Your search keyword '"RNA Polymerase II metabolism"' showing total 5,554 results

1. Isobaric crosslinking mass spectrometry technology for studying conformational and structural changes in proteins and complexes.

Author

Luo J and Ranish J

Subjects

Cross-Linking Reagents chemistry, RNA Polymerase II metabolism, RNA Polymerase II chemistry, Proteins chemistry, Proteins metabolism, Multiprotein Complexes chemistry, Multiprotein Complexes metabolism, Humans, Mass Spectrometry methods, Protein Conformation

Abstract

Dynamic conformational and structural changes in proteins and protein complexes play a central and ubiquitous role in the regulation of protein function, yet it is very challenging to study these changes, especially for large protein complexes, under physiological conditions. Here, we introduce a novel isobaric crosslinker, Qlinker, for studying conformational and structural changes in proteins and protein complexes using quantitative crosslinking mass spectrometry. Qlinkers are small and simple, amine-reactive molecules with an optimal extended distance of ~10 Å, which use MS2 reporter ions for relative quantification of Qlinker-modified peptides derived from different samples. We synthesized the 2-plex Q2linker and showed that the Q2linker can provide quantitative crosslinking data that pinpoints key conformational and structural changes in biosensors, binary and ternary complexes composed of the general transcription factors TBP, TFIIA, and TFIIB, and RNA polymerase II complexes., Competing Interests: JL, JR No competing interests declared, (© 2024, Luo and Ranish.)

Published

2024

2. Nucleolar Pol II interactome reveals TBPL1, PAF1, and Pol I at intergenic rDNA drive rRNA biogenesis.

Author

Khosraviani N, Yerlici VT, St-Germain J, Hou YY, Cao SB, Ghali C, Bokros M, Krishnan R, Hakem R, Lee S, Raught B, and Mekhail K

Subjects

Humans, RNA Polymerase II metabolism, RNA Polymerase II genetics, RNA, Untranslated metabolism, RNA, Untranslated genetics, DNA, Intergenic genetics, HeLa Cells, RNA Polymerase I metabolism, RNA Polymerase I genetics, RNA, Ribosomal metabolism, RNA, Ribosomal genetics, Cell Nucleolus metabolism, DNA, Ribosomal genetics, DNA, Ribosomal metabolism, Nuclear Proteins metabolism, Nuclear Proteins genetics, Transcription Factors metabolism, Transcription Factors genetics

Abstract

Ribosomal DNA (rDNA) repeats harbor ribosomal RNA (rRNA) genes and intergenic spacers (IGS). RNA polymerase (Pol) I transcribes rRNA genes yielding rRNA components of ribosomes. IGS-associated Pol II prevents Pol I from excessively synthesizing IGS non-coding RNAs (ncRNAs) that can disrupt nucleoli and rRNA production. Here, compartment-enriched proximity-dependent biotin identification (compBioID) revealed the TATA-less-promoter-binding TBPL1 and transcription-regulatory PAF1 with nucleolar Pol II. TBPL1 localizes to TCT motifs, driving Pol II and Pol I and maintaining its baseline ncRNA levels. PAF1 promotes Pol II elongation, preventing unscheduled R-loops that hyper-restrain IGS Pol I-associated ncRNAs. PAF1 or TBPL1 deficiency disrupts nucleolar organization and rRNA biogenesis. In PAF1-deficient cells, repressing unscheduled IGS R-loops rescues nucleolar organization and rRNA production. Depleting IGS Pol I-dependent ncRNAs is sufficient to compromise nucleoli. We present the nucleolar interactome of Pol II and show that its regulation by TBPL1 and PAF1 ensures IGS Pol I ncRNAs maintaining nucleolar structure and function., (© 2024. The Author(s).)

Published

2024

3. SUN2 mediates calcium-triggered nuclear actin polymerization to cluster active RNA polymerase II.

Author

Ulferts S and Grosse R

Subjects

Humans, Membrane Proteins metabolism, Membrane Proteins genetics, Cell Nucleus metabolism, Animals, Nuclear Envelope metabolism, Nuclear Proteins metabolism, Actin Cytoskeleton metabolism, HeLa Cells, Mice, Intracellular Signaling Peptides and Proteins, RNA Polymerase II metabolism, Calcium metabolism, Actins metabolism, Polymerization

Abstract

The nucleoskeleton is essential for nuclear architecture as well as genome integrity and gene expression. In addition to lamins, titin or spectrins, dynamic actin filament polymerization has emerged as a potential intranuclear structural element but its functions are less well explored. Here we found that calcium elevations trigger rapid nuclear actin assembly requiring the nuclear membrane protein SUN2 independently of its function as a component of the LINC complex. Instead, SUN2 colocalized and associated with the formin and actin nucleator INF2 in the nuclear envelope in a calcium-regulated manner. Moreover, SUN2 is required for active RNA polymerase II (RNA Pol II) clustering in response to calcium elevations. Thus, our data uncover a SUN2-formin module linking the nuclear envelope to intranuclear actin assembly to promote signal-dependent spatial reorganization of active RNA Pol II., (© 2024. The Author(s).)

Published

2024

4. The small RNA biogenesis in rice is regulated by MAP kinase-mediated OsCDKD phosphorylation.

Author

Singh D, Verma N, Rengasamy B, Banerjee G, and Sinha AK

Subjects

Phosphorylation, Cyclin-Dependent Kinases metabolism, Cyclin-Dependent Kinases genetics, RNA Polymerase II metabolism, Protein Binding, Amino Acid Sequence, RNA, Plant genetics, RNA, Plant metabolism, Transcription, Genetic, Oryza genetics, Plant Proteins metabolism, Plant Proteins genetics, Mitogen-Activated Protein Kinases metabolism, Mitogen-Activated Protein Kinases genetics, Gene Expression Regulation, Plant

Abstract

CDKs are the master regulator of cell division and their activity is controlled by the regulatory subunit cyclins and phosphorylation by the CAKs. However, the role of MAP kinases in regulating plant cell cycle or CDKs have not been explored. Here, we report that the MAP kinases OsMPK3, OsMPK4, and OsMPK6 physically interact and phosphorylate OsCDKD and its regulatory subunit OsCYCH in rice. MAP kinases phosphorylate CDKD at Ser-168 and Thr-235 residues in OsCDKD. The MAP kinase-mediated phosphorylation of OsCDKD is required for its activation to control the small RNA biogenesis. The phosphodead version of OsCDKD fails to activate the C-terminal domain of RNA Polymerase II, thereby negatively impacting small RNA transcription. Further, the overexpression lines of wild-type (WT) OsCDKD and phosphomimic OsCDKD show increased root growth, plant height, tiller number, panicle number, and seed number in comparison to WT, phosphodead OsCDKD-OE, and kinase-dead OsCDKD-OE plants. In a nutshell, our study establishes a novel regulation of OsCDKD by MAPK-mediated phosphorylation in rice. The phosphorylation of OsCDKD by MAPKs imparts a positive effect on rice growth and development by regulating miRNAs transcription., (© 2024 The Author(s). New Phytologist © 2024 New Phytologist Foundation.)

Published

2024

5. A simple, robust, cost-effective, and low-input ChIP-seq method for profiling histone modifications and Pol II in plants.

Author

Zhu D, Wen Y, Tan Y, Chen X, and Wu Z

Subjects

Cost-Benefit Analysis, Chromatin Immunoprecipitation methods, Arabidopsis genetics, Histones metabolism, Chromatin Immunoprecipitation Sequencing methods, RNA Polymerase II metabolism

Abstract

Chromatin immunoprecipitation and sequencing (vs ChIP-seq) is an essential tool for epigenetic and molecular genetic studies. Although being routinely used, ChIP-seq is expensive, requires grams of plant materials, and is challenging for samples that enrich fatty acids such as seeds. Here, we developed an Ultrasensitive Plant ChIP-seq (UP-ChIP) method based on native ChIP-seq combined with Tn5 tagmentation-based library construction strategy. UP-ChIP is generally applicable for profiling both histone modification and Pol II in a wide range of plant samples, such as a single Arabidopsis seedling, a few Arabidopsis seeds, and sorted nuclei. Compared with conventional ChIP-seq, UP-ChIP is much less labor intensive and only consumes 1 μg of antibody and 10 μl of Protein-A/G conjugated beads for each IP and can work effectively with the amount of starting material down to a few milligrams. By performing UP-ChIP in various conditions and genotypes, we showed that UP-ChIP is highly reliable, sensitive, and quantitative for studying histone modifications. Detailed UP-ChIP protocol is provided. We recommend UP-ChIP as an alternative to traditional ChIP-seq for profiling histone modifications and Pol II, offering the advantages of reduced labor intensity, decreased costs, and low-sample input., (© 2024 The Author(s). New Phytologist © 2024 New Phytologist Foundation.)

Published

2024

6. MOF-mediated acetylation of CDK9 promotes global transcription by modulating P-TEFb complex formation.

Author

Chen W, Chu J, Miao Y, Jiang W, Wang F, Zhang N, Jin J, and Cai Y

Subjects

Acetylation, Humans, Histone Deacetylase 1 metabolism, Histone Deacetylase 1 genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, HEK293 Cells, Lysine metabolism, HeLa Cells, Cyclin-Dependent Kinase 9 metabolism, Cyclin-Dependent Kinase 9 genetics, Positive Transcriptional Elongation Factor B metabolism, Positive Transcriptional Elongation Factor B genetics, Cyclin T metabolism, Cyclin T genetics, Histone Acetyltransferases metabolism, Histone Acetyltransferases genetics, Transcription, Genetic

Abstract

Cyclin-dependent kinase 9 (CDK9), a catalytic subunit of the positive transcription elongation factor b (P-TEFb) complex, is a global transcriptional elongation factor associated with cell proliferation. CDK9 activity is regulated by certain histone acetyltransferases, such as p300, GCN5 and P/CAF. However, the impact of males absent on the first (MOF) (also known as KAT8 or MYST1) on CDK9 activity has not been reported. Therefore, the present study aimed to elucidate the regulatory role of MOF on CDK9. We present evidence from systematic biochemical assays and molecular biology approaches arguing that MOF interacts with and acetylates CDK9 at the lysine 35 (i.e. K35) site, and that this acetyl-group can be removed by histone deacetylase HDAC1. Notably, MOF-mediated acetylation of CDK9 at K35 promotes the formation of the P-TEFb complex through stabilizing CDK9 protein and enhancing its association with cyclin T1, which further increases RNA polymerase II serine 2 residues levels and global transcription. Our study reveals for the first time that MOF promotes global transcription by acetylating CDK9, providing a new strategy for exploring the comprehensive mechanism of the MOF-CDK9 axis in cellular processes., (© 2024 Federation of European Biochemical Societies.)

Published

2024

7. Transcription start site scanning requires the fungi-specific hydrophobic loop of Tfb3.

Author

Yang C, Basnet P, Sharmin S, Shen H, Kaplan CD, and Murakami K

Subjects

Hydrophobic and Hydrophilic Interactions, Promoter Regions, Genetic, TATA Box genetics, Transcription Factor TFIIH metabolism, Transcription Factor TFIIH genetics, Transcription Factor TFIIH chemistry, RNA Polymerase II metabolism, RNA Polymerase II chemistry, RNA Polymerase II genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins chemistry, Transcription Initiation Site

Abstract

RNA polymerase II (pol II) initiates transcription from transcription start sites (TSSs) located ∼30-35 bp downstream of the TATA box in metazoans, whereas in the yeast Saccharomyces cerevisiae, pol II scans further downstream TSSs located ∼40-120 bp downstream of the TATA box. Previously, we found that removal of the kinase module TFIIK (Kin28-Ccl1-Tfb3) from TFIIH shifts the TSS in a yeast in vitro system upstream to the location observed in metazoans and that addition of recombinant Tfb3 back to TFIIH-ΔTFIIK restores the downstream TSS usage. Here, we report that this biochemical activity of yeast TFIIK in TSS scanning is attributable to the Tfb3 RING domain at the interface with pol II in the pre-initiation complex (PIC): especially, swapping Tfb3 Pro51-a residue conserved among all fungi-with Ala or Ser as in MAT1, the metazoan homolog of Tfb3, confers an upstream TSS shift in vitro in a similar manner to the removal of TFIIK. Yeast genetic analysis suggests that both Pro51 and Arg64 of Tfb3 are required to maintain the stability of the Tfb3-pol II interface in the PIC. Cryo-electron microscopy analysis of a yeast PIC lacking TFIIK reveals considerable variability in the orientation of TFIIH, which impairs TSS scanning after promoter opening., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

8. Sequence and structural determinants of RNAPII CTD phase-separation and phosphorylation by CDK7.

Author

Linhartova K, Falginella FL, Matl M, Sebesta M, Vácha R, and Stefl R

Subjects

Phosphorylation, Humans, Protein Domains, Amino Acid Sequence, Tyrosine metabolism, Tyrosine chemistry, Proline metabolism, Proline chemistry, RNA Polymerase II metabolism, RNA Polymerase II chemistry, Molecular Dynamics Simulation, Cyclin-Dependent Kinases metabolism, Cyclin-Dependent Kinases chemistry, Cyclin-Dependent Kinase-Activating Kinase

Abstract

The intrinsically disordered carboxy-terminal domain (CTD) of the largest subunit of RNA Polymerase II (RNAPII) consists of multiple tandem repeats of the consensus heptapeptide Y1-S2-P3-T4-S5-P6-S7. The CTD promotes liquid-liquid phase-separation (LLPS) of RNAPII in vivo. However, understanding the role of the conserved heptad residues in LLPS is hampered by the lack of direct biochemical characterization of the CTD. Here, we generated a systematic array of CTD variants to unravel the sequence-encoded molecular grammar underlying the LLPS of the human CTD. Using in vitro experiments and molecular dynamics simulations, we report that the aromaticity of tyrosine and cis-trans isomerization of prolines govern CTD phase-separation. The cis conformation of prolines and β-turns in the SPXX motif contribute to a more compact CTD ensemble, enhancing interactions among CTD residues. We further demonstrate that prolines and tyrosine in the CTD consensus sequence are required for phosphorylation by Cyclin-dependent kinase 7 (CDK7). Under phase-separation conditions, CDK7 associates with the surface of the CTD droplets, drastically accelerating phosphorylation and promoting the release of hyperphosphorylated CTD from the droplets. Our results highlight the importance of conformationally restricted local structures within spacer regions, separating uniformly spaced tyrosine stickers of the CTD heptads, which are required for CTD phase-separation., (© 2024. The Author(s).)

Published

2024

9. Clustering of RNA Polymerase II C-Terminal Domain Models upon Phosphorylation.

Author

Amith WD, Chen VT, and Dutagaci B

Subjects

Phosphorylation, Protein Domains, RNA Polymerase II metabolism, RNA Polymerase II chemistry, Molecular Dynamics Simulation

Abstract

RNA polymerase II (Pol II) C-terminal domain (CTD) is known to have crucial roles in regulating transcription. CTD has also been highly recognized for undergoing phase separation, which is further associated with its regulatory functions. However, the molecular interactions that the CTD forms to induce clustering to drive phase separations and how the phosphorylation of the CTD affects clustering are not entirely known. In this work, we studied the concentrated solutions of two heptapeptide repeat (2CTD) models at different phosphorylation patterns and protein and ion concentrations using all-atom molecular dynamics simulations to investigate clustering behavior and molecular interactions driving the cluster formation. Our results show that salt concentration and phosphorylation patterns play an important role in determining the clustering pattern, specifically at low protein concentrations. The balance between inter- and intrapeptide interactions and counterion coordination together impact the clustering behavior upon phosphorylation.

Published

2024

10. Spt5 orchestrates cryptic transcript suppression and transcriptional directionality.

Author

An H, Yang H, and Lee D

Subjects

Chromosomal Proteins, Non-Histone metabolism, Chromosomal Proteins, Non-Histone genetics, Humans, Gene Expression Regulation, Fungal, RNA Polymerase II metabolism, RNA Polymerase II genetics, Phosphorylation, RNA, Antisense genetics, RNA, Antisense metabolism, Histones metabolism, Promoter Regions, Genetic, Chromatin metabolism, Chromatin genetics, Transcriptional Elongation Factors metabolism, Transcriptional Elongation Factors genetics, Transcription, Genetic, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics

Abstract

Spt5 is a well-conserved factor that manipulates multiple stages of transcription from promoter-proximal pausing (PPP) to termination. Recent studies have revealed an unexpected increase of antisense transcripts near promoters in cells expressing mutant Spt5. Here, we identify Spt5p-restricted intragenic antisense transcripts and their close relationship with sense transcription in yeast. We confirm that Spt5 CTR phosphorylation is also important to retain Spt5's facility to regulate antisense transcription. The genes whose antisense transcription is strongly suppressed by Spt5p share strong endogenous sense transcription and weak antisense transcription, and this pattern is conserved in humans. Mechanistically, we found that Spt5p depletion increased histone acetylation to initiate intragenic antisense transcription by altering chromatin structure. We additionally identified termination factors that appear to be involved in the ability of Spt5p to restrict antisense transcription. By unveiling a new role of Spt5 in finely balancing the bidirectionality of transcription, we demonstrate that Spt5-mediated suppression of DSIF complex regulated-unstable transcripts (DUTs) is essential to sustain the accurate transcription by RNA polymerase II., (© 2024. The Author(s).)

Published

2024

11. ICP22-defined condensates mediate RNAPII deubiquitylation by UL36 and promote HSV-1 transcription.

Author

Qi H, Yin M, Xiong F, Ren X, Chen K, Qin HB, Wang E, Chen G, Yang L, Liu LD, Zhang H, Cao X, Fraser NW, Luo MH, Zeng WB, and Zhou J

Subjects

Animals, Humans, Biomolecular Condensates metabolism, Chlorocebus aethiops, Herpes Simplex virology, Herpes Simplex metabolism, Transcription, Genetic, Ubiquitin-Specific Proteases metabolism, Ubiquitin-Specific Proteases genetics, Ubiquitination, Herpesvirus 1, Human physiology, Immediate-Early Proteins metabolism, Immediate-Early Proteins genetics, RNA Polymerase II metabolism, Viral Proteins metabolism

Abstract

Herpes simplex virus type I (HSV-1) infection leads to RNA polymerase II (RNAPII) degradation and host transcription shutdown. We show that ICP22 defines the virus-induced chaperone-enriched (VICE) domain through liquid-liquid phase separation. Condensate-disrupting point mutations of ICP22 increase ubiquitin modification of RNAPII Ser-2P; reduce its level and occupancy on viral genes; impair viral gene expression, particularly late genes; and severely reduce viral titers. When proteasome activity is blocked, ubiquitinated RNAPII Ser-2P and the viral UL36 begin to accumulate in the ICP22 condensates. The ubiquitin-specific protease (USP) deubiquitinase domain of UL36 interacts with and erases ubiquitin modification from RNAPII Ser-2P, protecting it from degradation in infected cells. A virus carrying a catalytic mutant of the UL36 USP diminishes cellular RNAPII Ser-2P levels, viral transcription, and growth. Thus, ICP22 condensates are processing centers where RNAPII Ser-2P is recruited to be deubiquitinated to ensure viral transcription when host transcription is disrupted following infection., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

12. Base-excision repair pathway regulates transcription-replication conflicts in pancreatic ductal adenocarcinoma.

Author

Meng F, Li T, Singh AK, Wang Y, Attiyeh M, Kohram F, Feng Q, Li YR, Shen B, Williams T, Liu Y, and Raoof M

Subjects

Humans, Cell Line, Tumor, Ataxia Telangiectasia Mutated Proteins metabolism, Cell Proliferation, RNA Polymerase II metabolism, Checkpoint Kinase 1 metabolism, Checkpoint Kinase 1 genetics, Signal Transduction, Excision Repair, Carcinoma, Pancreatic Ductal pathology, Carcinoma, Pancreatic Ductal genetics, Carcinoma, Pancreatic Ductal metabolism, DNA Repair, Pancreatic Neoplasms pathology, Pancreatic Neoplasms genetics, Pancreatic Neoplasms metabolism, DNA Replication, Transcription, Genetic drug effects, DNA Damage

Abstract

Oncogenic mutations (such as in KRAS) can dysregulate transcription and replication, leading to transcription-replication conflicts (TRCs). Here, we demonstrate that TRCs are enriched in human pancreatic ductal adenocarcinoma (PDAC) compared to other common solid tumors or normal cells. Several orthogonal approaches demonstrated that TRCs are oncogene dependent. A small interfering RNA (siRNA) screen identified several factors in the base-excision repair (BER) pathway as main regulators of TRCs in PDAC cells. Inhibitors of BER pathway (methoxyamine and CRT) enhanced TRCs. Mechanistically, BER pathway inhibition severely altered RNA polymerase II (RNAPII) and R-loop dynamics at nascent DNA, causing RNAPII trapping and contributing to enhanced TRCs. The ensuing DNA damage activated the ATR-Chk1 pathway. Co-treatment with ATR inhibitor (VX970) and BER inhibitor (methoxyamine) at clinically relevant doses synergistically enhanced DNA damage and reduced cell proliferation in PDAC cells. The study provides mechanistic insights into the regulation of TRCs in PDAC by the BER pathway, which has biologic and therapeutic implications., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

13. RNA polymerase II transcription initiation in holo-TFIID-depleted mouse embryonic stem cells.

Author

Hisler V, Bardot P, Detilleux D, Bernardini A, Stierle M, Sanchez EG, Richard C, Arab LH, Ehrhard C, Morlet B, Hadzhiev Y, Jung M, Le Gras S, Négroni L, Müller F, Tora L, and Vincent SD

Subjects

Animals, Mice, Chromatin metabolism, Mouse Embryonic Stem Cells metabolism, Promoter Regions, Genetic genetics, TATA-Binding Protein Associated Factors metabolism, TATA-Binding Protein Associated Factors genetics, TATA-Box Binding Protein metabolism, TATA-Box Binding Protein genetics, Transcription Initiation, Genetic, Transcription, Genetic, RNA Polymerase II metabolism, Transcription Factor TFIID metabolism, Transcription Factor TFIID genetics

Abstract

The recognition of core promoter sequences by TFIID is the first step in RNA polymerase II (Pol II) transcription initiation. Metazoan holo-TFIID is a trilobular complex, composed of the TATA binding protein (TBP) and 13 TBP-associated factors (TAFs). Why and how TAFs are necessary for the formation of TFIID domains and how they contribute to transcription initiation remain unclear. Inducible TAF7 or TAF10 depletion, followed by comprehensive analysis of TFIID subcomplex formation, chromatin binding, and nascent transcription in mouse embryonic stem cells, result in the formation of a TAF7-lacking TFIID or a minimal core-TFIID complex, respectively. These partial complexes support TBP recruitment at promoters and nascent Pol II transcription at most genes early after depletion, but importantly, TAF10 is necessary for efficient Pol II pausing. We show that partially assembled TFIID complexes can sustain Pol II transcription initiation but cannot replace holo-TFIID over several cell divisions and/or development., Competing Interests: Declaration of interests The authors declare that they have no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

14. Isoginkgetin and Madrasin are poor splicing inhibitors.

Author

Tellier M, Ansa G, and Murphy S

Subjects

Humans, RNA Precursors genetics, RNA Precursors metabolism, Transcription, Genetic drug effects, RNA Polymerase II metabolism, RNA Splicing Factors metabolism, RNA Splicing Factors genetics, HeLa Cells, Phosphoproteins, Biflavonoids, RNA Splicing drug effects

Abstract

The production of eukaryotic mRNAs requires transcription by RNA polymerase (pol) II and co-transcriptional processing, including capping, splicing, and cleavage and polyadenylation. Pol II can positively affect co-transcriptional processing through interaction of factors with its carboxyl terminal domain (CTD), comprising 52 repeats of the heptapeptide Tyr1-Ser2-Pro3-Thr4-Ser5-Pro6-Ser7, and pol II elongation rate can regulate splicing. Splicing, in turn, can also affect transcriptional activity and transcription elongation defects are caused by some splicing inhibitors. Multiple small molecule inhibitors of splicing are now available, some of which specifically target SF3B1, a U2 snRNP component. SF3B1 inhibition results in a general downregulation of transcription elongation, including premature termination of transcription caused by increased use of intronic poly(A) sites. Here, we have investigated the effect of Madrasin and Isoginkgetin, two non-SF3B1 splicing inhibitors, on splicing and transcription. Surprisingly, we found that both Madrasin and Isoginkgetin affect transcription before any effect on splicing, indicating that their effect on pre-mRNA splicing is likely to be indirect. Both small molecules promote a general downregulation of transcription. Based on these and other published results, we conclude that these two small molecules should not be considered as primarily pre-mRNA splicing inhibitors., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Tellier et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

15. The Integrator complex: an emerging complex structure involved in the regulation of gene expression by targeting RNA polymerase II.

Author

Li T, Zeng F, Li Y, Li H, and Wu J

Subjects

Humans, Gene Expression Regulation, RNA, Small Nuclear genetics, RNA, Small Nuclear metabolism, Animals, Promoter Regions, Genetic, Transcription, Genetic, RNA Polymerase II metabolism, RNA Polymerase II genetics

Abstract

The Integrator complex is a multisubunit complex that participates in the processing of small nuclear RNA molecules in eukaryotic cells by cleaving the 3' end. In protein-coding genes, Integrator is a key regulator of promoter-proximal pausing, release, and recruitment of RNA polymerase II. Research on Integrator has revealed its critical role in the regulation of gene expression and RNA processing. Dysregulation of the Integrator complex has been implicated in a variety of human diseases including cancer and developmental disorders. Therefore, understanding the structure and function of the Integrator complex is critical to uncovering the mechanisms of gene expression and developing potential therapeutic strategies for related diseases., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2024

16. INO80 regulates chromatin accessibility to facilitate suppression of sex-linked gene expression during mouse spermatogenesis.

Author

Chakraborty P and Magnuson T

Subjects

Animals, Male, Mice, Sex Chromosomes genetics, DNA Repair genetics, ATPases Associated with Diverse Cellular Activities genetics, ATPases Associated with Diverse Cellular Activities metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Meiosis genetics, DNA Helicases genetics, DNA Helicases metabolism, Chromatin Assembly and Disassembly genetics, Gene Silencing, Pachytene Stage genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, Mice, Knockout, Histones metabolism, Histones genetics, Spermatogenesis genetics, Spermatocytes metabolism, Chromatin genetics, Chromatin metabolism

Abstract

The INO80 protein is the main catalytic subunit of the INO80-chromatin remodeling complex, which is critical for DNA repair and transcription regulation in murine spermatocytes. In this study, we explored the role of INO80 in silencing genes on meiotic sex chromosomes in male mice. INO80 immunolocalization at the XY body in pachytene spermatocytes suggested a role for INO80 in the meiotic sex body. Subsequent deletion of Ino80 resulted in high expression of sex-linked genes. Furthermore, the active form of RNA polymerase II at the sex chromosomes of Ino80-null pachytene spermatocytes indicates incomplete inactivation of sex-linked genes. A reduction in the recruitment of initiators of meiotic sex chromosome inhibition (MSCI) argues for INO80-facilitated recruitment of DNA repair factors required for silencing sex-linked genes. This role of INO80 is independent of a common INO80 target, H2A.Z. Instead, in the absence of INO80, a reduction in chromatin accessibility at DNA repair sites occurs on the sex chromosomes. These data suggest a role for INO80 in DNA repair factor localization, thereby facilitating the silencing of sex-linked genes during the onset of pachynema., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Chakraborty, Magnuson. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

17. DFF-ChIP: a method to detect and quantify complex interactions between RNA polymerase II, transcription factors, and chromatin.

Author

Spector BM, Santana JF, Pufall MA, and Price DH

Subjects

Humans, Receptors, Glucocorticoid metabolism, Receptors, Glucocorticoid genetics, DNA metabolism, DNA genetics, DNA-Binding Proteins metabolism, CCCTC-Binding Factor metabolism, Protein Binding, RNA Polymerase II metabolism, Chromatin metabolism, Chromatin genetics, Transcription Factors metabolism, Chromatin Immunoprecipitation methods

Abstract

Recently, we introduced a chromatin immunoprecipitation (ChIP) technique utilizing the human DNA Fragmentation Factor (DFF) to digest the DNA prior to immunoprecipitation (DFF-ChIP) that provides the precise location of transcription complexes and their interactions with neighboring nucleosomes. Here we expand the technique to new targets and provide useful information concerning purification of DFF, digestion conditions, and the impact of crosslinking. DFF-ChIP analysis was performed individually for subunits of Mediator, DSIF, and NELF that that do not interact with DNA directly, but rather interact with RNA polymerase II (Pol II). We found that Mediator was associated almost exclusively with preinitiation complexes (PICs). DSIF and NELF were associated with engaged Pol II and, in addition, potential intermediates between PICs and early initiation complexes. DFF-ChIP was then used to analyze the occupancy of a tight binding transcription factor, CTCF, and a much weaker binding factor, glucocorticoid receptor (GR), with and without crosslinking. These results were compared to those from standard ChIP-Seq that employs sonication and to CUT&RUN which utilizes MNase to fragment the genomic DNA. Our findings indicate that DFF-ChIP reveals details of occupancy that are not available using other methods including information revealing pertinent protein:protein interactions., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

18. Temporal transcriptional response of Candida glabrata during macrophage infection reveals a multifaceted transcriptional regulator CgXbp1 important for macrophage response and fluconazole resistance.

Author

Rai MN, Lan Q, Parsania C, Rai R, Shirgaonkar N, Chen R, Shen L, Tan K, and Wong KH

Subjects

Mice, Animals, Fungal Proteins genetics, Fungal Proteins metabolism, Candidiasis microbiology, Candidiasis genetics, Host-Pathogen Interactions genetics, Transcription Factors metabolism, Transcription Factors genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, Humans, Virulence genetics, Candida glabrata genetics, Candida glabrata drug effects, Macrophages microbiology, Macrophages metabolism, Macrophages immunology, Fluconazole pharmacology, Drug Resistance, Fungal genetics, Gene Expression Regulation, Fungal, Antifungal Agents pharmacology

Abstract

Candida glabrata can thrive inside macrophages and tolerate high levels of azole antifungals. These innate abilities render infections by this human pathogen a clinical challenge. How C. glabrata reacts inside macrophages and what is the molecular basis of its drug tolerance are not well understood. Here, we mapped genome-wide RNA polymerase II (RNAPII) occupancy in C. glabrata to delineate its transcriptional responses during macrophage infection in high temporal resolution. RNAPII profiles revealed dynamic C. glabrata responses to macrophages with genes of specialized pathways activated chronologically at different times of infection. We identified an uncharacterized transcription factor (CgXbp1) important for the chronological macrophage response, survival in macrophages, and virulence. Genome-wide mapping of CgXbp1 direct targets further revealed its multi-faceted functions, regulating not only virulence-related genes but also genes associated with drug resistance. Finally, we showed that CgXbp1 indeed also affects fluconazole resistance. Overall, this work presents a powerful approach for examining host-pathogen interaction and uncovers a novel transcription factor important for C. glabrata 's survival in macrophages and drug tolerance., Competing Interests: MR, QL, CP, RR, NS, RC, LS, KT, KW No competing interests declared, (© 2024, Rai, Lan et al.)

Published

2024

19. The zinc-finger transcription factor Sfp1 imprints specific classes of mRNAs and links their synthesis to cytoplasmic decay.

Author

Kelbert M, Jordán-Pla A, de Miguel-Jiménez L, García-Martínez J, Selitrennik M, Guterman A, Henig N, Granneman S, Pérez-Ortín JE, Chávez S, and Choder M

Subjects

RNA Stability, Promoter Regions, Genetic, Protein Binding, Zinc Fingers, Transcription, Genetic, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, Cytoplasm metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins, RNA, Messenger metabolism, RNA, Messenger genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, Transcription Factors metabolism, Transcription Factors genetics

Abstract

To function effectively as an integrated system, the transcriptional and post-transcriptional machineries must communicate through mechanisms that are still poorly understood. Here, we focus on the zinc-finger Sfp1, known to regulate transcription of proliferation-related genes. We show that Sfp1 can regulate transcription either by binding to promoters, like most known transcription activators, or by binding to the transcribed regions (gene bodies), probably via RNA polymerase II (Pol II). We further studied the first mode of Sfp1 activity and found that, following promoter binding, Sfp1 binds to gene bodies and affects Pol II configuration, manifested by dissociation or conformational change of its Rpb4 subunit and increased backtracking. Surprisingly, Sfp1 binds to a subset of mRNAs co-transcriptionally and stabilizes them. The interaction between Sfp1 and its client mRNAs is controlled by their respective promoters and coincides with Sfp1's dissociation from chromatin. Intriguingly, Sfp1 dissociation from the chromatin correlates with the extent of the backtracked Pol II. We propose that, following promoter recruitment, Sfp1 accompanies Pol II and regulates backtracking. The backtracked Pol II is more compatible with Sfp1's relocation to the nascent transcripts, whereupon Sfp1 accompanies these mRNAs to the cytoplasm and regulates their stability. Thus, Sfp1's co-transcriptional binding imprints the mRNA fate, serving as a paradigm for the cross-talk between the synthesis and decay of specific mRNAs, and a paradigm for the dual-role of some zinc-finger proteins. The interplay between Sfp1's two modes of transcription regulation remains to be examined., Competing Interests: MK, AJ, Ld, JG, MS, AG, NH, SG, JP, SC, MC No competing interests declared, (© 2023, Kelbert, Jordán-Pla, de Miguel-Jiménez et al.)

Published

2024

20. C-TERMINAL DOMAIN PHOSPHATASE-LIKE 1 promotes flowering with TAF15b by repressing the floral repressor gene FLOWERING LOCUS C.

Author

Kyung J, Jeong D, Eom H, Kim J, Kim JS, and Lee I

Subjects

MADS Domain Proteins metabolism, MADS Domain Proteins genetics, Phosphorylation, RNA Polymerase II metabolism, RNA Polymerase II genetics, Arabidopsis genetics, Arabidopsis metabolism, Arabidopsis Proteins metabolism, Arabidopsis Proteins genetics, Flowers genetics, Flowers metabolism, Gene Expression Regulation, Plant, Phosphoprotein Phosphatases metabolism, Phosphoprotein Phosphatases genetics, TATA-Binding Protein Associated Factors metabolism, TATA-Binding Protein Associated Factors genetics

Abstract

Arabidopsis TATA-BINDING PROTEIN-ASSOCIATED FACTOR15b (TAF15b) is a plant-specific component of the transcription factor IID complex. TAF15b is involved in the autonomous pathway for flowering and represses the transcription of FLOWERING LOCUS C (FLC), a major floral repressor in Arabidopsis. While components of the autonomous flowering pathway have been extensively studied, scant attention has been directed toward elucidating the direct transcriptional regulators responsible for repressing FLC transcription. Here, we demonstrate that C-TERMINAL DOMAIN PHOSPHATASE-LIKE 1 (CPL1) is a physical and functional partner of TAF15b, playing a role in FLC repression. CPL1 is a protein phosphatase that dephosphorylates the C-terminal domain of RNA polymerase II (Pol II). Through the immunoprecipitation and mass spectrometry technique, we identified CPL1 as an interacting partner of TAF15b. Similar to taf15b, the cpl1 mutant showed a late-flowering phenotype caused by an increase in FLC levels. Additionally, the increase in cpl1 was correlated with the enrichment of phosphorylated Pol II in the FLC chromatin, as expected. We also discovered that CPL1 and TAF15b share additional common target genes through transcriptome analysis. These results suggest that TAF15b and CPL1 cooperatively repress transcription through the dephosphorylation of Pol II, especially at the FLC locus., Competing Interests: Declaration of Competing Interests The authors declare no competing interests., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

21. Nuclear patterns of phosphatidylinositol 4,5- and 3,4-bisphosphate revealed by super-resolution microscopy differ between the consecutive stages of RNA polymerase II transcription.

Author

Hoboth P, Sztacho M, and Hozák P

Subjects

Humans, HeLa Cells, Phosphatidylinositol Phosphates metabolism, RNA Polymerase II metabolism, RNA Polymerase II genetics, Cell Nucleus metabolism, Transcription, Genetic, Phosphatidylinositol 4,5-Diphosphate metabolism

Abstract

Phosphatidylinositol phosphates are powerful signaling molecules that orchestrate signaling and direct membrane trafficking in the cytosol. Interestingly, phosphatidylinositol phosphates also localize within the membrane-less compartments of the cell nucleus, where they participate in the regulation of gene expression. Nevertheless, current models of gene expression, which include condensates of proteins and nucleic acids, do not include nuclear phosphatidylinositol phosphates. This gap is partly a result of the missing detailed analysis of the subnuclear distribution of phosphatidylinositol phosphates and their relationships with gene expression. Here, we used quantitative dual-color direct stochastic optical reconstruction microscopy to analyze the nanoscale co-patterning between RNA polymerase II transcription initiation and elongation markers with respect to phosphatidylinositol 4,5- or 3,4-bisphosphate in the nucleoplasm and nuclear speckles and compared it with randomized data and cells with inhibited transcription. We found specific co-patterning of the transcription initiation marker P-S5 with phosphatidylinositol 4,5-bisphosphate in the nucleoplasm and with phosphatidylinositol 3,4-bisphosphate at the periphery of nuclear speckles. We showed the specific accumulation of the transcription elongation marker PS-2 and of nascent RNA in the proximity of phosphatidylinositol 3,4-bisphosphate associated with nuclear speckles. Taken together, this shows that the distinct spatial associations between the consecutive stages of RNA polymerase II transcription and nuclear phosphatidylinositol phosphates exhibit specificity within the gene expression compartments. Thus, in analogy to the cellular membranes, where phospholipid composition orchestrates signaling pathways and directs membrane trafficking, we propose a model in which the phospholipid identity of gene expression compartments orchestrates RNA polymerase II transcription., (© 2024 The Authors. The FEBS Journal published by John Wiley & Sons Ltd on behalf of Federation of European Biochemical Societies.)

Published

2024

22. Multiple direct and indirect roles of the Paf1 complex in transcription elongation, splicing, and histone modifications.

Author

Francette AM and Arndt KM

Subjects

Nuclear Proteins metabolism, Nuclear Proteins genetics, Gene Expression Regulation, Fungal, Histones metabolism, Histone Code, Transcription, Genetic, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, RNA Splicing genetics, Transcription Elongation, Genetic, RNA Polymerase II metabolism

Abstract

The polymerase-associated factor 1 (Paf1) complex (Paf1C) is a conserved protein complex with critical functions during eukaryotic transcription. Previous studies showed that Paf1C is multi-functional, controlling specific aspects of transcription ranging from RNA polymerase II (RNAPII) processivity to histone modifications. However, it is unclear how specific Paf1C subunits directly impact transcription and coupled processes. We have compared conditional depletion to steady-state deletion for each Paf1C subunit to determine the direct and indirect contributions to gene expression in Saccharomyces cerevisiae. Using nascent transcript sequencing, RNAPII profiling, and modeling of transcription elongation dynamics, we have demonstrated direct effects of Paf1C subunits on RNAPII processivity and elongation rate and indirect effects on transcript splicing and repression of antisense transcripts. Further, our results suggest that the direct transcriptional effects of Paf1C cannot be readily assigned to any particular histone modification. This work comprehensively analyzes both the immediate and the extended roles of each Paf1C subunit in transcription elongation and transcript regulation., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

23. Protocol for the in vitro reconstruction of site-specifically phosphorylated RNA Pol II to identify the recruitment of novel transcription regulators.

Author

Hardtke HA, Moreno RY, and Zhang YJ

Subjects

Phosphorylation, Humans, Transcription, Genetic genetics, RNA Polymerase II metabolism, RNA Polymerase II chemistry

Abstract

The repetitive C-terminal domain (CTD) of the largest subunit of RNA polymerase II (RNAPII) becomes differentially phosphorylated throughout the transcription cycle. Here, we present a protocol to site-specifically phosphorylate the CTD of RNAPII by leveraging the specificity of well-characterized CTD kinases. We describe the steps for optimal phosphorylation of the CTD and the preparation of nuclear protein extract. This protocol can be used to identify the interactome of a phospho-CTD and has the potential to identify novel RNAPII-binding proteins. For complete details on the use and execution of this protocol, please refer to Moreno et al. 1 ., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

24. Variation of C-terminal domain governs RNA polymerase II genomic locations and alternative splicing in eukaryotic transcription.

Author

Zhang Q, Kim W, Panina SB, Mayfield JE, Portz B, and Zhang YJ

Subjects

Phosphorylation, Humans, Protein Domains, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, RNA, Messenger metabolism, RNA, Messenger genetics, Promoter Regions, Genetic, Protein Processing, Post-Translational, RNA Polymerase II metabolism, RNA Polymerase II genetics, Alternative Splicing, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Transcription, Genetic

Abstract

The C-terminal domain of RPB1 (CTD) orchestrates transcription by recruiting regulators to RNA Pol II upon phosphorylation. With CTD driving condensate formation on gene loci, the molecular mechanism behind how CTD-mediated recruitment of transcriptional regulators influences condensates formation remains unclear. Our study unveils that phosphorylation reversibly dissolves phase separation induced by the unphosphorylated CTD. Phosphorylated CTD, upon specific association with transcription regulators, forms distinct condensates from unphosphorylated CTD. Functional studies demonstrate CTD variants with diverse condensation properties exhibit differences in promoter binding and mRNA co-processing in cells. Notably, varying CTD lengths influence the assembly of RNA processing machinery and alternative splicing outcomes, which in turn affects cellular growth, linking the evolution of CTD variation/length with the complexity of splicing from yeast to human. These findings provide compelling evidence for a model wherein post-translational modification enables the transition of functionally specialized condensates, highlighting a co-evolution link between CTD condensation and splicing., (© 2024. The Author(s).)

Published

2024

25. Histone variant H2A.Z is needed for efficient transcription-coupled NER and genome integrity in UV challenged yeast cells.

Author

Gaillard H, Ciudad T, Aguilera A, and Wellinger RE

Subjects

RNA Polymerase II metabolism, RNA Polymerase II genetics, Genome, Fungal, DNA Breaks, Double-Stranded radiation effects, 4-Nitroquinoline-1-oxide pharmacology, Gene Expression Regulation, Fungal radiation effects, Ultraviolet Rays, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae radiation effects, DNA Repair genetics, Histones metabolism, Histones genetics, Genomic Instability radiation effects, Transcription, Genetic, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism, DNA Damage genetics

Abstract

The genome of living cells is constantly challenged by DNA lesions that interfere with cellular processes such as transcription and replication. A manifold of mechanisms act in concert to ensure adequate DNA repair, gene expression, and genome stability. Bulky DNA lesions, such as those induced by UV light or the DNA-damaging agent 4-nitroquinoline oxide, act as transcriptional and replicational roadblocks and thus represent a major threat to cell metabolism. When located on the transcribed strand of active genes, these lesions are handled by transcription-coupled nucleotide excision repair (TC-NER), a yet incompletely understood NER sub-pathway. Here, using a genetic screen in the yeast Saccharomyces cerevisiae, we identified histone variant H2A.Z as an important component to safeguard transcription and DNA integrity following UV irradiation. In the absence of H2A.Z, repair by TC-NER is severely impaired and RNA polymerase II clearance reduced, leading to an increase in double-strand breaks. Thus, H2A.Z is needed for proficient TC-NER and plays a major role in the maintenance of genome stability upon UV irradiation., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Gaillard et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

26. Differential processing of RNA polymerase II at DNA damage correlates with transcription-coupled repair syndrome severity.

Author

Gonzalo-Hansen C, Steurer B, Janssens RC, Zhou D, van Sluis M, Lans H, and Marteijn JA

Subjects

Humans, Transcription Factors metabolism, Transcription Factors genetics, Valosin Containing Protein metabolism, Valosin Containing Protein genetics, Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, Adenosine Triphosphatases metabolism, Adenosine Triphosphatases genetics, Ultraviolet Rays, Cell Line, Excision Repair, Carrier Proteins, RNA Polymerase II metabolism, RNA Polymerase II genetics, DNA Damage, DNA Repair, DNA Repair Enzymes metabolism, DNA Repair Enzymes genetics, Poly-ADP-Ribose Binding Proteins genetics, Poly-ADP-Ribose Binding Proteins metabolism, DNA Helicases metabolism, DNA Helicases genetics, Cockayne Syndrome genetics, Cockayne Syndrome metabolism, Transcription, Genetic

Abstract

DNA damage severely impedes gene transcription by RNA polymerase II (Pol II), causing cellular dysfunction. Transcription-Coupled Nucleotide Excision Repair (TC-NER) specifically removes such transcription-blocking damage. TC-NER initiation relies on the CSB, CSA and UVSSA proteins; loss of any results in complete TC-NER deficiency. Strikingly, UVSSA deficiency results in UV-Sensitive Syndrome (UVSS), with mild cutaneous symptoms, while loss of CSA or CSB activity results in the severe Cockayne Syndrome (CS), characterized by neurodegeneration and premature aging. Thus far the underlying mechanism for these contrasting phenotypes remains unclear. Live-cell imaging approaches reveal that in TC-NER proficient cells, lesion-stalled Pol II is swiftly resolved, while in CSA and CSB knockout (KO) cells, elongating Pol II remains damage-bound, likely obstructing other DNA transacting processes and shielding the damage from alternative repair pathways. In contrast, in UVSSA KO cells, Pol II is cleared from the damage via VCP-mediated proteasomal degradation which is fully dependent on the CRL4CSA ubiquitin ligase activity. This Pol II degradation might provide access for alternative repair mechanisms, such as GG-NER, to remove the damage. Collectively, our data indicate that the inability to clear lesion-stalled Pol II from the chromatin, rather than TC-NER deficiency, causes the severe phenotypes observed in CS., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

27. BOD1L mediates chromatin binding and non-canonical function of H3K4 methyltransferase SETD1A.

Author

Hoshii T, Kikuchi S, Kujirai T, Masuda T, Ito T, Yasuda S, Matsumoto M, Rahmutulla B, Fukuyo M, Murata T, Kurumizaka H, and Kaneda A

Subjects

Animals, Humans, Mice, Cell Line, Tumor, Leukemia genetics, Leukemia metabolism, Protein Binding, Protein Domains, RNA Polymerase II metabolism, Transcription Initiation Site, Transcription, Genetic, Chromatin metabolism, Histone-Lysine N-Methyltransferase metabolism, Histone-Lysine N-Methyltransferase genetics, Histones metabolism

Abstract

The H3K4 methyltransferase SETD1A plays an essential role in both development and cancer. However, essential components involved in SETD1A chromatin binding remain unclear. Here, we discovered that BOD1L exhibits the highest correlated SETD1A co-dependency in human cancer cell lines. BOD1L knockout reduces leukemia cells in vitro and in vivo, and mimics the transcriptional profiles observed in SETD1A knockout cells. The loss of BOD1L immediately reduced SETD1A distribution at transcriptional start sites (TSS), induced transcriptional elongation defect, and increased the RNA polymerase II content at TSS; however, it did not reduce H3K4me3. The Shg1 domain of BOD1L has a DNA binding ability, and a tryptophan residue (W104) in the domain recruits SETD1A to chromatin through the association with SETD1A FLOS domain. In addition, the BOD1L-SETD1A complex associates with transcriptional regulators, including E2Fs. These results reveal that BOD1L mediates chromatin and SETD1A, and regulates the non-canonical function of SETD1A in transcription., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

28. Thr 4 phosphorylation on RNA Pol II occurs at early transcription regulating 3'-end processing.

Author

Moreno RY, Panina SB, Irani S, Hardtke HA, Stephenson R, Floyd BM, Marcotte EM, Zhang Q, and Zhang YJ

Subjects

Phosphorylation, Humans, RNA 3' End Processing, Serine metabolism, Proteomics methods, RNA Polymerase II metabolism, RNA Polymerase II genetics, Threonine metabolism, Transcription, Genetic

Abstract

RNA polymerase II relies on a repetitive sequence domain (YSPTSPS) within its largest subunit to orchestrate transcription. While phosphorylation on serine-2/serine-5 of the carboxyl-terminal heptad repeats is well established, threonine-4's role remains enigmatic. Paradoxically, threonine-4 phosphorylation was only detected after transcription end sites despite functionally implicated in pausing, elongation, termination, and messenger RNA processing. Our investigation revealed that threonine-4 phosphorylation detection was obstructed by flanking serine-5 phosphorylation at the onset of transcription, which can be removed selectively. Subsequent proteomic analyses identified many proteins recruited to transcription via threonine-4 phosphorylation, which previously were attributed to serine-2. Loss of threonine-4 phosphorylation greatly reduces serine-2 phosphorylation, revealing a cross-talk between the two marks. Last, the function analysis of the threonine-4 phosphorylation highlighted its role in alternative 3'-end processing within pro-proliferative genes. Our findings unveil the true genomic location of this evolutionarily conserved phosphorylation mark and prompt a reassessment of functional assignments of the carboxyl-terminal domain.

Published

2024

29. Extracting regulatory active chromatin footprint from cell-free DNA.

Author

Lai K, Dilger K, Cunningham R, Lam KT, Boquiren R, Truong K, Louie MC, Rava R, and Abdueva D

Subjects

Humans, Promoter Regions, Genetic, Epigenesis, Genetic, Epigenomics methods, RNA Polymerase II metabolism, RNA Polymerase II genetics, Nucleosomes metabolism, Nucleosomes genetics, Chromatin genetics, Chromatin metabolism, Cell-Free Nucleic Acids blood, Cell-Free Nucleic Acids genetics

Abstract

Cell-free DNA (cfDNA) has emerged as a pivotal player in precision medicine, revolutionizing the diagnostic and therapeutic landscape. While its clinical applications have significantly increased in recent years, current cfDNA assays have limited ability to identify the active transcriptional programs that govern complex disease phenotypes and capture the heterogeneity of the disease. To address these limitations, we have developed a non-invasive platform to enrich and examine the active chromatin fragments (cfDNA ac ) in peripheral blood. The deconvolution of the cfDNA ac signal from traditional nucleosomal chromatin fragments (cfDNA nuc ) yields a catalog of features linking these circulating chromatin signals in blood to specific regulatory elements across the genome, including enhancers, promoters, and highly transcribed genes, mirroring the epigenetic data from the ENCODE project. Notably, these cfDNA ac counts correlate strongly with RNA polymerase II activity and exhibit distinct expression patterns for known circadian genes. Additionally, cfDNA ac signals across gene bodies and promoters show strong correlations with whole blood gene expression levels defined by GTEx. This study illustrates the utility of cfDNA ac analysis for investigating epigenomics and gene expression, underscoring its potential for a wide range of clinical applications in precision medicine., (© 2024. The Author(s).)

Published

2024

30. Cryo-EM structure and biochemical analyses of the nucleosome containing the cancer-associated histone H3 mutation E97K.

Author

Kimura T, Hirai S, Kujirai T, Fujita R, Ogasawara M, Ehara H, Sekine SI, Takizawa Y, and Kurumizaka H

Subjects

Humans, RNA Polymerase II metabolism, RNA Polymerase II genetics, DNA metabolism, DNA genetics, DNA chemistry, Nucleosomes metabolism, Nucleosomes ultrastructure, Nucleosomes genetics, Histones metabolism, Histones genetics, Cryoelectron Microscopy methods, Mutation, Neoplasms genetics, Neoplasms metabolism

Abstract

The Lys mutation of the canonical histone H3.1 Glu97 residue (H3E97K) is found in cancer cells. Previous biochemical analyses revealed that the nucleosome containing the H3E97K mutation is extremely unstable as compared to the wild-type nucleosome. However, the mechanism by which the H3E97K mutation causes nucleosome instability has not been clarified yet. In the present study, the cryo-electron microscopy structure of the nucleosome containing the H3E97K mutation revealed that the entry/exit DNA regions of the H3E97K nucleosome are disordered, probably by detachment of the nucleosomal DNA from the H3 N-terminal regions. This may change the intra-molecular amino acid interactions with the replaced H3 Lys97 residue, inducing structural distortion around the mutated position in the nucleosome. Consistent with the nucleosomal DNA end flexibility and the nucleosome instability, the H3E97K mutation exhibited reduced binding of linker histone H1 to the nucleosome, defective activation of PRC2 (the essential methyltransferase for facultative heterochromatin formation) with a poly-nucleosome, and enhanced nucleosome transcription by RNA polymerase II., (© 2024 The Author(s). Genes to Cells published by Molecular Biology Society of Japan and John Wiley & Sons Australia, Ltd.)

Published

2024

31. MediatorWeb: a protein-protein interaction network database for the RNA polymerase II Mediator complex.

Author

Maji S, Waseem M, Sharma MK, Singh M, Singh A, Dwivedi N, Thakur P, Cooper DG, Bisht NC, Fassler JS, Subbarao N, Khurana JP, Bhavesh NS, and Thakur JK

Subjects

Humans, RNA Polymerase II metabolism, RNA Polymerase II genetics, RNA Polymerase II chemistry, Protein Interaction Mapping, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins chemistry, Arabidopsis Proteins metabolism, Arabidopsis Proteins genetics, Arabidopsis Proteins chemistry, Mediator Complex metabolism, Mediator Complex genetics, Mediator Complex chemistry, Protein Interaction Maps genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Arabidopsis genetics, Arabidopsis metabolism, Databases, Protein

Abstract

The protein-protein interaction (PPI) network of the Mediator complex is very tightly regulated and depends on different developmental and environmental cues. Here, we present an interactive platform for comparative analysis of the Mediator subunits from humans, baker's yeast Saccharomyces cerevisiae, and model plant Arabidopsis thaliana in a user-friendly web-interface database called MediatorWeb. MediatorWeb provides an interface to visualize and analyze the PPI network of Mediator subunits. The database facilitates downloading the untargeted and unweighted network of Mediator complex, its submodules, and individual Mediator subunits to better visualize the importance of individual Mediator subunits or their submodules. Further, MediatorWeb offers network visualization of the Mediator complex and interacting proteins that are functionally annotated. This feature provides clues to understand functions of Mediator subunits in different processes. In an additional tab, MediatorWeb provides quick access to secondary and tertiary structures, as well as residue-level contact information for Mediator subunits in each of the three model organisms. Another useful feature of MediatorWeb is detection of interologs based on orthologous analyses, which can provide clues to understand the functions of Mediator complex in less explored kingdoms. Thus, MediatorWeb and its features can help the user to understand the role of Mediator complex and its subunits in the transcription regulation of gene expression., (© 2024 Federation of European Biochemical Societies.)

Published

2024

32. Uncovering the functions and mechanisms of regulatory elements-associated non-coding RNAs.

Author

Fosseprez O and Cuvier O

Subjects

Humans, Animals, Promoter Regions, Genetic, Transcription, Genetic, RNA Polymerase II metabolism, Chromatin metabolism, Gene Expression Regulation, RNA, Untranslated genetics, RNA, Untranslated metabolism, Enhancer Elements, Genetic

Abstract

Over the past decade, regulatory non-coding RNAs (ncRNAs) produced by RNA Pol II have been revealed as meaningful players in various essential cellular functions. In particular, thousands of ncRNAs are produced at transcriptional regulatory elements such as enhancers and promoters, where they may exert multiple functions to regulate proper development, cellular programming, transcription or genomic stability. Here, we review the mechanisms involving these regulatory element-associated ncRNAs, and particularly enhancer RNAs (eRNAs) and PROMoter uPstream Transcripts (PROMPTs). We contextualize the mechanisms described to the processing and degradation of these short lived RNAs. We summarize recent findings explaining how ncRNAs operate locally at promoters and enhancers, or further away, either shortly after their production by RNA Pol II, or through post-transcriptional stabilization. Such discoveries lead to a converging model accounting for how ncRNAs influence cellular fate, by acting on transcription and chromatin structure, which may further involve factors participating to 3D nuclear organization., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

33. Association with TFIIIC limits MYCN localisation in hubs of active promoters and chromatin accumulation of non-phosphorylated RNA polymerase II.

Author

Vidal R, Leen E, Herold S, Müller M, Fleischhauer D, Schülein-Völk C, Papadopoulos D, Röschert I, Uhl L, Ade CP, Gallant P, Bayliss R, Eilers M, and Büchel G

Subjects

Humans, Protein Binding, Transcription Factors, TFII metabolism, Transcription Factors, TFII genetics, Transcription, Genetic, Cell Line, Tumor, RNA Polymerase II metabolism, RNA Polymerase II genetics, N-Myc Proto-Oncogene Protein metabolism, N-Myc Proto-Oncogene Protein genetics, Promoter Regions, Genetic, Chromatin metabolism

Abstract

MYC family oncoproteins regulate the expression of a large number of genes and broadly stimulate elongation by RNA polymerase II (RNAPII). While the factors that control the chromatin association of MYC proteins are well understood, much less is known about how interacting proteins mediate MYC's effects on transcription. Here, we show that TFIIIC, an architectural protein complex that controls the three-dimensional chromatin organisation at its target sites, binds directly to the amino-terminal transcriptional regulatory domain of MYCN. Surprisingly, TFIIIC has no discernible role in MYCN-dependent gene expression and transcription elongation. Instead, MYCN and TFIIIC preferentially bind to promoters with paused RNAPII and globally limit the accumulation of non-phosphorylated RNAPII at promoters. Consistent with its ubiquitous role in transcription, MYCN broadly participates in hubs of active promoters. Depletion of TFIIIC further increases MYCN localisation to these hubs. This increase correlates with a failure of the nuclear exosome and BRCA1, both of which are involved in nascent RNA degradation, to localise to active promoters. Our data suggest that MYCN and TFIIIC exert an censoring function in early transcription that limits promoter accumulation of inactive RNAPII and facilitates promoter-proximal degradation of nascent RNA., Competing Interests: RV, EL, SH, MM, DF, CS, DP, IR, LU, CA, PG, RB, GB No competing interests declared, ME founder and shareholder of Tucana Biosciences, (© 2024, Vidal et al.)

Published

2024

34. CDK12 controls transcription at damaged genes and prevents MYC-induced transcription-replication conflicts.

Author

Curti L, Rohban S, Bianchi N, Croci O, Andronache A, Barozzi S, Mattioli M, Ricci F, Pastori E, Sberna S, Bellotti S, Accialini A, Ballarino R, Crosetto N, Wade M, Parazzoli D, and Campaner S

Subjects

Humans, DNA Breaks, Double-Stranded, Proto-Oncogene Proteins c-myc metabolism, Proto-Oncogene Proteins c-myc genetics, Cell Line, Tumor, RNA Polymerase II metabolism, RNA Polymerase II genetics, DNA Damage, Cyclin-Dependent Kinases metabolism, Cyclin-Dependent Kinases genetics, DNA Replication, Transcription, Genetic

Abstract

The identification of genes involved in replicative stress is key to understanding cancer evolution and to identify therapeutic targets. Here, we show that CDK12 prevents transcription-replication conflicts (TRCs) and the activation of cytotoxic replicative stress upon deregulation of the MYC oncogene. CDK12 was recruited at damaged genes by PARP-dependent DDR-signaling and elongation-competent RNAPII, to repress transcription. Either loss or chemical inhibition of CDK12 led to DDR-resistant transcription of damaged genes. Loss of CDK12 exacerbated TRCs in MYC-overexpressing cells and led to the accumulation of double-strand DNA breaks, occurring between co-directional early-replicating regions and transcribed genes. Overall, our data demonstrate that CDK12 protects genome integrity by repressing transcription of damaged genes, which is required for proper resolution of DSBs at oncogene-induced TRCs. This provides a rationale that explains both how CDK12 deficiency can promote tandem duplications of early-replicated regions during tumor evolution, and how CDK12 targeting can exacerbate replicative-stress in tumors., (© 2024. The Author(s).)

Published

2024

35. Coordination of transcription-coupled repair and repair-independent release of lesion-stalled RNA polymerase II.

Author

Zhu Y, Zhang X, Gao M, Huang Y, Tan Y, Parnas A, Wu S, Zhan D, Adar S, and Hu J

Subjects

Humans, Ubiquitin-Specific Peptidase 7 metabolism, Ubiquitin-Specific Peptidase 7 genetics, Valosin Containing Protein metabolism, Valosin Containing Protein genetics, Proteasome Endopeptidase Complex metabolism, Excision Repair, RNA Polymerase II metabolism, DNA Repair, Ubiquitination, Transcription, Genetic, DNA Damage

Abstract

Transcription-blocking lesions (TBLs) stall elongating RNA polymerase II (Pol II), which then initiates transcription-coupled repair (TCR) to remove TBLs and allow transcription recovery. In the absence of TCR, eviction of lesion-stalled Pol II is required for alternative pathways to address the damage, but the mechanism is unclear. Using Protein-Associated DNA Damage Sequencing (PADD-seq), this study reveals that the p97-proteasome pathway can evict lesion-stalled Pol II independently of repair. Both TCR and repair-independent eviction require CSA and ubiquitination. However, p97 is dispensable for TCR and Pol II eviction in TCR-proficient cells, highlighting repair's prioritization over repair-independent eviction. Moreover, ubiquitination of RPB1-K1268 is important for both pathways, with USP7's deubiquitinase activity promoting TCR without abolishing repair-independent Pol II release. In summary, this study elucidates the fate of lesion-stalled Pol II, and may shed light on the molecular basis of genetic diseases caused by the defects of TCR genes., (© 2024. The Author(s).)

Published

2024

36. Cell-type-specific loops linked to RNA polymerase II elongation in human neural differentiation.

Author

Titus KR, Simandi Z, Chandrashekar H, Paquet D, and Phillips-Cremins JE

Subjects

Humans, Promoter Regions, Genetic genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, Cell Differentiation genetics, Neural Stem Cells metabolism, Neural Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Induced Pluripotent Stem Cells cytology, Neurons metabolism, Neurons cytology

Abstract

DNA is folded into higher-order structures that shape and are shaped by genome function. The role of long-range loops in the establishment of new gene expression patterns during cell fate transitions remains poorly understood. Here, we investigate the link between cell-specific loops and RNA polymerase II (RNA Pol II) during neural lineage commitment. We find thousands of loops decommissioned or gained de novo upon differentiation of human induced pluripotent stem cells (hiPSCs) to neural progenitor cells (NPCs) and post-mitotic neurons. During hiPSC-to-NPC and NPC-to-neuron transitions, genes changing from RNA Pol II initiation to elongation are >4-fold more likely to anchor cell-specific loops than repressed genes. Elongated genes exhibit significant mRNA upregulation when connected in cell-specific promoter-enhancer loops but not invariant promoter-enhancer loops or promoter-promoter loops or when unlooped. Genes transitioning from repression to RNA Pol II initiation exhibit a slight mRNA increase independent of loop status. Our data link cell-specific loops and robust RNA Pol II-mediated elongation during neural cell fate transitions., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

37. Molecular insights into type I interferon suppression and enhanced pathogenicity by species B human adenoviruses B7 and B14.

Author

Graves D, Akkerman N, Fulham L, Helwer R, and Pelka P

Subjects

Humans, STAT2 Transcription Factor metabolism, STAT2 Transcription Factor genetics, Immunity, Innate, RNA Polymerase II metabolism, RNA Polymerase II genetics, Signal Transduction, Adenovirus Infections, Human virology, Adenovirus Infections, Human immunology, Virulence, Host-Pathogen Interactions immunology, Animals, Promoter Regions, Genetic, Immune Evasion, A549 Cells, Adenoviruses, Human genetics, Adenoviruses, Human pathogenicity, Adenoviruses, Human physiology, Adenoviruses, Human immunology, Interferon Type I immunology, Interferon Type I metabolism, Interferon Type I genetics

Abstract

Human adenoviruses (HAdVs) are small DNA viruses that generally cause mild disease. Certain strains, particularly those belonging to species B HAdVs, can cause severe pneumonia and have a relatively high mortality rate. Little is known about the molecular aspects of how these highly pathogenic species affect the infected cell and how they suppress innate immunity. The present study provides molecular insights into how species B adenoviruses suppress the interferon signaling pathway. Our study shows that these viruses, unlike HAdV-C2, are resistant to type I interferon. This resistance likely arises due to the highly efficient suppression of interferon-stimulated gene expression. Unlike in HAdV-C2, HAdV-B7 and B14 sequester STAT2 and RNA polymerase II from interferon-stimulated gene promoters in infected cells. This results in suppressed interferon- stimulated gene activation. In addition, we show that RuvBL1 and RuvBL2, cofactors important for RNA polymerase II recruitment to promoters and interferon-stimulated gene activation, are redirected to the cytoplasm forming high molecular weight complexes that, likely, are unable to associate with chromatin. Proteomic analysis also identified key differences in the way these viruses affect the host cell, providing insights into species B-associated high pathogenicity. Curiously, we observed that at the level of protein expression changes to the infected cell, HAdV-C2 and B7 were more similar than those of the same species, B7 and B14. Collectively, our study represents the first such study of innate immune suppression by the highly pathogenic HAdV-B7 and B14, laying an important foundation for future investigations.IMPORTANCEHuman adenoviruses form a large family of double-stranded DNA viruses known for a variety of usually mild diseases. Certain strains of human adenovirus cause severe pneumonia leading to much higher mortality and morbidity than most other strains. The reasons for this enhanced pathogenicity are unknown. Our study provides a molecular investigation of how these highly pathogenic strains might inactivate the interferon signaling pathway, highlighting the lack of sensitivity of these viruses to type I interferon in general while providing a global picture of how viral changes in cellular proteins drive worse disease outcomes., Competing Interests: The authors declare no conflict of interest.

Published

2024

38. Increased transcriptional elongation and RNA stability of GPCR ligand binding genes unveiled via RNA polymerase II degradation.

Author

Bao L, Zhu J, Shi T, Jiang Y, Li B, Huang J, and Ji X

Subjects

Humans, Ligands, Jumonji Domain-Containing Histone Demethylases metabolism, Jumonji Domain-Containing Histone Demethylases genetics, Alpha-Amanitin pharmacology, Phosphorylation, RNA, Messenger metabolism, RNA, Messenger genetics, Histones metabolism, Proteolysis, RNA Polymerase II metabolism, RNA Polymerase II genetics, RNA Stability, Transcription Elongation, Genetic

Abstract

RNA polymerase II drives mRNA gene expression, yet our understanding of Pol II degradation is limited. Using auxin-inducible degron, we degraded Pol II's RPB1 subunit, resulting in global repression. Surprisingly, certain genes exhibited increased RNA levels post-degradation. These genes are associated with GPCR ligand binding and are characterized by being less paused and comprising polycomb-bound short genes. RPB1 degradation globally increased KDM6B binding, which was insufficient to explain specific gene activation. In contrast, RPB2 degradation repressed nearly all genes, accompanied by decreased H3K9me3 and SUV39H1 occupancy. We observed a specific increase in serine 2 phosphorylated Pol II and RNA stability for RPB1 degradation-upregulated genes. Additionally, α-amanitin or UV treatment resulted in RPB1 degradation and global gene repression, unveiling subsets of upregulated genes. Our findings highlight the activated transcription elongation and increased RNA stability of signaling genes as potential mechanisms for mammalian cells to counter RPB1 degradation during stress., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

39. Blocker-SELEX: a structure-guided strategy for developing inhibitory aptamers disrupting undruggable transcription factor interactions.

Author

Li T, Liu X, Qian H, Zhang S, Hou Y, Zhang Y, Luo G, Zhu X, Tao Y, Fan M, Wang H, Sha C, Lin A, Qin J, Gu K, Chen W, Fu T, Wang Y, Wei Y, Wu Q, and Tan W

Subjects

Humans, Protein Binding, Cell Proliferation drug effects, RNA Polymerase II metabolism, HEK293 Cells, Proto-Oncogene Proteins c-myc metabolism, Proto-Oncogene Proteins c-myc genetics, Proto-Oncogene Proteins c-myc antagonists & inhibitors, Aptamers, Nucleotide pharmacology, Aptamers, Nucleotide chemistry, Aptamers, Nucleotide metabolism, Transcription Factors metabolism, SELEX Aptamer Technique

Abstract

Despite the well-established significance of transcription factors (TFs) in pathogenesis, their utilization as pharmacological targets has been limited by the inherent challenges in modulating their protein interactions. The lack of defined small-molecule binding pockets and the nuclear localization of TFs do not favor the use of traditional tools. Aptamers possess large molecular weights, expansive blocking surfaces and efficient cellular internalization, making them compelling tools for modulating TF interactions. Here, we report a structure-guided design strategy called Blocker-SELEX to develop inhibitory aptamers (iAptamers) that selectively block TF interactions. Our approach leads to the discovery of iAptamers that cooperatively disrupt SCAF4/SCAF8-RNAP2 interactions, dysregulating RNAP2-dependent gene expression, which impairs cell proliferation. This approach is further applied to develop iAptamers blocking WDR5-MYC interactions. Overall, our study highlights the potential of iAptamers in disrupting pathogenic TF interactions, implicating their potential utility in studying the biological functions of TF interactions and in nucleic acids drug discovery., (© 2024. The Author(s).)

Published

2024

40. Assessing contributions of DNA sequences at the 3' end of a yeast gene on yFACT, RNA polymerase II, and nucleosome occupancy.

Author

Byrd SE, Hoyt B, Ozersky SA, Crocker AW, Habenicht D, Nester MR, Prowse H, Turkal CE, Joseph L, and Duina AA

Subjects

Transcriptional Elongation Factors genetics, Transcriptional Elongation Factors metabolism, Histone Chaperones genetics, Histone Chaperones metabolism, DNA, Fungal genetics, DNA, Fungal metabolism, Alleles, Base Sequence, Gene Expression Regulation, Fungal, Transcription, Genetic, Nucleosomes metabolism, Nucleosomes genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism

Abstract

Objective: In past work in budding yeast, we identified a nucleosomal region required for proper interactions between the histone chaperone complex yFACT and transcribed genes. Specific histone mutations within this region cause a shift in yFACT occupancy towards the 3' end of genes, a defect that we have attributed to impaired yFACT dissociation from DNA following transcription. In this work we wished to assess the contributions of DNA sequences at the 3' end of genes in promoting yFACT dissociation upon transcription termination., Results: We generated fourteen different alleles of the constitutively expressed yeast gene PMA1, each lacking a distinct DNA fragment across its 3' end, and assessed their effects on occupancy of the yFACT component Spt16. Whereas most of these alleles conferred no defects on Spt16 occupancy, one did cause a modest increase in Spt16 binding at the gene's 3' end. Interestingly, the same allele also caused minor retention of RNA Polymerase II (Pol II) and altered nucleosome occupancy across the same region of the gene. These results suggest that specific DNA sequences at the 3' ends of genes can play roles in promoting efficient yFACT and Pol II dissociation from genes and can also contribute to proper chromatin architecture., (© 2024. The Author(s).)

Published

2024

41. A critical role for Pol II CTD phosphorylation in heterochromatic gene activation.

Author

Kainth AS, Zhang H, and Gross DS

Subjects

Phosphorylation, Transcriptional Activation, Gene Expression Regulation, Fungal, Histones metabolism, Serine metabolism, Heterochromatin metabolism, Heterochromatin genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, RNA Polymerase II metabolism, RNA Polymerase II genetics, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics

Abstract

How gene activation works in heterochromatin, and how the mechanism might differ from the one used in euchromatin, has been largely unexplored. Previous work has shown that in SIR-regulated heterochromatin of Saccharomyces cerevisiae, gene activation occurs in the absence of covalent histone modifications and other alterations of chromatin commonly associated with transcription.Here we demonstrate that such activation occurs in a substantial fraction of cells, consistent with frequent transcriptional bursting, and this raises the possibility that an alternative activation pathway might be used. We address one such possibility, Pol II CTD phosphorylation, and explore this idea using a natural telomere-linked gene, YFR057w, as a model. Unlike covalent histone modifications, we find that Ser2, Ser5 and Ser7 CTD phosphorylated Pol II is prevalent at the drug-induced heterochromatic gene. Particularly enriched relative to the euchromatic state is Ser2 phosphorylation. Consistent with a functional role for Ser2P, YFR057w is negligibly activated in cells deficient in the Ser2 CTD kinases Ctk1 and Bur1 even though the gene is strongly stimulated when it is placed in a euchromatic context. Collectively, our results are consistent with a critical role for Ser2 CTD phosphorylation in driving Pol II recruitment and transcription of a natural heterochromatic gene - an activity that may supplant the need for histone epigenetic modifications., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: David S. Gross reports financial support was provided by National Institutes of Health. David S. Gross reports financial support was provided by National Science Foundation Division of Molecular and Cellular Biosciences. If there are other authors, they declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

42. Structural basis of Cdk7 activation by dual T-loop phosphorylation.

Author

Düster R, Anand K, Binder SC, Schmitz M, Gatterdam K, Fisher RP, and Geyer M

Subjects

Phosphorylation, Humans, Cyclin H metabolism, Cyclin H chemistry, Cyclin H genetics, Crystallography, X-Ray, RNA Polymerase II metabolism, RNA Polymerase II chemistry, Transcription Factor TFIIH metabolism, Transcription Factor TFIIH chemistry, Transcription Factor TFIIH genetics, Models, Molecular, Transcription Factors metabolism, Transcription Factors chemistry, Transcription Factors genetics, Protein Domains, Cell Cycle Proteins, Cyclin-Dependent Kinases metabolism, Cyclin-Dependent Kinases chemistry, Cyclin-Dependent Kinases genetics, Cyclin-Dependent Kinase-Activating Kinase

Abstract

Cyclin-dependent kinase 7 (Cdk7) is required in cell-cycle and transcriptional regulation owing to its function as both a CDK-activating kinase (CAK) and part of transcription factor TFIIH. Cdk7 forms active complexes by associating with Cyclin H and Mat1, and is regulated by two phosphorylations in the activation segment (T loop): the canonical activating modification at T170 and another at S164. Here we report the crystal structure of the human Cdk7/Cyclin H/Mat1 complex containing both T-loop phosphorylations. Whereas pT170 coordinates basic residues conserved in other CDKs, pS164 nucleates an arginine network unique to the ternary Cdk7 complex, involving all three subunits. We identify differential dependencies of kinase activity and substrate recognition on the individual phosphorylations. CAK function is unaffected by T-loop phosphorylation, whereas activity towards non-CDK substrates is increased several-fold by T170 phosphorylation. Moreover, dual T-loop phosphorylation stimulates multisite phosphorylation of the RNA polymerase II (RNAPII) carboxy-terminal domain (CTD) and SPT5 carboxy-terminal repeat (CTR) region. In human cells, Cdk7 activation is a two-step process wherein S164 phosphorylation precedes, and may prime, T170 phosphorylation. Thus, dual T-loop phosphorylation can regulate Cdk7 through multiple mechanisms, with pS164 supporting tripartite complex formation and possibly influencing processivity, while pT170 enhances activity towards key transcriptional substrates., (© 2024. The Author(s).)

Published

2024

43. Transcription of damage-induced RNA in Arabidopsis was frequently initiated from DSB loci within the genic regions.

Author

Kawaguchi K, Satoh S, and Obokata J

Subjects

RNA, Plant genetics, RNA, Plant metabolism, Gene Expression Regulation, Plant, RNA Polymerase II metabolism, RNA Polymerase II genetics, Arabidopsis genetics, Arabidopsis metabolism, DNA Breaks, Double-Stranded, Transcription, Genetic, DNA Repair

Abstract

DNA double-strand breaks (DSBs) are the most severe DNA lesions and need to be removed immediately to prevent loss of genomic information. Recently, it has been revealed that DSBs induce novel transcription from the cleavage sites in various species, resulting in RNAs being referred to as damage-induced RNAs (diRNAs). While diRNA synthesis is an early event in the DNA damage response and plays an essential role in DSB repair activation, the location where diRNAs are newly generated in plants remains unclear, as does their transcriptional mechanism. Here, we performed the sequencing of polyadenylated (polyA) diRNAs that emerged around all DSB loci in Arabidopsis thaliana under the expression of the exogenous restriction enzyme Sbf I and observed 88 diRNAs transcribed via RNA polymerase II in 360 DSB loci. Most of the detected diRNAs originated within active genes and were transcribed from DSBs in a bidirectional manner. Furthermore, we found that diRNA elongation tends to terminate at the boundary of an endogenous gene located near DSB loci. Our results provide reliable evidence for understanding the importance of new transcription at DSBs and show that diRNA is a crucial factor for successful DSB repair., (© 2024 Molecular Biology Society of Japan and John Wiley & Sons Australia, Ltd.)

Published

2024

44. Transcription directionality is licensed by Integrator at active human promoters.

Author

Yang J, Li J, Miao L, Gao X, Sun W, Linghu S, Ren G, Peng B, Chen S, Liu Z, Wang B, Dong A, Huang D, Yuan J, Dang Y, and Lai F

Subjects

Humans, Phosphorylation, RNA Precursors metabolism, RNA Precursors genetics, HeLa Cells, Transcription Initiation Site, RNA Polymerase II metabolism, Promoter Regions, Genetic genetics, Transcription, Genetic

Abstract

A universal characteristic of eukaryotic transcription is that the promoter recruits RNA polymerase II (RNAPII) to produce both precursor mRNAs (pre-mRNAs) and short unstable promoter upstream transcripts (PROMPTs) toward the opposite direction. However, how the transcription machinery selects the correct direction to produce pre-mRNAs is largely unknown. Here, through multiple acute auxin-inducible degradation systems, we show that rapid depletion of an RNAPII-binding protein complex, Integrator, results in robust PROMPT accumulation throughout the genome. Interestingly, the accumulation of PROMPTs is compensated by the reduction of pre-mRNA transcripts in actively transcribed genes. Consistently, Integrator depletion alters the distribution of polymerase between the sense and antisense directions, which is marked by increased RNAPII-carboxy-terminal domain Tyr1 phosphorylation at PROMPT regions and a reduced Ser2 phosphorylation level at transcription start sites. Mechanistically, the endonuclease activity of Integrator is critical to suppress PROMPT production. Furthermore, our data indicate that the presence of U1 binding sites on nascent transcripts could counteract the cleavage activity of Integrator. In this process, the absence of robust U1 signal at most PROMPTs allows Integrator to suppress the antisense transcription and shift the transcriptional balance in favor of the sense direction., (© 2024. The Author(s), under exclusive licence to Springer Nature America, Inc.)

Published

2024

45. Human RNA Polymerase II Segregates from Genes and Nascent RNA and Transcribes in the Presence of DNA-Bound dCas9.

Author

Pessoa J and Carvalho C

Subjects

Humans, DNA metabolism, DNA genetics, Promoter Regions, Genetic, CRISPR-Associated Protein 9 metabolism, CRISPR-Associated Protein 9 genetics, CRISPR-Cas Systems, RNA genetics, RNA metabolism, RNA, Guide, CRISPR-Cas Systems genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Cell Line, RNA Polymerase II metabolism, RNA Polymerase II genetics, Transcription, Genetic, beta-Globins genetics, beta-Globins metabolism

Abstract

RNA polymerase II (Pol II) dysfunction is frequently implied in human disease. Understanding its functional mechanism is essential for designing innovative therapeutic strategies. To visualize its supra-molecular interactions with genes and nascent RNA, we generated a human cell line carrying ~335 consecutive copies of a recombinant β-globin gene. Confocal microscopy showed that Pol II was not homogeneously concentrated around these identical gene copies. Moreover, Pol II signals partially overlapped with the genes and their nascent RNA, revealing extensive compartmentalization. Using a cell line carrying a single copy of the β-globin gene, we also tested if the binding of catalytically dead CRISPR-associated system 9 (dCas9) to different gene regions affected Pol II transcriptional activity. We assessed Pol II localization and nascent RNA levels using chromatin immunoprecipitation and droplet digital reverse transcription PCR, respectively. Some enrichment of transcriptionally paused Pol II accumulated in the promoter region was detected in a strand-specific way of gRNA binding, and there was no decrease in nascent RNA levels. Pol II preserved its transcriptional activity in the presence of DNA-bound dCas9. Our findings contribute further insight into the complex mechanism of mRNA transcription in human cells.

Published

2024

46. Defining a chromatin architecture that supports transcription at RNA polymerase II promoters.

Author

Fisher MJ and Luse DS

Subjects

Humans, Animals, Transcription Initiation Site, RNA Polymerase II metabolism, RNA Polymerase II genetics, Promoter Regions, Genetic, Nucleosomes metabolism, Nucleosomes genetics, Histones metabolism, Histones genetics, Transcription, Genetic, Transcription Factor TFIID metabolism, Transcription Factor TFIID genetics, Chromatin metabolism, Chromatin genetics

Abstract

Mammalian RNA polymerase II preinitiation complexes assemble adjacent to a nucleosome whose proximal edge (NPE) is typically 40 to 50 bp downstream of the transcription start site. At active promoters, that +1 nucleosome is universally modified by trimethylation on lysine 4 of histone H3 (H3K4me3). The Pol II preinitiation complex only extends 35 bp beyond the transcription start site, but nucleosomal templates with an NPE at +51 are nearly inactive in vitro with promoters that lack a TATA element and thus depend on TFIID for promoter recognition. Significantly, this inhibition is relieved when the +1 nucleosome contains H3K4me3, which can interact with TFIID subunits. Here, we show that H3K4me3 templates with both TATA and TATA-less promoters are active with +35 NPEs when transcription is driven by TFIID. Templates with +20 NPE are also active but at reduced levels compared to +35 and +51 NPEs, consistent with a general inhibition of promoter function when the proximal nucleosome encroaches on the preinitiation complex. Remarkably, dinucleosome templates support transcription when H3K4me3 is only present in the distal nucleosome, suggesting that TFIID-H3K4me3 interaction does not require modification of the +1 nucleosome. Transcription reactions performed with an alternative protocol retaining most nuclear factors results primarily in early termination, with a minority of complexes successfully traversing the first nucleosome. In such reactions, the +1 nucleosome does not substantially affect the level of termination even with an NPE of +20, indicating that a nucleosome barrier is not a major driver of early termination by Pol II., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

47. 3D chromatin structures associated with ncRNA roX2 for hyperactivation and coactivation across the entire X chromosome.

Author

Tian SZ, Yang Y, Ning D, Fang K, Jing K, Huang G, Xu Y, Yin P, Huang H, Chen G, Deng Y, Zhang S, Zhang Z, Chen Z, Gao T, Chen W, Li G, Tian R, Ruan Y, Li Y, and Zheng M

Subjects

Animals, RNA, Untranslated genetics, Gene Expression Regulation, Dosage Compensation, Genetic, Promoter Regions, Genetic, Transcription Initiation Site, Chromatin metabolism, Chromatin genetics, X Chromosome genetics, RNA Polymerase II metabolism, RNA Polymerase II genetics

Abstract

The three-dimensional (3D) organization of chromatin within the nucleus is crucial for gene regulation. However, the 3D architectural features that coordinate the activation of an entire chromosome remain largely unknown. We introduce an omics method, RNA-associated chromatin DNA-DNA interactions, that integrates RNA polymerase II (RNAPII)-mediated regulome with stochastic optical reconstruction microscopy to investigate the landscape of noncoding RNA roX2 -associated chromatin topology for gene equalization to achieve dosage compensation. Our findings reveal that roX2 anchors to the target gene transcription end sites (TESs) and spreads in a distinctive boot-shaped configuration, promoting a more open chromatin state for hyperactivation. Furthermore, roX2 arches TES to transcription start sites to enhance transcriptional loops, potentially facilitating RNAPII convoying and connecting proximal promoter-promoter transcriptional hubs for synergistic gene regulation. These TESs cluster as roX2 compartments, surrounded by inactive domains for coactivation of multiple genes within the roX2 territory. In addition, roX2 structures gradually form and scaffold for stepwise coactivation in dosage compensation.

Published

2024

48. Elf1 promotes transcription-coupled repair in yeast by using its C-terminal domain to bind TFIIH.

Author

Selvam K, Xu J, Wilson HE, Oh J, Li Q, Wang D, and Wyrick JJ

Subjects

Protein Binding, Transcription, Genetic, Ultraviolet Rays, Protein Domains, RNA Polymerase II metabolism, RNA Polymerase II genetics, DNA Damage, Pyrimidine Dimers metabolism, Excision Repair, Transcription Factor TFIIH metabolism, Transcription Factor TFIIH genetics, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, DNA Repair, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics

Abstract

Transcription coupled-nucleotide excision repair (TC-NER) removes DNA lesions that block RNA polymerase II (Pol II) transcription. A key step in TC-NER is the recruitment of the TFIIH complex, which initiates DNA unwinding and damage verification; however, the mechanism by which TFIIH is recruited during TC-NER, particularly in yeast, remains unclear. Here, we show that the C-terminal domain (CTD) of elongation factor-1 (Elf1) plays a critical role in TC-NER in yeast by binding TFIIH. Analysis of genome-wide repair of UV-induced cyclobutane pyrimidine dimers (CPDs) using CPD-seq indicates that the Elf1 CTD in yeast is required for efficient TC-NER. We show that the Elf1 CTD binds to the pleckstrin homology (PH) domain of the p62 subunit of TFIIH in vitro, and identify a putative TFIIH-interaction region (TIR) in the Elf1 CTD that is important for PH binding and TC-NER. The Elf1 TIR shows functional, structural, and sequence similarities to a conserved TIR in the mammalian UV sensitivity syndrome A (UVSSA) protein, which recruits TFIIH during TC-NER in mammalian cells. These findings suggest that the Elf1 CTD acts as a functional counterpart to mammalian UVSSA in TC-NER by recruiting TFIIH in response to Pol II stalling at DNA lesions., (© 2024. The Author(s).)

Published

2024

49. An enhancer RNA recruits KMT2A to regulate transcription of Myb.

Author

Kim J, Diaz LF, Miller MJ, Leadem B, Krivega I, and Dean A

Subjects

Animals, Mice, RNA Polymerase II metabolism, RNA, Long Noncoding genetics, RNA, Long Noncoding metabolism, Humans, Cyclin-Dependent Kinase 9 metabolism, Cyclin-Dependent Kinase 9 genetics, Proto-Oncogene Mas, Protein Binding, Cell Differentiation genetics, Enhancer RNAs, Proto-Oncogene Proteins c-myb metabolism, Proto-Oncogene Proteins c-myb genetics, Myeloid-Lymphoid Leukemia Protein metabolism, Myeloid-Lymphoid Leukemia Protein genetics, Histone-Lysine N-Methyltransferase metabolism, Histone-Lysine N-Methyltransferase genetics, Enhancer Elements, Genetic genetics, Transcription, Genetic

Abstract

The Myb proto-oncogene encodes the transcription factor c-MYB, which is critical for hematopoiesis. Distant enhancers of Myb form a hub of interactions with the Myb promoter. We identified a long non-coding RNA (Myrlin) originating from the -81-kb murine Myb enhancer. Myrlin and Myb are coordinately regulated during erythroid differentiation. Myrlin TSS deletion using CRISPR-Cas9 reduced Myrlin and Myb expression and LDB1 complex occupancy at the Myb enhancers, compromising enhancer contacts and reducing RNA Pol II occupancy in the locus. In contrast, CRISPRi silencing of Myrlin left LDB1 and the Myb enhancer hub unperturbed, although Myrlin and Myb expressions were downregulated, decoupling transcription and chromatin looping. Myrlin interacts with the KMT2A/MLL1 complex. Myrlin CRISPRi compromised KMT2A occupancy in the Myb locus, decreasing CDK9 and RNA Pol II binding and resulting in Pol II pausing in the Myb first exon/intron. Thus, Myrlin directly participates in activating Myb transcription by recruiting KMT2A., Competing Interests: Declaration of interests The authors declare no competing interests., (Published by Elsevier Inc.)

Published

2024

50. Mechanomemory of nucleoplasm and RNA polymerase II after chromatin stretching by a microinjected magnetic nanoparticle force.

Author

Rashid F, Kabbo SA, and Wang N

Subjects

Animals, Humans, Magnetite Nanoparticles chemistry, Transcription, Genetic, Mice, Biomechanical Phenomena, RNA Polymerase II metabolism, Chromatin metabolism, Cell Nucleus metabolism

Abstract

Increasing evidence suggests that the mechanics of chromatin and nucleoplasm regulate gene transcription and nuclear function. However, how the chromatin and nucleoplasm sense and respond to forces remains elusive. Here, we employed a strategy of applying forces directly to the chromatin of a cell via a microinjected 200-nm anti-H2B-antibody-coated ferromagnetic nanoparticle (FMNP) and an anti-immunoglobulin G (IgG)-antibody-coated or an uncoated FMNP. The chromatin behaved as a viscoelastic gel-like structure and the nucleoplasm was a softer viscoelastic structure at loading frequencies of 0.1-5 Hz. Protein diffusivity of the chromatin, nucleoplasm, and RNA polymerase II (RNA Pol II) and RNA Pol II activity were upregulated in a chromatin-stretching-dependent manner and stayed upregulated for tens of minutes after force cessation. Chromatin stiffness increased, but the mechanomemory duration of chromatin diffusivity decreased, with substrate stiffness. These findings may provide a mechanomemory mechanism of transcription upregulation and have implications on cell and nuclear functions., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024