliceosome requires the
    participation of SR proteins.
  • The repeat regions (RS domains) are
    poly-phosphorylated by the SRPK and Clk/Sty
    families of kinases. The two families of kinases
    have distinct enzymatic properties, raising the
    question of how they may work to regulate the
    function of SR proteins in RNA metabolism in
    mammalian cells.
  • The authors report the first mass spectral
    analysis of the RS domain of ASF/SF2, a
    prototypical SR protein.
  • SRPK1 was responsible for efficient
    phosphorylation of a short stretch of amino acids
    in the N-terminal portion of the RS domain of
    ASF/SF2.
  • Clk/Sty was able to transfer phosphate to all
    available serine residues in the RS domain,
    indicating that SR proteins may be phosphorylated
    by different kinases in a stepwise manner.
  • Both kinases bind with high affinity and use
    fully processive catalytic mechanisms to achieve
    either restrictive or complete RS domain
    phosphorylation.
  • These findings have important implications on the
    regulation of SR proteins in vivo by the SRPK and
    Clk/Sty families of kinases.

35
Ordered Multi-site Phosphorylation of the
SplicingFactor ASF/SF2 By SRPK1Ma,
Velazquez-Dones, Hagopian Ghosh, Fu and AdamsJ.
Mol. Biol. (2008) 376, 5568
  • ASF/SF2, an SR protein is activated by multi-site
    phosphorylation of its C-terminal RS domain.
  • The protein kinase responsible for this
    modification, SRPK1, catalyzes the selective
    phosphorylation of approximately a dozen serines
    in only the N-terminal portion of the RS domain
    (RS1).
  • To unravel the nature of selective phosphate
    incorporation in ASF/SF2, region-specific
    phosphorylation in the RS domain was monitored as
    a function of reaction progress.
  • Arg-to-Lys mutations were made at several
    positions to produce unique protease cleavage
    sites that separate the RS domain into
    identifiable N- and C-terminal phosphopeptides
    upon treatment with lysyl endoproteinase.
  • These studies revealed that SRPK1 docks near the
    C-terminus of the RS1 segment and then moves in
    an N-terminal direction along the RS domain.
  • These data suggest that SRPK1 uses a unique
    grab-and-pull mechanism to control the
    region-specific phosphorylation of its protein
    substrate.

36
WT-ASF/SF2 structure and ASF(5R1K) cleavage
pattern. (a) Domain organization of wt-ASF/SF2
and expected LysC cleavage fragments of
ASF(5R1K). LysC protease cleavage sites are shown
using open arrows.(b) Identification of
phosphorylated peptide fragments by
autoradiography. ASF(5R1K) was phosphorylated
using SRPK1 and then treated with LysC before
incubation with Ni2-Sepharose resin.
37
C-terminal phosphorylation is favored in
pulsechase experiments.Kinetic analysis of
region-specific phosphorylation.ASF(5R1K) and
SRPK1 werepre-equilibrated before the reaction
was initiated with 1 or100 µM 32PATP. Further
32P incorporation was stopped at8 s or 10 min by
the addition of 10 mM cold ATP. The reaction was
treated immediately with LysC and the products
were analyzed byautoradiography. The ratio of
32P in the N-terminal fragment to 32P in the
C-terminal fragment was plotted against the
phospho-content of uncleaved ASF(5R1K).
38
Results Conclusions
  • After a reaction time of 8 s when only 2.2 sites
    are phosphorylated, approximately three times as
    much 32P is incorporated into the C-terminal
    compared to the N-terminal fragment.
  • After a reaction time of 10 min when nearly all
    sites are phosphorylated, the ratio of N- to
    C-terminal fragments is close to the expected
    ratio of 0.7
  • These findings suggest that phosphorylation in
    the C-terminal portion of RS1 is both
    thermodynamically and kinetically favored over
    N-terminal phosphorylation.

39
Grab-and-Pull Model
40
RNA Polymerase II Targets Pre-mRNA Splicing
Factors to Transcription Sites In Vivo
41
SR Proteins and Transcription
  • SR protein ASF/SF2 is a general pre-mRNA splicing
    factor.
  • ASF/SF2 is efficiently recruited to sites in the
    nucleus where adenovirus genes are transcribed
    and the resulting pre-mRNAs are processed.

Lindberg, M. Gama-Carvalho, M.Carmo-Fonseca and
J. Kreivi J. General Virology (2004), 85, 603608
42
very early
Cells were transfected with GFP-ASF/SF2 and
subsequently infected with Adenovirus. At
different times after infection, cells were fixed
and stained with an antibody to Ad-virus protein
that marks sites of Ad-virus transcription.
early
late
DRS
43
Phosphorylated RNA polymerase II stimulates
pre-mRNA splicing Y. Hirose, R, Tacke, and J. L.
Manley Genes Development 131234
Using reconstituted in vitro splicing assays, we
show that RNAP II functions directly in pre-mRNA
splicing by influencing very early steps in
assembly of the spliceosome. We demonstrate that
the phosphorylation status of the CTD
dramatically affects activity Hyperphosphorylated
RNAP II strongly activates splicing, whereas
hypophosphorylated RNAP II can inhibit the
reaction.
44
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45
SR Proteins Function in Coupling RNAP II
Transcription to Pre-mRNA SplicingR. Das, I. Yu,
Z. Zhang, M. P. Gygi, A.R. Krainer, S.P. Gygi,
and R.ReedMolecular Cell 26, 867881, 2007
  • Transcription and splicing are functionally
    coupled, resulting in highly efficient splicing
    of RNAP II transcripts.
  • To identify potential coupling factors, a
    comprehensive proteomic analysis of
    immuno-purified human RNAP II was carried out,
    and 100 specifically associated proteins were
    identified by Mass Spectroscopy.
  • Among these are the SR protein family of splicing
    factors and all of the components of U1 snRNP,
    but no other snRNPs or splicing factors.
  • It is shown that SR proteins function in coupling
    transcription to splicing and evidence is
    provided that the mechanism involves
    cotranscriptional recruitment of SR proteins to
    RNAP II transcripts.

46
Evidence that U1 snRNP and SR Proteins Are the
Splicing Factors Associated with RNAP II
47
(No Transcript)
48
Model for Cotranscriptional Recruitment of SR
Proteins/U1 snRNP to Nascent RNAP II Transcripts
A) SR proteins/U1 snRNP associate with RNAP II.
During transcription, these splicing factors are
transferred from RNAP II to the exon/5' splice
site. As a result, the spliceosome is efficiently
assembled and splicing is efficient. (B) SR
proteins/U1 snRNP compete with inhibitory hnRNP
proteins for binding to naked T7 transcripts,
resulting in a portion of the transcript binding
these splicing factors and a portion binding
inhibitory hnRNP proteins. The net result is that
T7 transcripts assemble into both the spliceosome
and the H complex, and the overall efficiency of
spliceosome assembly and splicing is lower with
the T7 versus RNAP II transcript.
49
SR Proteins help to define 5 and 3 splice sites
  • SR proteins bind to specific motifs within exons
    (ESE) to recruit the U1 snRNP to the 5 splice
    site and recruit U2AF35 to define the 3 splice
    site of some transcripts
  • SR proteins have different RNA binding
    specificities

50
Cross-intron versus cross-exon complexes (a) SR
proteins function in a cross-intron recognition
complex by bridging between the interactions of
U1 snRNP bound to the upstream 5ss and U2AF65
and 35-kDa subunits bound to the polypyrimidine
tract (PPT) and the AG dinucleotide of the
downstream 3ss, respectively. Then, U2AF65
recruits U2 to the branch site sequence (BS).
(b) SR proteins also facilitate a cross-exon
recognition complex. The exons contain exonic
splicing enhancers (ESEs) that are binding sites
for SR proteins. When an SR protein binds to an
ESE, the SR protein recruits U1 snRNP to the
downstream 5ss, and U2AF65 and 35-kDa subunits
to the PPT and the 3 ss-AG dinucleotide,
respectively. In turn, U2AF65 recruits U2 snRNP
to the BS.
51
SR Proteins have Different RNA specificities
52
The role of SR proteins in mRNA splicing
  • SR proteins bind to relatively short exonic and
    intronic sequences, usually 418 nt, which are
    generally found up to 150 bases from the
    regulated splice site.
  • The RS domains of SR proteins are phosphorylated
    by several different kinases. The phosphorylation
    modulates proteinprotein interactions within the
    spliceosome, thereby contributing to dynamic
    structural reorganization during splicing.
  • The binding of these proteins by means of their
    RNA recognition motif to the exonic and intronic
    sequences facilitates the recruitment of the
    basal splicing machinery to the splice junctions.

53
Substrate Specificities of SR Proteins in
Constitutive Splicing Are Determined by Their RNA
Recognition Motifs
54
(No Transcript)
55
SR Protein Family MembersDisplay Diverse
Activities in the Formationof Nascent and Mature
mRNPs In Vivo
  • Aparna K. Sapra, Minna-Liisa A nko , Inna
    Grishina, Mike Lorenz, Marta Pabis, Ina Poser,
    Jarod Rollins,Eva-Maria Weiland, and Karla M.
    Neugebauer
  • Mol Cell. 2009 Apr 2434(2)179-90

56
Stable Expression of GFP-Tagged Splicing Factors
from Recombineered BACs in HeLa Cells(A)
Proof-of-principle ChIP experiment, using a-GFP
antibodies to detect GFP-tagged U1-70K, U2AF65,
and Prp8 proteins, each expressed from BACs in
stable cell lines. The profiles show that the use
of the tag permits robust detection of each
splicing factor in the expected pattern along
activated FOS. Cartoon representing FOS gene
structure is shown.(B) Physiological expression
levels of tagged proteins were verified by
western blot analysis of different single-cell
stable clones and untransfected control cells
(HeLa), comparing expression levels of GFP-tagged
and endogenous proteins. Antibodies to SRp20
(7B4), all SR proteins (104), and U2AF65 (MC3)
were used.
57
Cotranscriptional Recruitment of SR Proteins to
the FOS Gene Is Transcription Dependent In Vivo
ChIP profiles of Pol II and GFP-tagged members of
the SR protein family (shown in key) on FOS
uninduced (top panel) and transcriptionally
induced (bottom panel). Cartoon representing FOS
gene structure is shown above the panels.
Amplicons distributed within each gene are marked
by horizontal black bars, which are centered over
the following positions in the gene 179, 945,
1373, and 2850. The y axis in each graph
denotes fold over intergenic, the signal obtained
from a region marked as gene desert. The x axis
shows the amplicons corresponding to the cartoon
above.
58
SRp55 Accumulation on the Active FOS Gene Is RNA
Dependent. ChIP results for (A) Pol II (mAb Pol
3/3), (B) SRp55-GFP (a-GFP), and (C) CBP80 on
induced FOS, following treatment of the
crosslinked extracts with (gray) or without
(black) RNase A.
59
SR Protein Interactions with Nascent and Mature
mRNPs(A) Cartoon depicting possible interactions
detectable in the coIP experiment RNA-dependent
interactions, both co- and posttranscriptional,
and direct protein-protein interactions.(B) CoIP
was carried out with nonspecific IgG and a-GFP
antibodies from RNase A-treated () or -untreated
(-) extracts prepared from different GFP-tagged
stable cell lines, as mentioned to the left of
each panel. Inputs (1/100) and the IPs were
analyzed by western blotting specificities of
the antibodies are indicated on the right side of
each panel. These include a-CBP20, a-CBP80, and
a-Pol II (mAbH5 specific for phosphorylated Ser2
of the CTD
60
Conclusions
  • Recruitment of SR proteins to nascent FOS RNA was
    transcription dependent and RNAse sensitive.
  • Unique patterns of SR proteins accumulated along
    the RNA specified by the RNA recognition motifs
    (RRMs).
  • All interactions of SR proteins with RNAP II were
    RNA dependent.

61
RNP RNA Recognition Domain
62
(No Transcript)
63
Determination of RNA-binding sequence or
structural specificity for RNA binding proteins
  • In vitro Functional SELEX

64
An increased specificity score matrix for the
prediction of SF2/ASF-specific exonic splicing
enhancers Philip J. Smith, Chaolin Zhang, Jinhua
Wang, Shern L. Chew, Michael Q. Zhang and Adrian
R. Krainer Human Molecular Genetics, 2006, Vol.
15, No. 16 24902508
  • A refined functional SELEX screen for motifs that
    can act as ESEs in response to the human SR
    protein SF2/ASF was developed.
  • 2. The test BRCA1 exon under selection was
    internal in the test gene. A naturally occurring
    heptameric ESE in BRCA1 exon 18 was replaced with
    two libraries of random sequences, one seven
    nucleotides in length, the other 14.
  • 3. Following three rounds of selection for in
    vitro splicing via internal exon inclusion, new
    consensus motifs were derived.
  • 4. Many winner sequences were demonstrated to be
    functional ESEs in S100-extract-complementation
    assays with recombinant SF2/ASF.

65
Experimental procedure for functional SELEX. The
SF2/ASF-specific BRCA1 exon 18 ESE was replaced
by 7 or 14 nt of randomized sequence by
overlap-extension PCR. In vitro-transcribed RNA
was incubated under splicing conditions in HeLa
S100 extract complemented by recombinant
SF2/ASF. Spliced mRNA molecules containing
SF2/ASF-responsive sequences (designated by the
white W in a black box) were purified from
denaturing polyacrylamide gels, and rebuilt into
full-length intron-containing constructs.
Following three rounds of selection, individual
ESE-containing clones (E) were sequenced and
consensus motifs and score matrices derived.
66
Splicing of the pre-mRNA pools following
selection (A) In vitro splicing of the n7 (lanes
79) and n14 (lanes 1012) winner pools following
three rounds of selection was performed in both
HeLa nuclear extract (NE), and S100 extract
complemented by recombinant SF2/ASF (A). As
controls, BRCA1 WT (lanes 13) and the nonsense
E1694X MT (lanes 46) were also spliced. The
structures of the precursor, intermediates and
products are indicated next to the autoradiogram.
The experiment was repeated three times and the
data normalized to BRCA1 WT levels of splicing
for exon inclusion (B) and inclusive splicing.
(C). Black boxes indicate splicing in nuclear
extract, white boxes splicing in S100
complemented by recombinant SF2/ASF.
67
The SELEX winners comprise functional ESEs
68
The SELEX winners comprise functional ESEs
The winner sequences are functional
SF2/ASF-dependent ESEs. In vitro splicing of 10
n14 round-three winner sequences in HeLa nuclear
extract, S100 extract alone and S100 complemented
by recombinant SF2/ASF. The structures of the
precursor, intermediates and products are
indicated next to the autoradiograms.
69
SR Proteins Splicing
  • SR proteins play essential roles in both
    constitutive and alternative splicing
  • SR proteins interact with each other and other RS
    domain containing proteins by protein-protein
    interactions in the RS domains
  • SR protein activity in splicing is modulated by
    phosphorylation
  • SR serve as molecular bridges in splicesome
    assembly
  • SR proteins bind to specific RNA sequences to
    recruit spliceosomal components to weak splice
    sites
  • SR proteins couple transcription splicing
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