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3. Real-time observation of DNA looping dynamics of type IIE restriction enzymes NaeI and NarI

Author

van den Broek, B., Vanzi, F., Normanno, D., Pavone, F. S., Wuite, G.J.L., van den Broek, B., Vanzi, F., Normanno, D., Pavone, F. S., and Wuite, G.J.L.

Abstract

Many restriction enzymes require binding of two copies of a recognition sequence for DNA cleavage, thereby introducing a loop in the DNA. We investigated looping dynamics of Type IIE restriction enzymes NaeI and NarI by tracking the Brownian motion of single tethered DNA molecules. DNA containing two endonuclease recognition sites spaced a few 100 bp apart connect small polystyrene beads to a glass surface. The position of a bead is tracked through video microscopy. Protein-mediated looping and unlooping is then observed as a sudden specific change in Brownian motion of the bead. With this method we are able to directly follow DNA looping kinetics of single protein-DNA complexes to obtain loop stability and loop formation times. We show that, in the absence of divalent cations, NaeI induces DNA loops of specific size. In contrast, under these conditions NarI mainly creates non-specific loops, resulting in effective DNA compaction for higher enzyme concentrations. Addition of Ca

Published
2006
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5. The Wnt-dependent master regulator NKX1-2 controls mouse pre-implantation development.

Author

Nakagawa S, Carnevali D, Tan X, Alvarez MJ, Parfitt DE, Di Vicino U, Arumugam K, Shin W, Aranda S, Normanno D, Sebastian-Perez R, Cannatá C, Cortes P, Neguembor MV, Shen MM, Califano A, and Cosma MP

Subjects
Animals, Mice, Blastocyst metabolism, Blastocyst cytology, Cell Nucleolus metabolism, Mouse Embryonic Stem Cells metabolism, Mouse Embryonic Stem Cells cytology, Tight Junctions metabolism, Wnt Proteins metabolism, Wnt Signaling Pathway, Embryonic Development genetics, Gene Expression Regulation, Developmental, Homeodomain Proteins metabolism, Homeodomain Proteins genetics, Transcription Factors metabolism, Transcription Factors genetics
Abstract

Embryo size, specification, and homeostasis are regulated by a complex gene regulatory and signaling network. Here we used gene expression signatures of Wnt-activated mouse embryonic stem cell (mESC) clones to reverse engineer an mESC regulatory network. We identify NKX1-2 as a novel master regulator of preimplantation embryo development. We find that Nkx1-2 inhibition reduces nascent RNA synthesis, downregulates genes controlling ribosome biogenesis, RNA translation, and transport, and induces severe alteration of nucleolus structure, resulting in the exclusion of RNA polymerase I from nucleoli. In turn, NKX1-2 loss of function leads to chromosome missegregation in the 2- to 4-cell embryo stages, severe decrease in blastomere numbers, alterations of tight junctions (TJs), and impairment of microlumen coarsening. Overall, these changes impair the blastocoel expansion-collapse cycle and embryo cavitation, leading to altered lineage specification and developmental arrest., Competing Interests: Declaration of interests A.C. is founder, equity holder, and consultant, and M.J.A. is Chief Scientific Officer at DarwinHealth Inc., a company that has licensed some of the algorithms used in this manuscript from Columbia University. Columbia University is also an equity holder in DarwinHealth Inc., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2024
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6. Branched microtubule nucleation and dynein transport organize RanGTP asters in Xenopus laevis egg extract.

Author

Scrofani J, Ruhnow F, Chew WX, Normanno D, Nedelec F, Surrey T, and Vernos I

Subjects
Animals, Xenopus laevis metabolism, Microtubules metabolism, Dynactin Complex, Microtubule-Associated Proteins metabolism, Xenopus Proteins metabolism, Dyneins metabolism, Spindle Apparatus metabolism
Abstract

Chromosome segregation relies on the correct assembly of a bipolar spindle. Spindle pole self-organization requires dynein-dependent microtubule (MT) transport along other MTs. However, during M-phase RanGTP triggers MT nucleation and branching generating polarized arrays with nonastral organization in which MT minus ends are linked to the sides of other MTs. This raises the question of how branched-MT nucleation and dynein-mediated transport cooperate to organize the spindle poles. Here, we used RanGTP-dependent MT aster formation in Xenopus laevis ( X. laevis ) egg extract to study the interplay between these two seemingly conflicting organizing principles. Using temporally controlled perturbations of MT nucleation and dynein activity, we found that branched MTs are not static but instead dynamically redistribute over time as poles self-organize. Our experimental data together with computer simulations suggest a model where dynein together with dynactin and NuMA directly pulls and move branched MT minus ends toward other MT minus ends.

Published
2024
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7. Probing the Structural Dynamics of a Bacterial Chaperone in Its Native Environment by Nitroxide-Based EPR Spectroscopy.

Author

Pierro A, Bonucci A, Normanno D, Ansaldi M, Pilet E, Ouari O, Guigliarelli B, Etienne E, Gerbaud G, Magalon A, Belle V, and Mileo E

Subjects
Electron Spin Resonance Spectroscopy methods, Spin Labels, Nitrogen Oxides chemistry, Molecular Chaperones chemistry
Abstract

One of the greatest current challenges in structural biology is to study protein dynamics over a wide range of timescales in complex environments, such as the cell. Among magnetic resonances suitable for this approach, electron paramagnetic resonance spectroscopy coupled to site-directed spin labeling (SDSL-EPR) has emerged as a promising tool to study protein local dynamics and conformational ensembles. In this work, we exploit the sensitivity of nitroxide labels to report protein local dynamics at room temperature. We demonstrate that such studies can be performed while preserving both the integrity of the cells and the activity of the protein under investigation. Using this approach, we studied the structural dynamics of the chaperone NarJ in its natural host, Escherichia coli. We established that spin-labeled NarJ is active inside the cell. We showed that the cellular medium affects NarJ structural dynamics in a site-specific way, while the structural flexibility of the protein is maintained. Finally, we present and discuss data on the time-resolved dynamics of NarJ in cellular context., (© 2022 Wiley-VCH GmbH.)

Published
2022
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8. Structural transitions in the GTP cap visualized by cryo-electron microscopy of catalytically inactive microtubules.

Author

LaFrance BJ, Roostalu J, Henkin G, Greber BJ, Zhang R, Normanno D, McCollum CO, Surrey T, and Nogales E

Subjects
Humans, Hydrolysis, Kinesins, Microtubule-Associated Proteins genetics, Microtubule-Associated Proteins metabolism, Microtubule-Associated Proteins ultrastructure, Microtubules genetics, Recombinant Proteins, Tubulin genetics, Tubulin metabolism, Tubulin ultrastructure, Cryoelectron Microscopy, Guanosine Triphosphate chemistry, Guanosine Triphosphate metabolism, Microtubules metabolism, Microtubules ultrastructure
Abstract

Microtubules (MTs) are polymers of αβ-tubulin heterodimers that stochastically switch between growth and shrinkage phases. This dynamic instability is critically important for MT function. It is believed that GTP hydrolysis within the MT lattice is accompanied by destabilizing conformational changes and that MT stability depends on a transiently existing GTP cap at the growing MT end. Here, we use cryo-electron microscopy and total internal reflection fluorescence microscopy of GTP hydrolysis-deficient MTs assembled from mutant recombinant human tubulin to investigate the structure of a GTP-bound MT lattice. We find that the GTP-MT lattice of two mutants in which the catalytically active glutamate in α-tubulin was substituted by inactive amino acids (E254A and E254N) is remarkably plastic. Undecorated E254A and E254N MTs with 13 protofilaments both have an expanded lattice but display opposite protofilament twists, making these lattices distinct from the compacted lattice of wild-type GDP-MTs. End-binding proteins of the EB family have the ability to compact both mutant GTP lattices and to stabilize a negative twist, suggesting that they promote this transition also in the GTP cap of wild-type MTs, thereby contributing to the maturation of the MT structure. We also find that the MT seam appears to be stabilized in mutant GTP-MTs and destabilized in GDP-MTs, supporting the proposal that the seam plays an important role in MT stability. Together, these structures of catalytically inactive MTs add mechanistic insight into the GTP state of MTs, the stability of the GTP- and GDP-bound lattice, and our overall understanding of MT dynamic instability., Competing Interests: The authors declare no competing interest., (Copyright © 2022 the Author(s). Published by PNAS.)

Published
2022
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9. Gradual compaction of the central spindle decreases its dynamicity in PRC1 and EB1 gene-edited cells.

Author

Asthana J, Cade NI, Normanno D, Lim WM, and Surrey T

Subjects
CRISPR-Cas Systems, Cell Cycle Proteins genetics, Cell Line, Transformed, Chromosome Segregation genetics, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Humans, Microtubule-Associated Proteins genetics, Microtubules metabolism, Protein Binding genetics, Transfection methods, Cell Cycle Proteins metabolism, Gene Editing methods, Microtubule-Associated Proteins metabolism, Mitosis genetics, Retinal Pigment Epithelium metabolism, Signal Transduction genetics, Spindle Apparatus metabolism
Abstract

During mitosis, the spindle undergoes morphological and dynamic changes. It reorganizes at the onset of the anaphase when the antiparallel bundler PRC1 accumulates and recruits central spindle proteins to the midzone. Little is known about how the dynamic properties of the central spindle change during its morphological changes in human cells. Using gene editing, we generated human cells that express from their endogenous locus fluorescent PRC1 and EB1 to quantify their native spindle distribution and binding/unbinding turnover. EB1 plus end tracking revealed a general slowdown of microtubule growth, whereas PRC1, similar to its yeast orthologue Ase1, binds increasingly strongly to compacting antiparallel microtubule overlaps. KIF4A and CLASP1 bind more dynamically to the central spindle, but also show slowing down turnover. These results show that the central spindle gradually becomes more stable during mitosis, in agreement with a recent "bundling, sliding, and compaction" model of antiparallel midzone bundle formation in the central spindle during late mitosis., (© 2021 Asthana et al.)

Published
2021
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11. Non-specific interactions govern cytosolic diffusion of nanosized objects in mammalian cells.

Author

Etoc F, Balloul E, Vicario C, Normanno D, Liße D, Sittner A, Piehler J, Dahan M, and Coppey M

Subjects
Diffusion, HeLa Cells, Humans, Particle Size, Quantum Dots chemistry, Quantum Dots metabolism, Cytosol metabolism, Nanoparticles chemistry
Abstract

The diffusivity of macromolecules in the cytoplasm of eukaryotic cells varies over orders of magnitude and dictates the kinetics of cellular processes. However, a general description that associates the Brownian or anomalous nature of intracellular diffusion to the architectural and biochemical properties of the cytoplasm has not been achieved. Here we measure the mobility of individual fluorescent nanoparticles in living mammalian cells to obtain a comprehensive analysis of cytoplasmic diffusion. We identify a correlation between tracer size, its biochemical nature and its mobility. Inert particles with size equal or below 50 nm behave as Brownian particles diffusing in a medium of low viscosity with negligible effects of molecular crowding. Increasing the strength of non-specific interactions of the nanoparticles within the cytoplasm gradually reduces their mobility and leads to subdiffusive behaviour. These experimental observations and the transition from Brownian to subdiffusive motion can be captured in a minimal phenomenological model.

Published
2018
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12. Mutational phospho-mimicry reveals a regulatory role for the XRCC4 and XLF C-terminal tails in modulating DNA bridging during classical non-homologous end joining.

Author

Normanno D, Négrel A, de Melo AJ, Betzi S, Meek K, and Modesti M

Subjects
Amino Acid Substitution, DNA Mutational Analysis, DNA Repair Enzymes genetics, DNA-Binding Proteins genetics, Humans, Phosphorylation, Protein Binding, Protein Processing, Post-Translational, DNA metabolism, DNA End-Joining Repair, DNA Repair Enzymes metabolism, DNA-Binding Proteins metabolism
Abstract

XRCC4 and DNA Ligase 4 (LIG4) form a tight complex that provides DNA ligase activity for classical non-homologous end joining (the predominant DNA double-strand break repair pathway in higher eukaryotes) and is stimulated by XLF. Independently of LIG4, XLF also associates with XRCC4 to form filaments that bridge DNA. These XRCC4/XLF complexes rapidly load and connect broken DNA, thereby stimulating intermolecular ligation. XRCC4 and XLF both include disordered C-terminal tails that are functionally dispensable in isolation but are phosphorylated in response to DNA damage by DNA-PK and/or ATM. Here we concomitantly modify the tails of XRCC4 and XLF by substituting fourteen previously identified phosphorylation sites with either alanine or aspartate residues. These phospho-blocking and -mimicking mutations impact both the stability and DNA bridging capacity of XRCC4/XLF complexes, but without affecting their ability to stimulate LIG4 activity. Implicit in this finding is that phosphorylation may regulate DNA bridging by XRCC4/XLF filaments.

Published
2017
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14. Human RAD52 Captures and Holds DNA Strands, Increases DNA Flexibility, and Prevents Melting of Duplex DNA: Implications for DNA Recombination.

Author

Brouwer I, Zhang H, Candelli A, Normanno D, Peterman EJG, Wuite GJL, and Modesti M

Subjects
DNA, Single-Stranded metabolism, Diffusion, Green Fluorescent Proteins metabolism, Humans, Protein Binding, DNA metabolism, Nucleic Acid Denaturation, Rad52 DNA Repair and Recombination Protein metabolism, Recombination, Genetic
Abstract

Human RAD52 promotes annealing of complementary single-stranded DNA (ssDNA). In-depth knowledge of RAD52-DNA interaction is required to understand how its activity is integrated in DNA repair processes. Here, we visualize individual fluorescent RAD52 complexes interacting with single DNA molecules. The interaction with ssDNA is rapid, static, and tight, where ssDNA appears to wrap around RAD52 complexes that promote intra-molecular bridging. With double-stranded DNA (dsDNA), interaction is slower, weaker, and often diffusive. Interestingly, force spectroscopy experiments show that RAD52 alters the mechanics dsDNA by enhancing DNA flexibility and increasing DNA contour length, suggesting intercalation. RAD52 binding changes the nature of the overstretching transition of dsDNA and prevents DNA melting, which is advantageous for strand clamping during or after annealing. DNA-bound RAD52 is efficient at capturing ssDNA in trans. Together, these effects may help key steps in DNA repair, such as second-end capture during homologous recombination or strand annealing during RAD51-independent recombination reactions., (Copyright © 2017 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2017
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15. Sliding sleeves of XRCC4-XLF bridge DNA and connect fragments of broken DNA.

Author

Brouwer I, Sitters G, Candelli A, Heerema SJ, Heller I, de Melo AJ, Zhang H, Normanno D, Modesti M, Peterman EJ, and Wuite GJ

Subjects
Diffusion, Humans, Microscopy, Fluorescence, Movement, Optical Tweezers, Translocation, Genetic, DNA Breaks, Double-Stranded, DNA End-Joining Repair, DNA Repair Enzymes metabolism, DNA-Binding Proteins metabolism
Abstract

Non-homologous end joining (NHEJ) is the primary pathway for repairing DNA double-strand breaks (DSBs) in mammalian cells. Such breaks are formed, for example, during gene-segment rearrangements in the adaptive immune system or by cancer therapeutic agents. Although the core components of the NHEJ machinery are known, it has remained difficult to assess the specific roles of these components and the dynamics of bringing and holding the fragments of broken DNA together. The structurally similar XRCC4 and XLF proteins are proposed to assemble as highly dynamic filaments at (or near) DSBs. Here we show, using dual- and quadruple-trap optical tweezers combined with fluorescence microscopy, how human XRCC4, XLF and XRCC4-XLF complexes interact with DNA in real time. We find that XLF stimulates the binding of XRCC4 to DNA, forming heteromeric complexes that diffuse swiftly along the DNA. Moreover, we find that XRCC4-XLF complexes robustly bridge two independent DNA molecules and that these bridges are able to slide along the DNA. These observations suggest that XRCC4-XLF complexes form mobile sleeve-like structures around DNA that can reconnect the broken ends very rapidly and hold them together. Understanding the dynamics and regulation of this mechanism will lead to clarification of how NHEJ proteins are involved in generating chromosomal translocations.

Published
2016
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16. Probing the target search of DNA-binding proteins in mammalian cells using TetR as model searcher.

Author

Normanno D, Boudarène L, Dugast-Darzacq C, Chen J, Richter C, Proux F, Bénichou O, Voituriez R, Darzacq X, and Dahan M

Subjects
Base Sequence, Cell Line, Tumor, DNA-Binding Proteins genetics, Gene Expression Regulation physiology, Humans, Kinetics, Protein Conformation, Protein Transport, Repressor Proteins genetics, DNA-Binding Proteins metabolism, Repressor Proteins metabolism
Abstract

Many cellular functions rely on DNA-binding proteins finding and associating to specific sites in the genome. Yet the mechanisms underlying the target search remain poorly understood, especially in the case of the highly organized mammalian cell nucleus. Using as a model Tet repressors (TetRs) searching for a multi-array locus, we quantitatively analyse the search process in human cells with single-molecule tracking and single-cell protein-DNA association measurements. We find that TetRs explore the nucleus and reach their target by 3D diffusion interspersed with transient interactions with non-cognate sites, consistent with the facilitated diffusion model. Remarkably, nonspecific binding times are broadly distributed, underlining a lack of clear delimitation between specific and nonspecific interactions. However, the search kinetics is not determined by diffusive transport but by the low association rate to nonspecific sites. Altogether, our results provide a comprehensive view of the recruitment dynamics of proteins at specific loci in mammalian cells.

Published
2015
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17. A general method to improve fluorophores for live-cell and single-molecule microscopy.

Author

Grimm JB, English BP, Chen J, Slaughter JP, Zhang Z, Revyakin A, Patel R, Macklin JJ, Normanno D, Singer RH, Lionnet T, and Lavis LD

Subjects
Azetidines chemistry, Chemistry Techniques, Synthetic, Coumarins chemistry, Fluorescein chemistry, Fluorescent Dyes analysis, Fluorescent Dyes chemical synthesis, HeLa Cells, Humans, Models, Molecular, Quantum Theory, Rhodamines chemistry, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet methods, Structure-Activity Relationship, Fluorescent Dyes chemistry, Microscopy, Ultraviolet methods, Molecular Imaging methods
Abstract

Specific labeling of biomolecules with bright fluorophores is the keystone of fluorescence microscopy. Genetically encoded self-labeling tag proteins can be coupled to synthetic dyes inside living cells, resulting in brighter reporters than fluorescent proteins. Intracellular labeling using these techniques requires cell-permeable fluorescent ligands, however, limiting utility to a small number of classic fluorophores. Here we describe a simple structural modification that improves the brightness and photostability of dyes while preserving spectral properties and cell permeability. Inspired by molecular modeling, we replaced the N,N-dimethylamino substituents in tetramethylrhodamine with four-membered azetidine rings. This addition of two carbon atoms doubles the quantum efficiency and improves the photon yield of the dye in applications ranging from in vitro single-molecule measurements to super-resolution imaging. The novel substitution is generalizable, yielding a palette of chemical dyes with improved quantum efficiencies that spans the UV and visible range.

Published
2015
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18. Single molecule study of non-specific binding kinetics of LacI in mammalian cells.

Author

Caccianini L, Normanno D, Izeddin I, and Dahan M

Subjects
Binding Sites, Cell Line, Tumor, DNA metabolism, Humans, Kinetics, Lac Repressors metabolism, Molecular Dynamics Simulation, Spectrometry, Fluorescence, Cells metabolism, DNA chemistry, Lac Repressors chemistry
Abstract

Many key cellular processes are controlled by the association of DNA-binding proteins (DBPs) to specific sites. The kinetics of the search process leading to the binding of DBPs to their target locus are largely determined by transient interactions with non-cognate DNA. Using single-molecule microscopy, we studied the dynamics and non-specific binding to DNA of the Lac repressor (LacI) in the environment of mammalian nuclei. We measured the distribution of the LacI-DNA binding times at non-cognate sites and determined the mean residence time to be τ(1D) = 182 ms. This non-specific interaction time, measured in the context of an exogenous system such as that of human U2OS cells, is remarkably different compared to that reported for the LacI in its native environment in E. coli (<5 ms). Such a striking difference (more than 30 fold) suggests that the genome, its organization, and the nuclear environment of mammalian cells play important roles on the dynamics of DBPs and their non-specific DNA interactions. Furthermore, we found that the distribution of off-target binding times follows a power law, similar to what was reported for TetR in U2OS cells. We argue that a possible molecular origin of such a power law distribution of residence times is the large variability of non-cognate sequences found in the mammalian nucleus by the diffusing DBPs.

Published
2015
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19. Intra-nuclear mobility and target search mechanisms of transcription factors: a single-molecule perspective on gene expression.

Author

Normanno D, Dahan M, and Darzacq X

Subjects
Cell Survival, DNA genetics, DNA metabolism, Eukaryota genetics, Eukaryota metabolism, Genome, Humans, Transcription, Genetic, Active Transport, Cell Nucleus genetics, Cell Nucleus genetics, Cell Nucleus metabolism, Gene Expression Regulation, Developmental, Transcription Factors genetics, Transcription Factors metabolism
Abstract

Precise expression of specific genes in time and space is at the basis of cellular viability as well as correct development of organisms. Understanding the mechanisms of gene regulation is fundamental and still one of the great challenges for biology. Gene expression is regulated also by specific transcription factors that recognize and bind to specific DNA sequences. Transcription factors dynamics, and especially the way they sample the nucleoplasmic space during the search for their specific target in the genome, are a key aspect for regulation and it has been puzzling researchers for forty years. The scope of this review is to give a state-of-the-art perspective over the intra-nuclear mobility and the target search mechanisms of specific transcription factors at the molecular level. Going through the seminal biochemical experiments that have raised the first questions about target localization and the theoretical grounds concerning target search processes, we describe the most recent experimental achievements and current challenges in understanding transcription factors dynamics and interactions with DNA using in vitro assays as well as in live prokaryotic and eukaryotic cells. This article is part of a Special Issue entitled: Nuclear Transport and RNA Processing., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published
2012
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21. Single-molecule manipulation reveals supercoiling-dependent modulation of lac repressor-mediated DNA looping.

Author

Normanno D, Vanzi F, and Pavone FS

Subjects
DNA, Superhelical metabolism, Genetic Techniques, Kinetics, Lac Repressors, Microspheres, Nucleic Acid Conformation, Bacterial Proteins metabolism, DNA, Superhelical chemistry, Repressor Proteins metabolism
Abstract

Gene expression regulation is a fundamental biological process which deploys specific sets of genomic information depending on physiological or environmental conditions. Several transcription factors (including lac repressor, LacI) are present in the cell at very low copy number and increase their local concentration by binding to multiple sites on DNA and looping the intervening sequence. In this work, we employ single-molecule manipulation to experimentally address the role of DNA supercoiling in the dynamics and stability of LacI-mediated DNA looping. We performed measurements over a range of degrees of supercoiling between -0.026 and +0.026, in the absence of axial stretching forces. A supercoiling-dependent modulation of the lifetimes of both the looped and unlooped states was observed. Our experiments also provide evidence for multiple structural conformations of the LacI-DNA complex, depending on torsional constraints. The supercoiling-dependent modulation demonstrated here adds an important element to the model of the lac operon. In fact, the complex network of proteins acting on the DNA in a living cell constantly modifies its topological and mechanical properties: our observations demonstrate the possibility of establishing a signaling pathway from factors affecting DNA supercoiling to transcription factors responsible for the regulation of specific sets of genes.

Published
2008
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22. Real-time observation of DNA looping dynamics of Type IIE restriction enzymes NaeI and NarI.

Author

van den Broek B, Vanzi F, Normanno D, Pavone FS, and Wuite GJ

Subjects
Calcium pharmacology, Deoxyribonucleases, Type II Site-Specific chemistry, Kinetics, Models, Molecular, Nucleic Acid Conformation, DNA chemistry, DNA metabolism, Deoxyribonucleases, Type II Site-Specific metabolism
Abstract

Many restriction enzymes require binding of two copies of a recognition sequence for DNA cleavage, thereby introducing a loop in the DNA. We investigated looping dynamics of Type IIE restriction enzymes NaeI and NarI by tracking the Brownian motion of single tethered DNA molecules. DNA containing two endonuclease recognition sites spaced a few 100 bp apart connect small polystyrene beads to a glass surface. The position of a bead is tracked through video microscopy. Protein-mediated looping and unlooping is then observed as a sudden specific change in Brownian motion of the bead. With this method we are able to directly follow DNA looping kinetics of single protein-DNA complexes to obtain loop stability and loop formation times. We show that, in the absence of divalent cations, NaeI induces DNA loops of specific size. In contrast, under these conditions NarI mainly creates non-specific loops, resulting in effective DNA compaction for higher enzyme concentrations. Addition of Ca2+ increases the NaeI-DNA loop lifetime by two orders of magnitude and stimulates specific binding by NarI. Finally, for both enzymes we observe exponentially distributed loop formation times, indicating that looping is dominated by (re)binding the second recognition site.

Published
2006
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23. High-precision measurements of light-induced torque on absorbing microspheres.

Author

Capitanio M, Normanno D, and Pavone FS

Abstract

Laser beams have been demonstrated to be capable of exerting torque as well as forces on microparticles. Using a custom magneto-optic manipulator, we directly measured the torque exerted by laser light on absorbing microspheres as a result of the transfer of spin angular momentum. A general method for measuring torque has been developed, and the experimental apparatus has shown a sensitivity of approximately 1 pN/nm.

Published
2004
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