49 research outputs found

    Programmable in situ amplification for multiplexed imaging of mRNA expression

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    In situ hybridization methods enable the mapping of mRNA expression within intact biological samples. With current approaches, it is challenging to simultaneously map multiple target mRNAs within whole-mount vertebrate embryos, representing a significant limitation in attempting to study interacting regulatory elements in systems most relevant to human development and disease. Here, we report a multiplexed fluorescent in situ hybridization method based on orthogonal amplification with hybridization chain reactions (HCR). With this approach, RNA probes complementary to mRNA targets trigger chain reactions in which fluorophore-labeled RNA hairpins self-assemble into tethered fluorescent amplification polymers. The programmability and sequence specificity of these amplification cascades enable multiple HCR amplifiers to operate orthogonally at the same time in the same sample. Robust performance is achieved when imaging five target mRNAs simultaneously in fixed whole-mount and sectioned zebrafish embryos. HCR amplifiers exhibit deep sample penetration, high signal-to-background ratios and sharp signal localization

    Design of Novel Relaxase Substrates Based on Rolling Circle Replicases for Bioconjugation to DNA Nanostructures

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    During bacterial conjugation and rolling circle replication, HUH endonucleases, respectively known as relaxases and replicases, form a covalent bond with ssDNA when they cleave their target sequence (nic site). Both protein families show structural similarity but limited amino acid identity. Moreover, the organization of the inverted repeat (IR) and the loop that shape the nic site differs in both proteins. Arguably, replicases cleave their target site more efficiently, while relaxases exert more biochemical control over the process. Here we show that engineering a relaxase target by mimicking the replicase target, results in enhanced formation of protein-DNA covalent complexes. Three widely different relaxases, which belong to MOBF, MOBQ and MOBP families, can properly cleave DNA sequences with permuted target sequences. Collaterally, the secondary structure that the permuted targets acquired within a supercoiled plasmid DNA resulted in poor conjugation frequencies underlying the importance of relaxase accessory proteins in conjugative DNA processing. Our results reveal that relaxase and replicase targets can be interchangeable in vitro. The new Rep substrates provide new bioconjugation tools for the design of sophisticated DNA-protein nanostructures.This work was financed by grants BFU2014-55534-C2-1-P from the Spanish Ministry of Economy and Competitiveness and 612146/FP7-ICT- 2013 and 282004/FP7-HEALTH.2011.2.3.1-2 from the European Union Seventh Framework Programme to FC and grant BFU2014-55534-C2-2-P from the Spanish Ministry of Economy and Competitiveness to GM. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript

    A DNA-fuelled molecular machine made of DNA.

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    Molecular recognition between complementary strands of DNA allows construction on a nanometre length scale. For example, DNA tags may be used to organize the assembly of colloidal particles, and DNA templates can direct the growth of semiconductor nanocrystals and metal wires. As a structural material in its own right, DNA can be used to make ordered static arrays of tiles, linked rings and polyhedra. The construction of active devices is also possible--for example, a nanomechanical switch, whose conformation is changed by inducing a transition in the chirality of the DNA double helix. Melting of chemically modified DNA has been induced by optical absorption, and conformational changes caused by the binding of oligonucleotides or other small groups have been shown to change the enzymatic activity of ribozymes. Here we report the construction of a DNA machine in which the DNA is used not only as a structural material, but also as 'fuel'. The machine, made from three strands of DNA, has the form of a pair of tweezers. It may be closed and opened by addition of auxiliary strands of 'fuel' DNA; each cycle produces a duplex DNA waste product

    DNA fuel for free-running nanomachines.

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    We describe kinetic control of DNA hybridization: loop complexes are used to inhibit the hybridization of complementary oligonucleotides; rationally designed DNA catalysts are shown to be effective in promoting their hybridization. This is the basis of a strategy for using DNA as a fuel to drive free-running artificial molecular machines

    The unnatural order of things

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    Distance Dependence of Single-Fluorophore Quenching by Gold Nanoparticles Studied on DNA Origami

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    We study the distance-dependent quenching of fluorescence due to a metallic nanoparticle in proximity of a fluorophore. In our single-molecule measurements, we achieve excellent control over structure and stoichiometry by using self-assembled DNA structures (DNA origami) as a breadboard where both the fluorophore and the 10 nm metallic nanoparticle are positioned with nanometer precision. The single-molecule spectroscopy method employed here reports on the co-localization of particle and dye, while fluorescence lifetime imaging is used to directly obtain the correlation of intensity and fluorescence lifetime for varying particle to dye distances. Our data can be well explained by exact calculations that include dipole dipole orientation and distances. Fitting with a more practical model for nanosurface energy transfer yields 10.4 nm as the characteristic distance of 50% energy transfer. The use of DNA nanotechnology together with minimal sample usage by attaching the particles to the DNA origami directly on the microscope coverslip paves the way for more complex experiments exploiting dye nanoparticle interactions.Fil: Acuna, Guillermo P.. Technische Universität Braunschweig; AlemaniaFil: Bucher, Martina. Ludwig Maximilians Universitat; AlemaniaFil: Stein, Ingo H.. Ludwig Maximilians Universitat; AlemaniaFil: Steinhauer, Christian. Ludwig Maximilians Universitat; AlemaniaFil: Kuzyk, Anton. Technische Universitat Munchen; AlemaniaFil: Holzmeister, Phil. Technische Universität Braunschweig; AlemaniaFil: Schreiber, Robert. Ludwig Maximilians Universitat; AlemaniaFil: Moroz, Alexander.Fil: Stefani, Fernando Daniel. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Ciudad Universitaria. Instituto de Física de Buenos Aires. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales. Instituto de Física de Buenos Aires; ArgentinaFil: Liedl, Tim. Ludwig Maximilians Universitat; AlemaniaFil: Simmel, Friedrich C.. Technische Universitat Munchen; AlemaniaFil: Tinnefeld, Philip. Technische Universität Braunschweig; Alemani

    On Low Energy Barrier Folding Pathways for Nucleic Acid Sequences

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    Abstract. Secondary structure folding pathways correspond to the ex-ecution of DNA programs such as DNA strand displacement systems. It is helpful to understand the full diversity of features that such pathways can have, when designing novel folding pathways. In this work, we show that properties of folding pathways over a 2-base strand (a strand with either A and T, or C and G, but not all four bases) may be quite different than those over a 4-base alphabet. Our main result is that, for a simple energy model in which each base pair contributes −1, 2-base sequences of length n always have a folding pathway of length O(n3) with energy barrier at most 2. We provide an efficient algorithm for constructing such a pathway. In contrast, it is unknown whether minimum energy barrier pathways for 4-base sequences can be found efficiently, and such path-ways can have barrier Θ(n). We also present several results that show how folding pathways with temporary and/or repeated base pairs can have lower energy barrier than pathways without such base pairs.
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