Identification and Characterization of the CDK12/Cyclin L1 Complex Involved in Alternative Splicing Regulation

CrkRS is a Cdc2-related protein kinase that contains an arginine-and serine-rich (SR) domain, a characteristic of the SR proteinfamily of splicing factors, and is proposed to be involved inRNA processing. However, whether it acts together with a cyclinand at which steps it may function to regulate RNA processingare not clear. Here, we report that CrkRS interacts with cyclinL1 and cyclin L2, and thus rename it as the long form of cyclin-dependentkinase 12 (CDK12^L). A shorter isoform of CDK12, CDK12^S, thatdiffers from CDK12^L only at the carboxyl end, was also identified.Both isoforms associate with cyclin L1 through interactionsmediated by the kinase domain and the cyclin domain, suggestinga bona fide CDK/cyclin partnership. Furthermore, CDK12 isoformsalter the splicing pattern of an E1a minigene, and the effectis potentiated by the cyclin domain of cyclin L1. When expressionof CDK12 isoforms is perturbed by small interfering RNAs, areversal of the splicing choices is observed. The activity ofCDK12 on splicing is counteracted by SF2/ASF and SC35, but notby SRp40, SRp55, and SRp75. Together, our findings indicatethat CDK12 and cyclin L1/L2 are cyclin-dependent kinase andcyclin partners and regulate alternative splicing.

INTRODUCTION

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Introduction

It is estimated that fewer than 30,000 genes are present inthe human genome (13). The heterogeneity generated by this numberof genes is not enough to account for the complexity that specifieshuman organs. One way to create more proteomic variations isthrough alternative splicing (2, 21). About 38 to 74% of humangenes are subject to alternative splicing (3, 14, 15), and mutationsthat affect splicing patterns are the underlying causes of somecancers and neurodegenerative diseases (10, 29). It is estimatedthat $~$ 15% of disease-causing mutations in human genes involvemisregulation of alternative splicing (25). Thus, unravelingthe pathways and the molecules involved in alternative splicingis crucial to an understanding of various intricate cellularfunctions and for the management of human diseases.

Although cyclin-dependent kinases (CDKs) and their associatedcyclins are pivotal for cell cycle progression and RNA transcription(23), evidence has emerged that they also engage in the regulationof RNA splicing (19, 27). For example, CDK11^p110 colocalizeswith the general splicing factor RNPS1 (20) and serine- andarginine-rich (SR) proteins, such as 9G8 (12). Moreover, depletionof CDK11^p110 immune complex impedes the efficiency of an invitro splicing assay (12). Similarly, blocking the activityof cyclin L1, a cyclin partner of CDK11^p110, inhibits the secondstep (cutting of the lariat-exon intermediate and ligation ofadjacent exons) of pre-mRNA splicing in an in vitro assay (7).

A recently identified Cdc2-related kinase, CrkRS, is also implicatedin the regulation of RNA splicing (16). CrkRS contains an arginine-and serine-rich (RS) domain, a characteristic found in the SRprotein family of splicing factors. Furthermore, CrkRS localizesin nuclear speckles and CrkRS-immunoprecipitated complexes phosphorylatethe C-terminal domain of RNA polymerase II and the splicingfactor SF2/ASF in vitro, suggesting its roles in transcriptionand splicing. However, whether CrkRS has a cyclin partner isnot clear, nor is it known to be involved in alternative splicingmachinery.

In a previous study, we surveyed the expression profiles ofprotein kinases in cultured neurons and in early developingneural tissues by reverse transcription (RT)-PCR using primerscorresponding to conserved amino acids in the kinase domain(18). Several PCR fragments whose sequences corresponded tonovel kinases at that time were identified. One of the fragmentscontains sequences similar to the CDC2 kinase domain. In thisstudy, we characterized this kinase and showed that it is ashorter isoform of CrkRS.

Based on coprecipitation experiments as well as colocalizationstudies, we demonstrated that both isoforms of CrkRS interactwith cyclin L1 and cyclin L2 and renamed these isoforms CDK12^L(the long isoform of CDK12) and CDK12^S (the short isoform ofCDK12). Furthermore, overexpression of CDK12 isoforms, cyclinL1, and cyclin L2 affects the splicing pattern of the E1a minigene,and perturbation of CDK12 expression changes the splicing patternin a reverse manner. We also demonstrated that the effect ofCDK12 on the E1a splicing pattern is inhibited by overexpressionof SF2/ASF and SC35. These results provide initial evidencethat CDK12 and its cyclin partners are involved in alternativeRNA splicing.

MATERIALS AND METHODS

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Materials and Methods

Animals and reagents. Pregnant and postnatal Sprague-Dawley rats were obtained fromthe animal facility of National Yang-Ming University. Handlingof the animals was according to university guidelines and wasapproved by the National Yang-Ming University Animal Care andUse Committee. Superscript reverse transcriptase II and chemicalsused in tissue culture were purchased from Gibco-BRL (GrandIsland, NY). Expand high-fidelity Taq DNA polymerase, dATP,dCTP, dGTP, dTTP, 4',6'-diamidino-2-phenylindole (DAPI), andthe protease inhibitor cocktail were obtained from Roche (Mannheim,Germany). RNase inhibitor (RNasin) and Taq DNA polymerase werepurchased from Promega (Madison, WI). Hybond-N⁺ nylon membranes,mRNA purification kits, and Rediprime II kits were purchasedfrom Amersham Pharmacia (Buckinghamshire, England). The primersused in PCR were synthesized by MDBioMed (Taipei, Republic ofChina). The Marathon kits were from Clontech (Palo Alto, CA).All other chemicals, unless otherwise specified, were purchasedfrom Merck (Darmstadt, Germany).

cDNA cloning of CDK12^S. Total RNA was prepared as described previously (5). A fragmentof rat CDK12^S was obtained by degenerated RT-PCR from embryonicday 14.5 (E14.5) cortical neurons (18). To obtain 5' and 3'fragments of rat CDK12^S, 5' and 3' rapid amplification of cDNAends (RACE) was performed using the Marathon kit according tothe manufacturer's instructions. The 5'- and 3'-RACE productswere cloned into pCR II (Invitrogen, Carlsbad, CA) for DNA sequencing.

Northern blotting analysis. Polyadenylated mRNAs or total RNAs were separated on a 1% denaturingagarose gel and transferred to Hybond-N⁺ nylon membranes. Themembranes were prehybridized at 65°C for 2 h in prehybridizationsolution (0.125 M Na₃PO₄ [pH 7], 0.25 M NaCl, 1 mM EDTA, 10%PEG-6000, 7% sodium dodecyl sulfate, 1% bovine serum albumin)and then hybridized with probes corresponding to nucleotidesequence 90 to 786 (probe 1) of the rat CDK12^S (accession numberNM_138916), 3814 to 4381 (probe 2) of the rat CDK12^S or 3951to 4268 (probe 3) of the rat CDK12^L (accession number AY962568).After hybridization at 65°C for 20 h, membranes were washedthree times in 0.5x SSC (1x SSC is 0.15 M NaCl plus 0.015 Msodium citrate) and 0.1% sodium dodecyl sulfate at 65°Cfor 30 min before autoradiography. For normalization, blotswere stripped and reprobed with a cyclophilin probe.

Vector construction. To construct pCDK12^S, the CDK12^S coding region was amplifiedfrom E14.5 rat brain cDNA by RT-PCR and cloned into pHA (a giftfrom C.-J. Huang, Academia Sinica, Taipei, Republic of China).To construct the pEGFP-Myc expression vector, the enhanced greenfluorescent protein (EGFP) coding region was amplified fromvector pCRG and ligated into vector pEF (Invitrogen). CDK12^Sand truncated CDK12 fragments were amplified by PCR using pCDK12^Sas a template and cloned into pEGFP-Myc, such that the vectorswere able to express EGFP-fused CDK12^S and truncated CDK12 proteinstagged with Myc and His tags. Human CDK12^S and CDK12^L were amplifiedfrom cDNA of HeLa cells and cloned into pEF. The resulting vectors(phCDK12^S and phCDK12^L) express untagged human CDK12^S and CDK12^Lproteins.

To construct pcyclin L1 ${alpha}$ -Flag, pcyclin L1ß-Flag, andpcyclin L2 ${alpha}$ -Flag expression vectors, the coding regions wereamplified from E14.5 rat cDNA using primer sets containing Flagand the stop codon sequence and cloned into pEF. Cyclin L1 ${alpha}$ -Flagand cyclin L1ß-Flag were also cloned into pEGFP aspEGFP-cyclin L1 ${alpha}$ -Flag and pEGFP-cyclin L1ß-Flag.

The SR protein expression vectors, including pSF2/ASF, pSC35,pSRp40, pSRp55, and pSRp75, were kindly provided by W.-Y. Tarn.These vectors were derived from pCEP4 and express hemagglutinin(HA)-tagged SR proteins. RNA recognition motifs 1 and 2 of SF2/ASF,the RS domain of SF2/ASF, the RNA recognition motif of SC35,and the RS domain of SC35 were amplified by PCR and then clonedinto pCEP4 for truncated HA-tagged SR proteins. For RNA interferenceexperiments, synthesized double-stranded DNA fragments correspondingto 1488 to 1513 (pCDK12si1) and 2809 to 2834 (pCDK12si2) ofmouse CDK12 (accession number NM_138916) were cloned into vectorpmU6 (32). For antigen expression in Escherichia coli, cDNAfragments were cloned into pET29a (Clontech). All constructswere verified by sequencing.

Cell cultures and transfection. HEK293T cells were cultured at 37°C in Dulbecco's modifiedEagle's medium supplemented with 10% fetal bovine serum in a5% CO₂ incubator. P19 cells were cultured in ${alpha}$ minimal essentialmedium supplemented with 2.5% fetal bovine serum and 7.5% newborncalf serum. To introduce various constructs into HEK293T andP19 cells, calcium phosphate transfection cocktails (5 mg/mlHEPES, 5 mg/ml NaCl, 0.37 mg/ml KCl, 1 mg/ml D-glucose, 0.1mg/ml Na₂HPO₄, pH 7.05, 125 µM calcium chloride, and 20µg expression vector) were added to cells grown at 70%confluence in 10-cm culture dishes. Alternatively, cells weretransfected using FuGENE6 (Roche) according to the manufacturer'sinstructions. The medium was changed 18 h after transfection.Cells were harvested 24 to 48 h after transfection. For thesmall interfering RNA experiments, pBiCS2-Puro/GFP (a gift fromD. L. Turner, University of Michigan) was cotransfected withother plasmids into P19 cells. The P19 cells were then selectedusing 5 µg/ml of puromycin 18 h after transfection. Cellswere harvested 48 h after transfection.

Antibodies. DNA fragments corresponding to amino acid residues 1040 to 1212of rat CDK12 (peptide 1) and amino acid residues 1297 to 1402of CDK12^L (peptide 2) were amplified and cloned into pET29a.The recombinant proteins produced by the two bacterial strainswere purified by a Ni²⁺ column. Peptide 1 was injected intorabbit spleen to produce rabbit antiserum. The resulting antiserum(r ${alpha}$ CDK12) was used at 1:2,000 dilution for immunofluorescencestaining. Peptide 1 and peptide 2 were separately injected intoBALB/c mice seven times before collection of the two antisera.The mouse antisera (m ${alpha}$ CDK12 and m ${alpha}$ CDK12^L) were diluted at 1:2,000for Western blots. Mouse anti-Flag M2 monoclonal antibody wasfrom Kodak (New Haven, CT). Mouse anti-Myc monoclonal antibody(9E10) and mouse anti-ß-tubulin antibody (E7) wereobtained from the Developmental Studies Hybridoma Bank (Universityof Iowa, IA), and rabbit anti-Myc antibody was from Bethyl (Montgomery,TX). Rhodamine-conjugated goat anti-mouse immunoglobulin G waspurchased from Caltag Laboratories (Burlingame, CA). Other secondaryantisera were from Cappel (Aurora, Ohio).

Protein extraction, immunoprecipitation, and Western blotting analysis. Rat tissues were homogenized in Laemmli lysis buffer (25 mMTris-HCl, pH 7.4, 50 mM NaCl, 0.5% sodium deoxycholate, 2% NP-40,0.2% sodium dodecyl sulfate, 50 mM NaF, and the protease inhibitorcocktail) for Western analysis. Transfected cells were washedonce with phosphate-buffered saline and dissolved in radioimmunoprecipitationassay (RIPA) lysis buffer (20 mM HEPES, pH 7.8, 150 mM NaCl,1 mM EDTA, 0.1% Triton X-100, 50 mM NaF, 1 mM dithiothreitol,and protease inhibitor cocktail). The cell lysates were clearedby centrifuging at 13,000 x g force for 10 min, and supernatantswere used for Western blotting analysis or immunoprecipitation.The protein concentration was determined using a BCA kit (Pierce,Rockford, IL).

Immunoprecipitation was performed with 300 µg of proteinextract and 2 µl of undiluted primary antibodies in areaction volume of 500 µl at 4°C on a rotator forat least 12 h. The immune complex was absorbed onto 15 µlprotein A/G beads (Calbiochem, Cambridge, MA) at 4°C ona rotator for 30 min. Samples were spun down by low-speed centrifugationand washed 5 times with RIPA lysis buffer. For Western blottinganalysis, equal amounts of either tissue or cell lysate weresubjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresisand transferred to polyvinylidene difluoride membranes. Themembrane was blocked with 5% skimmed milk and probed with primaryantibodies at 4°C overnight. After the membrane was washedand incubated with horseradish peroxidase-conjugated secondaryantibodies at room temperature for 1 h, it was developed withan ECL kit (Amersham Pharmacia). Membranes were then strippedand reprobed with an anti-ß-tubulin antibody.

In vivo splicing assay. The pCEP4-E1a minigene vector was kindly provided by W.-Y. Tarn.HEK293T or P19 cells cultured in six-well plates were cotransfectedwith 0.4 µg of pCEP4-E1a and different amounts of Myc-taggedCDK12 isoform plasmids, Flag-tagged cyclin L1 ${alpha}$ plasmids, and/orSR plasmids. The amounts of plasmid were equalized in each wellby the addition of the backbone vector (pEGFP, pEF, or pCEP4).Total RNAs from the transfected cells were extracted 32 to 48h after transfection by the RNeasy minikit (QIAGEN, Valencia,CA) according to the manufacturer's instructions.

RT-PCR was then performed to amplify the various transcriptsof E1a minigene. To detect the RT-PCR products, standard Southernblotting was performed. The 9S RT-PCR fragment of E1a minigenewas used as the probe. Intensities of 13S, 12S, and 9S in theautoradiography were measured by the ImageQuant (version 1.1,Molecular Dynamics, Sunnyvale, CA) or the Scion image (Beta4.0.2, PC format of NIH Image by Wayne Rasband of National Institutesof Health) program. The percentage of each isoform relativeto the total amount of three isoforms in each sample was calculatedand further normalized to the control. Each experiment was performedat least three times. Statistical analysis was performed bypaired t test, and the P value for statistical significancewas set at 0.05.

Immunofluorescence microscopy. Transfected HEK293T cells grown on coverslips were rinsed oncewith phosphate-buffered saline and then fixed in ice-cold methanolfor 10 min. The samples were stained with appropriate primaryantibodies and then with rhodamine-conjugated goat anti-rabbitantiserum or rhodamine-conjugated goat anti-mouse antiserum.The cells were finally stained with DAPI (1 µg/ml) for10 min. The coverslips were examined by a fluorescence microscope(Eclipse E800M, Nikon) or a confocal microscope (TCS NT, Leica).

RESULTS

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Results

Cloning and sequence analysis of CDK12^S. In a previous study, the expression profile of various proteinkinases in rat cortical neurons was analyzed using degenerateRT-PCR and a nucleotide sequence identified as a novel CDC2-likekinase was isolated (18). Using RACE, we obtained a contiguousnucleotide sequence of 4,381 bp encoding an open reading frameof 1,258 amino acids. A polyadenylation signal was found atbp 4231 (Fig. 1C). Functional domains present in the deducedamino acid sequences were predicted by MotifScan search (http://hits.isb-sib.ch/cgi-bin/PFSCAN?)and included a bipartite nuclear localization signal, an RSdomain, and a CDC2-like serine/threonine kinase domain (Fig.1A). According to the characteristics of the sequence and thefollowing data, we named the protein the short form of cyclin-dependentkinase 12 (CDK12^S, accession number NM_138916). The sequencesof the human and mouse CDK12^S were then acquired by databasecomparison and were confirmed by RT-PCR and DNA sequencing.The deduced protein sequences of CDK12^S are highly conservedamong these species, with 90.7% identity between human and mouse,91.8% identity between human and rat, and 96.5% identity betweenmouse and rat.

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FIG. 1. Protein, mRNA, and genomic structures of CDK12^S and CDK12^L. (A) Protein domains of CDK12^S and CDK12^L. The amino acid sequences of rat CDK12^S and CDK12^L were analyzed by the MotifScan program. CDK12^S and CDK12^L share 1,249 amino acids of sequence. They contain a bipartite nuclear localization signal (NLS), an arginine- and serine-rich motif (RS), and a CDC2-like kinase domain (gray boxes). CDK12^S and CDK12^L display 9 (hatched box) and 235 (blank box) distinct amino acid residues, respectively, at their carboxyl termini. Peptides 1 and 2 were used to generate antisera. (B) Genomic organization of CDK12. The exons were identified by comparing the cDNA sequences with the genomic sequences. The genomic structure of CDK12 contains 14 exons and is conserved between human, mouse, and rat. (C) mRNAs of CDK12^S and CDK12^L. The CDK12^S and CDK12^L transcripts share exons 1 to 13, and the CDK12^S transcript reads through exon 13', while the CDK12^L transcript splices exon 13 directly to exon 14. The probes used in Northern analysis are underlined. Stop codons are labeled with asterisks. The position of the polyadenylation signal is also indicated.

A search of the nonredundant sequence database revealed thatthe cDNA sequences of the human Crkrs (NM_016507) and humanCDK12^S genes are identical at their 5' ends (16). This suggeststhat they are alternatively spliced isoforms of the same gene.To confirm that the alternative splicing event is conserved,we cloned rat Crkrs cDNA, which encodes a protein of 1,484 aminoacids, from E14.5 brain by RT-PCR. Alignment of the rat CDK12^Sand Crkrs cDNA sequences and comparison of these two sequencesto rat genomic sequences indicates that CDK12^S and Crkrs cDNAsare transcripts of the same gene, CDK12, and differ at the 3'end (Fig. 1B and C).

There are 14 exons in the CDK12 gene. The CDK12^S transcriptskips the 5' splice site at the end of exon 13 and containsexon 13'. As there is an in-frame stop codon in exon 13', thisresults in a shortened open reading frame for CDK12^S. In contrast,crkrs transcript splices out exon 13' and connects exon 13 and14, resulting in a longer open reading frame. For clarity, werenamed CrkRS CDK12^L. Thus, the rat CDK12^S and rat CDK12^L proteinsshare the same 1,249 amino acids of the amino termini, but havean additional 9 and 235 distinct amino acid residues, respectively,at the carboxyl termini. An identical exon organization forthe CDK12 gene is observed in the human and rodent genomes,albeit with different lengths of introns in the three species(Fig. 1B). The CDK12 gene is located on human chromosome 17q12(AC009283) and on mouse chromosome 11 (AL591205). The closesthomologous protein to human CDK12 is human CDC2L5 (22), whichalso contains a CDC2-like protein kinase domain and an RS domain.

Expression analyses of rat CDK12. Previously, Ko et al. detected CDK12 expression by Northernblotting using adult human tissues. Its expression in embryonictissues was not analyzed. Moreover, the sizes of CDK12^L andCDK12^S transcripts were not determined. Thus, the expressionof rat CDK12^L and CDK12^S transcripts in various tissues duringembryonic development was analyzed using a probe (probe 1) thatrecognizes both transcripts. When total RNAs derived from E14.5tissues were analyzed, two transcripts of CDK12 with sizes of9.3 and 6.8 kb were detected (Fig. 2A). The CDK12 mRNAs wereubiquitously expressed in E14.5 tissues, including brain, spinalcord, heart, lung, liver, gut, and limb (Fig. 2A). We also examinedthe temporal expression pattern of CDK12 during the developmentof the nervous system. The CDK12 mRNAs were expressed in E10.5neural tube, which was the earliest time point examined (Fig.2B). The levels of CDK12 expression in rat brain are more abundantin the embryonic stages, gradually decrease as development proceeds,and became barely detectable at the adult stage (Fig. 2B).

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FIG. 2. Expression of CDK12 in embryonic rat tissues. (A) We used 5 µg of total RNA from various E14.5 rat tissues analyzed by Northern blotting using probe 1 depicted in Fig. 1C. Two major transcripts, 6.8 kb and 9.3 kb (arrowheads), were detected. Ethidium bromide staining of 28S rRNA was used as the loading control. (B) We used 30 µg of total RNA derived from E10.5 neural tube and brain at various developmental stages analyzed by Northern blotting. The membrane was stripped and reprobed with cyclophilin for the loading control. (C) Polyadenylated mRNA from E14.5 rat brain analyzed by Northern blotting using probe 1, probe 2, or probe 3. Probe 1 and probe 3 detected two transcripts, while probe 2 detected only the 6.8-kb transcript. (D) We used 20 µg of cell extracts of HEK293T transfected with control vector (pEF), phCDK12^S and phCDK12^L to examine the specificity of the m ${alpha}$ CDK12 and the m ${alpha}$ CDK12^L antisera. The m ${alpha}$ CDK12 antiserum recognizes both CDK12^S and CDK12^L, and the m ${alpha}$ CDK12^L antiserum recognizes only CDK12^L. (E) Western analysis of 15 µg of E14.5 rat tissue extracts performed using m ${alpha}$ CDK12 (left panel). The sizes of CDK12^S and CDK12^L detected in the E14.5 brain by the m ${alpha}$ CDK12 antiserum are the same as those detected in 4 µg of CDK12^S- or CDK12^L-overexpressed HEK293T cell lysates (right panel). (F) Western analysis of 15 µg of E14.5 rat tissue extracts performed using m ${alpha}$ CDK12^L (left panel). The size of CDK12^L detected in the E14.5 brain by the m ${alpha}$ CDK12^L antiserum is the same as that detected in 4 µg of CDK12^L-overexpressed HEK293T cell lysates (right panel). Membranes were reprobed with the anti- ${alpha}$ -actin antibody as the loading control.

To distinguish which transcripts correspond to CDK12^S and CDK12^LmRNAs in Northern blots, we designed probe 2 and probe 3, whichspecifically hybridize to the CDK12^S and CDK12^L mRNAs, respectively(Fig. 1C). In the Northern blots using CDK12^S-specific probe2, only the 6.8-kb band could be observed (Fig. 2C). Surprisingly,CDK12^L-specific probe 3 could hybridize both the 9.3-kb and6.8-kb bands, a pattern identical to that observed by probe1 (Fig. 2C). The data indicate that two transcripts, with sizesof 9.3 and 6.8 kb, encode CDK12^L; and a transcript with a sizeof 6.8 kb encodes CDK12^S.

To verify that CDK12^S and CDK12^L transcripts can be translatedto proteins and to examine endogenous protein expression ofCDK12 in rat embryonic tissues by Western blotting, rabbit andmouse antisera (r ${alpha}$ CDK12 and m ${alpha}$ CDK12) were raised against peptidesequences 1040 to 1212 of rat CDK12 (peptide 1 in Fig. 1A) suchthat the antisera recognize both CDK12^S and CDK12^L. Mouse antisera(m ${alpha}$ CDK12^L) against amino acids 1297 to 1402 (peptide 2 in Fig.1A) were also generated to detect only CDK12^L. The specificityof the antibodies was determined by Western blotting using lysatesof HEK293T cells transfected with a control vector (pEF), phCDK12^Sor phCDK12^L. The latter two vectors were able to express humanCDK12^S and CDK12^L protein, respectively.

In cells transfected with pEF, both m ${alpha}$ CDK12 and m ${alpha}$ CDK12^L identifieda 200-kDa band, suggesting that this band corresponds to CDK12^L(Fig. 2D, lanes 1 and 4). m ${alpha}$ CDK12, but not m ${alpha}$ CDK12^L, bound anadditional 180-kDa band, suggesting that this band correspondsto CDK12^S (Fig. 2D, lane 1). The data also indicated that HEK293Tcells express CDK12^S and CDK12^L endogenously. The specificityof antibodies was further validated when CDK12^S- or CDK12^L-overexpressingHEK293T cell lysates were analyzed by Western blotting (Fig.2D). The sizes of CDK12^S and CDK12^L are larger than those predicted(140.0 kDa for CDK12^S and 163.9 kDa for CDK12^L), possibly dueto posttranslational modification such as phosphorylation (16).

We then used these two antibodies to analyze the expressionpattern of CDK12 in E14.5 rat tissues (Fig. 2E and F). BothCDK12^S and CDK12^L proteins were detected in E14.5 brain, spinalcord, heart, lung, liver, gut, and limb. The sizes of thesetwo bands are identical to those found in HEK293T cells.

Interaction between CDK12, and cyclins L1 and L2. It is possible that activation of CDK12 requires a cyclin. Examinationof the cellular localization of known cyclins points to membersof cyclin class L, cyclin L1 and cyclin L2, as good candidatesfor the cyclin partner of CDK12, as they contain an RS domainand are located in the nuclear speckles (6, 7, 31). To testthis hypothesis, we determined whether CDK12 interacts withthe cyclin L members.

CDK12^S and EGFP-tagged cyclin L1 ${alpha}$ (the longest isoform of cyclinL1) were overexpressed in HEK293T cells. The subcellular localizationof CDK12^S, recognized by r ${alpha}$ CDK12, is in nuclear speckles andappears similar to the subcellular pattern of CDK12^L reportedpreviously (Fig. 3A) (16). As expected from previous studies(1, 7), EGFP-tagged cyclin L1 ${alpha}$ is located in the nuclear speckles(Fig. 3B) and is colocalized with CDK12^S (Fig. 3C). CDK12^S andcyclin L2 ${alpha}$ are also colocalized in nuclear speckles when overexpressedtogether in HEK293T cells (Fig. 2D to F).

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FIG. 3. Interaction between CDK12 and cyclin L1 and cyclin L2. (A to C) HEK293T cells transfected with pCDK12^S-Myc and pEGFP-cyclin L1 ${alpha}$ -Flag were stained with the r ${alpha}$ CDK12 antiserum (A) and examined for EGFP fluorescence (B). The merged photograph shows that CDK12^S colocalizes with cyclin L1 ${alpha}$ in nuclear speckles (C). (D to F) HEK293T cells transfected with pEGFP-CDK12^S and pcyclin L2 ${alpha}$ -Flag were examined for EGFP fluorescence (D) and stained with anti-Flag antibody (E). The merged photograph shows that CDK12^S colocalizes with cyclin L2 ${alpha}$ in nuclear speckles (F). (G and H) Lysates of HEK293T cells transfected with the vectors indicated above the panels were immunoprecipitated with the anti-Flag antibody. The immunoprecipitates were subjected to immunoblot analysis with the anti-Flag antibody or the r ${alpha}$ CDK12 antiserum. The expected positions of cyclin L1 ${alpha}$ , cyclin L2 ${alpha}$ , CDK12^L and CDK12^S are shown by arrows.

To demonstrate the possibility that CDK12 can associate withcyclin L1 and cyclin L2, immunoprecipitation experiments wereperformed. Cell lysates containing overexpressed CDK12^S or CDK12^Land Flag-tagged cyclin L1 ${alpha}$ or Flag-tagged cyclin L2 ${alpha}$ were immunoprecipitatedby an anti-Flag antibody. The immune complex was then subjectedto Western blotting. Both CDK12^S and CDK12^L were coimmunoprecipitatedwith cyclin L1 ${alpha}$ or L2 ${alpha}$ (Fig. 3G and H). Similarly, when cell lysatescontaining overexpressed Myc-tagged CDK12^S and Flag-tagged cyclinL1 ${alpha}$ were immunoprecipitated by an anti-Myc antibody, it was shownthat cyclin L1 ${alpha}$ was coimmunoprecipitated with CDK12^S (Fig. 4B,lane 2).

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FIG. 4. Mapping of interaction domains between CDK12 and cyclin L1. (A) Schematic structures of CDK12^L, Myc-tagged CDK12^S, various Myc-tagged CDK12 truncated constructs, Flag-tagged cyclin L1 ${alpha}$ , and Flag-tagged cyclin L1ß. (B) Lysates of HEK293T cells transfected with various CDK12 truncated constructs and pcyclin L1 ${alpha}$ -Flag were immunoprecipitated with the anti-Myc antibody. The immunoprecipitates were subjected to immunoblot analysis with the anti-Flag antibody or the rabbit anti-Myc antiserum (left panels). The same lysates were also immunoprecipitated with the anti-Flag antibody. The immunoprecipitates were subjected to immunoblot analysis with the anti-Flag antibody or the rabbit anti-Myc antiserum (right panels). A nonspecific band was recognized by the rabbit anti-Myc antiserum (asterisk). (C) Lysates of HEK293T cells transfected with the plasmids listed above the panel and immunoprecipitated with the anti-Flag antibody. The resulting proteins were then immunoblotted using the rabbit anti-Flag antiserum or the r ${alpha}$ CDK12 antiserum (left panels). The same lysates were immunoprecipitated with the r ${alpha}$ CDK12 antiserum. The resulting proteins were then immunoblotted using the m ${alpha}$ CDK12 antiserum or the anti-Flag antibody (right panels). A faint band corresponding to the heavy chain (HC) of antibodies used in the immunoprecipitation was detected by the secondary antibodies. (D) Lysates of HEK293T cell transfected with pCDK12K-Myc and pEF or pcyclin L1ß-Flag were immunoprecipitated with the anti-Flag antibody. The resulting proteins were then immunoblotted using the anti-Flag antibody or the rabbit anti-Myc antiserum.

To study further the interaction between CDK12 and cyclin L1,we next mapped the domains involved in the interaction. SinceCDK12^S is sufficient to bind cyclin L1 ${alpha}$ and the amino acid sequenceof CDK12^S is included in CDK12^L (except the last 9 amino acids),we used CDK12^S as the starting template to study the interactionbetween CDK12 and cyclin L1. The Myc-tagged CDK12^S or Myc-taggedtruncated proteins (Fig. 4A) were coexpressed with Flag-taggedcyclin L1 ${alpha}$ in HEK293T cells. Immunoprecipitation with the anti-Flagantibody and Western blotting were then performed. The resultsshowed that cyclin L1 ${alpha}$ protein was coprecipitated with CDK12^Sand the truncated CDK12 protein containing the kinase domainand the carboxyl-terminal domain (CDK12^SKC, Fig. 4B, left panel).

In the reverse immunoprecipitation experiment, CDK12^S and thekinase domain (CDK12K), carboxyl terminus (CDK12^SC) or CDK12^SKCwere coprecipitated with cyclin L1 ${alpha}$ protein by the anti-Flagantibody (Fig. 4B, right panel). The cause for the discrepancyobserved between these two immunoprecipitation experiments isunclear. One possibility is that binding of the anti-Myc antibodyto CDK12K and CDK12^SC during immunoprecipitation may generatesteric hindrance that inhibits interaction between these proteinsand cyclin L1 ${alpha}$ . Together, these results suggest that the kinasedomain and carboxyl-terminal domain of CDK12^S interact withcyclin L1 ${alpha}$ . In a control experiment, the anti-Flag antibody wasunable to pull down CDK12^S or truncated proteins using lysatesof cells transfected with the CDK12 constructs but without pcyclinL1 ${alpha}$ -Flag (data not shown).

As many cyclins interact with CDK through the cyclin domain,we cloned a naturally occurring cyclin L1 isoform, cyclin L1ß,which contains the cyclin domain but no carboxyl-terminal RSdomain (Fig. 4A), and examined its interaction with CDK12 byimmunoprecipitation. The results showed that cyclin L1ßcan interact with CDK12^S (Fig. 4C). The kinase domain of CDK12can also interact with cyclin L1ß in the immunoprecipitationexperiment (Fig. 4D).

CDK12 and cyclin L1 are regulators of alternative splicing. It was reported that human CDK12^L immune complex contains akinase activity that phosphorylates SF2/ASF in vitro (16). Wealso found that immunoprecipitated rat CDK12^S can phosphorylateSF2/ASF, although CDK12^S does not directly phosphorylate SF2/ASF(see Fig. S1 in the supplemental material). As SF2/ASF is amember of the SR proteins, which are involved in the regulationof constitutive splicing as well as alternative splicing (9),we tested whether CDK12 and cyclin L1 change splicing site selectionof an E1a minigene in HEK293T cells.

The pre-mRNA of the E1a minigene can be processed into fivemRNAs. Three major forms, 13S, 12S, and 9S, derive from selectionof one of three 5' splice sites, and two minor forms, 11S and10S, involve additional splicing using an upstream 3' splicesite (Fig. 5A). We transfected the E1a minigene together withpCDK12^S or pCDK12^L and then quantified the intensity ratiosof the 13S, 12S, and 9S products after RT-PCR and Southern blotting.We normalized the percentages of the three major bands to thosein the control experiments, so that changes in the splicingpatterns are easily visualized.

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FIG. 5. Regulation of alternative splicing by CDK12 and cyclin L1. (A) A schematic diagram illustrating the splicing pattern of the E1a reporter gene. The alternative 5' splice sites and splicing events that generate 13S, 12S, and 9S mRNAs are indicated above the diagram. The locations of the primers used for PCR analysis are marked by arrowheads. (B) HEK293T cells were transfected with 0.4 µg of pCEP4-E1a and 1.6 µg of phCDK12^L or phCDK12^S. The splicing assays were then performed as described under Materials and Methods. The upper panel shows a representative autoradiograph of the results. The positions of the 13S, 12S, 10S, and 9S transcripts are indicated on the left. The mean values and standard deviations from three independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control by paired t test. (C) HEK293T cells were transfected with 0.4 µg of pCEP4-E1a and the indicated amounts of pCDK12^S-Myc. The upper panel shows a representative autoradiograph result. The mean values and standard deviations from three independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control by paired t test. (D) Splicing assays of HEK293T cells transfected with pCEP4-E1a (0.4 µg) and the indicated amounts of pcyclin L1 ${alpha}$ -Flag were performed. The upper panel shows a representative autoradiograph result. The mean values and standard deviations from three independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control by paired t test. (E) Splicing assays of HEK293T cells transfected with 0.4 µg of pCEP4-E1a and 2.8 µg of pCDK12^S-Myc or pCDK12^L-Myc and/or 0.8 µg of pcyclin L1ß-Flag were performed. The upper panel shows a representative autoradiograph result. The mean values and standard deviations from four independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control and # indicates P < 0.05 between the pairs marked by connecting lines.

In HEK293T cells, both CDK12^S and CDK12^L decreased the 13S transcriptand increased the 9S transcript (Fig. 5B). Moreover, this effectof CDK12 on E1a splicing pattern is dosage dependent (Fig. 5C).Similar dosage-dependent increases of the 9S transcript anddecrease of the 12S and 13S transcripts were also observed whencyclin L1 ${alpha}$ and cyclin L2 ${alpha}$ were transfected into HEK293T cells(Fig. 5D; see Fig. S2B in the supplemental material). Changesof the splicing pattern of the E1a minigene were also observedwhen CDK12^S and cyclin L1 ${alpha}$ were overexpressed in P19 cells (Fig.6C, lanes 1 and 2). P19 cells are a mouse embryonic carcinomacell line (8).

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FIG. 6. Changes in the alternative splicing pattern in cells with decreased expression of CDK12. (A and B) Proteins and RNAs of P19 cells transfected with 0.4 µg of pCEP4-E1a and 1.2 µg of pmU6, pCDK12si1, and pCDK12si2 were prepared. Proteins were subjected to Western analysis using the m ${alpha}$ CDK12^L antiserum (A). The membrane was reprobed with the anti-ß-tubulin antibody. RNAs were subjected to splicing assays (B). The upper panel shows a representative autoradiograph result. Quantitative results derived from three independent experiments are shown in the lower panel. Standard deviations are indicated. * indicates P < 0.05 in comparison to the control by paired t test. (C) Splicing assays of P19 cells transfected with 0.4 µg of pCEP4-E1a and 0.6 µg of the plasmid indicated above each lane. The upper panel shows a representative autoradiograph result. The mean values and standard deviations from three independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control (lane 1) and # indicates P < 0.05 between the pairs marked by connecting lines.

As cyclin L1ß, which contains mainly the cyclin domain,had lower activity in the E1a splicing assay (see Fig. S2A inthe supplemental material), we examined whether it could potentiatethe effects of CDK12. There was no change in the splicing patternwhen 0.8 µg of pcyclin L1ß was transfected intoHEK293T cells (Fig. 5E, lane 4). However, this dose of pcyclinL1ß potentiated the effects induced by 2.8 µgof phCDK12^S and phCDK12^L (Fig. 5E, compare lanes 5 and 6 tolanes 2 and 3).

To further confirm that CDK12 proteins are involved in alternativesplicing, we knocked down mouse CDK12 in P19 cells, in whichthe expression of endogenous CDK12 is higher than that in HEK293Tcells (data not shown). Two small interfering RNA constructs,pCDK12si1 and pCDK12si2, were transfected into P19 cells. Bothconstructs decreased endogenous CDK12 proteins by at least 40%(Fig. 6A). When the E1a minigene splicing assay was performedin P19 cells, fewer of the 13S transcripts and more of the 9Stranscripts were detected in the control conditions (Fig. 6B,lane 1) compared to the levels in HEK293T cells. When CDK12was knocked down, there were increases in the 13S transcriptand decreases in the 9S transcript levels (Fig. 6B, lanes 2and 3), a pattern opposite what was observed for the CDK12-overexpressedexperiments. The small interfering RNAs also completely blockedany effect on the alternative splicing pattern generated byoverexpression of CDK12^S (Fig. 6C, compare lane 5 to lane 2).Moreover, when the expression of endogenous CDK12 was suppressed,the effect of overexpressed cyclin L1 ${alpha}$ on alternative splicingwas also partially inhibited (Fig. 6C, compare lane 6 to lane3), suggesting that the effects of cyclin L1 on alternativesplicing, at least in part, are mediated by CDK12.

Effect of CDK12 on E1a splicing pattern is compromised by overexpression of SF2/ASF and SC35. Many SR splicing factors have been shown to increase the 13Sand 12S transcripts and to decrease the 9S transcript, a patternopposite what was observed in the case of CDK12 in the E1a splicingassay (26, 28, 33). We thus hypothesized that CDK12 may depletethe activities of SR proteins in the splicing machinery by indirectphosphorylation or sequestration of SR proteins and change theway in which the splicing machinery selects splice sites. Ifthis hypothesis is correct, we reasoned that overexpressionof SR proteins may counteract the effects of CDK12 on the E1asplicing pattern.

We examined this possibility by overexpressing five SR splicingfactors, including SF2/ASF, SC35, SRp40, SRp55, and SRp75, withor without CDK12^S in HEK293T cells for the E1a assay. In HEK293Tcells, due to their already greater amounts of the 13S transcript,no further increase of the 13S transcript was observed by overexpressionof SR proteins alone (Fig. 7A, lanes 3 to 6), except the minorincrease caused by overexpression of SF2/ASF (Fig. 7A, lane2). Among the five SR proteins tested, SF2/ASF partially inhibitedand SC35 almost eliminated the effect of CDK12^S in the E1a assay(Fig. 7A, compare lanes 8 and 9 to lane 7). The other threeSR proteins had no influence on CDK12^S activity. Some of theHEK293T cell lysates used for the splicing assay were used inWestern analyses to detect the overexpressed proteins. The resultsshowed that SR proteins were expressed as expected and ectopicexpression of SR proteins did not affect synthesis of CDK12^Sproteins (see Fig. S3 in the supplemental material). Moreover,no changes in the molecular weights of all the SR proteins testedwere observed when SR proteins and CDK12^S proteins were coexpressed.

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FIG. 7. Inhibition of CDK12 alternative splicing activity by SR proteins. (A and B) Splicing assays of HEK293T cells transfected with 0.4 µg of pCEP4-E1a and 1.8 µg of the plasmids listed above the panels were performed. The splicing assays were then performed as described under Materials and Methods. The upper panel shows a representative autoradiograph of the results. The positions of the 13S, 12S, 10S, and 9S transcripts are indicated on the right. The mean values and standard deviations from three independent experiments are shown in the lower panel. * indicates P < 0.05 in comparison to the control (lane 1) and # indicates P < 0.05 between the pairs marked by connecting lines by paired t test.

Previous reports had shown that the RNA recognition motifs (RRMs),but not the RS domain, mediate the effect of SF2/ASF in theE1a splicing assay (4, 30). We thus tested whether the RRMsof SF2/ASF are sufficient to block the effect of CDK12^S in theE1a assay. As expected, the RRMs of SF2/ASF, but not the RSdomain, changed the E1a splicing pattern (Fig. 7B, lanes 2 and3) and eliminated the effect of CDK12^S (Fig. 7B, compare lane7 to lane 6). However, neither the RRM nor the RS domain ofSC35 offset the effect of CDK12^S, suggesting that both domainsof SC35 were required to counteract CDK12^S (Fig. 7B, lanes 9and 10). Together, these data suggested that one of the mechanismsby which CDK12 regulates alternative splicing is mediated byblockage of the activities of SF2/ASF and SC35.

DISCUSSION

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Discussion

In this report, we describe the cloning of a shorter isoformof crkrs and demonstrate that both isoforms interact with cyclinL1, and we renamed them as isoforms of CDK12. Based on a comparisonof genomic DNA sequences, these isoforms result from alternativesplicing. Unlike canonical CDKs, CDK12^S and CDK12^L are proteinswith high molecular weights and have an extended amino-terminalregion that contains an RS domain. By Northern and Western analyses,both isoforms of CDK12 are ubiquitously expressed in embryonictissues. A lower level of CDK12 proteins is detected in adultrat tissues (data not shown). In the present report, both CDK12^Sand CDK12^L proteins are shown to associate with members of thecyclin L class and act similarly in the splicing assay. Furtherexperiments are needed to reveal whether there are functionaldifferences between the CDK12^S and CDK12^L proteins in termsof these activities.

Our results from the coprecipitation and colocalization experimentsshow that CDK12 associates with cyclin L1 and cyclin L2. Wefurther demonstrate that this interaction occurs mainly betweenthe kinase domain of CDK12 and the cyclin domain of cyclin L1,albeit the carboxyl-terminal region of CDK12^S also interactsweakly with cyclin L1 (Fig. 4B). In the E1a minigene splicingassay, CDK12, cyclin L1 ${alpha}$ , and cyclin L2 ${alpha}$ increase formation ofthe 9S transcript at the expense of the 13S transcript in HEK293Tcells. Furthermore, addition of a very small amount of the cyclindomain of cyclin L1 potentiates the effect of CDK12^S on thechange in alternative splicing, suggesting that these two proteinscollaborate. Note that there is endogenous expression of CDK12and cyclin L1 ${alpha}$ in HEK293T cells and P19 cells, which makes itdifficult to display a strong synergistic effect between cyclinL1 and CDK12.

The cooperation between CDK12 and cyclin L1 is further suggestedby the small interfering RNA experiments. Introduction of CDK12small interfering RNAs into cultured cells not only partiallydecreases endogenous CDK12 expression, hence increasing the13S transcript in the E1a minigene assay, but also eliminatesthe effect of overexpressed CDK12 in the splicing assay. Moreover,in the presence of CDK12 small interfering RNAs, the effectsof overexpressed cyclin L1 ${alpha}$ are also partially blocked (Fig.6C), which further substantiates the interaction between CDK12and cyclin L1. The fact that blockage of the cyclin L1 ${alpha}$ effectby the CDK12 small interfering RNAs is incomplete is not unexpected,as cyclin L1 ${alpha}$ may associate with other CDKs, in addition to CDK12,to regulate RNA processing. At least one known CDK, CDK11^p110,has been demonstrated to interact with cyclin L1 ${alpha}$ , and this proteinis involved in constitutive splicing as measured by an in vitroassay (12). It is possible that CDK11^p110 regulates alternativesplicing in the same manner as CDK12, and by acting with CDK11^p110the overexpressed cyclin L1 ${alpha}$ protein may still be able to changethe splicing pattern even in the absence of CDK12.

The protein sequence of human CDK12 is very similar to thatof a recently identified kinase, CDC2L5 (22). There is 92% aminoacid identity in the kinase domain and 52% identity overallbetween human CDK12^L and human CDC2L5. Like CDK12, CDC2L5 containsan RS domain at the amino-terminal region. It has thus beensuggested that these two genes belong to a new subfamily inthe CDC2-like protein kinase family (22). In view of the structuralsimilarity between CDK12 and CDC2L5, it is likely that CDC2L5may interact with cyclin L1 or a related cyclin(s) and regulateRNA processing.

The observed effects of CDK12/cyclin L1 on the E1a minigene,with a decrease of the 13S transcript and a concurrent increaseof the 9S transcript, are opposite those exerted by SR proteins(26, 28). Interestingly, we found that overexpression of SF2/ASFand SC35, but not SRp40, SRp55, and SRp75, offsets the effectof CDK12 on alternative splicing (Fig. 7A). The relationshipbetween CDK12, SF2/ASF, and SC35 is currently unclear. Thereis no direct phosphorylation of SF2/ASF in vitro by CDK12 (seeFig. S1 in the supplemental material), and no molecular weightincrease of SR proteins is observed when SR proteins are coexpressedwith CDK12 (see Fig. S3 in the supplemental material). Moreover,there was no increase of phosphorylated endogenous SR proteinsdetected by the 1H4 antibody, which recognizes phosphoserinein the RS domain, when CDK12 was overexpressed in cultured cells(data not shown). One possibility is that CDK12 affects splicingpatterns by sequestering SR proteins by its interaction withSR proteins. It has been suggested that nuclear factors SAF-Band YT521-B bind and sequester SR proteins to affect splicesite selection (11, 24). By saturating the CDK12 binding sites,overexpression of SF2/ASF and SC35 thus eliminates the CDK12effect. CDK12 deletion constructs and mutations are needed tosort out whether sequestration of SR proteins by CDK12 is likely.As SF2/ASF and SC35 are essential for constitutive splicingand alternative splicing and are involved in maintaining genomestability (17), our results may also show another way to controlthe activities of these two splicing factors.

ACKNOWLEDGMENTS

We thank Woan-Yuh Tarn, Chang-Jen Huang, and David L. Turnerfor providing reagents and Shu-Fen Tsai, Yui-Ing Yu and Shu-HueiWang for assistance with the confocal microscopy. We thank Zi-JayShan, I-Jan Shan, and Hsin-I Yu for generating m ${alpha}$ CDK12^L antiseraand Shu-Fen Lin for cloning mouse CDK12^S. We are also gratefulto Lung-Sen Kao, Chen-Kung Chou, and Woan-Yuh Tarn for criticalreading of the manuscript and to other laboratory members fortheir help in manuscript preparation.

This work was supported by grants from the National Health ResearchInstitute (NHRI-GT-EX89S732C), Yen Tjing Ling Medical Foundation,and the Program for Promoting Academic Excellence from Ministryof Education, ROC, to M.-J.F.

FOOTNOTES

* Corresponding author. Mailing address: Faculty of Life Sciences, National Yang-Ming University, Taipei, Taiwan 11221. Phone: 886-2-2826-7184. Fax: 886-2-2820-0259. E-mail: mjfann{at}ym.edu.tw.

Supplemental material for this article may be found at http://mcb.asm.org/.

REFERENCES

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