Your search keyword '"Zarnack K"' showing total 89 results

51. iCLIP data analysis: A complete pipeline from sequencing reads to RBP binding sites.

Author

Busch A, Brüggemann M, Ebersberger S, and Zarnack K

Subjects

Binding Sites genetics, Gene Expression Regulation genetics, Humans, Protein Binding genetics, RNA chemistry, RNA genetics, High-Throughput Nucleotide Sequencing methods, Immunoprecipitation methods, RNA isolation & purification

Abstract

Precise knowledge on the binding sites of an RNA-binding protein (RBP) is key to understanding the complex post-transcriptional regulation of gene expression. This information can be obtained from individual-nucleotide resolution UV crosslinking and immunoprecipitation (iCLIP) experiments. Here, we present a complete data analysis workflow to reliably detect RBP binding sites from iCLIP data. The workflow covers all steps from the initial quality control of the sequencing reads up to peak calling and quantification of RBP binding. For each tool, we explain the specific requirements for iCLIP data analysis and suggest optimised parameter settings., (Copyright © 2019 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2020

52. Muscleblind-like 2 controls the hypoxia response of cancer cells.

Author

Fischer S, Di Liddo A, Taylor K, Gerhardus JS, Sobczak K, Zarnack K, and Weigand JE

Subjects

Breast Neoplasms metabolism, Breast Neoplasms pathology, Cell Line, Tumor, Cell Proliferation genetics, Female, Gene Expression Regulation, Neoplastic genetics, Humans, Lung Neoplasms metabolism, Lung Neoplasms pathology, Transcriptome genetics, Breast Neoplasms genetics, Lung Neoplasms genetics, RNA-Binding Proteins genetics, Tumor Hypoxia genetics, Vascular Endothelial Growth Factor A genetics

Abstract

Hypoxia is a hallmark of solid cancers, supporting proliferation, angiogenesis, and escape from apoptosis. There is still limited understanding of how cancer cells adapt to hypoxic conditions and survive. We analyzed transcriptome changes of human lung and breast cancer cells under chronic hypoxia. Hypoxia induced highly concordant changes in transcript abundance, but divergent splicing responses, underlining the cell type-specificity of alternative splicing programs. While RNA-binding proteins were predominantly reduced, hypoxia specifically induced muscleblind-like protein 2 (MBNL2). Strikingly, MBNL2 induction was critical for hypoxia adaptation by controlling the transcript abundance of hypoxia response genes, such as vascular endothelial growth factor A ( VEGFA) MBNL2 depletion reduced the proliferation and migration of cancer cells, demonstrating an important role of MBNL2 as cancer driver. Hypoxia control is specific for MBNL2 and not shared by its paralog MBNL1. Thus, our study revealed MBNL2 as central mediator of cancer cell responses to hypoxia, regulating the expression and alternative splicing of hypoxia-induced genes., (© 2020 Fischer et al.; Published by Cold Spring Harbor Laboratory Press for the RNA Society.)

Published

2020

53. Exon Definition Facilitates Reliable Control of Alternative Splicing in the RON Proto-Oncogene.

Author

Enculescu M, Braun S, Thonta Setty S, Busch A, Zarnack K, König J, and Legewie S

Subjects

Exons genetics, Introns genetics, Alternative Splicing, Proto-Oncogenes

Abstract

Alternative splicing is a key step in eukaryotic gene expression that allows for the production of multiple transcript and protein isoforms from the same gene. Even though splicing is perturbed in many diseases, we currently lack insights into regulatory mechanisms promoting its precision and efficiency. We analyze high-throughput mutagenesis data obtained for an alternatively spliced exon in the proto-oncogene RON and determine the functional units that control this splicing event. Using mathematical modeling of distinct splicing mechanisms, we show that alternative splicing is based in RON on a so-called "exon definition" mechanism. Here, the recognition of the adjacent exons by the spliceosome is required for removal of an intron. We use our model to analyze the differences between the exon and intron definition scenarios and find that exon definition prevents the accumulation of deleterious, partially spliced retention products during alternative splicing regulation. Furthermore, it modularizes splicing control, as multiple regulatory inputs are integrated into a common net input, irrespective of the location and nature of the corresponding cis-regulatory elements in the pre-messenger RNA. Our analysis suggests that exon definition promotes robust and reliable splicing outcomes in RON splicing., (Copyright © 2020 Biophysical Society. Published by Elsevier Inc. All rights reserved.)

Published

2020

54. An autoinhibitory intramolecular interaction proof-reads RNA recognition by the essential splicing factor U2AF2.

Author

Kang HS, Sánchez-Rico C, Ebersberger S, Sutandy FXR, Busch A, Welte T, Stehle R, Hipp C, Schulz L, Buchbender A, Zarnack K, König J, and Sattler M

Subjects

Animals, Cattle, Chromatin Immunoprecipitation methods, Humans, Magnetic Resonance Spectroscopy, Mice, RNA Recognition Motif, Ribonucleoside Diphosphate Reductase metabolism, RNA metabolism, Splicing Factor U2AF metabolism

Abstract

The recognition of cis -regulatory RNA motifs in human transcripts by RNA binding proteins (RBPs) is essential for gene regulation. The molecular features that determine RBP specificity are often poorly understood. Here, we combined NMR structural biology with high-throughput iCLIP approaches to identify a regulatory mechanism for U2AF2 RNA recognition. We found that the intrinsically disordered linker region connecting the two RNA recognition motif (RRM) domains of U2AF2 mediates autoinhibitory intramolecular interactions to reduce nonproductive binding to weak Py-tract RNAs. This proofreading favors binding of U2AF2 at stronger Py-tracts, as required to define 3' splice sites at early stages of spliceosome assembly. Mutations that impair the linker autoinhibition enhance the affinity for weak Py-tracts result in promiscuous binding of U2AF2 along mRNAs and impact on splicing fidelity. Our findings highlight an important role of intrinsically disordered linkers to modulate RNA interactions of multidomain RBPs., Competing Interests: The authors declare no competing interest.

Published

2020

55. Polypyrimidine tract-binding proteins are essential for B cell development.

Author

Monzón-Casanova E, Matheson LS, Tabbada K, Zarnack K, Smith CW, and Turner M

Subjects

Animals, Cell Cycle, Cell Differentiation, Cell Proliferation, Female, Flow Cytometry, Gene Expression Regulation, Heterogeneous-Nuclear Ribonucleoproteins metabolism, Male, Mice, Nerve Tissue Proteins metabolism, Nerve Tissue Proteins physiology, Polypyrimidine Tract-Binding Protein metabolism, RNA-Binding Proteins metabolism, RNA-Binding Proteins physiology, B-Lymphocytes metabolism, Heterogeneous-Nuclear Ribonucleoproteins physiology, Polypyrimidine Tract-Binding Protein physiology

Abstract

Polypyrimidine tract-binding protein 1 (PTBP1) is a RNA-binding protein (RBP) expressed throughout B cell development. Deletion of Ptbp1 in mouse pro-B cells results in upregulation of PTBP2 and normal B cell development. We show that PTBP2 compensates for PTBP1 in B cell ontogeny as deletion of both Ptbp1 and Ptbp2 results in a complete block at the pro-B cell stage and a lack of mature B cells. In pro-B cells PTBP1 ensures precise synchronisation of the activity of cyclin dependent kinases at distinct stages of the cell cycle, suppresses S-phase entry and promotes progression into mitosis. PTBP1 controls mRNA abundance and alternative splicing of important cell cycle regulators including CYCLIN-D2, c-MYC, p107 and CDC25B. Our results reveal a previously unrecognised mechanism mediated by a RBP that is essential for B cell ontogeny and integrates transcriptional and post-translational determinants of progression through the cell cycle., Competing Interests: EM, LM, KT, KZ, CS, MT No competing interests declared, (© 2020, Monzón-Casanova et al.)

Published

2020

56. Makorin 1 controls embryonic patterning by alleviating Bruno1-mediated repression of oskar translation.

Author

Dold A, Han H, Liu N, Hildebrandt A, Brüggemann M, Rücklé C, Hänel H, Busch A, Beli P, Zarnack K, König J, Roignant JY, and Lasko P

Subjects

3' Untranslated Regions, Animals, Cell Line, Drosophila Proteins genetics, Drosophila melanogaster, Female, Gene Expression Regulation, Developmental, Humans, Intracellular Signaling Peptides and Proteins genetics, Ovary metabolism, Protein Binding, Body Patterning, Drosophila Proteins metabolism, Intracellular Signaling Peptides and Proteins metabolism, RNA-Binding Proteins metabolism

Abstract

Makorins are evolutionary conserved proteins that contain C3H-type zinc finger modules and a RING E3 ubiquitin ligase domain. In Drosophila, maternal Makorin 1 (Mkrn1) has been linked to embryonic patterning but the mechanism remained unsolved. Here, we show that Mkrn1 is essential for axis specification and pole plasm assembly by translational activation of oskar (osk). We demonstrate that Mkrn1 interacts with poly(A) binding protein (pAbp) and binds specifically to osk 3' UTR in a region adjacent to A-rich sequences. Using Drosophila S2R+ cultured cells we show that this binding site overlaps with a Bruno1 (Bru1) responsive element (BREs) that regulates osk translation. We observe increased association of the translational repressor Bru1 with osk mRNA upon depletion of Mkrn1, indicating that both proteins compete for osk binding. Consistently, reducing Bru1 dosage partially rescues viability and Osk protein level in ovaries from Mkrn1 females. We conclude that Mkrn1 controls embryonic patterning and germ cell formation by specifically activating osk translation, most likely by competing with Bru1 to bind to osk 3' UTR., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

57. A combined computational pipeline to detect circular RNAs in human cancer cells under hypoxic stress.

Author

Di Liddo A, de Oliveira Freitas Machado C, Fischer S, Ebersberger S, Heumüller AW, Weigand JE, Müller-McNicoll M, and Zarnack K

Subjects

A549 Cells, Cell Hypoxia genetics, Cell Line, Tumor, Computational Biology, Exons genetics, HeLa Cells, Humans, Introns genetics, MCF-7 Cells, MicroRNAs genetics, RNA-Seq, Cell Hypoxia physiology, RNA, Circular genetics

Abstract

Hypoxia is associated with several diseases, including cancer. Cells that are deprived of adequate oxygen supply trigger transcriptional and post-transcriptional responses, which control cellular pathways such as angiogenesis, proliferation, and metabolic adaptation. Circular RNAs (circRNAs) are a novel class of mainly non-coding RNAs, which have been implicated in multiple cancers and attract increasing attention as potential biomarkers. Here, we characterize the circRNA signatures of three different cancer cell lines from cervical (HeLa), breast (MCF-7), and lung (A549) cancer under hypoxia. In order to reliably detect circRNAs, we integrate available tools with custom approaches for quantification and statistical analysis. Using this consolidated computational pipeline, we identify ~12000 circRNAs in the three cancer cell lines. Their molecular characteristics point to an involvement of complementary RNA sequences as well as trans-acting factors in circRNA biogenesis, such as the RNA-binding protein HNRNPC. Notably, we detect a number of circRNAs that are more abundant than their linear counterparts. In addition, 64 circRNAs significantly change in abundance upon hypoxia, in most cases in a cell type-specific manner. In summary, we present a comparative circRNA profiling in human cancer cell lines, which promises novel insights into the biogenesis and function of circRNAs under hypoxic stress., (© The Author(s) (2019). Published by Oxford University Press on behalf of Journal of Molecular Cell Biology, IBCB, SIBS, CAS.)

Published

2019

58. The RNA-binding ubiquitin ligase MKRN1 functions in ribosome-associated quality control of poly(A) translation.

Author

Hildebrandt A, Brüggemann M, Rücklé C, Boerner S, Heidelberger JB, Busch A, Hänel H, Voigt A, Möckel MM, Ebersberger S, Scholz A, Dold A, Schmid T, Ebersberger I, Roignant JY, Zarnack K, König J, and Beli P

Subjects

3' Untranslated Regions, HEK293 Cells, Humans, Poly(A)-Binding Protein I metabolism, RNA, Messenger metabolism, Ubiquitination, Nerve Tissue Proteins metabolism, Protein Biosynthesis, Ribonucleoproteins metabolism

Abstract

Background: Cells have evolved quality control mechanisms to ensure protein homeostasis by detecting and degrading aberrant mRNAs and proteins. A common source of aberrant mRNAs is premature polyadenylation, which can result in non-functional protein products. Translating ribosomes that encounter poly(A) sequences are terminally stalled, followed by ribosome recycling and decay of the truncated nascent polypeptide via ribosome-associated quality control., Results: Here, we demonstrate that the conserved RNA-binding E3 ubiquitin ligase Makorin Ring Finger Protein 1 (MKRN1) promotes ribosome stalling at poly(A) sequences during ribosome-associated quality control. We show that MKRN1 directly binds to the cytoplasmic poly(A)-binding protein (PABPC1) and associates with polysomes. MKRN1 is positioned upstream of poly(A) tails in mRNAs in a PABPC1-dependent manner. Ubiquitin remnant profiling and in vitro ubiquitylation assays uncover PABPC1 and ribosomal protein RPS10 as direct ubiquitylation substrates of MKRN1., Conclusions: We propose that MKRN1 mediates the recognition of poly(A) tails to prevent the production of erroneous proteins from prematurely polyadenylated transcripts, thereby maintaining proteome integrity.

Published

2019

59. uORF-Tools-Workflow for the determination of translation-regulatory upstream open reading frames.

Author

Scholz A, Eggenhofer F, Gelhausen R, Grüning B, Zarnack K, Brüne B, Backofen R, and Schmid T

Subjects

5' Untranslated Regions, Gene Expression Regulation, Humans, Protein Biosynthesis, Protein Processing, Post-Translational, RNA, Messenger, Software, Workflow, Gene Expression Profiling methods, Open Reading Frames genetics, Ribosomes genetics

Abstract

Ribosome profiling (ribo-seq) provides a means to analyze active translation by determining ribosome occupancy in a transcriptome-wide manner. The vast majority of ribosome protected fragments (RPFs) resides within the protein-coding sequence of mRNAs. However, commonly reads are also found within the transcript leader sequence (TLS) (aka 5' untranslated region) preceding the main open reading frame (ORF), indicating the translation of regulatory upstream ORFs (uORFs). Here, we present a workflow for the identification of translation-regulatory uORFs. Specifically, uORF-Tools uses Ribo-TISH to identify uORFs within a given dataset and generates a uORF annotation file. In addition, a comprehensive human uORF annotation file, based on 35 ribo-seq files, is provided, which can serve as an alternative input file for the workflow. To assess the translation-regulatory activity of the uORFs, stimulus-induced changes in the ratio of the RPFs residing in the main ORFs relative to those found in the associated uORFs are determined. The resulting output file allows for the easy identification of candidate uORFs, which have translation-inhibitory effects on their associated main ORFs. uORF-Tools is available as a free and open Snakemake workflow at https://github.com/Biochemistry1-FFM/uORF-Tools. It is easily installed and all necessary tools are provided in a version-controlled manner, which also ensures lasting usability. uORF-Tools is designed for intuitive use and requires only limited computing times and resources., Competing Interests: The authors have declared that no competing interests exist.

Published

2019

60. Phenotypic Plasticity of Fibroblasts during Mammary Carcinoma Development.

Author

Elwakeel E, Brüggemann M, Fink AF, Schulz MH, Schmid T, Savai R, Brüne B, Zarnack K, and Weigert A

Subjects

Animals, Female, Fibroblasts pathology, Mammary Glands, Animal pathology, Mammary Neoplasms, Animal genetics, Mammary Neoplasms, Animal pathology, Mice, Mice, Transgenic, Fibroblasts metabolism, Gene Expression Regulation, Neoplastic, Mammary Glands, Animal metabolism, Mammary Neoplasms, Animal metabolism, Transcription, Genetic

Abstract

: Cancer-associated fibroblasts (CAFs) in the tumor microenvironment contribute to all stages of tumorigenesis and are usually considered to be tumor-promoting cells. CAFs show a remarkable degree of heterogeneity, which is attributed to developmental origin or to local environmental niches, resulting in distinct CAF subsets within individual tumors. While CAF heterogeneity is frequently investigated in late-stage tumors, data on longitudinal CAF development in tumors are lacking. To this end, we used the transgenic polyoma middle T oncogene-induced mouse mammary carcinoma model and performed whole transcriptome analysis in FACS-sorted fibroblasts from early- and late-stage tumors. We observed a shift in fibroblast populations over time towards a subset previously shown to negatively correlate with patient survival, which was confirmed by multispectral immunofluorescence analysis. Moreover, we identified a transcriptomic signature distinguishing CAFs from early- and late-stage tumors. Importantly, the signature of early-stage CAFs correlated well with tumor stage and survival in human mammary carcinoma patients. A random forest analysis suggested predictive value of the complete set of differentially expressed genes between early- and late-stage CAFs on bulk tumor patient samples, supporting the clinical relevance of our findings. In conclusion, our data show transcriptome alterations in CAFs during tumorigenesis in the mammary gland, which suggest that CAFs are educated by the tumor over time to promote tumor development. Moreover, we show that murine CAF gene signatures can harbor predictive value for human cancer., Competing Interests: Funding: This research was funded by Deutsche Forschungsgemeinschaft (SFB 1039 TP B04 and B06; FOR 2438), Deutsche Krebshilfe (70112451), and Else Kröner Fresenius-Foundation (Graduate school Translational Research Innovation—Pharma (TRIP) and Else Kröner Fresenius Graduate School). The APC was funded by the ‘Open-Access-Publikationsfonds’ of Goethe-University Frankfurt.

Published

2019

61. Membrane-Associated RNA-Binding Proteins Orchestrate Organelle-Coupled Translation.

Author

Béthune J, Jansen RP, Feldbrügge M, and Zarnack K

Subjects

Animals, Humans, Protein Transport, RNA, Messenger genetics, RNA, Messenger metabolism, Endoplasmic Reticulum metabolism, Endosomes metabolism, Membrane Proteins metabolism, Mitochondria metabolism, Protein Biosynthesis, RNA-Binding Proteins metabolism

Abstract

Proteins are positioned and act at defined subcellular locations. This is particularly important in eukaryotic cells that deliver proteins to membrane-bound organelles such as the endoplasmic reticulum (ER), mitochondria, or endosomes. It is axiomatic that organelle targeting depends mainly on polypeptide signals. However, recent results demonstrate that targeting elements within the encoding transcripts are essential for efficient protein localisation. Key readers of these elements are membrane-associated RNA-binding proteins (memRBPs) that orchestrate organelle-coupled translation. The translation products then either cross the membrane for organelle entry or hitchhike on organelle surfaces for complex assembly and co-transport. Understanding the interaction of protein- and RNA-based targeting signals is essential to decipher the molecular basis for mutant phenotypes in disease., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2019

62. The key protein of endosomal mRNP transport Rrm4 binds translational landmark sites of cargo mRNAs.

Author

Olgeiser L, Haag C, Boerner S, Ule J, Busch A, Koepke J, König J, Feldbrügge M, and Zarnack K

Subjects

Binding Sites, Biological Transport genetics, Endosomes genetics, Gene Expression Regulation, Microtubules genetics, RNA Transport genetics, RNA, Messenger genetics, Transcriptome genetics, Fungal Proteins genetics, RNA-Binding Proteins genetics, Ribonucleoproteins genetics, Ustilago genetics

Abstract

RNA-binding proteins (RBPs) determine spatiotemporal gene expression by mediating active transport and local translation of cargo mRNAs. Here, we cast a transcriptome-wide view on the transported mRNAs and cognate RBP binding sites during endosomal messenger ribonucleoprotein (mRNP) transport in Ustilago maydis Using individual-nucleotide resolution UV crosslinking and immunoprecipitation (iCLIP), we compare the key transport RBP Rrm4 and the newly identified endosomal mRNP component Grp1 that is crucial to coordinate hyphal growth. Both RBPs bind predominantly in the 3' untranslated region of thousands of shared cargo mRNAs, often in close proximity. Intriguingly, Rrm4 precisely binds at stop codons, which constitute landmark sites of translation, suggesting an intimate connection of mRNA transport and translation. Towards uncovering the code of recognition, we identify UAUG as specific binding motif of Rrm4 that is bound by its third RRM domain. Altogether, we provide first insights into the positional organisation of co-localising RBPs on individual cargo mRNAs., (© 2018 The Authors.)

Published

2019

63. Decoding a cancer-relevant splicing decision in the RON proto-oncogene using high-throughput mutagenesis.

Author

Braun S, Enculescu M, Setty ST, Cortés-López M, de Almeida BP, Sutandy FXR, Schulz L, Busch A, Seiler M, Ebersberger S, Barbosa-Morais NL, Legewie S, König J, and Zarnack K

Subjects

Base Sequence, Binding Sites, Exons genetics, HEK293 Cells, Heterogeneous-Nuclear Ribonucleoprotein Group F-H metabolism, Humans, Introns genetics, Linear Models, MCF-7 Cells, Mutation genetics, Proto-Oncogene Mas, RNA-Binding Proteins metabolism, Regulatory Sequences, Nucleic Acid genetics, Sequence Analysis, RNA, Alternative Splicing genetics, Mutagenesis genetics, Neoplasms genetics, Receptor Protein-Tyrosine Kinases genetics

Abstract

Mutations causing aberrant splicing are frequently implicated in human diseases including cancer. Here, we establish a high-throughput screen of randomly mutated minigenes to decode the cis-regulatory landscape that determines alternative splicing of exon 11 in the proto-oncogene MST1R (RON). Mathematical modelling of splicing kinetics enables us to identify more than 1000 mutations affecting RON exon 11 skipping, which corresponds to the pathological isoform RON∆165. Importantly, the effects correlate with RON alternative splicing in cancer patients bearing the same mutations. Moreover, we highlight heterogeneous nuclear ribonucleoprotein H (HNRNPH) as a key regulator of RON splicing in healthy tissues and cancer. Using iCLIP and synergy analysis, we pinpoint the functionally most relevant HNRNPH binding sites and demonstrate how cooperative HNRNPH binding facilitates a splicing switch of RON exon 11. Our results thereby offer insights into splicing regulation and the impact of mutations on alternative splicing in cancer.

Published

2018

64. High-Throughput Screens for cis-Acting RNA Sequence Elements That Promote Nuclear Retention.

Author

Zarnack K and Müller-McNicoll M

Subjects

Animals, Base Sequence, Binding Sites, Cell Nucleus chemistry, Humans, Nucleic Acid Conformation, RNA chemistry, RNA Transport, RNA-Binding Proteins chemistry, RNA-Binding Proteins metabolism, Regulatory Sequences, Ribonucleic Acid, Cell Nucleus metabolism, RNA metabolism

Published

2018

65. In vitro iCLIP-based modeling uncovers how the splicing factor U2AF2 relies on regulation by cofactors.

Author

Sutandy FXR, Ebersberger S, Huang L, Busch A, Bach M, Kang HS, Fallmann J, Maticzka D, Backofen R, Stadler PF, Zarnack K, Sattler M, Legewie S, and König J

Subjects

Binding Sites genetics, HeLa Cells, Humans, Introns genetics, Models, Genetic, RNA Precursors genetics, RNA Splicing Factors genetics, RNA Splicing Factors metabolism, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, Spliceosomes metabolism, Splicing Factor U2AF metabolism, RNA Splice Sites genetics, RNA Splicing, Spliceosomes genetics, Splicing Factor U2AF genetics

Abstract

Alternative splicing generates distinct mRNA isoforms and is crucial for proteome diversity in eukaryotes. The RNA-binding protein (RBP) U2AF2 is central to splicing decisions, as it recognizes 3' splice sites and recruits the spliceosome. We establish "in vitro iCLIP" experiments, in which recombinant RBPs are incubated with long transcripts, to study how U2AF2 recognizes RNA sequences and how this is modulated by trans -acting RBPs. We measure U2AF2 affinities at hundreds of binding sites and compare in vitro and in vivo binding landscapes by mathematical modeling. We find that trans -acting RBPs extensively regulate U2AF2 binding in vivo, including enhanced recruitment to 3' splice sites and clearance of introns. Using machine learning, we identify and experimentally validate novel trans -acting RBPs (including FUBP1, CELF6, and PCBP1) that modulate U2AF2 binding and affect splicing outcomes. Our study offers a blueprint for the high-throughput characterization of in vitro mRNP assembly and in vivo splicing regulation., (© 2018 Sutandy et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2018

66. Interaction profiling of RNA-binding ubiquitin ligases reveals a link between posttranscriptional regulation and the ubiquitin system.

Author

Hildebrandt A, Alanis-Lobato G, Voigt A, Zarnack K, Andrade-Navarro MA, Beli P, and König J

Subjects

Humans, Mass Spectrometry, Protein Binding, Protein Interaction Mapping, RNA-Binding Proteins metabolism, Ubiquitin metabolism, Ubiquitinated Proteins metabolism, Ubiquitination, Proteomics methods, Ubiquitin-Protein Ligases metabolism

Abstract

RNA-binding ubiquitin ligases (RBULs) have the potential to link RNA-mediated mechanisms to protein ubiquitylation. Despite this, the cellular functions, substrates and interaction partners of most RBULs remain poorly characterized. Affinity purification (AP) combined with quantitative mass spectrometry (MS)-based proteomics is a powerful approach for analyzing protein functions. Mapping the physiological interaction partners of RNA-binding proteins has been hampered by their intrinsic properties, in particular the existence of low-complexity regions, which are prone to engage in non-physiological interactions. Here, we used an adapted AP approach to identify the interaction partners of human RBULs harboring different RNA-binding domains. To increase the likelihood of recovering physiological interactions, we combined control and bait-expressing cells prior to lysis. In this setup, only stable interactions that were originally present in the cell will be identified. We exploit gene function similarity between the bait proteins and their interactors to benchmark our approach in its ability to recover physiological interactions. We reveal that RBULs engage in stable interactions with RNA-binding proteins involved in different steps of RNA metabolism as well as with components of the ubiquitin conjugation machinery and ubiquitin-binding proteins. Our results thus demonstrate their capacity to link posttranscriptional regulation with the ubiquitin system.

Published

2017

67. Erratum to: Insights into the design and interpretation of iCLIP experiments.

Author

Haberman N, Huppertz I, Attig J, König J, Wang Z, Hauer C, Hentze MW, Kulozik AE, Le Hir H, Curk T, Sibley CR, Zarnack K, and Ule J

Published

2017

68. Cellular differentiation state modulates the mRNA export activity of SR proteins.

Author

Botti V, McNicoll F, Steiner MC, Richter FM, Solovyeva A, Wegener M, Schwich OD, Poser I, Zarnack K, Wittig I, Neugebauer KM, and Müller-McNicoll M

Subjects

Active Transport, Cell Nucleus, Animals, Arginine, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, HeLa Cells, Humans, Immunoprecipitation, Methylation, Mice, Neurogenesis, Phenotype, Phosphorylation, Protein Binding, Protein Processing, Post-Translational, RNA Interference, RNA, Messenger genetics, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, Repressor Proteins genetics, Repressor Proteins metabolism, Serine-Arginine Splicing Factors genetics, Tandem Mass Spectrometry, Transcription Factors genetics, Transcription Factors metabolism, Transfection, Cell Differentiation, Cell Nucleus metabolism, Pluripotent Stem Cells metabolism, RNA, Messenger metabolism, Serine-Arginine Splicing Factors metabolism

Abstract

SR proteins function in nuclear pre-mRNA processing, mRNA export, and translation. To investigate their cellular dynamics, we developed a quantitative assay, which detects differences in nucleocytoplasmic shuttling among seven canonical SR protein family members. As expected, SRSF2 and SRSF5 shuttle poorly in HeLa cells but surprisingly display considerable shuttling in pluripotent murine P19 cells. Combining individual-resolution cross-linking and immunoprecipitation (iCLIP) and mass spectrometry, we show that elevated arginine methylation of SRSF5 and lower phosphorylation levels of cobound SRSF2 enhance shuttling of SRSF5 in P19 cells by modulating protein-protein and protein-RNA interactions. Moreover, SRSF5 is bound to pluripotency-specific transcripts such as Lin28a and Pou5f1/Oct4 in the cytoplasm. SRSF5 depletion reduces and overexpression increases their cytoplasmic mRNA levels, suggesting that enhanced mRNA export by SRSF5 is required for the expression of pluripotency factors. Remarkably, neural differentiation of P19 cells leads to dramatically reduced SRSF5 shuttling. Our findings indicate that posttranslational modification of SR proteins underlies the regulation of their mRNA export activities and distinguishes pluripotent from differentiated cells., (© 2017 Botti et al.)

Published

2017

69. Differential Binding of Mitochondrial Transcripts by MRB8170 and MRB4160 Regulates Distinct Editing Fates of Mitochondrial mRNA in Trypanosomes.

Author

Dixit S, Müller-McNicoll M, David V, Zarnack K, Ule J, Hashimi H, and Lukeš J

Subjects

Protein Binding, Mitochondria metabolism, Protozoan Proteins metabolism, RNA Editing, RNA Precursors metabolism, Trypanosoma brucei brucei metabolism

Abstract

A dozen mRNAs are edited by multiple insertions and/or deletions of uridine residues in the mitochondrion of Trypanosoma brucei Several protein complexes have been implicated in performing this type of RNA editing, including the mitochondrial RNA-binding complex 1 (MRB1). Two paralogous novel RNA-binding proteins, MRB8170 and MRB4160, are loosely associated with the core MRB1 complex. Their roles in RNA editing and effects on target mRNAs are so far not well understood. In this study, individual-nucleotide-resolution UV-cross-linking and affinity purification (iCLAP) revealed a preferential binding of both proteins to mitochondrial mRNAs, which was positively correlated with their extent of editing. Integrating additional in vivo and in vitro data, we propose that binding of MRB8170 and/or MRB4160 onto pre-mRNA marks it for the initiation of editing and that initial binding of both proteins may facilitate the recruitment of other components of the RNA editing/processing machinery to ensure efficient editing. Surprisingly, MRB8170 also binds never-edited mRNAs, suggesting that at least this paralog has an additional role outside RNA editing to shape the mitochondrial transcriptome., Importance: Trypanosoma brucei mitochondrial mRNAs undergo maturation by RNA editing, a unique process involving decrypting open reading frames by the precise deletion and/or insertion of uridine (U) residues at specific positions on an mRNA. This process is catalyzed by multiprotein complexes, such as the RNA editing core complex, which provides the enzymatic activities needed for U insertion/deletion at a single editing site. Less well understood is how RNA editing occurs throughout an mRNA bearing multiple sites. To address this question, we mapped at single-nucleotide resolution the RNA interactions of two unique RNA-binding proteins (RBPs). These RBPs are part of the mitochondrial RNA-binding complex 1, hypothesized to mediate multiple rounds of RNA editing. Both RBPs were shown to mark mRNAs for the process in correlation with the number of editing sites on the transcript. Surprisingly, one also binds mRNAs that bypass RNA editing, indicating that it may have an additional role outside RNA editing., (Copyright © 2017 Dixit et al.)

Published

2017

70. Insights into the design and interpretation of iCLIP experiments.

Author

Haberman N, Huppertz I, Attig J, König J, Wang Z, Hauer C, Hentze MW, Kulozik AE, Le Hir H, Curk T, Sibley CR, Zarnack K, and Ule J

Subjects

Binding Sites, Computational Biology methods, DNA, Complementary genetics, DNA, Complementary metabolism, Exons, Heterogeneous-Nuclear Ribonucleoproteins metabolism, Humans, Introns, Nucleotide Motifs, Protein Binding, Ribonuclease, Pancreatic metabolism, Ultraviolet Rays, Immunoprecipitation methods, RNA genetics, RNA metabolism, RNA-Binding Proteins metabolism

Abstract

Background: Ultraviolet (UV) crosslinking and immunoprecipitation (CLIP) identifies the sites on RNAs that are in direct contact with RNA-binding proteins (RBPs). Several variants of CLIP exist, which require different computational approaches for analysis. This variety of approaches can create challenges for a novice user and can hamper insights from multi-study comparisons. Here, we produce data with multiple variants of CLIP and evaluate the data with various computational methods to better understand their suitability., Results: We perform experiments for PTBP1 and eIF4A3 using individual-nucleotide resolution CLIP (iCLIP), employing either UV-C or photoactivatable 4-thiouridine (4SU) combined with UV-A crosslinking and compare the results with published data. As previously noted, the positions of complementary DNA (cDNA)-starts depend on cDNA length in several iCLIP experiments and we now find that this is caused by constrained cDNA-ends, which can result from the sequence and structure constraints of RNA fragmentation. These constraints are overcome when fragmentation by RNase I is efficient and when a broad cDNA size range is obtained. Our study also shows that if RNase does not efficiently cut within the binding sites, the original CLIP method is less capable of identifying the longer binding sites of RBPs. In contrast, we show that a broad size range of cDNAs in iCLIP allows the cDNA-starts to efficiently delineate the complete RNA-binding sites., Conclusions: We demonstrate the advantage of iCLIP and related methods that can amplify cDNAs that truncate at crosslink sites and we show that computational analyses based on cDNAs-starts are appropriate for such methods.

Published

2017

71. Splicing repression allows the gradual emergence of new Alu-exons in primate evolution.

Author

Attig J, Ruiz de Los Mozos I, Haberman N, Wang Z, Emmett W, Zarnack K, König J, and Ule J

Subjects

HEK293 Cells, Heterogeneous-Nuclear Ribonucleoprotein Group C metabolism, Humans, Nonsense Mediated mRNA Decay, Alu Elements, Evolution, Molecular, Exons, RNA Splicing

Abstract

Alu elements are retrotransposons that frequently form new exons during primate evolution. Here, we assess the interplay of splicing repression by hnRNPC and nonsense-mediated mRNA decay (NMD) in the quality control and evolution of new Alu-exons. We identify 3100 new Alu-exons and show that NMD more efficiently recognises transcripts with Alu-exons compared to other exons with premature termination codons. However, some Alu-exons escape NMD, especially when an adjacent intron is retained, highlighting the importance of concerted repression by splicing and NMD. We show that evolutionary progression of 3' splice sites is coupled with longer repressive uridine tracts. Once the 3' splice site at ancient Alu-exons reaches a stable phase, splicing repression by hnRNPC decreases, but the exons generally remain sensitive to NMD. We conclude that repressive motifs are strongest next to cryptic exons and that gradual weakening of these motifs contributes to the evolutionary emergence of new alternative exons., Competing Interests: The authors declare that no competing interests exist.

Published

2016

72. SR proteins are NXF1 adaptors that link alternative RNA processing to mRNA export.

Author

Müller-McNicoll M, Botti V, de Jesus Domingues AM, Brandl H, Schwich OD, Steiner MC, Curk T, Poser I, Zarnack K, and Neugebauer KM

Subjects

3' Untranslated Regions, Active Transport, Cell Nucleus genetics, Animals, Cell Line, Mice, Nuclear Proteins metabolism, Protein Binding, Reproducibility of Results, Ribonucleoproteins metabolism, Serine-Arginine Splicing Factors, Alternative Splicing genetics, Nucleocytoplasmic Transport Proteins metabolism, RNA, Messenger metabolism, RNA-Binding Proteins metabolism

Abstract

Nuclear export factor 1 (NXF1) exports mRNA to the cytoplasm after recruitment to mRNA by specific adaptor proteins. How and why cells use numerous different export adaptors is poorly understood. Here we critically evaluate members of the SR protein family (SRSF1-7) for their potential to act as NXF1 adaptors that couple pre-mRNA processing to mRNA export. Consistent with this proposal, >1000 endogenous mRNAs required individual SR proteins for nuclear export in vivo. To address the mechanism, transcriptome-wide RNA-binding profiles of NXF1 and SRSF1-7 were determined in parallel by individual-nucleotide-resolution UV cross-linking and immunoprecipitation (iCLIP). Quantitative comparisons of RNA-binding sites showed that NXF1 and SR proteins bind mRNA targets at adjacent sites, indicative of cobinding. SRSF3 emerged as the most potent NXF1 adaptor, conferring sequence specificity to RNA binding by NXF1 in last exons. Interestingly, SRSF3 and SRSF7 were shown to bind different sites in last exons and regulate 3' untranslated region length in an opposing manner. Both SRSF3 and SRSF7 promoted NXF1 recruitment to mRNA. Thus, SRSF3 and SRSF7 couple alternative splicing and polyadenylation to NXF1-mediated mRNA export, thereby controlling the cytoplasmic abundance of transcripts with alternative 3' ends., (© 2016 Müller-McNicoll et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2016

73. Recognition of distinct RNA motifs by the clustered CCCH zinc fingers of neuronal protein Unkempt.

Author

Murn J, Teplova M, Zarnack K, Shi Y, and Patel DJ

Subjects

Animals, Crystallography, X-Ray, Mice, Models, Molecular, Protein Binding, Protein Conformation, Carrier Proteins chemistry, Carrier Proteins metabolism, Nucleotide Motifs, RNA metabolism, RNA-Binding Proteins metabolism, Zinc Fingers

Abstract

Unkempt is an evolutionarily conserved RNA-binding protein that regulates translation of its target genes and is required for the establishment of the early bipolar neuronal morphology. Here we determined the X-ray crystal structure of mouse Unkempt and show that its six CCCH zinc fingers (ZnFs) form two compact clusters, ZnF1-3 and ZnF4-6, that recognize distinct trinucleotide RNA substrates. Both ZnF clusters adopt a similar overall topology and use distinct recognition principles to target specific RNA sequences. Structure-guided point mutations reduce the RNA binding affinity of Unkempt both in vitro and in vivo, ablate Unkempt's translational control and impair the ability of Unkempt to induce a bipolar cellular morphology. Our study unravels a new mode of RNA sequence recognition by clusters of CCCH ZnFs that is critical for post-transcriptional control of neuronal morphology.

Published

2016

74. Intergenic Alu exonisation facilitates the evolution of tissue-specific transcript ends.

Author

Tajnik M, Vigilante A, Braun S, Hänel H, Luscombe NM, Ule J, Zarnack K, and König J

Subjects

Cell Line, DNA metabolism, DNA, Intergenic chemistry, Heterogeneous-Nuclear Ribonucleoprotein Group C metabolism, Humans, Introns, Nuclear Proteins metabolism, Organ Specificity, Polyadenylation, Protein Isoforms genetics, Protein Isoforms metabolism, RNA metabolism, RNA Splicing, Ribonucleoproteins metabolism, Splicing Factor U2AF, 3' Untranslated Regions, Alu Elements, Evolution, Molecular, Exons

Abstract

The 3' untranslated regions (3' UTRs) of transcripts serve as important hubs for posttranscriptional gene expression regulation. Here, we find that the exonisation of intergenic Alu elements introduced new terminal exons and polyadenylation sites during human genome evolution. While Alu exonisation from introns has been described previously, we shed light on a novel mechanism to create alternative 3' UTRs, thereby opening opportunities for differential posttranscriptional regulation. On the mechanistic level, we show that intergenic Alu exonisation can compete both with alternative splicing and polyadenylation in the upstream gene. Notably, the Alu-derived isoforms are often expressed in a tissue-specific manner, and the Alu-derived 3' UTRs can alter mRNA stability. In summary, we demonstrate that intergenic elements can affect processing of preceding genes, and elucidate how intergenic Alu exonisation can contribute to tissue-specific posttranscriptional regulation by expanding the repertoire of 3' UTRs., (© The Author(s) 2015. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2015

75. The RNA-binding protein HuR is essential for the B cell antibody response.

Author

Diaz-Muñoz MD, Bell SE, Fairfax K, Monzon-Casanova E, Cunningham AF, Gonzalez-Porta M, Andrews SR, Bunik VI, Zarnack K, Curk T, Heggermont WA, Heymans S, Gibson GE, Kontoyiannis DL, Ule J, and Turner M

Subjects

Acyltransferases genetics, Acyltransferases immunology, Alternative Splicing immunology, Animals, Antigens administration & dosage, Antigens immunology, B-Lymphocytes cytology, B-Lymphocytes drug effects, Cell Death, Cell Differentiation, Cell Proliferation, ELAV Proteins genetics, Erythrocytes immunology, Germinal Center cytology, Germinal Center drug effects, Immunization, Immunoglobulin Class Switching, Lipopolysaccharides pharmacology, Mice, Mice, Inbred C57BL, Mice, Knockout, Mitochondria genetics, Mitochondria immunology, RNA, Messenger genetics, Reactive Oxygen Species immunology, Reactive Oxygen Species metabolism, Sheep, B-Lymphocytes immunology, ELAV Proteins immunology, Germinal Center immunology, Immunity, Humoral, Immunoglobulins biosynthesis, RNA, Messenger immunology

Abstract

Post-transcriptional regulation of mRNA by the RNA-binding protein HuR (encoded by Elavl1) is required in B cells for the germinal center reaction and for the production of class-switched antibodies in response to thymus-independent antigens. Transcriptome-wide examination of RNA isoforms and their abundance and translation in HuR-deficient B cells, together with direct measurements of HuR-RNA interactions, revealed that HuR-dependent splicing of mRNA affected hundreds of transcripts, including that encoding dihydrolipoamide S-succinyltransferase (Dlst), a subunit of the 2-oxoglutarate dehydrogenase (α-KGDH) complex. In the absence of HuR, defective mitochondrial metabolism resulted in large amounts of reactive oxygen species and B cell death. Our study shows how post-transcriptional processes control the balance of energy metabolism required for the proliferation and differentiation of B cells.

Published

2015

76. Control of a neuronal morphology program by an RNA-binding zinc finger protein, Unkempt.

Author

Murn J, Zarnack K, Yang YJ, Durak O, Murphy EA, Cheloufi S, Gonzalez DM, Teplova M, Curk T, Zuber J, Patel DJ, Ule J, Luscombe NM, Tsai LH, Walsh CA, and Shi Y

Subjects

Animals, Brain metabolism, Cell Line, Embryo, Mammalian, Gene Expression Profiling, HeLa Cells, Humans, Mice, Protein Binding, RNA, Messenger, Cell Shape genetics, Gene Expression Regulation, Developmental, Neurons cytology

Abstract

Cellular morphology is an essential determinant of cellular function in all kingdoms of life, yet little is known about how cell shape is controlled. Here we describe a molecular program that controls the early morphology of neurons through a metazoan-specific zinc finger protein, Unkempt. Depletion of Unkempt in mouse embryos disrupts the shape of migrating neurons, while ectopic expression confers neuronal-like morphology to cells of different nonneuronal lineages. We found that Unkempt is a sequence-specific RNA-binding protein and identified its precise binding sites within coding regions of mRNAs linked to protein metabolism and trafficking. RNA binding is required for Unkempt-induced remodeling of cellular shape and is directly coupled to a reduced production of the encoded proteins. These findings link post-transcriptional regulation of gene expression with cellular shape and have general implications for the development and disease of multicellular organisms., (© 2015 Murn et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2015

77. Direct competition between hnRNP C and U2AF65 protects the transcriptome from the exonization of Alu elements.

Author

Zarnack K, König J, Tajnik M, Martincorena I, Eustermann S, Stévant I, Reyes A, Anders S, Luscombe NM, and Ule J

Subjects

Evolution, Molecular, Exons, Gene Expression Profiling, Gene Knockdown Techniques, HeLa Cells, Heterogeneous-Nuclear Ribonucleoprotein Group C genetics, High-Throughput Nucleotide Sequencing, Humans, Immunoprecipitation, RNA Splice Sites, Sequence Analysis, RNA, Splicing Factor U2AF, Alu Elements, Heterogeneous-Nuclear Ribonucleoprotein Group C metabolism, Nuclear Proteins metabolism, Ribonucleoproteins metabolism, Transcriptome

Abstract

There are ~650,000 Alu elements in transcribed regions of the human genome. These elements contain cryptic splice sites, so they are in constant danger of aberrant incorporation into mature transcripts. Despite posing a major threat to transcriptome integrity, little is known about the molecular mechanisms preventing their inclusion. Here, we present a mechanism for protecting the human transcriptome from the aberrant exonization of transposable elements. Quantitative iCLIP data show that the RNA-binding protein hnRNP C competes with the splicing factor U2AF65 at many genuine and cryptic splice sites. Loss of hnRNP C leads to formation of previously suppressed Alu exons, which severely disrupt transcript function. Minigene experiments explain disease-associated mutations in Alu elements that hamper hnRNP C binding. Thus, by preventing U2AF65 binding to Alu elements, hnRNP C plays a critical role as a genome-wide sentinel protecting the transcriptome. The findings have important implications for human evolution and disease., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

78. Protein-RNA interactions: new genomic technologies and perspectives.

Author

König J, Zarnack K, Luscombe NM, and Ule J

Subjects

Animals, Computational Biology, High-Throughput Nucleotide Sequencing, Humans, Ribonucleoproteins metabolism, Genomics methods, RNA metabolism, RNA-Binding Proteins metabolism

Abstract

RNA-binding proteins are key players in the regulation of gene expression. In this Progress article, we discuss state-of-the-art technologies that can be used to study individual RNA-binding proteins or large complexes such as the ribosome. We also describe how these approaches can be used to study interactions with different types of RNAs, including nascent transcripts, mRNAs, microRNAs and ribosomal RNAs, in order to investigate transcription, RNA processing and translation. Finally, we highlight current challenges in data analysis and the future steps that are needed to obtain a quantitative and high-resolution picture of protein-RNA interactions on a genome-wide scale.

Published

2012

79. The RNA-binding protein Rrm4 is essential for efficient secretion of endochitinase Cts1.

Author

Koepke J, Kaffarnik F, Haag C, Zarnack K, Luscombe NM, König J, Ule J, Kellner R, Begerow D, and Feldbrügge M

Subjects

Amino Acid Sequence, Cell Membrane metabolism, Fungal Proteins metabolism, Gene Knockout Techniques, Molecular Sequence Data, Phylogeny, Protein Binding, Protein Transport, RNA Transport, RNA, Messenger metabolism, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, Ribonucleoproteins metabolism, Two-Dimensional Difference Gel Electrophoresis, Ustilago genetics, Ustilago growth & development, Chitinases metabolism, Fungal Proteins physiology, RNA Processing, Post-Transcriptional, RNA-Binding Proteins physiology, Ustilago enzymology

Abstract

Long-distance transport of mRNAs is crucial in determining spatio-temporal gene expression in eukaryotes. The RNA-binding protein Rrm4 constitutes a key component of microtubule-dependent mRNA transport in filaments of Ustilago maydis. Although a number of potential target mRNAs could be identified, cellular processes that depend on Rrm4-mediated transport remain largely unknown. Here, we used differential proteomics to show that ribosomal, mitochondrial, and cell wall-remodeling proteins, including the bacterial-type endochitinase Cts1, are differentially regulated in rrm4Δ filaments. In vivo UV crosslinking and immunoprecipitation and fluorescence in situ hybridization revealed that cts1 mRNA represents a direct target of Rrm4. Filaments of cts1Δ mutants aggregate in liquid culture suggesting an altered cell surface. In wild type cells Cts1 localizes predominantly at the growth cone, whereas it accumulates at both poles in rrm4Δ filaments. The endochitinase is secreted and associates most likely with the cell wall of filaments. Secretion is drastically impaired in filaments lacking Rrm4 or conventional kinesin Kin1 as well as in filaments with disrupted microtubules. Thus, Rrm4-mediated mRNA transport appears to be essential for efficient export of active Cts1, uncovering a novel molecular link between mRNA transport and the mechanism of secretion.

Published

2011

80. Analysis of alternative splicing associated with aging and neurodegeneration in the human brain.

Author

Tollervey JR, Wang Z, Hortobágyi T, Witten JT, Zarnack K, Kayikci M, Clark TA, Schweitzer AC, Rot G, Curk T, Zupan B, Rogelj B, Shaw CE, and Ule J

Subjects

Adolescent, Adult, Age Factors, Aged, Aged, 80 and over, Antigens, Neoplasm genetics, Antigens, Neoplasm metabolism, Cell Adhesion Molecules genetics, Down-Regulation, Exons, Gene Expression Profiling, Humans, Ion Channels genetics, Middle Aged, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Neuro-Oncological Ventral Antigen, Oligonucleotide Array Sequence Analysis, Polypyrimidine Tract-Binding Protein metabolism, Principal Component Analysis, Protein Isoforms metabolism, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, Synaptic Transmission genetics, Temporal Lobe metabolism, Transcription, Genetic, Young Adult, Aging, Alternative Splicing, Alzheimer Disease genetics, Frontotemporal Lobar Degeneration genetics

Abstract

Age is the most important risk factor for neurodegeneration; however, the effects of aging and neurodegeneration on gene expression in the human brain have most often been studied separately. Here, we analyzed changes in transcript levels and alternative splicing in the temporal cortex of individuals of different ages who were cognitively normal, affected by frontotemporal lobar degeneration (FTLD), or affected by Alzheimer's disease (AD). We identified age-related splicing changes in cognitively normal individuals and found that these were present also in 95% of individuals with FTLD or AD, independent of their age. These changes were consistent with increased polypyrimidine tract binding protein (PTB)-dependent splicing activity. We also identified disease-specific splicing changes that were present in individuals with FTLD or AD, but not in cognitively normal individuals. These changes were consistent with the decreased neuro-oncological ventral antigen (NOVA)-dependent splicing regulation, and the decreased nuclear abundance of NOVA proteins. As expected, a dramatic down-regulation of neuronal genes was associated with disease, whereas a modest down-regulation of glial and neuronal genes was associated with aging. Whereas our data indicated that the age-related splicing changes are regulated independently of transcript-level changes, these two regulatory mechanisms affected expression of genes with similar functions, including metabolism and DNA repair. In conclusion, the alternative splicing changes identified in this study provide a new link between aging and neurodegeneration.

Published

2011

81. iCLIP--transcriptome-wide mapping of protein-RNA interactions with individual nucleotide resolution.

Author

Konig J, Zarnack K, Rot G, Curk T, Kayikci M, Zupan B, Turner DJ, Luscombe NM, and Ule J

Subjects

DNA, Complementary genetics, DNA, Complementary metabolism, Immunoprecipitation methods, RNA genetics, RNA metabolism, RNA radiation effects, RNA Splicing, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, RNA-Binding Proteins radiation effects, Ultraviolet Rays, Gene Expression Profiling methods, RNA analysis, RNA-Binding Proteins analysis

Abstract

The unique composition and spatial arrangement of RNA-binding proteins (RBPs) on a transcript guide the diverse aspects of post-transcriptional regulation. Therefore, an essential step towards understanding transcript regulation at the molecular level is to gain positional information on the binding sites of RBPs. Protein-RNA interactions can be studied using biochemical methods, but these approaches do not address RNA binding in its native cellular context. Initial attempts to study protein-RNA complexes in their cellular environment employed affinity purification or immunoprecipitation combined with differential display or microarray analysis (RIP-CHIP). These approaches were prone to identifying indirect or non-physiological interactions. In order to increase the specificity and positional resolution, a strategy referred to as CLIP (UV cross-linking and immunoprecipitation) was introduced. CLIP combines UV cross-linking of proteins and RNA molecules with rigorous purification schemes including denaturing polyacrylamide gel electrophoresis. In combination with high-throughput sequencing technologies, CLIP has proven as a powerful tool to study protein-RNA interactions on a genome-wide scale (referred to as HITS-CLIP or CLIP-seq). Recently, PAR-CLIP was introduced that uses photoreactive ribonucleoside analogs for cross-linking. Despite the high specificity of the obtained data, CLIP experiments often generate cDNA libraries of limited sequence complexity. This is partly due to the restricted amount of co-purified RNA and the two inefficient RNA ligation reactions required for library preparation. In addition, primer extension assays indicated that many cDNAs truncate prematurely at the crosslinked nucleotide. Such truncated cDNAs are lost during the standard CLIP library preparation protocol. We recently developed iCLIP (individual-nucleotide resolution CLIP), which captures the truncated cDNAs by replacing one of the inefficient intermolecular RNA ligation steps with a more efficient intramolecular cDNA circularization (Figure 1). Importantly, sequencing the truncated cDNAs provides insights into the position of the cross-link site at nucleotide resolution. We successfully applied iCLIP to study hnRNP C particle organization on a genome-wide scale and assess its role in splicing regulation.

Published

2011

82. iCLIP predicts the dual splicing effects of TIA-RNA interactions.

Author

Wang Z, Kayikci M, Briese M, Zarnack K, Luscombe NM, Rot G, Zupan B, Curk T, and Ule J

Subjects

Base Sequence, Exons, Genome, Human, HeLa Cells, Humans, Molecular Sequence Data, Poly(A)-Binding Proteins genetics, Protein Binding, RNA Splice Sites, RNA, Small Interfering genetics, RNA, Small Interfering metabolism, RNA-Binding Proteins genetics, T-Cell Intracellular Antigen-1, Alternative Splicing, Poly(A)-Binding Proteins metabolism, RNA genetics, RNA metabolism, RNA-Binding Proteins metabolism

Abstract

The regulation of alternative splicing involves interactions between RNA-binding proteins and pre-mRNA positions close to the splice sites. T-cell intracellular antigen 1 (TIA1) and TIA1-like 1 (TIAL1) locally enhance exon inclusion by recruiting U1 snRNP to 5' splice sites. However, effects of TIA proteins on splicing of distal exons have not yet been explored. We used UV-crosslinking and immunoprecipitation (iCLIP) to find that TIA1 and TIAL1 bind at the same positions on human RNAs. Binding downstream of 5' splice sites was used to predict the effects of TIA proteins in enhancing inclusion of proximal exons and silencing inclusion of distal exons. The predictions were validated in an unbiased manner using splice-junction microarrays, RT-PCR, and minigene constructs, which showed that TIA proteins maintain splicing fidelity and regulate alternative splicing by binding exclusively downstream of 5' splice sites. Surprisingly, TIA binding at 5' splice sites silenced distal cassette and variable-length exons without binding in proximity to the regulated alternative 3' splice sites. Using transcriptome-wide high-resolution mapping of TIA-RNA interactions we evaluated the distal splicing effects of TIA proteins. These data are consistent with a model where TIA proteins shorten the time available for definition of an alternative exon by enhancing recognition of the preceding 5' splice site. Thus, our findings indicate that changes in splicing kinetics could mediate the distal regulation of alternative splicing., Competing Interests: The authors have declared that no competing interests exist.

Published

2010

83. Microtubule-dependent mRNA transport in fungi.

Author

Zarnack K and Feldbrügge M

Subjects

Actins metabolism, Fungi metabolism, RNA, Fungal genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Fungi cytology, Fungi genetics, Microtubules metabolism, RNA Transport, RNA, Fungal metabolism

Abstract

The localization and local translation of mRNAs constitute an important mechanism to promote the correct subcellular targeting of proteins. mRNA localization is mediated by the active transport of mRNPs, large assemblies consisting of mRNAs and associated factors such as RNA-binding proteins. Molecular motors move mRNPs along the actin or microtubule cytoskeleton for short-distance or long-distance trafficking, respectively. In filamentous fungi, microtubule-based long-distance transport of vesicles, which are involved in membrane and cell wall expansion, supports efficient hyphal growth. Recently, we discovered that the microtubule-mediated transport of mRNAs is essential for the fast polar growth of infectious filaments in the corn pathogen Ustilago maydis. Combining in vivo UV cross-linking and RNA live imaging revealed that the RNA-binding protein Rrm4, which constitutes an integral part of the mRNP transport machinery, mediates the transport of distinct mRNAs encoding polarity factors, protein synthesis factors, and mitochondrial proteins. Moreover, our results indicate that microtubule-dependent mRNA transport is evolutionarily conserved from fungi to higher eukaryotes. This raises the exciting possibility of U. maydis as a model system to uncover basic concepts of long-distance mRNA transport.

Published

2010

84. Tandem KH domains of Khd4 recognize AUACCC and are essential for regulation of morphology as well as pathogenicity in Ustilago maydis.

Author

Vollmeister E, Haag C, Zarnack K, Baumann S, König J, Mannhaupt G, and Feldbrügge M

Subjects

Amino Acid Sequence, Base Sequence, Fungal Proteins chemistry, Fungal Proteins genetics, Gene Expression Regulation, Fungal, Molecular Sequence Data, Mutation, RNA, Messenger chemistry, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, Sequence Alignment, Sequence Homology, Amino Acid, Ustilago cytology, Ustilago genetics, Ustilago pathogenicity, Fungal Proteins metabolism, RNA, Messenger metabolism, RNA-Binding Proteins metabolism, Ustilago chemistry

Abstract

RNA-binding proteins constitute key factors of the post-transcriptional machinery. These regulatory proteins recognize specific elements within target transcripts to promote, for example, maturation, translation, or stability of mRNAs. In Ustilago maydis, evidence is accumulating that post-transcriptional processes are important to determine pathogenicity. Deletion of khd4, encoding a predicted RNA-binding protein with five K homology (KH) domains, causes aberrant cell morphology and reduced virulence. Here, we demonstrate that Khd4 recognizes the sequence AUACCC in vivo via its tandem KH domains 3 and 4. This sequence most likely functions as a regulatory RNA element in U. maydis, since it accumulates in 3' untranslated regions. Consistently, an independent mRNA expression profiling approach revealed that the binding motif is significantly enriched in transcripts showing altered expression levels in khd4Delta strains. Since the vast majority of potential Khd4 target mRNAs exhibit increased amounts in deletion mutants, Khd4 might promote mRNA instability. Mutants that fail to bind AUACCC resemble deletion mutants, which exhibit altered cell morphology, disturbed filamentous growth, and severely reduced virulence. Hence, RNA binding is essential for function of Khd4, stressing the importance of post-transcriptional control in regulating morphology and pathogenicity.

Published

2009

85. The fungal RNA-binding protein Rrm4 mediates long-distance transport of ubi1 and rho3 mRNAs.

Author

König J, Baumann S, Koepke J, Pohlmann T, Zarnack K, and Feldbrügge M

Subjects

Base Sequence, Binding Sites, Cloning, Molecular, Cytoskeleton metabolism, Escherichia coli K12 genetics, Fungal Proteins analysis, Molecular Sequence Data, Mutation, RNA, Messenger analysis, RNA, Messenger genetics, RNA-Binding Proteins analysis, RNA-Binding Proteins genetics, Ubiquitin genetics, Ustilago genetics, rho GTP-Binding Proteins genetics, Fungal Proteins metabolism, Microtubules metabolism, RNA Transport, RNA, Messenger metabolism, RNA-Binding Proteins metabolism, Ustilago metabolism

Abstract

Cytoskeletal transport promotes polar growth in filamentous fungi. In Ustilago maydis, the RNA-binding protein Rrm4 shuttles along microtubules and is crucial for polarity in infectious filaments. Mutations in the RNA-binding domain cause loss of function. However, it was unclear which RNAs are bound and transported. Here, we applied in vivo RNA binding studies and live imaging to determine the molecular function of Rrm4. This new combination revealed that Rrm4 mediates microtubule-dependent transport of distinct mRNAs encoding, for example, the ubiquitin fusion protein Ubi1 and the small G protein Rho3. These transcripts accumulate in ribonucleoprotein particles (mRNPs) that move bidirectionally along microtubules and co-localise with Rrm4. Importantly, the 3' untranslated region of ubi1 containing a CA-rich binding site functions as zipcode during mRNA transport. Furthermore, motile mRNPs are not formed when the RNA-binding domain of Rrm4 is deleted, although the protein is still shuttling. Thus, Rrm4 constitutes an integral component of the transport machinery. We propose that microtubule-dependent mRNP trafficking is crucial for hyphal growth introducing U. maydis as attractive model for studying mRNA transport in higher eukaryotes.

Published

2009

86. The posttranscriptional machinery of Ustilago maydis.

Author

Feldbrügge M, Zarnack K, Vollmeister E, Baumann S, Koepke J, König J, Münsterkötter M, and Mannhaupt G

Subjects

Fungal Proteins metabolism, Gene Expression Regulation, Fungal, Ustilago metabolism, Fungal Proteins genetics, Genome, Fungal, RNA Processing, Post-Transcriptional, Ustilago genetics

Abstract

Eukaryotic gene expression begins with transcription and maturation of mRNAs in the nucleus and ends with their translation and degradation in the cytoplasm. Here, we present an inventory of the posttranscriptional machinery of Ustilago maydis that is based on the recently sequenced genome and its comprehensive manual annotation. We used the detailed knowledge available for Saccharomyces cerevisiae and higher eukaryotes to predict posttranscriptional components in this plant pathogen. The comparison to S. cerevisiae revealed that most core components are shared. Both fungi belong to the small group of organisms lacking components of the RNAi machinery. However, a striking difference exists at the level of splicing. U. maydis harbors substantially more intron-containing genes and this correlates with the presence of numerous splice components with human orthologues that are absent or less conserved in S. cerevisiae. In particular, U. maydis contains three out of four core proteins of the exon junction complex, which marks spliced exons and is involved in cytoplasmic mRNA transport. In this context, it is also remarkable that the U. maydis genome displays components involved in microtubule- rather than actin-dependent mRNA transport. Thus, U. maydis might serve as an attractive model system to gain novel insights into posttranscriptional processes.

Published

2008

87. Pheromone-regulated target genes respond differentially to MAPK phosphorylation of transcription factor Prf1.

Author

Zarnack K, Eichhorn H, Kahmann R, and Feldbrügge M

Subjects

Cyclic AMP-Dependent Protein Kinases metabolism, Gene Expression Profiling, Genes, Mating Type, Fungal drug effects, High Mobility Group Proteins genetics, Pheromones pharmacology, Phosphorylation, Plant Proteins genetics, Signal Transduction, Transcription Factors genetics, Transcription, Genetic drug effects, Ustilago metabolism, Gene Expression Regulation, Fungal, High Mobility Group Proteins metabolism, Mitogen-Activated Protein Kinase Kinases metabolism, Pheromones metabolism, Plant Proteins metabolism, Protein Processing, Post-Translational, Transcription Factors metabolism, Ustilago genetics

Abstract

Pheromone signalling during mating is essential for pathogenicity of Ustilago maydis. The activity of the key transcription factor Prf1 is controlled at the transcriptional level and post-translationally by mitogen-activated protein kinase (MAPK) and protein kinase A (PKA) phosphorylation. However, the precise contribution of these regulatory mechanisms to the transcriptional output is unknown. Here, we genetically dissected the three levels of Prf1 regulation. We performed transcriptional profiling of respective mutants to identify and classify targets. This approach revealed that transcriptional regulation of prf1 had only minor influence on target gene expression stressing the importance of post-translational control. PKA regulation of Prf1 was sufficient to control expression of nine pheromone-responsive genes including the major transcription factor regulating pathogenicity. MAPK regulation was necessary for the pheromone response of a set of 57 genes. In 35 cases, pheromone responsiveness was completely lost, while in the remaining 22 cases regulation was alleviated. This indicated a novel level of complexity in MAPK signalling suggesting that target genes respond differentially to MAPK phosphorylation of the respective transcription factors.

Published

2008

88. mRNA trafficking in fungi.

Author

Zarnack K and Feldbrügge M

Subjects

Biological Transport, Cell Division physiology, Microtubules physiology, Mitochondrial Proteins metabolism, Models, Biological, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Fungi genetics, Fungi metabolism, RNA, Messenger metabolism

Abstract

Fungal growth depends on active transport of macromolecules along the actin and/or microtubule cytoskeleton. Thereby, molecular cargo such as proteins, lipids, and mRNAs is targeted to defined subcellular regions. Active transport and localisation of mRNAs mediate localised translation so that protein synthesis occurs where protein function is required. In Saccharomyces cerevisiae, actomyosin-dependent mRNA trafficking participates in polar growth, asymmetric cell division, targeting of membrane proteins and import of mitochondrial proteins. The best-understood example is transport of ASH1 mRNA to the distal pole of the incipient daughter cell. cis-acting RNA sequences are recognised by the RNA-binding protein She2p that is connected via the adaptor She3p to the molecular motor Myo4p. Local translation at the poles of daughter cells causes Ash1p to accumulate predominantly in nuclei of daughter cells, where this transcription factor inhibits mating-type switching. Recently, it was also shown that actomyosin-dependent ASH1 mRNA transport directs tip cell-specific gene expression in filaments of the human pathogen Candida albicans. Furthermore, in the plant pathogen Ustilago maydis microtubule-dependent shuttling of the RNA-binding protein Rrm4 is essential to determine the axis of polarity in infectious filaments. Thus, mRNA trafficking appears to be universally required for polar growth of fungi.

Published

2007

89. Tetracycline-regulated gene expression in the pathogen Ustilago maydis.

Author

Zarnack K, Maurer S, Kaffarnik F, Ladendorf O, Brachmann A, Kämper J, and Feldbrügge M

Subjects

Anti-Bacterial Agents pharmacology, Base Sequence genetics, Dose-Response Relationship, Drug, Enhancer Elements, Genetic genetics, Gene Expression Regulation, Fungal drug effects, Genes, Synthetic genetics, Pheromones pharmacology, Plant Diseases microbiology, Protein Structure, Tertiary genetics, Sequence Deletion genetics, Tetracycline pharmacology, Tetracycline Resistance genetics, Ustilago pathogenicity, Zea mays microbiology, Gene Expression Regulation, Fungal genetics, Polyadenylation genetics, Promoter Regions, Genetic genetics, Transcription Factors genetics, Transgenes genetics, Ustilago genetics

Abstract

A powerful approach to explore gene function is the use of tetracycline-regulated expression. Here, we report the establishment of this titratable gene expression system for Ustilago maydis. Obstacles of premature polyadenylation of the native tetR gene, high basal activity of the tetracycline-responsive promoter, and toxicity of the viral activation domain were overcome by designing a synthetic tetR* gene according to context-dependent codon usage, removing cryptic enhancer elements from the promoter, and using an acidic minimal activation domain, respectively. We verified tetracycline-dependent dose-response using optimised components and applied a straightforward single-step promoter replacement cassette to regulate expression of pheromone response factor, a key transcription factor regulating mating. Pheromone response in liquid culture and mating on solid media was abolished in the presence of tetracycline and doxycycline. Thus, functionality of this versatile new tool for the plant pathogen was proven in a biological context.

Published

2006