Single-Molecule Pull-Down FRET to Dissect the Mechanisms of Biomolecular Machines

Kahlscheuer, Matthew L.; Widom, Julia R.; Walter, Nils G.

doi:10.1016/bs.mie.2015.01.009

Cited by 7 publications

(5 citation statements)

References 64 publications

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“…Hoskins et al revealed the order of spliceosome assembly during pre-mRNA maturation in cell extract via single-molecule multi-color fluorescence [22,23]. Single-molecule pull-down FRET allowed Nils et al to visualize in real time the splicing of pre-mRNA by the spliceosome [24,25]. Lee et al used a single-molecule co-immunoprecipitation approach to investigate weak interactions between different proteins [26,27].…”

Section: Introductionmentioning

confidence: 99%

Single-molecule pull-down for investigating protein–nucleic acid interactions

Fareh

Loeff

Szczepaniak

et al. 2016

Methods

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The genome and transcriptome are constantly modified by proteins in the cell. Recent advances in single-molecule techniques allow for high spatial and temporal observations of these interactions between proteins and nucleic acids. However, due to the difficulty of obtaining functional protein complexes, it remains challenging to study the interactions between macromolecular protein complexes and nucleic acids. Here, we combined singlemolecule fluorescence with various protein complex pull-down techniques and determined the function and stoichiometry of ribonucleoprotein complexes. Through the use of three examples from eukaryotic cells (Drosha, Dicer, and TUT4 protein complexes), we provide step-by-step guidance for using novel single-molecule techniques. Our single-molecule methods provide sub-second and nanometer resolution and can be applied to other nucleoprotein complexes that are essential for cellular processes. Highlights : Single-molecule pull-down provides a real-time view of the interactions between protein complexes and nucleic acids. Single-molecule pull-down can be used to determine the stoichiometry of nucleoprotein complexes. Tandem affinity purification yields protein complexes that are suitable for singlemolecule kinetics studies. Various tactics have to be considered for the surface immobilization of nucleoprotein complexes.

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Section: Introductionmentioning

confidence: 99%

Single-molecule pull-down for investigating protein–nucleic acid interactions

Fareh

Loeff

Szczepaniak

et al. 2016

Methods

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“…Single-molecule pull down (SiMPull) and its derivatives SNAP-SiMPull and SiMPull-FRET fuse conventional pull-down assays with single-molecule fluorescence microscopy or single-molecule fluorescence resonance energy transfer (FRET) to allow direct visualization of individual protein complexes. − Using these methods, studies have demonstrated the ability to detect single molecules of U1 snRNP and to investigate the dynamic nature of the mammalian target of rapamycin (mTOR)-containing complex (mTORC) dimerization and the selectivity of rapamycin on mTORC stoichiometry. , The ability to understand the dynamics of mTORC1 and mTORC2 is promising as mTOR is a regulatory protein associated with many cellular pathways like mRNA translation, ribosome biogenesis, autophagy, and metabolism. Additionally, mTOR deregulation has been linked to several types of cancer .…”

Section: Novel Methods Supporting Additional Mechanistic and Function...mentioning

confidence: 99%

“…Additionally, mTOR deregulation has been linked to several types of cancer . SiMPull-FRET was utilized to investigate pre-mRNA splicing dynamics and revealed that the spliceosome achieves an accurate initial splice through a biased Brownian ratcheting mechanism. , Because deregulated alternative splicing has been identified in ALS, SMA, AD, and even cancer, the capability to monitor spliceosome dynamics is a strong first step toward understanding the beginning of splicing defects and their proliferation through the cell.…”

Section: Novel Methods Supporting Additional Mechanistic and Function...mentioning

confidence: 99%

Defective Ribonucleoproteins, Mistakes in RNA Processing, and Diseases

et al. 2017

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Ribonucleoproteins (RNPs) are vital to many cellular events. To this end, many neurodegenerative diseases and cancers have been linked to RNP malfunction, particularly as this relates to defective processing of cellular RNA. The connection of RNPs and diseases has also propagated a shift of focus onto RNA targeting from traditional protein targeting treatments. However, therapeutic development in this area has been limited by incomplete molecular insight into the specific contributions of RNPs to disease. This review outlines the role of several RNPs in diseases, focusing on molecular defects in processes that affect proper RNA handling in the cell. This work also evaluates the contributions of recently developed methods to understanding RNP association and function. We review progress in this area by focusing on molecular malfunctions of RNPs associated with the onset and progression of several neurodegenerative diseases and cancer and conclude with a brief discussion of RNA-based therapeutic efforts.

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“…On the basis of these results, the authors concluded that spliceosome activation proceeds via a Brownian ratchet mechanism, in which ATP hydrolysis by Prp2 unlocks reversible fluctuations in the conformation of the pre-mRNA (and likely other components of the spliceosome), with Cwc25 acting as a pawl that facilitates the first step of splicing by trapping the conformation in which the BP and 5′SS are in close proximity. 143,260…”

Section: Single Molecule Fluorescence Studies Of Rna-protein Assemmentioning

confidence: 99%

“…Further addition of Cwc25 yielded a population of complexes that remained stably in the high-FRET state, which was confirmed by additional experiments to result from C complexes that have completed the first chemical reaction of splicing. On the basis of these results, the authors concluded that spliceosome activation proceeds via a Brownian ratchet mechanism, in which ATP hydrolysis by Prp2 unlocks reversible fluctuations in the conformation of the pre-mRNA (and likely other components of the spliceosome), with Cwc25 acting as a pawl that facilitates the first step of splicing by trapping the conformation in which the BP and 5′SS are in close proximity. , …”

Section: Single Molecule Fluorescence Studies Of Rna-protein Assembliesmentioning

confidence: 99%

Life under the Microscope: Single-Molecule Fluorescence Highlights the RNA World

2018

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The emergence of single-molecule (SM) fluorescence techniques has opened up a vast new toolbox for exploring the molecular basis of life. The ability to monitor individual biomolecules in real time enables complex, dynamic folding pathways to be interrogated without the averaging effect of ensemble measurements. In parallel, modern biology has been revolutionized by our emerging understanding of the many functions of RNA. In this comprehensive review, we survey SM fluorescence approaches and discuss how the application of these tools to RNA and RNA-containing macromolecular complexes in vitro has yielded significant insights into the underlying biology. Topics covered include the three-dimensional folding landscapes of a plethora of isolated RNA molecules, their assembly and interactions in RNA-protein complexes, and the relation of these properties to their biological functions. In all of these examples, the use of SM fluorescence methods has revealed critical information beyond the reach of ensemble averages.

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Single-Molecule Pull-Down FRET to Dissect the Mechanisms of Biomolecular Machines

Cited by 7 publications

References 64 publications

Single-molecule pull-down for investigating protein–nucleic acid interactions

Single-molecule pull-down for investigating protein–nucleic acid interactions

Defective Ribonucleoproteins, Mistakes in RNA Processing, and Diseases

Life under the Microscope: Single-Molecule Fluorescence Highlights the RNA World

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