Asymmetric Arginine Dimethylation of Heterogeneous Nuclear Ribonucleoprotein K by Protein-arginine Methyltransferase 1 Inhibits Its Interaction with c-Src

Ostareck-Lederer, Antje; Ostareck, Dirk H.; Rücknagel, Karl Peter; Schierhorn, Angelika; Moritz, Bodo; Hüttelmaier, Stefan; Flach, Nadine; Handoko, Lusy; Wahle, Elmar

doi:10.1074/jbc.m513053200

Cited by 99 publications

(137 citation statements)

References 74 publications

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“…hnRNP K contains three prolinerich motifs which have been shown to interact with the isolated SH3 domain of the Src kinase family members c-Src, Fyn, and Lyn in vitro (49,53,54). The arginine residues (R256, 258, 268, 296, 299) of hnRNP K, which are located between the prolinerich motifs, are asymmetrically dimethylated by the protein arginine methyltransferase 1 (PRMT1) (40). The methylation of those arginine residues inhibits the activation of c-Src by hnRNP K, suggesting that the proline-rich motifs are important for the activation of c-Src in vitro and in vivo (40).…”

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confidence: 99%

“…The arginine residues (R256, 258, 268, 296, 299) of hnRNP K, which are located between the prolinerich motifs, are asymmetrically dimethylated by the protein arginine methyltransferase 1 (PRMT1) (40). The methylation of those arginine residues inhibits the activation of c-Src by hnRNP K, suggesting that the proline-rich motifs are important for the activation of c-Src in vitro and in vivo (40). Thus, hnRNP K acts as a scaffold protein that integrates signaling cascades by facilitating cross talk between ERK, c-Src, and PRMT1 with factors that mediate mRNA-directed processes.…”

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confidence: 99%

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Deciphering the Cross Talk between hnRNP K and c-Src: the c-Src Activation Domain in hnRNP K Is Distinct from a Second Interaction Site

Adolph

Flach

Mueller

et al. 2007

Molecular and Cellular Biology

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The protein tyrosine kinase c-Src is regulated by two intramolecular interactions. The repressed state is achieved through the interaction of the Src homology 2 (SH2) domain with the phosphorylated C-terminal tail and the association of the SH3 domain with a polyproline type II helix formed by the linker region between SH2 and the kinase domain. hnRNP K, the founding member of the KH domain protein family, is involved in chromatin remodeling, regulation of transcription, and translation of specific mRNAs and is a target in different signal transduction pathways. In particular, it functions as a specific activator and a substrate of the tyrosine kinase c-Src. Here we address the question how hnRNP K interacts with and activates c-Src. We define the proline residues in hnRNP K in the proline-rich motifs P2 (amino acids [aa] 285 to 297) and P3 (aa 303 to 318), which are necessary and sufficient for the specific activation of c-Src, and we dissect the amino acid sequence (aa 216 to 226) of hnRNP K that mediates a second interaction with c-Src. Our findings indicate that the interaction with c-Src and the activation of the kinase are separable functions of hnRNP K. hnRNP K acts as a scaffold protein that integrates signaling cascades by facilitating the cross talk between kinases and factors that mediate nucleic acid-directed processes.

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confidence: 99%

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confidence: 99%

Deciphering the Cross Talk between hnRNP K and c-Src: the c-Src Activation Domain in hnRNP K Is Distinct from a Second Interaction Site

Adolph

Flach

Mueller

et al. 2007

Molecular and Cellular Biology

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“…Coupled with the observation that many PRMT targets have multiple arginines that are methylated (39,40), the diversity of potential protein products is large and suggests the possibility for a methylarginine code. The biological relevance of such a code has most recently been validated as part of the complex set of post-translational histone modifications affecting gene expression (2,6,7).…”

Section: Discussionmentioning

confidence: 99%

Investigation of the Molecular Origins of Protein-arginine Methyltransferase I (PRMT1) Product Specificity Reveals a Role for Two Conserved Methionine Residues

Gui

Wooderchak

Daly

et al. 2011

Journal of Biological Chemistry

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Protein-arginine methyltransferases aid in the regulation of many biological processes by methylating specific arginyl groups within targeted proteins. The varied nature of the response to methylation is due in part to the diverse product specificity displayed by the protein-arginine methyltransferases. In addition to site location within a protein, biological response is also determined by the degree (mono-/dimethylation) and type of arginine dimethylation (asymmetric/symmetric). Here, we have identified two strictly conserved methionine residues in the PRMT1 active site that are not only important for activity but also control substrate specificity. Mutation of Met-155 or Met-48 results in a loss in activity and a change in distribution of mono-and dimethylated products. The altered substrate specificity of M155A and M48L mutants is also evidenced by automethylation. Investigation into the mechanistic basis of altered substrate recognition led us to consider each methyl transfer step separately. Single turnover experiments reveal that the rate of transfer of the second methyl group is much slower than transfer of the first methyl group in M48L, especially for arginine residues located in the center of the peptide substrate where turnover of the monomethylated species is negligible. Thus, altered product specificity in M48L originates from the differential effect of the mutation on the two rates. Characterization of the two active-site methionines provides the first insight into how the PRMT1 active site is engineered to control product specificity.Protein methylation is a significant post-translational modification in eukaryotic organisms. Protein arginine residues can be methylated on the guanidino nitrogens by protein-arginine methyltransferases (PRMTs), 2 which use S-adenosyl-L-methionine (AdoMet) as a methyl group donor. This post-translational modification is important in a wide variety of fundamental biological processes, including transcription, RNA splicing, signal transduction, DNA repair, viral replication (reviewed in Ref. 1), and chromatin remodeling (2). In recent years, the significance of PRMTs in human diseases has been increasingly studied, especially in cardiovascular disease (3) and cancer (4). In all, PRMTs play a crucial role in many biological processes.Although the biological importance of PRMTs has become well accepted, the current knowledge of the fundamental biochemistry of these enzymes is limited, due in part to the complexity of the system. So far, 11 PRMT isoforms have been identified. In mammalian cells, nine PRMTs catalyze monomethyl arginine (MMA) formation, and they can be categorized into two major types as follows: PRMT1, -2-4, -6, and -8 additionally catalyze asymmetric dimethyl arginine (ADMA) formation, demonstrating type I activity; and PRMT5, -7, and -9 catalyze symmetric dimethyl arginine (SDMA) formation, demonstrating type II activity (Fig. 1A). PRMT10 and -11 were identified as putative PRMT genes with no methylation activity shown as yet (5). As with other enzyme f...

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“…8). HnRNPs are known to undergo posttranslational modifications such as phosphorylation [49,50], methylation [51,52], and sumoylation [53]. In the case of hnRNP K, phosphorylation can regulate RNA binding [49].…”

Section: Discussionmentioning

confidence: 99%

Identification of hnRNPs K, L and A2/B1 as candidate proteins involved in the nutritional regulation of mRNA splicing

Griffith¹,

Walsh²,

Szeszel-Fedorowicz³

et al. 2006

Biochimica et Biophysica Acta (BBA) - Gene Structure and Expres

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SummaryNutrient regulation of glucose-6-phosphate dehydrogenase (G6PD) expression occurs through changes in the rate of splicing of G6PD pre-mRNA. This posttranscriptional mechanism accounts for the 12-to 15-fold increase in G6PD expression in livers of mice that were starved and then refed a high-carbohydrate diet. Regulation of G6PD pre-mRNA splicing requires a cis-acting element in exon 12 of the pre-mRNA. Using RNA probes to exon 12 and nuclear extracts from livers of mice that were starved or refed, proteins of 60 kDa and 37 kDa were detected bound to nucleotides 65-79 of exon 12 and this binding was decreased by 50% with nuclear extracts from refed mice. The proteins were identified as hnRNP K, and L, and hnRNP A2/B1 by LC-MS/MS. The decrease in binding of these proteins to exon 12 during refeeding was not accompanied by a decrease in the total amount of these proteins in total nuclear extract. HnRNPs K, L and A2/B1 have known roles in the regulation of mRNA splicing. The decrease in binding of these proteins during treatments that increase G6PD expression is consistent with a role for these proteins in the inhibition of G6PD mRNA splicing.

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Asymmetric Arginine Dimethylation of Heterogeneous Nuclear Ribonucleoprotein K by Protein-arginine Methyltransferase 1 Inhibits Its Interaction with c-Src

Cited by 99 publications

References 74 publications

Deciphering the Cross Talk between hnRNP K and c-Src: the c-Src Activation Domain in hnRNP K Is Distinct from a Second Interaction Site

Deciphering the Cross Talk between hnRNP K and c-Src: the c-Src Activation Domain in hnRNP K Is Distinct from a Second Interaction Site

Investigation of the Molecular Origins of Protein-arginine Methyltransferase I (PRMT1) Product Specificity Reveals a Role for Two Conserved Methionine Residues

Identification of hnRNPs K, L and A2/B1 as candidate proteins involved in the nutritional regulation of mRNA splicing

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