Your search keyword '"Drosophila Proteins chemistry"' showing total 3,193 results

1. Structural basis of endo-siRNA processing by Drosophila Dicer-2 and Loqs-PD.

Author

Cao N, Wang J, Deng T, Fan B, Su S, Ma J, and Wang HW

Subjects

Animals, RNA-Binding Proteins metabolism, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, Models, Molecular, Adenosine Triphosphate metabolism, Cryoelectron Microscopy, RNA, Double-Stranded metabolism, RNA, Double-Stranded chemistry, RNA, Double-Stranded genetics, Protein Binding, RNA Precursors metabolism, RNA Precursors chemistry, Ribonuclease III metabolism, Ribonuclease III chemistry, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, RNA Helicases metabolism, RNA Helicases chemistry, RNA Helicases genetics, RNA, Small Interfering metabolism, RNA, Small Interfering genetics, RNA, Small Interfering chemistry, Drosophila melanogaster genetics, Drosophila melanogaster metabolism

Abstract

Endogenous small interfering RNAs (endo-siRNAs or esiRNAs) originate from either elongated endogenous transcripts capable of forming complex fold-back structures or from double-stranded regions generated through intermolecular base pairing of convergently transcribed mRNAs. The mechanism of maturation and functionality of esiRNAs exhibit significant variation across diverse species. In Drosophila melanogaster, esiRNAs reside in both somatic and germline cells, where they serve as post-transcriptional modulators for specific target RNAs. Their maturation process critically relies on Dicer-2 (Dcr-2), with the assistance of its cofactor Loqs-PD. In this study, we have successfully elucidated the cryo-EM structures of Dcr-2/Loqs-PD complex bound to esiRNA precursors (pre-esiRNAs) in various states. Our structural and biochemical results reveal that ATP is essential for the cleavage of esiRNAs by the Dcr-2/Loqs-PD complex, a process analogous to the cleavage of double-stranded RNA (dsRNA). When Loqs-PD is present, pre-esiRNAs are preferentially loaded onto the Helicase domain of Dcr-2. Moreover, as the Helicase domain exhibits a preference for binding to the rigid end of double-stranded RNA, Dcr-2 tends to cleave pre-esiRNA from the small closed loop end, rather than the loose and flexible open end., (© The Author(s) 2025. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2025

2. Chemical and temporal manipulation of early steps in protein assembly tunes the structure and intermolecular interactions of protein-based materials.

Author

Italia V, Jons A, Kaparthi B, Faulk B, Maccarini M, Bertoncello P, Meissner K, Martin DK, and Bondos SE

Subjects

Animals, Tyrosine chemistry, Tyrosine analogs & derivatives, Intrinsically Disordered Proteins chemistry, Intrinsically Disordered Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins metabolism

Abstract

The Drosophila intrinsically disordered protein Ultrabithorax (Ubx) undergoes a series of phase transitions, beginning with noncovalent interactions between apparently randomly organized monomers, and evolving over time to form increasingly ordered coacervates. This assembly process ends when specific dityrosine covalent bonds lock the monomers in place, forming macroscale materials. Inspired by this hierarchical, multistep assembly process, we analyzed the impact of protein concentration, assembly time, and subphase composition on the early, noncovalent stages of Ubx assembly, which are extremely sensitive to their environment. We discovered that in low salt buffers, we can generate a new type of Ubx material from early coacervates using 5-fold less protein, and 100-fold less assembly time. Comparison of the new materials with standard Ubx fibers also revealed differences in the extent of wrinkling on the fiber surface. A new image analysis technique based on autocorrelation of scanning electron microscopy (SEM) images was developed to quantify these structural differences. These differences extend to the molecular level: new materials form more dityrosine covalent cross-links per monomer, but without requiring the specific tyrosine residues necessary for crosslinking previously established materials. We conclude that varying the assembly conditions represents a facile and inexpensive process for creating new materials. Most new biopolymers are created by changing the composition of the monomers or the method used to drive assembly. In contrast, in this study we used the same monomers and assembly approach, but altered the assembly time and chemical environment to create a new material with unique properties., (© 2025 The Protein Society.)

Published

2025

3. Cryo-EM structures reveal the H + /citrate symport mechanism of Drosophila INDY.

Author

Kim S, Park JG, Choi SH, Kim JW, and Jin MS

Subjects

Animals, Models, Molecular, Drosophila melanogaster metabolism, Protein Conformation, Symporters metabolism, Symporters chemistry, Drosophila metabolism, Cryoelectron Microscopy methods, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Citric Acid metabolism

Abstract

Drosophila I'm Not Dead Yet (INDY) functions as a transporter for citrate, a key metabolite in the citric acid cycle, across the plasma membrane. Partial deficiency of INDY extends lifespan, akin to the effects of caloric restriction. In this work, we use cryo-electron microscopy to determine structures of INDY in the presence and absence of citrate and in complex with the well-known inhibitor 4,4'-diisothiocyano-2,2'-disulfonic acid stilbene (DIDS) at resolutions ranging from 2.7 to 3.6 Å. Together with functional data obtained in vitro, the INDY structures reveal the H + /citrate co-transport mechanism, in which aromatic residue F119 serves as a one-gate element. They also provide insight into how protein-lipid interactions at the dimerization interface affect the stability and function of the transporter, and how DIDS disrupts the transport cycle., (© 2025 Kim et al.)

Published

2025

4. Structural basis for the interaction between the Drosophila RTK Sevenless (dROS1) and the GPCR BOSS.

Author

Zhang J, Tsutsui Y, Li H, Li T, Wang Y, Laraki S, Alarcon-Frias S, Stayrook SE, and Klein DE

Subjects

Animals, Drosophila melanogaster metabolism, Receptors, G-Protein-Coupled metabolism, Receptors, G-Protein-Coupled chemistry, Receptors, G-Protein-Coupled genetics, Models, Molecular, Humans, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Cryoelectron Microscopy, Receptor Protein-Tyrosine Kinases metabolism, Receptor Protein-Tyrosine Kinases genetics, Receptor Protein-Tyrosine Kinases chemistry, Protein Binding

Abstract

Sevenless, the Drosophila homologue of ROS1 (University of Rochester Sarcoma) (herein, dROS1) is a receptor tyrosine kinase (RTK) essential for the differentiation of Drosophila R7 photoreceptor cells. Activation of dROS1 is mediated by binding to the extracellular region (ECR) of the GPCR (G protein coupled receptor) BOSS (Bride Of Sevenless) on adjacent cells. Activation of dROS1 by BOSS leads to subsequent downstream signaling pathways including SOS (Son of Sevenless). However, the physical basis for how dROS1 interacts with BOSS has long remained unknown. Here we provide a cryo-EM structure of dROS1's extracellular region, which mediates ligand binding. We show that the extracellular region of dROS1 adopts a folded-over conformation stabilized by an N-terminal domain comprised of two disulfide stapled helical hairpins. We further narrowed down the interacting binding epitopes on both dROS1 and BOSS using hydrogen-deuterium exchange mass spectrometry (HDX-MS). This includes beta-strands in dROS1's third Fibronectin type III (FNIII) domain and a C-terminal peptide in BOSS' ECR. Our mutagenesis studies, coupled with AlphaFold complex predictions, support a binding interaction mediated by a hydrophobic interaction and beta-strand augmentation between these regions. Our findings provide a fundamental understanding of the regulatory function of dROS1 and further provide mechanistic insight into the human ortholog and oncogene ROS1., Competing Interests: Competing interests: The authors declare no competing interests., (© 2025. The Author(s).)

Published

2025

5. Unique and Common Agonists Activate the Insect Juvenile Hormone Receptor and the Human AHR.

Author

Sedlak D, Tuma R, Kolla JN, Mokhamatam RB, Bahrova L, Lisova M, Bittova L, and Jindra M

Subjects

Animals, Humans, Signal Transduction drug effects, Ligands, Cell Line, Protein Binding, Transcription Factors metabolism, Transcription Factors genetics, Juvenile Hormones metabolism, Juvenile Hormones pharmacology, Receptors, Aryl Hydrocarbon agonists, Receptors, Aryl Hydrocarbon metabolism, Receptors, Aryl Hydrocarbon genetics, Drosophila melanogaster metabolism, Drosophila melanogaster genetics, Drosophila melanogaster drug effects, Basic Helix-Loop-Helix Transcription Factors metabolism, Basic Helix-Loop-Helix Transcription Factors genetics, Basic Helix-Loop-Helix Transcription Factors agonists, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry

Abstract

Transcription factors of the bHLH-PAS family play vital roles in animal development, physiology, and disease. Two members of the family require binding of low-molecular weight ligands for their activity: the vertebrate aryl hydrocarbon receptor (AHR) and the insect juvenile hormone receptor (JHR). In the fly Drosophila melanogaster, the paralogous proteins GCE and MET constitute the ligand-binding component of JHR complexes. Whilst GCE/MET and AHR are phylogenetically heterologous, their mode of action is similar. JHR is targeted by several synthetic agonists that serve as insecticides disrupting the insect endocrine system. AHR is an important regulator of human endocrine homeostasis, and it responds to environmental pollutants and endocrine disruptors. Whether AHR signaling is affected by compounds that can activate JHR has not been reported. To address this question, we screened a chemical library of 50,000 compounds to identify 93 novel JHR agonists in a reporter system based on Drosophila cells. Of these compounds, 26% modulated AHR signaling in an analogous reporter assay in a human cell line, indicating a significant overlap in the agonist repertoires of the two receptors. To explore the structural features of agonist-dependent activation of JHR and AHR, we compared the ligand-binding cavities and their interactions with selective and common ligands of AHR and GCE. Molecular dynamics modeling revealed ligand-specific as well as conserved side chains within the respective cavities. Significance of predicted interactions was supported through site-directed mutagenesis. The results have indicated that synthetic insect juvenile hormone agonists might interfere with AHR signaling in human cells., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: “DS and MJ have co-founded a start-up Preagon Biotech, s.r.o”., (Copyright © 2024 Elsevier Ltd. All rights reserved.)

Published

2025

6. Nanoscale Visualization of Drosophila E-cadherin Ectodomain Fragments and Their Interactions Using DNA Origami Nanoblocks.

Author

Oda H, Nishiguchi S, Song C, Murata K, Uchihashi T, and Suzuki Y

Subjects

Animals, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila metabolism, Biotin chemistry, Biotin metabolism, Protein Domains, Cell Adhesion, Nanostructures chemistry, Protein Binding, Drosophila melanogaster metabolism, Microscopy, Electron, Transmission, Streptavidin chemistry, Streptavidin metabolism, Cadherins chemistry, Cadherins metabolism, Cadherins genetics, DNA metabolism, DNA chemistry, Microscopy, Atomic Force methods

Abstract

The adhesive function of cell surface proteins can be visually assessed through direct observation; however, the underlying structures that mediate adhesion typically remain invisible at the nanoscale level. This hinders knowledge on the diversity of molecular architectures responsible for cell-cell adhesion. Drosophila E-cadherin (DE-cadherin), a classical cadherin with a unique domain structure, demonstrates adhesive function; however, it lacks a structural model that explains its adhesion mechanism. Here, we present a novel application of DNA origami technology to create a cell-free, flat environment in which full DE-cadherin ectodomains are anchored using SNAP-tags and biotin-streptavidin interactions. DNA origami was assembled into a 120 nm long block, bearing 5 or 14 biotin:streptavidin sites that were evenly spaced on one lateral face. DE-cadherin ectodomain fragments were attached via biotinylated SNAP-tags. These decorated DNA origami nanoblocks were subjected to transmission electron and high-speed atomic force microscopy, which revealed a hinge-like site that separated the membrane-distal and -proximal portions of the DE-cadherin ectodomain, suggesting a role in mechanical flexibility. We also observed interactions between DE-cadherin ectodomains via their membrane-distal portions on single DNA origami nanoblocks. We reconstituted an adhesion-like process via pairing DNA origami nanoblocks using DE-cadherin ectodomain interactions. Homophilic associations of functional DE-cadherin ectodomains between the paired DNA origami nanoblocks were visualized at the nanoscale, displaying strand-like molecular configurations, likely representing the extracellular cadherin repeats without regular arrays of structural elements. This study introduces a DNA origami-based platform for reconstituting and visualizing cadherin ectodomain interactions, with potential applications for a broader range of adhesion molecules., 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 Elsevier Ltd. All rights reserved.)

Published

2025

7. Morphogen-induced kinase condensates transduce Hh signal by allosterically activating Gli.

Author

Han Y, Zhou M, Wang B, and Jiang J

Subjects

Animals, Allosteric Regulation, Phosphorylation, Transcription Factors metabolism, Transcription Factors genetics, Transcription Factors chemistry, Protein Serine-Threonine Kinases metabolism, Protein Serine-Threonine Kinases chemistry, Protein Serine-Threonine Kinases genetics, Zinc Finger Protein GLI1 metabolism, Zinc Finger Protein GLI1 genetics, Protein Binding, Humans, Hedgehog Proteins metabolism, Signal Transduction, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics

Abstract

Hedgehog (Hh) morphogen governs embryonic development and tissue homeostasis through the Ci/Gli family transcription factors. Here we report that Hh induces phase separation of the fused (Fu)/Ulk family kinases to allosterically regulate Ci/Gli. We find that Hh-induced phosphorylation of Fu/Ulk3 promotes SUMOylation of their inverted phosphorylation-dependent SUMOylation motifs. Subsequent interaction between SUMO and SUMO-interacting motif drives Fu/Ulk3 self-assembly to form biomolecular condensates that recruit Ci-Sufu and Gli-Sufu in the cytoplasm and primary cilium, respectively. Within the condensates, Fu/Ulk3 undergoes a conformational change to expose Ci/Gli for Fu/Ulk3-mediated phosphorylation and activation, leading to gradual accumulation of nuclear Ci A /Gli A transcriptional complexes in proportion to ligand dose and exposure time. Our findings provide mechanistic insights into the spatiotemporal control of Hh signal transduction, reveal previously unexplored regulatory mechanism and function for biomolecular condensation, and establish a paradigm for kinase-mediated signal transduction whereby a kinase allosterically activates its substrate through ligand-induced and condensation-driven conformational change.

Published

2025

8. Structure of an ex vivoDrosophila TOM complex determined by single-particle cryoEM.

Author

Periasamy A, Ornelas P, Bausewein T, Mitchell N, Zhao J, Quinn LM, Kuehlbrandt W, and Gulbis JM

Subjects

Animals, Humans, Models, Molecular, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Mitochondrial Precursor Protein Import Complex Proteins, Protein Conformation, Cryoelectron Microscopy methods, Drosophila melanogaster

Abstract

Most mitochondrial precursor proteins are encoded in the cell nucleus and synthesized on cytoplasmic ribosomes. The translocase of the outer membrane (TOM) is the main protein-import pore of mitochondria, recognizing nascent precursors of mitochondrially targeted proteins and transferring them across the outer membrane. A 3.3 Å resolution map and molecular model of a TOM complex from Drosophila melanogaster, obtained by single-particle electron cryomicroscopy, is presented. As the first reported structure of a transgenic protein expressed and purified ex vivo from Drosophila, the method provides impetus for parallel structural and genetic analyses of protein complexes linked to human pathology. The core TOM complex extracted from native membranes of the D. melanogaster retina contains transgenic Tom40 co-assembled with four endogenous TOM components: Tom22, Tom5, Tom6 and Tom7. The Drosophila TOM structure presented here shows that the human and Drosophila TOM are very similar, with small conformational changes at two subunit interfaces attributable to variation in lipid-binding residues. The new structure provides an opportunity to pinpoint general features that differentiate the TOM structures of higher and unicellular eukaryotes. While the quaternary fold of the assembly is retained, local nuances of structural elements implicated in precursor import are indicative of subtle evolutionary change., (open access.)

Published

2025

9. Patterning Functional Proteins in Ultrabithorax-Based Materials.

Author

Faulk B, Jons A, Fong BL, Lara M, Irion AR, and Bondos SE

Subjects

Animals, Biocompatible Materials chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Drosophila melanogaster metabolism, Homeodomain Proteins genetics, Homeodomain Proteins metabolism, Transcription Factors metabolism, Transcription Factors genetics

Abstract

The ability to add bioactivities, such as cell signaling or ligand recognition, to biomaterials has generated the potential to include multiple bioactivities into a single material. In some cases, it is desirable to localize these activities to different areas of the biomaterial, creating functional patterns. While photolithography and 3D printing have been effective techniques for patterning functions in many materials, patterning remains a challenge in materials composed of protein, in part due to how these materials are artificially assembled. Protein fibers are often produced from protein films that co-acervate at the air-water interface. This chapter describes methods to leverage this coacervation process to pattern materials, using the Drosophila melanogaster Hox protein Ultrabithorax (Ubx) as a model self-assembling protein. Through gene fusion, Ubx and a functional protein are produced as a single polypeptide, capable of both forming materials and performing the activity of interest. This functionality is retained in the final materials. In this chapter, we describe how to use multiple Ubx fusion proteins to not only imbue the final materials with multiple functions, but also to create macroscale patterns of the appended proteins in fibrous protein-based materials. These patterned materials include striped fibers, bifunctional-faced fibers, gradient fibers, and core-shell fibers., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

10. The Drosophila RNA binding protein Hrp48 binds a specific RNA sequence of the msl-2 mRNA 3' UTR to regulate translation.

Author

Lomoschitz A, Meyer J, Guitart T, Krepl M, Lapouge K, Hayn C, Schweimer K, Simon B, Šponer J, Gebauer F, and Hennig J

Subjects

Animals, Protein Biosynthesis, RNA, Messenger metabolism, RNA, Messenger genetics, RNA, Messenger chemistry, Molecular Dynamics Simulation, Protein Binding, Binding Sites, Transcription Factors metabolism, Transcription Factors chemistry, Transcription Factors genetics, DNA-Binding Proteins, Heterogeneous-Nuclear Ribonucleoproteins, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, 3' Untranslated Regions, RNA-Binding Proteins metabolism, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, Drosophila melanogaster metabolism, Drosophila melanogaster genetics

Abstract

Repression of msl-2 mRNA translation is essential for viability of Drosophila melanogaster females to prevent hypertranscription of both X chromosomes. This translational control event is coordinated by the female-specific protein Sex-lethal (Sxl) which recruits the RNA binding proteins Unr and Hrp48 to the 3' untranslated region (UTR) of the msl-2 transcript and represses translation initiation. The mechanism exerted by Hrp48 during translation repression and its interaction with msl-2 are not well understood. Here we investigate the RNA binding specificity and affinity of the tandem RNA recognition motifs of Hrp48. Using NMR spectroscopy, molecular dynamics simulations and isothermal titration calorimetry, we identified the exact region of msl-2 3' UTR recognized by Hrp48. Additional biophysical experiments and translation assays give further insights into complex formation of Hrp48, Unr, Sxl and RNA. Our results show that Hrp48 binds independent of Sxl and Unr downstream of the E and F binding sites of Sxl and Unr to msl-2., 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 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2025

11. Enzyme fragment complementation driven by nucleic acid hybridization sans self-labeling protein.

Author

Xu Z, Zhang X, Pal C, Rozners E, and Callahan BP

Subjects

Animals, RNA metabolism, RNA chemistry, Biosensing Techniques methods, Luciferases metabolism, Luciferases chemistry, Luciferases genetics, DNA, Single-Stranded chemistry, DNA, Single-Stranded metabolism, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Nucleic Acid Hybridization

Abstract

A modified enzyme fragment complementation assay has been designed and validated as a turn-on biosensor for nucleic acid detection in dilute aqueous solution. The assay is target sequence-agonistic and uses fragments of NanoBiT, the split luciferase reporter enzyme, that are esterified enzymatically at their C-termini to steramers, sterol-linked oligonucleotides. The Drosophila hedgehog autoprocessing domain, DHhC, serves as the self-cleaving enzyme for the NanoBiT-steramer bioconjugations. Unlike current approaches, the final bioconjugate generated by DHhC and used for nucleic acid detection is free of self-labeling passenger protein. In the presence of single stranded (ss) DNA or RNA template with adjacent segments complementary to the Nano-BiT steramer oligonucleotides, the two NanoBiT fragments associate productively, reconstituting NanoBiT's luciferase activity. In samples containing ssDNA or RNA template at low nM concentrations, NanoBiT luminescence exceeded background signal by 30- to 60-fold. The steramer probe sequences used to prepare these sensors are unconstrained in length and composition. In the absence of sequence constraints of the probe element and without the added bulk of a self-labeling protein, these NanoBiT-steramer bioconjugates open new applications in the programmable detection of small fragments of coding and noncoding DNA and RNA., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Brian Callahan has patent #US 10,738,338 B2 issued to SUNY Research Foundation of New York. Brian Callahan has patent #U.S. 12,077,795 issued to SUNY Research Foundation of New York. 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 Elsevier Inc. All rights reserved.)

Published

2025

12. N-terminus of Drosophila melanogaster MSL1 is critical for dosage compensation.

Author

Babosha V, Klimenko N, Revel-Muroz A, Tikhonova E, Georgiev P, and Maksimenko O

Subjects

Animals, Male, Female, Transcription Factors metabolism, Transcription Factors genetics, Transcription Factors chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, DNA-Binding Proteins chemistry, Protein Binding, Nuclear Proteins, Dosage Compensation, Genetic, Drosophila Proteins genetics, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, X Chromosome genetics

Abstract

The male-specific lethal complex (MSL), which consists of five proteins and two non-coding roX RNAs, is involved in the transcriptional enhancement of X-linked genes to compensate for the sex chromosome monosomy in Drosophila XY males compared with XX females. The MSL1 and MSL2 proteins form the heterotetrameric core of the MSL complex and are critical for the specific recruitment of the complex to the high-affinity 'entry' sites (HAS) on the X chromosome. In this study, we demonstrated that the N-terminal region of MSL1 is critical for stability and functions of MSL1. Amino acid deletions and substitutions in the N-terminal region of MSL1 strongly affect both the interaction with roX2 RNA and the MSL complex binding to HAS on the X chromosome. In particular, substitution of the conserved N-terminal amino-acids 3-7 in MSL1 (MSL1 GS ) affects male viability similar to the inactivation of genes encoding roX RNAs. In addition, MSL1 GS binds to promoters such as MSL1 WT but does not co-bind with MSL2 and MSL3 to X chromosomal HAS. However, overexpression of MSL2 partially restores the dosage compensation. Thus, the interaction of MSL1 with roX RNA is critical for the efficient assembly of the MSL complex on HAS of the male X chromosome., Competing Interests: VB, NK, AR, ET, PG, OM No competing interests declared, (© 2024, Babosha et al.)

Published

2024

13. The Drosophila toothrin Gene Related to the d4 Family Genes: An Evolutionary View on Origin and Function.

Author

Kuvaeva EE, Cherezov RO, Kulikova DA, and Mertsalov IB

Subjects

Animals, Drosophila melanogaster genetics, Multigene Family, Transcription Factors genetics, Transcription Factors metabolism, Gene Duplication, Protein Domains, Evolution, Molecular, Drosophila Proteins genetics, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Phylogeny

Abstract

D. melanogaster has two paralogs, tth and dd4 , related to the evolutionarily conserved d4 family genes. In mammals, the family consists of Dpf1-3 , encoding transcription co-factors involved in the regulation of development and cell fate determination. The function of tth and dd4 in Drosophila remains unclear. The typical domain structure of the proteins encoded by the d4 family consists of an N-terminal 2/3 domain (Requiem_N), a central Kruppel-type zinc finger, and a C-terminal D4 domain of paired PHD zinc fingers (DPFs). In Drosophila , both paralogs lack the Kruppel-type ZF, and tth encodes a protein that contains only Requiem_N. In contrast, vertebrate Dpf1-3 paralogs encode all the domains, but some paralogs have specific splice isoforms. For example, the DPF3a isoform lacks the D4 domain necessary for histone reading. The occurrence of proteins without the D4 domain in mammals and flies implies functional significance and analogous roles across animal taxa. In this study, we reconstructed the evolutionary events that led to the emergence of Drosophila tth by analyzing the divergence of d4 paralogs across different evolutionary lineages. Our genomic and transcriptomic data analysis revealed duplications and gene copy loss events. Among insects, gene duplication was only observed in Diptera. In other lineages, we found the specialization of paralogs for producing isoforms and further specialization for coding proteins with specific domain organizations. We hypothesize that this pathway is a common mechanism for the emergence of paralogues lacking the D4 domain across different evolutionary lineages. We, thus, postulate that TTH may function as a splice isoform of the ancestral single-copy gene, possibly a DPF3a-like isoform characteristic of related insect species. Our analysis provides insights into the possible impact of paralogue divergence, emphasizing the functional significance of the 2/3 domain and the potential roles of isoforms lacking the D4 domain.

Published

2024

14. Structures and pH-dependent dimerization of the sevenless receptor tyrosine kinase.

Author

Cerutti G, Arias R, Bahna F, Mannepalli S, Katsamba PS, Ahlsen G, Kloss B, Bruni R, Tomlinson A, and Shapiro L

Subjects

Animals, Hydrogen-Ion Concentration, Receptor Protein-Tyrosine Kinases metabolism, Receptor Protein-Tyrosine Kinases chemistry, Receptor Protein-Tyrosine Kinases genetics, Humans, Protein Binding, Models, Molecular, Signal Transduction, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Cryoelectron Microscopy, Protein Multimerization, Drosophila melanogaster genetics

Abstract

Sevenless (Sev) is a Drosophila receptor tyrosine kinase (RTK) required for the specification of the R7 photoreceptor. It is cleaved into α and β subunits and binds the ectodomain of the G-protein-coupled receptor bride of sevenless (Boss). Previous work showed that the Boss ectodomain could bind but not activate Sev; rather, the whole seven-pass transmembrane Boss was required. Here, we show that Sev does not need to be cleaved to function and that a single-pass transmembrane form of Boss activates Sev. We use cryo-electron microscopy and biophysical methods to determine the structural basis of ligand binding and pH-dependent dimerization of Sev, and we discuss the implications in the process of Sev activation. The Sev human homolog, receptor oncogene from sarcoma 1 (ROS1), is associated with oncogenic transformations, and we discuss their structural similarities., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

15. NMR chemical shift assignment of Drosophila odorant binding protein 44a in complex with 8(Z)-eicosenoic acid.

Author

Cotten ML, Starich MR, He Y, Yin J, Yuan Q, and Tjandra N

Subjects

Animals, Protein Binding, Fatty Acids, Monounsaturated chemistry, Fatty Acids, Monounsaturated metabolism, Amino Acid Sequence, Nuclear Magnetic Resonance, Biomolecular, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Drosophila melanogaster, Receptors, Odorant chemistry, Receptors, Odorant metabolism

Abstract

The odorant binding protein, OBP44a is one of the most abundant proteins expressed in the brain of the developing fruit fly Drosophila melanogaster. Its cellular function has not yet been determined. The OBP family of proteins is well established to recognize hydrophobic molecules. In this study, NMR is employed to structurally characterize OBP44a. NMR chemical shift perturbation measurements confirm that OBP44a binds to fatty acids. Complete assignments of the backbone chemical shifts and secondary chemical shift analysis demonstrate that the apo state of OBP44a is comprised of six α-helices. Upon binding 8(Z)-eicosenoic acid (8(Z)-C20:1), the OBP44a C-terminal region undergoes a conformational change, from unstructured to α-helical. In addition to C-terminal restructuring upon ligand binding, some hydrophobic residues show dramatic chemical shift changes. Surprisingly, several charged residues are also strongly affected by lipid binding. Some of these residues could represent key structural features that OBP44a relies on to perform its cellular function. The NMR chemical shift assignment is the first step towards characterizing the structure of OBP44a and how specific residues might play a role in lipid binding and release. This information will be important in deciphering the biological function of OBP44a during fly brain development., (© 2024. This is a U.S. Government work and not under copyright protection in the US; foreign copyright protection may apply.)

Published

2024

16. Biochemical Analysis of the Regulatory Role of Gα o in the Conformational Transitions of Drosophila Pins.

Author

Song Y, Ji J, Liu C, and Wang W

Subjects

Animals, Drosophila melanogaster metabolism, Protein Binding, Cell Cycle Proteins chemistry, Cell Cycle Proteins metabolism, Guanosine Diphosphate metabolism, Guanosine Diphosphate chemistry, Binding Sites, Drosophila Proteins chemistry, Drosophila Proteins metabolism, GTP-Binding Protein alpha Subunits, Gi-Go metabolism, GTP-Binding Protein alpha Subunits, Gi-Go chemistry, GTP-Binding Protein alpha Subunits, Gi-Go genetics, Protein Conformation

Abstract

Drosophila Pins (and its mammalian homologue LGN) play a crucial role in the process of asymmetric cell division (ACD). Extensive research has established that Pins/LGN functions as a conformational switch primarily through intramolecular interactions involving the N-terminal TPR repeats and the C-terminal GoLoco (GL) motifs. The GL motifs served as binding sites for the α subunit of the trimeric G protein (Gα), which facilitates the release of the autoinhibited conformation of Pins/LGN. While LGN has been observed to specifically bind to Gα i ·GDP, Pins has been found to associate with both Drosophila Gα i ( d Gα i ) and Gα o ( d Gα o ) isoforms. Moreover, d Gα o was reported to be able to bind Pins in both the GDP- and GTP-bound forms. However, the precise mechanism underlying the influence of d Gα o on the conformational states of Pins remains unclear, despite extensive investigations into the Gα i ·GDP-mediated regulatory conformational changes in LGN/Pins. In this study, we conducted a comprehensive characterization of the interactions between Pins-GL motifs and d Gα o in both GDP- and GTP-loaded forms. Our findings reveal that Pins-GL specifically binds to GDP-loaded d Gα o . Through biochemical characterization, we determined that the intramolecular interactions of Pins primarily involve the entire TPR domain and the GL23 motifs. Additionally, we observed that Pins can simultaneously bind three molecules of d Gα o ·GDP, leading to a partial opening of the autoinhibited conformation. Furthermore, our study presents evidence contrasting with previous observations indicating the absence of binding between d Gα i and Pins-GLs, thus implying the pivotal role of d Gα o as the principal participant in the ACD pathway associated with Pins.

Published

2024

17. Two Forms of Thick Filament in the Flight Muscle of Drosophila melanogaster .

Author

Rastegarpouyani H, Hojjatian A, and Taylor KA

Subjects

Animals, Cryoelectron Microscopy, Filamins metabolism, Muscle Proteins metabolism, Muscle Proteins chemistry, Muscle Proteins ultrastructure, Drosophila melanogaster metabolism, Drosophila melanogaster ultrastructure, Myosins metabolism, Flight, Animal physiology, Drosophila Proteins metabolism, Drosophila Proteins chemistry

Abstract

Invertebrate striated muscle myosin filaments are highly variable in structure. The best characterized myosin filaments are those found in insect indirect flight muscle (IFM) in which the flight-powering muscles are not attached directly to the wings. Four insect orders, Hemiptera, Diptera, Hymenoptera, and Coleoptera, have evolved IFM. IFM thick filaments from the first three orders have highly similar myosin arrangements but differ significantly among their non-myosin proteins. The cryo-electron microscopy of isolated IFM myosin filaments from the Dipteran Drosophila melanogaster described here revealed the coexistence of two distinct filament types, one presenting a tubular backbone like in previous work and the other a solid backbone. Inside an annulus of myosin tails, tubular filaments show no noticeable densities; solid filaments show four paired paramyosin densities. Both myosin heads of the tubular filaments are disordered; solid filaments have one completely and one partially immobilized head. Tubular filaments have the protein stretchin-klp on their surface; solid filaments do not. Two proteins, flightin and myofilin, are identifiable in all the IFM filaments previously determined. In Drosophila , flightin assumes two conformations, being compact in solid filaments and extended in tubular filaments. Nearly identical solid filaments occur in the large water bug Lethocerus indicus , which flies infrequently. The Drosophila tubular filaments occur in younger flies, and the solid filaments appear in older flies, which fly less frequently if at all, suggesting that the solid filament form is correlated with infrequent muscle use. We suggest that the solid form is designed to conserve ATP when the muscle is not in active use.

Published

2024

18. Structural requirements for activity of Mind bomb1 in Notch signaling.

Author

Cao R, Gozlan O, Airich A, Tveriakhina L, Zhou H, Jiang H, Cole PA, Aster JC, Klein T, Sprinzak D, and Blacklow SC

Subjects

Animals, Humans, Binding Sites, Crystallography, X-Ray, Drosophila melanogaster metabolism, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Models, Molecular, Protein Binding, Protein Multimerization, Ubiquitin-Conjugating Enzymes metabolism, Ubiquitin-Conjugating Enzymes chemistry, Ubiquitin-Conjugating Enzymes genetics, Ubiquitination, Receptors, Notch metabolism, Receptors, Notch chemistry, Signal Transduction, Ubiquitin-Protein Ligases metabolism, Ubiquitin-Protein Ligases chemistry, Ubiquitin-Protein Ligases genetics

Abstract

Mind bomb 1 (MIB1) is a RING E3 ligase that ubiquitinates Notch ligands, a necessary step for induction of Notch signaling. The structural basis for binding of the JAG1 ligand by the N-terminal region of MIB1 is known, yet how the ankyrin (ANK) and RING domains of MIB1 cooperate to catalyze ubiquitin transfer from E2∼Ub to Notch ligands remains unclear. Here, we show that the third RING domain and adjacent coiled coil region (ccRING3) drive MIB1 dimerization and that MIB1 ubiquitin transfer activity relies solely on ccRING3. We report X-ray crystal structures of a UbcH5B-ccRING3 complex and the ANK domain. Directly tethering the MIB1 N-terminal region to ccRING3 forms a minimal MIB1 protein sufficient to induce a Notch response in receiver cells and rescue mib knockout phenotypes in flies. Together, these studies define the functional elements of an E3 ligase needed for ligands to induce a Notch signaling response., Competing Interests: Declaration of interests S.C.B. is on the board of directors of the non-profit Institute for Protein Innovation and the Revson Foundation, is on the scientific advisory board for and receives funding from Erasca, Inc. for an unrelated project, is an advisor to MPM Capital, and is a consultant for IFM, Scorpion Therapeutics, Odyssey Therapeutics, Droia Ventures, and Ayala Pharmaceuticals for unrelated projects. J.C.A. is a consultant for Ayala Pharmaceuticals, Cellestia, Inc., SpringWorks Therapeutics, and Remix Therapeutics. P.A.C. has been a consultant for Scorpion Therapeutics, Nested Therapeutics, and Intonation Research Labs., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

19. Architecture of CTPS filament networks revealed by cryo-electron tomography.

Author

Fu Y, Guo CJ, Liu ZJ, and Liu JL

Subjects

Animals, Cytoskeleton ultrastructure, Cytoskeleton metabolism, Organelles ultrastructure, Organelles metabolism, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins ultrastructure, Female, Carbon-Nitrogen Ligases, Electron Microscope Tomography methods, Cryoelectron Microscopy methods, Drosophila melanogaster ultrastructure

Abstract

The cytoophidium is a novel type of membraneless organelle, first observed in the ovaries of Drosophila using fluorescence microscopy. In vitro, purified Drosophila melanogaster CTPS (dmCTPS) can form metabolic filaments under the presence of either substrates or products, and their structures that have been analyzed using cryo-electron microscopy (cryo-EM). These dmCTPS filaments are considered the fundamental units of cytoophidia. However, due to the resolution gap between light and electron microscopy, the precise assembly pattern of cytoophidia remains unclear. In this study, we find that dmCTPS filaments can spontaneously assemble in vitro, forming network structures that reach micron-scale dimensions. Using cryo-electron tomography (cryo-ET), we reconstruct the network structures formed by dmCTPS filaments under substrate or product binding conditions and elucidate their assembly process. The dmCTPS filaments initially form structural bundles, which then further assemble into larger networks. By identifying, tracking, and statistically analyzing the filaments, we observed distinct characteristics of the structural bundles formed under different conditions. This study provides the first systematic analysis of dmCTPS filament networks, offering new insights into the relationship between cytoophidia and metabolic filaments., Competing Interests: Declaration of competing interest The authors declare that no interest exists., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

20. Drosophila Protein Z4 Possesses ZAD Dimerization Domain.

Author

Bonchuk AN and Georgiev PG

Subjects

Animals, Protein Domains, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Drosophila Proteins metabolism, Protein Multimerization, Transcription Factors chemistry, Transcription Factors genetics, Transcription Factors metabolism

Abstract

The transcription factor Z4 (putzig) is one of the key proteins that determine the chromatin structure in Drosophila. Z4 is found at the boundaries of bands on polytene chromosomes, and the bands are currently thought to correlate with chromatin domains. Z4 is a component of a protein complex that additionally includes Chromator and BEAF-32, and a conserved domain is necessary to occur at the N end of Z4 to ensure its interaction with the two proteins. In this study, a zinc finger-associated domain (ZAD) domain was identified in Z4. The capability of dimerization was confirmed for the domain by biochemical methods. A dimer model of the domain was obtained using AlphaFold2, and the model structure was confirmed using small-angle X-ray scattering (SAXS). The dimer structure shows a fold typical of ZAD domains., (© 2024. Pleiades Publishing, Ltd.)

Published

2024

21. Wnt target gene activation requires β-catenin separation into biomolecular condensates.

Author

Stewart RA, Ding Z, Jeon US, Goodman LB, Tran JJ, Zientko JP, Sabu M, and Cadigan KM

Subjects

Animals, Humans, Biomolecular Condensates metabolism, Transcriptional Activation, Cell Nucleus metabolism, HEK293 Cells, Mutation, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Intrinsically Disordered Proteins metabolism, Intrinsically Disordered Proteins genetics, beta Catenin metabolism, Wnt Signaling Pathway, Lymphoid Enhancer-Binding Factor 1 metabolism, Lymphoid Enhancer-Binding Factor 1 genetics, Drosophila melanogaster metabolism, Drosophila melanogaster genetics

Abstract

The Wnt/β-catenin signaling pathway plays numerous essential roles in animal development and tissue/stem cell maintenance. The activation of genes regulated by Wnt/β-catenin signaling requires the nuclear accumulation of β-catenin, a transcriptional co-activator. β-catenin is recruited to many Wnt-regulated enhancers through direct binding to T-cell factor/lymphoid enhancer factor (TCF/LEF) family transcription factors. β-catenin has previously been reported to form phase-separated biomolecular condensates (BMCs), which was implicated as a component of β-catenin's mechanism of action. This function required aromatic amino acid residues in the intrinsically disordered regions (IDRs) at the N- and C-termini of the protein. In this report, we further explore a role for β-catenin BMCs in Wnt target gene regulation. We find that β-catenin BMCs are miscible with LEF1 BMCs in vitro and in cultured cells. We characterized a panel of β-catenin mutants with different combinations of aromatic residue mutations in human cell culture and Drosophila melanogaster. Our data support a model in which aromatic residues across both IDRs contribute to BMC formation and signaling activity. Although different Wnt targets have different sensitivities to loss of β-catenin's aromatic residues, the activation of every target examined was compromised by aromatic substitution. These mutants are not defective in nuclear import or co-immunoprecipitation with several β-catenin binding partners. In addition, residues in the N-terminal IDR with no previously known role in signaling are clearly required for the activation of various Wnt readouts. Consistent with this, deletion of the N-terminal IDR results in a loss of signaling activity, which can be rescued by the addition of heterologous IDRs enriched in aromatic residues. Overall, our work supports a model in which the ability of β-catenin to form biomolecular condensates in the nucleus is tightly linked to its function as a transcriptional co-regulator., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Stewart 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

22. Bound ion effects: Using machine learning method to study the kinesin Ncd's binding with microtubule.

Author

Guo W, Du D, Zhang H, Sanchez JE, Sun S, Xu W, Peng Y, and Li L

Subjects

Protein Multimerization, Ions chemistry, Static Electricity, Solvents chemistry, Animals, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Machine Learning, Kinesins chemistry, Kinesins metabolism, Microtubules metabolism, Microtubules chemistry, Protein Binding, Molecular Dynamics Simulation, Tubulin chemistry, Tubulin metabolism

Abstract

Drosophila Ncd proteins are motor proteins that play important roles in spindle organization. Ncd and the tubulin dimer are highly charged. Thus, it is crucial to investigate Ncd-tubulin dimer interactions in the presence of ions, especially ions that are bound or restricted at the Ncd-tubulin dimer binding interfaces. To consider the ion effects, widely used implicit solvent models treat ions implicitly in the continuous solvent environment without focusing on the individual ions' effects. But highly charged biomolecules such as the Ncd and tubulin dimer may capture some ions at highly charged regions as bound ions. Such bound ions are restricted to their binding sites; thus, they can be treated as part of the biomolecules. By applying multiscale computational methods, including the machine-learning-based Hybridizing Ions Treatment-2 program, molecular dynamics simulations, DelPhi, and DelPhiForce, we studied the interaction between the Ncd motor domain and the tubulin dimer using a hybrid solvent model, which considers the bound ions explicitly and the other ions implicitly in the solvent environment. To identify the importance of treating bound ions explicitly, we also performed calculations using the implicit solvent model without considering the individual bound ions. We found that the calculations of the electrostatic features differ significantly between those of the hybrid solvent model and the pure implicit solvent model. The analyses show that treating bound ions at highly charged regions explicitly is crucial for electrostatic calculations. This work proposes a machine-learning-based approach to handle the bound ions using the hybrid solvent model. Such an approach is not only capable of handling kinesin-tubulin complexes but is also appropriate for other highly charged biomolecules, such as DNA/RNA, viral capsid proteins, etc., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 Biophysical Society. Published by Elsevier Inc. All rights reserved.)

Published

2024

23. ISWI catalyzes nucleosome sliding in condensed nucleosome arrays.

Author

Vizjak P, Kamp D, Hepp N, Scacchetti A, Gonzalez Pisfil M, Bartho J, Halic M, Becker PB, Smolle M, Stigler J, and Mueller-Planitz F

Subjects

Animals, Chromatin Assembly and Disassembly, Adenosine Triphosphate metabolism, Drosophila melanogaster metabolism, Drosophila melanogaster genetics, Hydrolysis, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, DNA metabolism, DNA chemistry, Chromatin metabolism, Chromatin chemistry, Drosophila metabolism, Nucleosomes metabolism, Nucleosomes chemistry, Adenosine Triphosphatases metabolism, Adenosine Triphosphatases chemistry, Adenosine Triphosphatases genetics, Molecular Dynamics Simulation, Transcription Factors metabolism, Transcription Factors chemistry, Transcription Factors genetics

Abstract

How chromatin enzymes work in condensed chromatin and how they maintain diffusional mobility inside remains unexplored. Here we investigated these challenges using the Drosophila ISWI remodeling ATPase, which slides nucleosomes along DNA. Folding of chromatin fibers did not affect sliding in vitro. Catalytic rates were also comparable in- and outside of chromatin condensates. ISWI cross-links and thereby stiffens condensates, except when ATP hydrolysis is possible. Active hydrolysis is also required for ISWI's mobility in condensates. Energy from ATP hydrolysis therefore fuels ISWI's diffusion through chromatin and prevents ISWI from cross-linking chromatin. Molecular dynamics simulations of a 'monkey-bar' model in which ISWI grabs onto neighboring nucleosomes, then withdraws from one before rebinding another in an ATP hydrolysis-dependent manner, qualitatively agree with our data. We speculate that monkey-bar mechanisms could be shared with other chromatin factors and that changes in chromatin dynamics caused by mutations in remodelers could contribute to pathologies., (© 2024. The Author(s), under exclusive licence to Springer Nature America, Inc.)

Published

2024

24. Cryo-EM structure of the dopamine transporter with a novel atypical non-competitive inhibitor bound to the orthosteric site.

Author

Pedersen CN, Yang F, Ita S, Xu Y, Akunuri R, Trampari S, Neumann CMT, Desdorf LM, Schiøtt B, Salvino JM, Mortensen OV, Nissen P, and Shahsavar A

Subjects

Animals, Binding Sites drug effects, Dopamine Uptake Inhibitors pharmacology, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins antagonists & inhibitors, Cocaine pharmacology, Dopamine Plasma Membrane Transport Proteins metabolism, Dopamine Plasma Membrane Transport Proteins antagonists & inhibitors, Dopamine Plasma Membrane Transport Proteins chemistry, Cryoelectron Microscopy methods, Drosophila melanogaster

Abstract

The regulation of dopamine (DA) removal from the synaptic cleft is a crucial process in neurotransmission and is facilitated by the sodium- and chloride-coupled dopamine transporter DAT. Psychostimulant drugs, cocaine, and amphetamine, both block the uptake of DA, while amphetamine also triggers the release of DA. As a result, they prolong or even amplify neurotransmitter signaling. Atypical inhibitors of DAT lack cocaine-like rewarding effects and offer a promising strategy for the treatment of drug use disorders. Here, we present the 3.2 Å resolution cryo-electron microscopy structure of the Drosophila melanogaster dopamine transporter (dDAT) in complex with the atypical non-competitive inhibitor AC-4-248. The inhibitor partially binds at the central binding site, extending into the extracellular vestibule, and locks the transporter in an outward open conformation. Our findings propose mechanisms for the non-competitive inhibition of DAT and attenuation of cocaine potency by AC-4-248 and provide a basis for the rational design of more efficacious atypical inhibitors., (© 2024 The Author(s). Journal of Neurochemistry published by John Wiley & Sons Ltd on behalf of International Society for Neurochemistry.)

Published

2024

25. Chromosome structure in Drosophila is determined by boundary pairing not loop extrusion.

Author

Bing X, Ke W, Fujioka M, Kurbidaeva A, Levitt S, Levine M, Schedl P, and Jaynes JB

Subjects

Animals, Drosophila melanogaster genetics, Chromatin chemistry, Chromatin metabolism, Cohesins, Chromosomal Proteins, Non-Histone metabolism, Chromosomal Proteins, Non-Histone chemistry, Chromosomal Proteins, Non-Histone genetics, Chromosome Structures, Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, Cell Cycle Proteins chemistry, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Drosophila genetics

Abstract

Two different models have been proposed to explain how the endpoints of chromatin looped domains ('TADs') in eukaryotic chromosomes are determined. In the first, a cohesin complex extrudes a loop until it encounters a boundary element roadblock, generating a stem-loop. In this model, boundaries are functionally autonomous: they have an intrinsic ability to halt the movement of incoming cohesin complexes that is independent of the properties of neighboring boundaries. In the second, loops are generated by boundary:boundary pairing. In this model, boundaries are functionally non-autonomous, and their ability to form a loop depends upon how well they match with their neighbors. Moreover, unlike the loop-extrusion model, pairing interactions can generate both stem-loops and circle-loops. We have used a combination of MicroC to analyze how TADs are organized, and experimental manipulations of the even skipped TAD boundary, homie , to test the predictions of the 'loop-extrusion' and the 'boundary-pairing' models. Our findings are incompatible with the loop-extrusion model, and instead suggest that the endpoints of TADs in flies are determined by a mechanism in which boundary elements physically pair with their partners, either head-to-head or head-to-tail, with varying degrees of specificity. Although our experiments do not address how partners find each other, the mechanism is unlikely to require loop extrusion., Competing Interests: XB currently employed by a biotech company; however, this author's experimental contributions to the paper were done prior to taking the biotech job, WK, MF, AK, SL, ML, PS, JJ No competing interests declared, (© 2024, Bing, Ke, Fujioka et al.)

Published

2024

26. Sequence, Structure, and Functional Space of Drosophila De Novo Proteins.

Author

Middendorf L, Ravi Iyengar B, and Eicholt LA

Subjects

Animals, Evolution, Molecular, Machine Learning, Drosophila genetics, Drosophila melanogaster genetics, Protein Folding, Biomolecular Condensates metabolism, Biomolecular Condensates chemistry, Drosophila Proteins genetics, Drosophila Proteins chemistry, Drosophila Proteins metabolism

Abstract

During de novo emergence, new protein coding genes emerge from previously nongenic sequences. The de novo proteins they encode are dissimilar in composition and predicted biochemical properties to conserved proteins. However, functional de novo proteins indeed exist. Both identification of functional de novo proteins and their structural characterization are experimentally laborious. To identify functional and structured de novo proteins in silico, we applied recently developed machine learning based tools and found that most de novo proteins are indeed different from conserved proteins both in their structure and sequence. However, some de novo proteins are predicted to adopt known protein folds, participate in cellular reactions, and to form biomolecular condensates. Apart from broadening our understanding of de novo protein evolution, our study also provides a large set of testable hypotheses for focused experimental studies on structure and function of de novo proteins in Drosophila., (© The Author(s) 2024. Published by Oxford University Press on behalf of Society for Molecular Biology and Evolution.)

Published

2024

27. Organization of microtubule plus-end dynamics by phase separation in mitosis.

Author

Yang F, Ding M, Song X, Chen F, Yang T, Wang C, Hu C, Hu Q, Yao Y, Du S, Yao PY, Xia P, Adams G Jr, Fu C, Xiang S, Liu D, Wang Z, Yuan K, and Liu X

Subjects

Animals, Humans, Acetylation, HeLa Cells, Drosophila melanogaster metabolism, p300-CBP Transcription Factors metabolism, Kinesins metabolism, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Spindle Apparatus metabolism, Phase Separation, Microtubules metabolism, Mitosis, Microtubule-Associated Proteins metabolism, Chromosome Segregation, Kinetochores metabolism

Abstract

In eukaryotes, microtubule polymers are essential for cellular plasticity and fate decisions. End-binding (EB) proteins serve as scaffolds for orchestrating microtubule polymer dynamics and are essential for cellular dynamics and chromosome segregation in mitosis. Here, we show that EB1 forms molecular condensates with TIP150 and MCAK through liquid-liquid phase separation to compartmentalize the kinetochore-microtubule plus-end machinery, ensuring accurate kinetochore-microtubule interactions during chromosome segregation in mitosis. Perturbation of EB1-TIP150 polymer formation by a competing peptide prevents phase separation of the EB1-mediated complex and chromosome alignment at the metaphase equator in both cultured cells and Drosophila embryos. Lys220 of EB1 is dynamically acetylated by p300/CBP-associated factor in early mitosis, and persistent acetylation at Lys220 attenuates phase separation of the EB1-mediated complex, dissolves droplets in vitro, and harnesses accurate chromosome segregation. Our data suggest a novel framework for understanding the organization and regulation of eukaryotic spindle for accurate chromosome segregation in mitosis., (© The Author(s) (2024). Published by Oxford University Press on behalf of Journal of Molecular Cell Biology, CEMCS, CAS.)

Published

2024

28. Cooperative Gsx2-DNA binding requires DNA bending and a novel Gsx2 homeodomain interface.

Author

Webb JA, Farrow E, Cain B, Yuan Z, Yarawsky AE, Schoch E, Gagliani EK, Herr AB, Gebelein B, and Kovall RA

Subjects

Animals, Binding Sites, Nucleic Acid Conformation, Models, Molecular, Transcription Factors metabolism, Transcription Factors chemistry, DNA-Binding Proteins metabolism, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Humans, Thermodynamics, DNA metabolism, DNA chemistry, Homeodomain Proteins metabolism, Homeodomain Proteins chemistry, Homeodomain Proteins genetics, Protein Binding

Abstract

The conserved Gsx homeodomain (HD) transcription factors specify neural cell fates in animals from flies to mammals. Like many HD proteins, Gsx factors bind A/T-rich DNA sequences prompting the following question: How do HD factors that bind similar DNA sequences in vitro regulate specific target genes in vivo? Prior studies revealed that Gsx factors bind DNA both as a monomer on individual A/T-rich sites and as a cooperative homodimer to two sites spaced precisely 7 bp apart. However, the mechanistic basis for Gsx-DNA binding and cooperativity is poorly understood. Here, we used biochemical, biophysical, structural and modeling approaches to (i) show that Gsx factors are monomers in solution and require DNA for cooperative complex formation, (ii) define the affinity and thermodynamic binding parameters of Gsx2/DNA interactions, (iii) solve a high-resolution monomer/DNA structure that reveals that Gsx2 induces a 20° bend in DNA, (iv) identify a Gsx2 protein-protein interface required for cooperative DNA binding and (v) determine that flexible spacer DNA sequences enhance Gsx2 cooperativity on dimer sites. Altogether, our results provide a mechanistic basis for understanding the protein and DNA structural determinants that underlie cooperative DNA binding by Gsx factors., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

29. Discerning the Role of DNA Sequence, Shape, and Flexibility in Recognition by Drosophila Transcription Factors.

Author

Murthy S, Dey U, Olymon K, Abbas E, Yella VR, and Kumar A

Subjects

Animals, Binding Sites, Protein Binding, Base Sequence, Nucleic Acid Conformation, Transcription Factors metabolism, Transcription Factors chemistry, DNA metabolism, DNA chemistry, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry

Abstract

The precise spatial and temporal orchestration of gene expression is crucial for the ontogeny of an organism and is mainly governed by transcription factors (TFs). The mechanism of recognition of cognate sites amid millions of base pairs in the genome by TFs is still incompletely understood. In this study, we focus on DNA sequence composition, shape, and flexibility preferences of 28 quintessential TFs from Drosophila melanogaster that are critical to development and body patterning mechanisms. Our study finds that TFs exhibit distinct predilections for DNA shape, flexibility, and sequence compositions in the proximity of transcription factor binding sites (TFBSs). Notably, certain zinc finger proteins prefer GC-rich areas with less negative propeller twist, while homeodomains mainly seek AT-rich regions with a more negative propeller twist at their sites. Intriguingly, while numerous cofactors share similar binding site preferences and bind closer to each other in the genome, some cofactors that have different preferences bind farther apart. These findings shed light on TF DNA recognition and provide novel insights into possible cofactor binding and transcriptional regulation mechanisms.

Published

2024

30. The CNK-HYP scaffolding complex promotes RAF activation by enhancing KSR-MEK interaction.

Author

Maisonneuve P, Sahmi M, Bergeron-Labrecque F, Ma XI, Queguiner J, Arseneault G, Lefrançois M, Kurinov I, Fronzes R, Sicheri F, and Therrien M

Subjects

Animals, Humans, Cryoelectron Microscopy, raf Kinases metabolism, raf Kinases chemistry, Protein Binding, Protein Multimerization, Models, Molecular, Drosophila melanogaster metabolism, Mitogen-Activated Protein Kinase Kinases metabolism, Protein Kinases, ras Proteins, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics

Abstract

The RAS-MAPK pathway regulates cell proliferation, differentiation and survival, and its dysregulation is associated with cancer development. The pathway minimally comprises the small GTPase RAS and the kinases RAF, MEK and ERK. Activation of RAF by RAS is notoriously intricate and remains only partially understood. There are three RAF isoforms in mammals (ARAF, BRAF and CRAF) and two related pseudokinases (KSR1 and KSR2). RAS-mediated activation of RAF depends on an allosteric mechanism driven by the dimerization of its kinase domain. Recent work on human RAFs showed that MEK binding to KSR1 promotes KSR1-BRAF heterodimerization, which leads to the phosphorylation of free MEK molecules by BRAF. Similar findings were made with the single Drosophila RAF homolog. Here we show that the fly scaffold proteins CNK and HYP stabilize the KSR-MEK interaction, which in turn enhances RAF-KSR heterodimerization and RAF activation. The cryogenic electron microscopy structure of the minimal KSR-MEK-CNK-HYP complex reveals a ring-like arrangement of the CNK-HYP complex allowing CNK to simultaneously engage KSR and MEK, thus stabilizing the binary interaction. Together, these results illuminate how CNK contributes to RAF activation by stimulating the allosteric function of KSR and highlight the diversity of mechanisms impacting RAF dimerization as well as the regulatory potential of the KSR-MEK interaction., (© 2024. The Author(s).)

Published

2024

31. Key arginine residues in R2D2 dsRBD1 and dsRBD2 lead the siRNA recognition in Drosophila melanogaster RNAi pathway.

Author

Aute R, Waghela N, and Deshmukh MV

Subjects

Animals, Nuclear Magnetic Resonance, Biomolecular, Protein Folding, Protein Domains, Mutation, Mutagenesis, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, RNA Interference, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, Drosophila Proteins chemistry, Drosophila Proteins genetics, Arginine chemistry, Arginine genetics

Abstract

In Drosophila melanogaster, Dcr-2:R2D2 heterodimer binds to the 21 nucleotide siRNA duplex to form the R2D2/Dcr-2 Initiator (RDI) complex, which is critical for the initiation of siRNA-induced silencing complex (RISC) assembly. During RDI complex formation, R2D2, a protein that contains three dsRNA binding domains (dsRBD), senses two aspects of the siRNA: thermodynamically more stable end (asymmetry sensing) and the 5'-phosphate (5'-P) recognition. Despite several detailed studies to date, the molecular determinants arising from R2D2 for performing these two tasks remain elusive. In this study, we have performed structural, biophysical, and biochemical characterization of R2D2 dsRBDs. We found that the solution NMR-derived structure of R2D2 dsRBD1 yielded a canonical α1-β1-β2-β3-α2 fold, wherein two arginine salt bridges provide additional stability to the R2D2 dsRBD1. Furthermore, we show that R2D2 dsRBD1 interacts with thermodynamically asymmetric siRNA duplex independent of its 5'-phosphorylation state, whereas R2D2 dsRBD2 prefers to interact with 5'-P siRNA duplex. The mutation of key arginine residues, R53 and R101, in concatenated dsRBDs of R2D2 results in a significant loss of siRNA duplex recognition. Our study deciphers the active roles of R2D2 dsRBDs by showing that dsRBD1 initiates siRNA recognition, whereas dsRBD2 senses 5'-phosphate as an authentic mark on functional siRNA., Competing Interests: Declaration of competing interest The authors declare that they have no conflict of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

32. Structural Analysis of the Drosophila melanogaster GSTome.

Author

Petiot N, Schwartz M, Delarue P, Senet P, Neiers F, and Nicolaï A

Subjects

Animals, Binding Sites, Amino Acid Sequence, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Drosophila Proteins genetics, Models, Molecular, Crystallography, X-Ray, Glutathione metabolism, Glutathione chemistry, Protein Multimerization, Drosophila melanogaster enzymology, Glutathione Transferase chemistry, Glutathione Transferase metabolism, Glutathione Transferase genetics

Abstract

Glutathione transferase (GST) is a superfamily of ubiquitous enzymes, multigenic in numerous organisms and which generally present homodimeric structures. GSTs are involved in numerous biological functions such as chemical detoxification as well as chemoperception in mammals and insects. GSTs catalyze the conjugation of their cofactor, reduced glutathione (GSH), to xenobiotic electrophilic centers. To achieve this catalytic function, GSTs are comprised of a ligand binding site and a GSH binding site per subunit, which is very specific and highly conserved; the hydrophobic substrate binding site enables the binding of diverse substrates. In this work, we focus our interest in a model organism, the fruit fly Drosophila melanogaster ( D. mel ), which comprises 42 GST sequences distributed in six classes and composing its GSTome. The goal of this study is to describe the complete structural GSTome of D. mel to determine how changes in the amino acid sequence modify the structural characteristics of GST, particularly in the GSH binding sites and in the dimerization interface. First, we predicted the 3D atomic structures of each GST using the AlphaFold (AF) program and compared them with X-ray crystallography structures, when they exist. We also characterized and compared their global and local folds. Second, we used multiple sequence alignment coupled with AF-predicted structures to characterize the relationship between the conservation of amino acids in the sequence and their structural features. Finally, we applied normal mode analysis to estimate thermal B-factors of all GST structures of D. mel . Particularly, we extracted flexibility profiles of GST and identify key residues and motifs that are systematically involved in the ligand binding/dimerization processes and thus playing a crucial role in the catalytic function. This methodology will be extended to guide the in silico design of synthetic GST with new/optimal catalytic properties for detoxification applications.

Published

2024

33. Structural and Thermodynamic Insights into Dimerization Interfaces of Drosophila Glutathione Transferases.

Author

Schwartz M, Petiot N, Chaloyard J, Senty-Segault V, Lirussi F, Senet P, Nicolai A, Heydel JM, Canon F, Sonkaria S, Khare V, Didierjean C, and Neiers F

Subjects

Animals, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Crystallography, X-Ray, Drosophila melanogaster enzymology, Models, Molecular, Amino Acid Sequence, Drosophila enzymology, Thermodynamics, Glutathione Transferase chemistry, Glutathione Transferase metabolism, Glutathione Transferase genetics, Protein Multimerization

Abstract

This study presents a comprehensive analysis of the dimerization interfaces of fly GSTs through sequence alignment. Our investigation revealed GSTE1 as a particularly intriguing target, providing valuable insights into the variations within Delta and Epsilon GST interfaces. The X-ray structure of GSTE1 was determined, unveiling remarkable thermal stability and a distinctive dimerization interface. Utilizing circular dichroism, we assessed the thermal stability of GSTE1 and other Drosophila GSTs with resolved X-ray structures. The subsequent examination of GST dimer stability correlated with the dimerization interface supported by findings from X-ray structural analysis and thermal stability measurements. Our discussion extends to the broader context of GST dimer interfaces, offering a generalized perspective on their stability. This research enhances our understanding of the structural and thermodynamic aspects of GST dimerization, contributing valuable insights to the field.

Published

2024

34. Molecular mechanism of BMP signal control by Twisted gastrulation.

Author

Malinauskas T, Moore G, Rudolf AF, Eggington H, Belnoue-Davis HL, El Omari K, Griffiths SC, Woolley RE, Duman R, Wagner A, Leedham SJ, Baldock C, Ashe HL, and Siebold C

Subjects

Animals, Mice, Humans, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Glycoproteins metabolism, Glycoproteins genetics, Intercellular Signaling Peptides and Proteins metabolism, Intercellular Signaling Peptides and Proteins genetics, Binding Sites, Protein Domains, Protein Binding, Organoids metabolism, Organoids embryology, HEK293 Cells, Gastrulation genetics, Mutation, Crystallography, X-Ray, Drosophila melanogaster embryology, Drosophila melanogaster metabolism, Drosophila melanogaster genetics, Proteins, Bone Morphogenetic Proteins metabolism, Bone Morphogenetic Proteins genetics, Signal Transduction

Abstract

Twisted gastrulation (TWSG1) is an evolutionarily conserved secreted glycoprotein which controls signaling by Bone Morphogenetic Proteins (BMPs). TWSG1 binds BMPs and their antagonist Chordin to control BMP signaling during embryonic development, kidney regeneration and cancer. We report crystal structures of TWSG1 alone and in complex with a BMP ligand, Growth Differentiation Factor 5. TWSG1 is composed of two distinct, disulfide-rich domains. The TWSG1 N-terminal domain occupies the BMP type 1 receptor binding site on BMPs, whereas the C-terminal domain binds to a Chordin family member. We show that TWSG1 inhibits BMP function in cellular signaling assays and mouse colon organoids. This inhibitory function is abolished in a TWSG1 mutant that cannot bind BMPs. The same mutation in the Drosophila TWSG1 ortholog Tsg fails to mediate BMP gradient formation required for dorsal-ventral axis patterning of the early embryo. Our studies reveal the evolutionarily conserved mechanism of BMP signaling inhibition by TWSG1., (© 2024. The Author(s).)

Published

2024

35. Structure and Dynamics of Drk-SH2 Domain and Its Site-Specific Interaction with Sev Receptor Tyrosine Kinase.

Author

Sayeesh PM, Iguchi M, Inomata K, Ikeya T, and Ito Y

Subjects

Animals, Humans, Amino Acid Sequence, Binding Sites, GRB2 Adaptor Protein metabolism, GRB2 Adaptor Protein chemistry, Magnetic Resonance Spectroscopy, Molecular Docking Simulation, Receptor Protein-Tyrosine Kinases chemistry, Receptor Protein-Tyrosine Kinases metabolism, Drosophila melanogaster, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Molecular Dynamics Simulation, Protein Binding, src Homology Domains

Abstract

The Drosophila downstream receptor kinase (Drk), a homologue of human GRB2, participates in the signal transduction from the extracellular to the intracellular environment. Drk receives signals through the interaction of its Src homology 2 (SH2) domain with the phosphorylated tyrosine residue in the receptor tyrosine kinases (RTKs). Here, we present the solution NMR structure of the SH2 domain of Drk (Drk-SH2), which was determined in the presence of a phosphotyrosine (pY)-containing peptide derived from a receptor tyrosine kinase, Sevenless (Sev). The solution structure of Drk-SH2 possess a common SH2 domain architecture, consisting of three β strands imposed between two α helices. Additionally, we interpret the site-specific interactions of the Drk-SH2 domain with the pY-containing peptide through NMR titration experiments. The dynamics of Drk-SH2 were also analysed through NMR-relaxation experiments as well as the molecular dynamic simulation. The docking simulations of the pY-containing peptide onto the protein surface of Drk-SH2 provided the orientation of the peptide, which showed a good agreement with the analysis of the SH2 domain of GRB2.

Published

2024

36. Random, de novo, and conserved proteins: How structure and disorder predictors perform differently.

Author

Middendorf L and Eicholt LA

Subjects

Animals, Conserved Sequence, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Databases, Protein, Models, Molecular, Computational Biology methods, Proteins chemistry, Proteins metabolism, Intrinsically Disordered Proteins chemistry, Intrinsically Disordered Proteins metabolism, Protein Conformation, Amino Acid Sequence, Algorithms, Drosophila chemistry, Protein Folding

Abstract

Understanding the emergence and structural characteristics of de novo and random proteins is crucial for unraveling protein evolution and designing novel enzymes. However, experimental determination of their structures remains challenging. Recent advancements in protein structure prediction, particularly with AlphaFold2 (AF2), have expanded our knowledge of protein structures, but their applicability to de novo and random proteins is unclear. In this study, we investigate the structural predictions and confidence scores of AF2 and protein language model-based predictor ESMFold for de novo and conserved proteins from Drosophila and a dataset of comparable random proteins. We find that the structural predictions for de novo and random proteins differ significantly from conserved proteins. Interestingly, a positive correlation between disorder and confidence scores (pLDDT) is observed for de novo and random proteins, in contrast to the negative correlation observed for conserved proteins. Furthermore, the performance of structure predictors for de novo and random proteins is hampered by the lack of sequence identity. We also observe fluctuating median predicted disorder among different sequence length quartiles for random proteins, suggesting an influence of sequence length on disorder predictions. In conclusion, while structure predictors provide initial insights into the structural composition of de novo and random proteins, their accuracy and applicability to such proteins remain limited. Experimental determination of their structures is necessary for a comprehensive understanding. The positive correlation between disorder and pLDDT could imply a potential for conditional folding and transient binding interactions of de novo and random proteins., (© 2024 The Authors. Proteins: Structure, Function, and Bioinformatics published by Wiley Periodicals LLC.)

Published

2024

37. Carbohydrate-binding ability of a recombinant protein containing the DM9 motif from Drosophila melanogaster.

Author

Hatakeyama T, Kojima F, Ohkawachi I, Sawai H, and Unno H

Subjects

Animals, Amino Acid Motifs, Mannose metabolism, Binding Sites, Protein Binding, Drosophila melanogaster metabolism, Recombinant Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Drosophila Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics

Abstract

Proteins containing DM9 motifs, which were originally identified in the Drosophila melanogaster genome, are widely distributed in various organisms and are assumed to be involved in their innate immune response. In this study, we produced a recombinant protein of CG13321 (rCG13321) from D. melanogaster, which consists of four DM9 motifs, in Escherichia coli cells. In affinity chromatography using a mannose-immobilized column, rCG13321 exhibited mannose-binding ability and was separated into high-affinity and low-affinity fractions, named HA and LA, respectively, based on its binding ability to the column. In addition to having a higher affinity for the column, HA exhibited self-oligomerization ability, suggesting slight differences in tertiary structure. Both LA and HA showed hemagglutinating activity and were able to agglutinate an oligomannose-containing dendrimer, indicating that they have multiple carbohydrate-binding sites. Glycan array analysis suggested that rCG13321 primarily recognizes d-mannose and d-rhamnose through hydrogen bonding with the 2-, 3- and 4-hydroxy groups. Isothermal titration calorimetry demonstrated that rCG13321 has a comparable affinity to typical lectins. These findings suggest that CG13321 functions as a carbohydrate-binding protein or lectin that recognizes mannose and related carbohydrate-containing molecules on the surface of foreign organisms as a pattern recognition molecule., (© The Author(s) 2024. Published by Oxford University Press on behalf of the Japanese Biochemical Society. All rights reserved.)

Published

2024

38. The polarity protein Yurt associates with the plasma membrane via basic and hydrophobic motifs embedded in its FERM domain.

Author

Gamblin CL, Alende C, Corriveau F, Jetté A, Parent-Prévost F, Biehler C, Majeau N, Laurin M, and Laprise P

Subjects

Animals, Amino Acid Motifs, Drosophila melanogaster metabolism, Hydrophobic and Hydrophilic Interactions, Membrane Proteins metabolism, Membrane Proteins genetics, Membrane Proteins chemistry, Phospholipids metabolism, Protein Binding, Cell Membrane metabolism, Cell Polarity, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Protein Domains

Abstract

The subcellular distribution of the polarity protein Yurt (Yrt) is subjected to a spatio-temporal regulation in Drosophila melanogaster embryonic epithelia. After cellularization, Yrt binds to the lateral membrane of ectodermal cells and maintains this localization throughout embryogenesis. During terminal differentiation of the epidermis, Yrt accumulates at septate junctions and is also recruited to the apical domain. Although the mechanisms through which Yrt associates with septate junctions and the apical domain have been deciphered, how Yrt binds to the lateral membrane remains as an outstanding puzzle. Here, we show that the FERM domain of Yrt is necessary and sufficient for membrane localization. Our data also establish that the FERM domain of Yrt directly binds negatively charged phospholipids. Moreover, we demonstrate that positively charged amino acid motifs embedded within the FERM domain mediates Yrt membrane association. Finally, we provide evidence suggesting that Yrt membrane association is functionally important. Overall, our study highlights the molecular basis of how Yrt associates with the lateral membrane during the developmental time window where it is required for segregation of lateral and apical domains., Competing Interests: Competing interests The authors declare no competing or financial interests., (© 2024. Published by The Company of Biologists Ltd.)

Published

2024

39. The origin recognition complex requires chromatin tethering by a hypervariable intrinsically disordered region that is functionally conserved from sponge to man.

Author

Adiji OA, McConnell BS, and Parker MW

Subjects

Animals, Humans, Adenosine Triphosphate metabolism, DNA metabolism, DNA chemistry, DNA genetics, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Phosphorylation, Phylogeny, Protein Binding, Evolution, Molecular, Chromatin metabolism, Chromatin genetics, Intrinsically Disordered Proteins metabolism, Intrinsically Disordered Proteins genetics, Intrinsically Disordered Proteins chemistry, Origin Recognition Complex metabolism, Origin Recognition Complex genetics

Abstract

The first step toward eukaryotic genome duplication is loading of the replicative helicase onto chromatin. This 'licensing' step initiates with the recruitment of the origin recognition complex (ORC) to chromatin, which is thought to occur via ORC's ATP-dependent DNA binding and encirclement activity. However, we have previously shown that ATP binding is dispensable for the chromatin recruitment of fly ORC, raising the question of how metazoan ORC binds chromosomes. We show here that the intrinsically disordered region (IDR) of fly Orc1 is both necessary and sufficient for recruitment of ORC to chromosomes in vivo and demonstrate that this is regulated by IDR phosphorylation. Consistently, we find that the IDR confers the ORC holocomplex with ATP-independent DNA binding activity in vitro. Using phylogenetic analysis, we make the surprising observation that metazoan Orc1 IDRs have diverged so markedly that they are unrecognizable as orthologs and yet we find that these compositionally homologous sequences are functionally conserved. Altogether, these data suggest that chromatin is recalcitrant to ORC's ATP-dependent DNA binding activity, necessitating IDR-dependent chromatin tethering, which we propose poises ORC to opportunistically encircle nucleosome-free regions as they become available., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

40. Evolutionary analyses of intrinsically disordered regions reveal widespread signals of conservation.

Author

Singleton MD and Eisen MB

Subjects

Drosophila melanogaster genetics, Evolution, Molecular, Sequence Homology, Amino Acid Sequence, Intrinsically Disordered Proteins chemistry, Intrinsically Disordered Proteins genetics, Intrinsically Disordered Proteins metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Drosophila Proteins metabolism

Abstract

Intrinsically disordered regions (IDRs) are segments of proteins without stable three-dimensional structures. As this flexibility allows them to interact with diverse binding partners, IDRs play key roles in cell signaling and gene expression. Despite the prevalence and importance of IDRs in eukaryotic proteomes and various biological processes, associating them with specific molecular functions remains a significant challenge due to their high rates of sequence evolution. However, by comparing the observed values of various IDR-associated properties against those generated under a simulated model of evolution, a recent study found most IDRs across the entire yeast proteome contain conserved features. Furthermore, it showed clusters of IDRs with common "evolutionary signatures," i.e. patterns of conserved features, were associated with specific biological functions. To determine if similar patterns of conservation are found in the IDRs of other systems, in this work we applied a series of phylogenetic models to over 7,500 orthologous IDRs identified in the Drosophila genome to dissect the forces driving their evolution. By comparing models of constrained and unconstrained continuous trait evolution using the Brownian motion and Ornstein-Uhlenbeck models, respectively, we identified signals of widespread constraint, indicating conservation of distributed features is mechanism of IDR evolution common to multiple biological systems. In contrast to the previous study in yeast, however, we observed limited evidence of IDR clusters with specific biological functions, which suggests a more complex relationship between evolutionary constraints and function in the IDRs of multicellular organisms., Competing Interests: I have read the journal’s policy and the authors of this manuscript have the following competing interests: MBE is a founder and former member of the board of directors of PLOS., (Copyright: © 2024 Singleton, Eisen. 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

41. Functional Role of C-terminal Domains in the MSL2 Protein of Drosophila melanogaster.

Author

Tikhonova EA, Georgiev PG, and Maksimenko OG

Subjects

Animals, Male, Female, Transcription Factors metabolism, Transcription Factors genetics, Transcription Factors chemistry, Ubiquitination, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins chemistry, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Drosophila melanogaster metabolism, Drosophila melanogaster genetics, Protein Domains

Abstract

Dosage compensation complex (DCC), which consists of five proteins and two non-coding RNAs roX, specifically binds to the X chromosome in males, providing a higher level of gene expression necessary to compensate for the monosomy of the sex chromosome in male Drosophila compared to the two X chromosomes in females. The MSL2 protein contains the N-terminal RING domain, which acts as an E3 ligase in ubiquitination of proteins and is the only subunit of the complex expressed only in males. Functional role of the two C-terminal domains of the MSL2 protein, enriched with proline (P-domain) and basic amino acids (B-domain), was investigated. As a result, it was shown that the B-domain destabilizes the MSL2 protein, which is associated with the presence of two lysines ubiquitination of which is under control of the RING domain of MSL2. The unstructured proline-rich domain stimulates transcription of the roX2 gene, which is necessary for effective formation of the dosage compensation complex.

Published

2024

42. Role of Mod(mdg4)-67.2 Protein in Interactions between Su(Hw)-Dependent Complexes and Their Recruitment to Chromatin.

Author

Melnikova LS, Molodina VV, Georgiev PG, and Golovnin AK

Subjects

Animals, Protein Binding, Nuclear Proteins metabolism, DNA-Binding Proteins metabolism, Zinc Fingers, Microtubule-Associated Proteins, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Chromatin metabolism, Transcription Factors metabolism, Drosophila melanogaster metabolism, Repressor Proteins metabolism, Repressor Proteins genetics

Abstract

Su(Hw) belongs to the class of proteins that organize chromosome architecture, determine promoter activity, and participate in formation of the boundaries/insulators between the regulatory domains. This protein contains a cluster of 12 zinc fingers of the C2H2 type, some of which are responsible for binding to the consensus site. The Su(Hw) protein forms complex with the Mod(mdg4)-67.2 and the CP190 proteins, where the last one binds to all known Drosophila insulators. To further study functioning of the Su(Hw)-dependent complexes, we used the previously described su(Hw) E8 mutation with inactive seventh zinc finger, which produces mutant protein that cannot bind to the consensus site. The present work shows that the Su(Hw) E8 protein continues to directly interact with the CP190 and Mod(mdg4)-67.2 proteins. Through interaction with Mod(mdg4)-67.2, the Su(Hw) E8 protein can be recruited into the Su(Hw)-dependent complexes formed on chromatin and enhance their insulator activity. Our results demonstrate that the Su(Hw) dependent complexes without bound DNA can be recruited to the Su(Hw) binding sites through the specific protein-protein interactions that are stabilized by Mod(mdg4)-67.2.

Published

2024

43. Structural basis for sugar perception by Drosophila gustatory receptors.

Author

Ma D, Hu M, Yang X, Liu Q, Ye F, Cai W, Wang Y, Xu X, Chang S, Wang R, Yang W, Ye S, Su N, Fan M, Xu H, and Guo J

Subjects

Animals, Protein Conformation, Sugars, Taste physiology, Taste Perception physiology, Drosophila melanogaster physiology, Drosophila Proteins chemistry

Abstract

Insects rely on a family of seven transmembrane proteins called gustatory receptors (GRs) to encode different taste modalities, such as sweet and bitter. We report structures of Drosophila sweet taste receptors GR43a and GR64a in the apo and sugar-bound states. Both GRs form tetrameric sugar-gated cation channels composed of one central pore domain (PD) and four peripheral ligand-binding domains (LBDs). Whereas GR43a is specifically activated by the monosaccharide fructose that binds to a narrow pocket in LBDs, disaccharides sucrose and maltose selectively activate GR64a by binding to a larger and flatter pocket in LBDs. Sugar binding to LBDs induces local conformational changes, which are subsequently transferred to the PD to cause channel opening. Our studies reveal a structural basis for sugar recognition and activation of GRs.

Published

2024

44. Molecular characterization of Drosophila melanogaster thymidylate kinase.

Author

Hu Frisk J and Wang L

Subjects

Animals, Amino Acid Sequence, Models, Molecular, Phosphorylation, Drosophila Proteins metabolism, Drosophila Proteins genetics, Drosophila Proteins chemistry, Substrate Specificity, Cloning, Molecular, Drosophila melanogaster enzymology, Drosophila melanogaster genetics, Nucleoside-Phosphate Kinase metabolism, Nucleoside-Phosphate Kinase genetics, Nucleoside-Phosphate Kinase chemistry

Abstract

Drosophila has been used as an animal model to study pathogenic mechanism of neurological disorders. Thymidylate kinase (TMPK) is an essential enzyme in dTTP synthesis catalyzing the phosphorylation of dTMP to dTDP. Loss of function mutations in the DTYMK gene, coding for TMPK, cause severe microcephaly in human patients. In this study, Drosophila melanogaster TMPK (DmTMPK) was cloned, expressed, purified and characterized. Unlike human TMPK, DmTMPK phosphorylated not only dTMP and dUMP but also dGMP and dIMP although with low efficiency. ATP and dATP are the most efficient phosphate donor but at higher concentration (>1 mM) ATP inhibited DmTMPK activity. Sequence and structural model analysis explain why DmTMPK could phosphorylate purine nucleoside monophosphates. This study has laid a solid foundation for future study of TMPK function in Drosophila .

Published

2024

45. Chemical shift assignments of dsRBD1 and linker region of R2D2, a siRNA binding protein in the Drosophila RNAi pathway.

Author

Aute R and Deshmukh MV

Subjects

Animals, RNA, Small Interfering chemistry, RNA, Small Interfering genetics, RNA, Small Interfering metabolism, RNA Interference, RNA, Double-Stranded metabolism, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Carrier Proteins metabolism, RNA-Binding Proteins chemistry, Nuclear Magnetic Resonance, Biomolecular, Phosphates metabolism, RNA Helicases genetics, RNA Helicases metabolism, Drosophila genetics, Drosophila metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Drosophila Proteins metabolism

Abstract

In the model organism Drosophila melanogaster, one of the Dicer homologs, Dcr-2, initiates the RNA interference pathway by cleaving long double-stranded RNA into small interfering RNA (siRNA). The Dcr-2:R2D2 heterodimer subsequently binds to the 21-nucleotide siRNA to form the R2D2:Dcr-2 Initiator (RDI) complex, which is critical for initiating the assembly of the RNA-induced silencing complex containing guide siRNA strand. During RDI complex formation, R2D2 senses the stability of the 5' end of the siRNA and a 5'-phosphate group, although the underlying mechanism of siRNA asymmetry sensing and 5'-phosphate recognition by R2D2 is elusive. In this study, we present nearly complete chemical shift assignments of the backbone and the side chain of a construct that comprises the N-terminus dsRBD1 and linker of R2D2 (~ 10.3 kDa; henceforth: R2D2D1L). Our study would further aid in the structural and functional characterization of R2D2., (© 2023. The Author(s), under exclusive licence to Springer Nature B.V.)

Published

2023

46. Drosophila class-I myosins that can impact left-right asymmetry have distinct ATPase kinetics.

Author

Báez-Cruz FA and Ostap EM

Subjects

Animals, Actins metabolism, Kinetics, Protein Domains, Myosin Type I chemistry, Myosin Type I metabolism, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Drosophila melanogaster anatomy & histology, Drosophila melanogaster enzymology, Functional Laterality

Abstract

Myosin-1D (myo1D) is important for Drosophila left-right asymmetry, and its effects are modulated by myosin-1C (myo1C). De novo expression of these myosins in nonchiral Drosophila tissues promotes cell and tissue chirality, with handedness depending on the paralog expressed. Remarkably, the identity of the motor domain determines the direction of organ chirality, rather than the regulatory or tail domains. Myo1D, but not myo1C, propels actin filaments in leftward circles in in vitro experiments, but it is not known if this property contributes to establishing cell and organ chirality. To further explore if there are differences in the mechanochemistry of these motors, we determined the ATPase mechanisms of myo1C and myo1D. We found that myo1D has a 12.5-fold higher actin-activated steady-state ATPase rate, and transient kinetic experiments revealed myo1D has an 8-fold higher MgADP release rate compared to myo1C. Actin-activated phosphate release is rate limiting for myo1C, whereas MgADP release is the rate-limiting step for myo1D. Notably, both myosins have among the tightest MgADP affinities measured for any myosin. Consistent with ATPase kinetics, myo1D propels actin filaments at higher speeds compared to myo1C in in vitro gliding assays. Finally, we tested the ability of both paralogs to transport 50 nm unilamellar vesicles along immobilized actin filaments and found robust transport by myo1D and actin binding but no transport by myo1C. Our findings support a model where myo1C is a slow transporter with long-lived actin attachments, whereas myo1D has kinetic properties associated with a transport motor., Competing Interests: Conflict of interest The authors declare no conflict of interest with the contents of this article., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

47. Widespread regulatory specificities between transcriptional co-repressors and enhancers in Drosophila .

Author

Jacobs J, Pagani M, Wenzl C, and Stark A

Subjects

Animals, Chromatin metabolism, Gene Expression Regulation, Developmental, Amino Acid Motifs, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Drosophila Proteins chemistry, Drosophila Proteins genetics, Drosophila Proteins metabolism, Enhancer Elements, Genetic, Repressor Proteins chemistry, Repressor Proteins genetics, Repressor Proteins metabolism

Abstract

Gene expression is controlled by the precise activation and repression of transcription. Repression is mediated by specialized transcription factors (TFs) that recruit co-repressors (CoRs) to silence transcription, even in the presence of activating cues. However, whether CoRs can dominantly silence all enhancers or display distinct specificities is unclear. In this work, we report that most enhancers in Drosophila can be repressed by only a subset of CoRs, and enhancers classified by CoR sensitivity show distinct chromatin features, function, TF motifs, and binding. Distinct TF motifs render enhancers more resistant or sensitive to specific CoRs, as we demonstrate by motif mutagenesis and addition. These CoR-enhancer compatibilities constitute an additional layer of regulatory specificity that allows differential regulation at close genomic distances and is indicative of distinct mechanisms of transcriptional repression.

Published

2023

48. Cryptochrome-Timeless structure reveals circadian clock timing mechanisms.

Author

Lin C, Feng S, DeOliveira CC, and Crane BR

Subjects

Animals, Light, Mammals metabolism, Cryoelectron Microscopy, Active Transport, Cell Nucleus radiation effects, alpha Karyopherins metabolism, Circadian Clocks physiology, Circadian Clocks radiation effects, Circadian Rhythm physiology, Circadian Rhythm radiation effects, Cryptochromes chemistry, Cryptochromes metabolism, Cryptochromes ultrastructure, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Drosophila melanogaster radiation effects, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Drosophila Proteins ultrastructure

Abstract

Circadian rhythms influence many behaviours and diseases 1,2 . They arise from oscillations in gene expression caused by repressor proteins that directly inhibit transcription of their own genes. The fly circadian clock offers a valuable model for studying these processes, wherein Timeless (Tim) plays a critical role in mediating nuclear entry of the transcriptional repressor Period (Per) and the photoreceptor Cryptochrome (Cry) entrains the clock by triggering Tim degradation in light 2,3 . Here, through cryogenic electron microscopy of the Cry-Tim complex, we show how a light-sensing cryptochrome recognizes its target. Cry engages a continuous core of amino-terminal Tim armadillo repeats, resembling how photolyases recognize damaged DNA, and binds a C-terminal Tim helix, reminiscent of the interactions between light-insensitive cryptochromes and their partners in mammals. The structure highlights how the Cry flavin cofactor undergoes conformational changes that couple to large-scale rearrangements at the molecular interface, and how a phosphorylated segment in Tim may impact clock period by regulating the binding of Importin-α and the nuclear import of Tim-Per 4,5 . Moreover, the structure reveals that the N terminus of Tim inserts into the restructured Cry pocket to replace the autoinhibitory C-terminal tail released by light, thereby providing a possible explanation for how the long-short Tim polymorphism adapts flies to different climates 6,7 ., (© 2023. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2023

49. PK1 from Drosophila obscurin is an inactive pseudokinase with scaffolding properties.

Author

Zacharchenko T, Dorendorf T, Locker N, Van Dijk E, Katzemich A, Diederichs K, Bullard B, and Mayans O

Subjects

Animals, Drosophila Proteins chemistry, Drosophila Proteins metabolism, Protein Structure, Tertiary, Sarcomeres chemistry, Sarcomeres metabolism, Drosophila metabolism, Muscle Proteins metabolism

Abstract

Obscurins are large filamentous proteins with crucial roles in the assembly, stability and regulation of muscle. Characteristic of these proteins is a tandem of two C-terminal kinase domains, PK1 and PK2, that are separated by a long intrinsically disordered sequence. The significance of this conserved domain arrangement is unknown. Our study of PK1 from Drosophila obscurin shows that this is a pseudokinase with features typical of the CAM-kinase family, but which carries a minimalistic regulatory tail that no longer binds calmodulin or has mechanosensory properties typical of other sarcomeric kinases. PK1 binds ATP with high affinity, but in the absence of magnesium and lacks detectable phosphotransfer activity. It also has a highly diverged active site, strictly conserved across arthropods, that might have evolved to accommodate an unconventional binder. We find that PK1 interacts with PK2, suggesting a functional relation to the latter. These findings lead us to speculate that PK1/PK2 form a pseudokinase/kinase dual system, where PK1 might act as an allosteric regulator of PK2 and where mechanosensing properties, akin to those described for regulatory tails in titin-like kinases, might now reside on the unstructured interkinase segment. We propose that the PK1-interkinase-PK2 region constitutes an integrated functional unit in obscurin proteins.

Published

2023

50. Disordered proteins mitigate the temperature dependence of site-specific binding free energies.

Author

Thole JF, Waudby CA, and Pielak GJ

Subjects

Animals, Binding Sites, Entropy, Peptides metabolism, Protein Binding, src Homology Domains, Temperature, Son of Sevenless Protein, Drosophila chemistry, Drosophila melanogaster metabolism, Intrinsically Disordered Proteins chemistry, Drosophila Proteins chemistry

Abstract

Biophysical characterization of protein-protein interactions involving disordered proteins is challenging. A common simplification is to measure the thermodynamics and kinetics of disordered site binding using peptides containing only the minimum residues necessary. We should not assume, however, that these few residues tell the whole story. Son of sevenless, a multidomain signaling protein from Drosophila melanogaster, is critical to the mitogen-activated protein kinase pathway, passing an external signal to Ras, which leads to cellular responses. The disordered 55 kDa C-terminal domain of Son of sevenless is an autoinhibitor that blocks guanidine exchange factor activity. Activation requires another protein, Downstream of receptor kinase (Drk), which contains two Src homology 3 domains. Here, we utilized NMR spectroscopy and isothermal titration calorimetry to quantify the thermodynamics and kinetics of the N-terminal Src homology 3 domain binding to the strongest sites incorporated into the flanking disordered sequences. Comparing these results to those for isolated peptides provides information about how the larger domain affects binding. The affinities of sites on the disordered domain are like those of the peptides at low temperatures but less sensitive to temperature. Our results, combined with observations showing that intrinsically disordered proteins become more compact with increasing temperature, suggest a mechanism for this effect., Competing Interests: Conflict of interest The authors declare no conflicts of interests with the contents of this article., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023