TFIIH kinase phosphorylates Serine 7

Cyclin-dependent kinases (Cdk) are promiscuous enzymes and their substrate choices are governed by cyclins that recruit specific target proteins (Nigg, 1996; Schulman et al., 1998). The substrate preference of Cdk7, the human homolog of Kin28, is specified by other subunits of the TFIIH complex (Feaver et al., 1994; Svejstrup et al., 1994; Watanabe et al., 2000). Thus, Kin28 within the TFIIH complex could display altered substrate selectivity and might not phosphorylate Ser7. We therefore examined if the TFIIH-associated Kin28 would phosphorylate Ser7 residue of the CTD. Kin28 associates with the cyclin Ccl1 and a third partner (Tfb3) to form an active TFIIK complex that phosphorylates Ser5 of the CTD (Feaver et al., 1994, Feaver et al., 1997). TFIIK further associates with the “core” seven-subunit complex to form the TFIIH complex (Figure 2A) (Feaver et al., 1994; Svejstrup et al., 1994; Ranish et al., 2004). As part of the TFIIH complex, the kinase shows a high degree of substrate specificity and selectively phosphorylates the CTD, two subunits of transcriptional machinery (Med4 and Rgr1), and the transcription activator Gal4 (Feaver et al., 1994; Watanabe et al., 2000; Guidi et al., 2004; Hirst et al., 1999; Liu et al., 2004; Muratani et al., 2005; Sadowski et al., 1991). We purified TFIIH using TAP-fusions to different subunits of the complex. In each case, the associated Kin28 kinase robustly phosphorylates Ser7 as well as Ser5 (Figure 2A). These results indicate that TFIIH-associated Kin28, despite its increased substrate-specificity, phosphorylates Ser7.

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Figure 2

TFIIH-associated Kin28 phosphorylates the Ser7 of Pol II CTD

(A) The schematic diagram (top left) shows the different subunits of TFIIK and the core TFIIH complex. Dot blot and ELISA of GST-CTD phosphorylated by TFIIH purified using TAP-tagged Kin28, Ccl1, Rad3 or Rad25.

(B) The diagram (top) illustrates the docking of ATP into the catalytic pocket of wild type kinase. Dot blot (bottom) of GST-CTD phosphorylated by Kin28 and its analog sensitive mutant Kin28as (Kin28-L83G) in the presence and absence of an inhibitor was probed with αSer5-P and αSer7-P antibodies.

(C) Dot blot of GST-CTD and its various mutants at positions 2, 5, and 7 phosphorylated by purified Kin28 and probed with αSer5-P and αSer7-P antibodies.

(D) The diagram (top) illustrates the ability of Kin28as to use of the ATP analog (N⁶-benzyl ATP) as a co-factor. Dot blot (bottom) of GST-CTD phosphorylated by Kin28 and Kin28as in presence and absence of the N⁶- benzyl ATP was probed with αSer5-P and αSer7-P antibodies.

TFIIH complex itself associates with numerous protein partners and even with the U1-snRNA (Esnault et al., 2008; Roeder, 2005; Kwek et al., 2002; Zurita and Merino, 2003). Hence, rather than Kin28, it is possible that an unrelated kinase that sub-stoichiometrically associates with TFIIH is responsible for the Ser7 modification. To address this concern we engineered the TAP-tagged Kin28 to accept a bulky analog of a kinase inhibitor (Figure S2). This bulky analog is incapable of docking into ATP binding pockets of unmodified kinases (Bishop et al., 2000; Bishop et al., 2001). In contrast, the engineered Kin28as (analog sensitized) is inhibited at micro-molar concentrations of the designed inhibitor, 1-NAPP1 (Kanin et al., 2007; Liu et al., 2004). The TAP-tagged Kin28as (Kin28-L83G) enzyme is unable to phosphorylate Ser5 or Ser7 in the presence of the inhibitor but is as active as the wild type kinase in the presence of ATP (Figure 2B). As expected, due to the inability of the inhibitor to dock in an unmodified ATP binding pocket, the activity of wild-type Kin28 is not detectably perturbed by the inhibitor. These results suggest that Kin28 directly phosphorylates Ser7. However, Ser7 phosphorylation might be dependent on prior phosphorylation of Ser5 by Kin28 (Chapman et al., 2007). We therefore examined the ability of Kin28 to phosphorylate recombinant CTD substrates wherein Ser2, 5 or 7 have been substituted by an alanine residue (Fig. 2C). The data show that an alanine at positions 2 or 7 does not detectably affect the ability of Kin28 to phosphorylate Ser5. In contrast, replacing Ser5 with an alanine dramatically reduces the ability of Kin28 to phosphorylate Ser7. In other words, inhibiting Ser5 phosphorylation by chemical inhibition could block subsequent phosphorylation of Ser7 by a different kinase. To directly test if Kin28 can phosphorylate both Ser5 and Ser7, we used N⁶-benzyl-ATP as a phospho-donor in kinase reactions with Kin28 or Kin28as (Figure 2D and Figure S2). This modified ATP docks into the expanded ATP binding pocket of Kin28as but is not used efficiently by unmodified kinases. The enlargement of the ATP binding site does not alter substrate specificity of the kinase (Liu et al., 1998; Bishop et al., 2000; Bishop et al., 2001; Liu et al., 2004). In this context, the appearance of Ser7-P mark with N⁶-benzyl-ATP therefore confirms that Kin28as phosphorylates both Ser7 and Ser5 residues of the CTD heptad (Figure 2D).

Chemical genomics evidence for Ser7 phosphorylation by Kin28 in vivo

We examined the consequences of chemically inhibiting Kin28 on Ser7 phosphorylation patterns across the genome. The growth of cells bearing the Kin28as allele is greatly attenuated by micro-molar concentrations of the cell-permeable inhibitor (Figure S3) (Kanin et al., 2007; Liu et al., 2004). Chromatin immunoprecipitation (ChIP) assays show that within 20 minutes of inhibition, the Ser5-P marks of CTD are dramatically reduced in Kin28as strains (Kanin et al., 2007; Liu et al., 2004). Using high-resolution genome tiling microarrays, we examined the genome-wide profiles of Ser5-P and Ser7-P CTD modifications (Figure 3). We focused on the snRNA genes that code for spliceosomal transcripts because of the key role of Ser7 phosphorylation in the expression of these genes (Figure 3A). At all five snRNA genes the profiles of Ser7-P closely mirror those of Ser5-P (Figure 3 and Figure S4). SNR6 (U6), which is transcribed by Pol III, serves as negative control with background levels of Pol II and Ser5/7 phosphorylation profiles. Strikingly, inhibition of Kin28 eliminates both Ser7-P and Ser5-P peaks. A similar remodeling of the profiles is also seen at protein-coding genes (Figure 3B). We focused on protein-coding genes with uniformly robust Pol II occupancy across the entire open reading frame (Steinmetz et al., 2006). Of these 415 genes, 308 with well-defined transcription start sites were clustered based on the CTD modification profiles. Upon Kin28 inhibition, the attenuation of Ser7-P and Ser5-P profiles is clearly evident (Figure 3B). The results across the genome reflect this loss of Ser7-P phosphorylation at the promoter regions and are consistent with the ability of Kin28 to phosphorylate Ser7. The results strongly implicate Kin28 in the phosphorylation of Ser7 and Ser5 residues of the CTD in vivo.

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Figure 3

In vivo inhibition of Kin28 affects the Ser7 phosphorylation pattern

(A) ChIP-chip profiles for two snRNAs (remaining three are in the supplemental figures). The occupancy profiles of Pol II (blue), Ser7-P (purple) and Ser5-P (red) at SNR14 and SNR6 (control) are shown. Uninhibited profiles are shown as solid lines and profiles in chemically inhibited cells are shown as dashed lines. TSS and 3′ processing sites are marked by an arrow and a red bar respectively. All x-axes are shown as the distance in base pairs relative to the TSS and y-axes are shown on a log2 scale for ChIP-chip enrichment (IP/input).

(B) Heat maps of 308 protein-coding genes showing Ser7-P and Ser5-P occupancy profiles over a 1kb region centered over the TSS (white bar) for the Kin28as strain with and without inhibition. The change in profiles upon inhibition is shown on the right. Yellow profiles indicate enrichment and blue profiles indicate depletion of the phosphorylated CTD.

In vitro kinase assay detected by dot blot

The substrate, GST-CTD3 (three repeats of YSPTSPS attached to GST), GST-CTD16, GST-CTD4 (and its respective alanine mutants, 2A,5A and 7A) purifications and enzymatic assays were carried out as described previously (Ansari et al., 2005; Patturajan et al., 1998). For inhibition assays, the kinase was pre-incubated for 5 minutes with an inhibitor (6μM of 1-NA-PP1) or synthetic analog of ATP (0.6mM of N⁶-benzyl ATP) prior to the reaction. For the assay, 1:200 dilution of primary rat IgG (αSer2-P or αSer5-P or αSer7-P) and 1:10000 dilution of secondary HRP anti-rat IgG (Southern Biotech) antibodies were used.

In vitro kinase assay detected by ELISA

Recombinant kinase (100ng) was incubated with excess CTD-peptide linked to 96-well plates and phosphorylation of CTD was quantitated via ELISA experiments after incubation with αSer2-P, αSer5-P and αSer7-P specific antibodies (for details see supplementary materials).

We are grateful to J. Rodriguez-Molina and S. Boeing for helpful discussions, A. Flatley and E. Kremmer for technical support and to A. Gasch, A. Kumar, J. Corden, K. Shokat, S. Hahn, P. Fisher and D. Barilla for strains and plasmids. This work was funded by the NSF-CAREER (MCB07147), the W.M. Keck, Shaw Scholar and Vilas associate awards to A. Z. Ansari and grant from the Deutsche Forschungsgemeinschaft (SFB/TR5 and SFB684) to D. Eick. M. Heidemann was funded by Boehringer Ingelheim Fonds travel grant and J. Tietjen was supported by the NHGRI training grant of the Genome Sciences Training program (5T32HG002760).