Single-molecule study of the CUG repeat–MBNL1 interaction and its inhibition by small molecules

Jahromi, Amin Haghighat; Honda, Masayoshi; Zimmerman, Steven C.; Spies, Maria

doi:10.1093/nar/gkt330

Cited by 28 publications

(32 citation statements)

References 42 publications

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“…At the beginning of imaging, use 5 seconds excitation with 640 nm laser, then switch the excitation source to 532 nm laser for the rest of the recording. In this scheme, the MatLab program for extraction of the fluorescence trajectories only needs to consider the first 5 seconds of the recording to map the possible locations of surface-tethered molecules, aiding in the selection of trajectories (Boehm et al, 2016, Haghighat Jahromi et al, 2013). When the unlabeled neutravidin is used for surface-tethering, the MatLab code needs to be set to scan the entire movie in Cy3 channel to identify the locations where the Cy3 signal associated with the binding of the freely diffusing Cy3-labeled ligand appears.…”

Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

“…More complex binding patterns can be observed if the surface-tethered molecule contains multiple binding sites for the fluorescently-labeled binding partner(s), which may bind independently or oligomerize upon binding to the surface-tethered substarte. An example of the interaction involving multiple independent binding sites can be found in a study examining the interaction of muscleblind-like 1 protein (MBNL1) with RNA molecules containing CUG repeats (Haghighat Jahromi et al, 2013). The protein bound the surface-tethered (CUG) 4 construct with 1:1 stoichiometry.…”

Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

“…Even in its simplest one-color version, TIRFM-based single-molecule co-localization provides a suite of powerful approaches to develop a comprehensive understanding of the inhibition mechanism and the kinetics of the macromolecular interactions in the presence of an inhibitor (Haghighat Jahromi et al, 2013). In this section we provide a guide on how to design and carry this type of analysis.…”

Section: Binary Interactions In the Presence Of Inhibitorsmentioning

confidence: 99%

“…In this section we provide a guide on how to design and carry this type of analysis. We will use a study of the non-competitive inhibition of the interaction between muscleblind-like 1 protein (MBNL1) and the CUG repeat containing RNA (Haghighat Jahromi et al, 2013), but the overall approach can be generally applied to competitive and non-competitive inhibitors, as well as the allosteric effectors of protein-protein and protein nucleic acid interactions. The major advantage of this approach is that it is model-independent, i.e.…”

Section: Binary Interactions In the Presence Of Inhibitorsmentioning

confidence: 99%

“…Global analysis of these trajectories allows for accurate determination of the kinetic rate constants and interaction affinities (Wang et al, 2009, Elenko et al, 2009, Huppa et al, 2010, Joshi et al, 2012, Haghighat Jahromi et al, 2013, Chen et al, 2014), helps to reveal populations of conformers with different binding or catalytic properties (Amrute-Nayak et al, 2014, Chen et al, 2016, Honda et al, 2014), allows the investigator to distinguish different orders of complex assembly, and provides the tools to infer the mechanisms of competition or cooperation in the assembly of the higher order complexes (Boehm, 2016, Hoskins et al, 2016). With the advent of commercially available TIRFM systems, the methodology is becoming less arcane and hopefully will become a routine technique in biophysics and biochemistry laboratories.…”

Section: Introductionmentioning

confidence: 99%

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Quantifying the Assembly of Multicomponent Molecular Machines by Single-Molecule Total Internal Reflection Fluorescence Microscopy

Boehm

Subramanyam

Ghoneim

et al. 2016

Methods in Enzymology

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Large, dynamic macromolecular complexes play essential roles in many cellular processes. Knowing how the components of these complexes associate with one another and undergo structural rearrangements is critical to understanding how they function. Single-molecule total internal reflection fluorescence (TIRF) microscopy is a powerful approach for addressing these fundamental issues. In this article, we first discuss single-molecule TIRF microscopes and strategies to immobilize and fluorescently label macromolecules. We then review the use of single-molecule TIRF microscopy to study the formation of binary macromolecular complexes using one-color imaging and inhibitors. We conclude with a discussion of the use of TIRF microscopy to examine the formation of higher-order (i.e., ternary, quaternary, etc.) complexes using multi-color setups. The focus throughout this article is on experimental design, controls, data acquisition, and data analysis. We hope that single-molecule TIRF microscopy, which has largely been the province of specialists, will soon become as common in the tool box of biophysicists and biochemists as structural approaches has become today.

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Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

Section: Binary Interactions In the Presence Of Inhibitorsmentioning

confidence: 99%

Section: Binary Interactions In the Presence Of Inhibitorsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Quantifying the Assembly of Multicomponent Molecular Machines by Single-Molecule Total Internal Reflection Fluorescence Microscopy

Boehm

Subramanyam

Ghoneim

et al. 2016

Methods in Enzymology

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A Potent Inhibitor of Protein Sequestration by Expanded Triplet (CUG) Repeats that Shows Phenotypic Improvements in a Drosophila Model of Myotonic Dystrophy

et al. 2016

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Myotonic dystrophy is the most common form of the adult-onset muscular dystrophy, originating in a CTG repeat expansion in the DMPK gene. The expanded CUG transcript sequesters MBNL1 a key regulator of alternative splicing, leading to the misregulation of numerous pre-mRNAs. We report an RNA-targeted agent as a possible lead compound for the treatment of DM1 that reveals both the promise and challenges for this type of small molecule approach. The agent is a potent inhibitor of the MBNL1-rCUG complex with an inhibition constant, KI of 25 ± 8 nM, and is also relatively non-toxic to HeLa cells, able to dissolve nuclear foci, and correct the IR splicing defect in DM1 model cells. Moreover, treatment with this compound improves two separate disease phenotypes in a DM1 Drosophila model, the adult external eye degeneration and larval crawling defect. However, the compound has a relatively low maximum tolerated dose in mice and its cell uptake may be limited, providing insights into directions for future development.

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Myotonic Dystrophy and Developmental Regulation of RNA Processing

Thomas

Oliveira

Sznajder

et al. 2018

Comprehensive Physiology

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Myotonic dystrophy (DM) is a multisystemic disorder caused by microsatellite expansion mutations in two unrelated genes leading to similar, yet distinct, diseases. DM disease presentation is highly variable and distinguished by differences in age-of-onset and symptom severity. In the most severe form, DM presents with congenital onset and profound developmental defects. At the molecular level, DM pathogenesis is characterized by a toxic RNA gain-of-function mechanism that involves the transcription of noncoding microsatellite expansions. These mutant RNAs disrupt key cellular pathways, including RNA processing, localization, and translation. In DM, these toxic RNA effects are predominantly mediated through the modulation of the muscleblind-like and CUGBP and ETR-3-like factor families of RNA binding proteins (RBPs). Dysfunction of these RBPs results in widespread RNA processing defects culminating in the expression of developmentally inappropriate protein isoforms in adult tissues. The tissue that is the focus of this review, skeletal muscle, is particularly sensitive to mutant RNA-responsive perturbations, as patients display a variety of developmental, structural, and functional defects in muscle. Here, we provide a comprehensive overview of DM1 and DM2 clinical presentation and pathology as well as the underlying cellular and molecular defects associated with DM disease onset and progression. Additionally, fundamental aspects of skeletal muscle development altered in DM are highlighted together with ongoing and potential therapeutic avenues to treat this muscular dystrophy. © 2018 American Physiological Society. Compr Physiol 8:509-553, 2018.

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Single-molecule study of the CUG repeat–MBNL1 interaction and its inhibition by small molecules

Cited by 28 publications

References 42 publications

Quantifying the Assembly of Multicomponent Molecular Machines by Single-Molecule Total Internal Reflection Fluorescence Microscopy

Quantifying the Assembly of Multicomponent Molecular Machines by Single-Molecule Total Internal Reflection Fluorescence Microscopy

A Potent Inhibitor of Protein Sequestration by Expanded Triplet (CUG) Repeats that Shows Phenotypic Improvements in a Drosophila Model of Myotonic Dystrophy

Myotonic Dystrophy and Developmental Regulation of RNA Processing

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