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Dive into the research topics where Jessica S. Lamb is active.

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Featured researches published by Jessica S. Lamb.


Nucleic Acids Research | 2009

Both helix topology and counterion distribution contribute to the more effective charge screening in dsRNA compared with dsDNA

Suzette A. Pabit; Xiangyun Qiu; Jessica S. Lamb; Li Li; Steve P. Meisburger; Lois Pollack

The recent discovery of the RNA interference mechanism emphasizes the biological importance of short, isolated, double-stranded (ds) RNA helices and calls for a complete understanding of the biophysical properties of dsRNA. However, most previous studies of the electrostatics of nucleic acid duplexes have focused on DNA. Here, we present a comparative investigation of electrostatic effects in RNA and DNA. Using resonant (anomalous) and non-resonant small-angle X-ray scattering, we characterized the charge screening efficiency and counterion distribution around short (25 bp) dsDNA and RNA molecules of comparable sequence. Consistent with theoretical predictions, we find counterion mediated screening to be more efficient for dsRNA than dsDNA. Furthermore, the topology of the RNA A-form helix alters the spatial distribution of counterions relative to B-form DNA. The experimental results reported here agree well with ion-size-corrected non-linear Poisson–Boltzmann calculations. We propose that differences in electrostatic properties aid in selective recognition of different types of short nucleic acid helices by target binding partners.


Journal of Molecular Biology | 2009

Illuminating solution responses of a LOV domain protein with photocoupled small-angle X-ray scattering.

Jessica S. Lamb; Brian D. Zoltowski; Suzette A. Pabit; Li Li; Brian R. Crane; Lois Pollack

The PAS-LOV domain is a signal-transducing component found in a large variety of proteins that is responsible for sensing different stimuli such as light, oxygen, and voltage. The LOV protein VVD regulates blue light responses in the filamentous fungi Neurospora crassa. Using photocoupled, time-resolved small-angle X-ray scattering, we extract the solution protein structure in both dark-adapted and light-activated states. Two distinct dark-adapted conformations are detected in the wild-type protein: a compact structure that corresponds to the crystal structure of the dark-state monomer as well as an extended structure that is well modeled by introducing conformational disorder at the N-terminus of the protein. These conformations are accentuated in carefully selected variants, in which a key residue for propagating structural transitions, Cys71, has been mutated or oxidized. Despite different dark-state conformations, all proteins form a common dimer in response to illumination. Taken together, these data support a reaction scheme that describes the mechanism for light-induced dimerization of VVD. Envelope reconstructions of the transient light-state dimer reveal structures that are best described by a parallel arrangement of subunits that have significantly changed conformation compared to the crystal structure.


Journal of Molecular Biology | 2008

Hinge stiffness is a barrier to RNA folding

Jörg C. Schlatterer; Lisa W. Kwok; Jessica S. Lamb; Hye Yoon Park; Kurt Andresen; Michael Brenowitz; Lois Pollack

Cation-mediated RNA folding from extended to compact, biologically active conformations relies on a temporal balance of forces. The Mg2 +-mediated folding of the Tetrahymena thermophila ribozyme is characterized by rapid nonspecific collapse followed by tertiary-contact-induced compaction. This article focuses on an autonomously folding portion of the Tetrahymena ribozyme, its P4-P6 domain, in order to probe one facet of the rapid collapse: chain flexibility. The time evolution of P4-P6 folding was followed by global and local measures as a function of Mg2 + concentration. While all concentrations of Mg2 + studied are sufficient to screen the charge on the helices, the rates of compaction and tertiary contact formation diverge as the concentration of Mg2 + increases; collapse is greatly accelerated by Mg2 +, while tertiary contact formation is not. These studies highlight the importance of chain stiffness to RNA folding; at 10 mM Mg2 +, a stiff hinge limits the rate of P4-P6 folding. At higher magnesium concentrations, the rate-limiting step shifts from hinge bending to tertiary contact formati


Biophysical Journal | 2008

Mono- and trivalent ions around DNA: a small-angle scattering study of competition and interactions.

Kurt Andresen; Xiangyun Qiu; Suzette A. Pabit; Jessica S. Lamb; Hye Yoon Park; Lisa W. Kwok; Lois Pollack

The presence of small numbers of multivalent ions in DNA-containing solutions results in strong attractive forces between DNA strands. Despite the biological importance of this interaction, e.g., DNA condensation, its physical origin remains elusive. We carried out a series of experiments to probe interactions between short DNA strands as small numbers of trivalent ions are included in a solution containing DNA and monovalent ions. Using resonant (anomalous) and nonresonant small angle x-ray scattering, we coordinated measurements of the number and distribution of each ion species around the DNA with the onset of attractive forces between DNA strands. DNA-DNA interactions occur as the number of trivalent ions increases. Surprisingly good agreement is found between data and size-corrected numerical Poisson-Boltzmann predictions of ion competition for non- and weakly interacting DNAs. We also obtained an estimate for the minimum number of trivalent ions needed to initiate DNA-DNA attraction.


Journal of the American Chemical Society | 2008

Time-resolved dimerization of a PAS-LOV protein measured with photocoupled small angle x-ray scattering

Jessica S. Lamb; Brian D. Zoltowski; Suzette A. Pabit; Brian R. Crane; Lois Pollack

Time-resolved small-angle X-ray scattering (SAXS) has been used to probe photoexcitation of the blue-light signal transduction protein Vivid (VVD). Laser excitation of sample in a continuous flow cell enables time-resolved measurement of the initial response of VVD to illumination. Good signal-to-noise is achieved without relying on multiple exposures of the same sample or limiting exposure times to prevent radiation damage. The SAXS data demonstrate that VVD dimerizes within tens of milliseconds of light-state activation. Time-resolved SAXS in a flow cell format is a general method for connecting chemical changes in photoreceptors to conformationally driven output signals.


Journal of Applied Crystallography | 2008

Reconstructing three-dimensional shape envelopes from time-resolved small-angle X-ray scattering data

Jessica S. Lamb; Lisa W. Kwok; Xiangyun Qiu; Kurt Andresen; Hye Yoon Park; Lois Pollack

Modern computing power has made it possible to reconstruct low-resolution, three-dimensional shapes from solution small-angle X-ray scattering (SAXS) data on biomolecules without a priori knowledge of the structure. In conjunction with rapid mixing techniques, SAXS has been applied to time resolve conformational changes accompanying important biological processes, such as biomolecular folding. In response to the widespread interest in SAXS reconstructions, their value in conjunction with such time-resolved data has been examined. The group I intron from Tetrahymena thermophila and its P4-P6 subdomain are ideal model systems for investigation owing to extensive previous studies, including crystal structures. The goal of this paper is to assay the quality of reconstructions from time-resolved data given the sacrifice in signal-to-noise required to obtain sharp time resolution.


Applied Physics Letters | 2008

Closing the lid on DNA end-to-end stacking interactions

Li Li; Suzette A. Pabit; Jessica S. Lamb; Hye Yoon Park; Lois Pollack

Recent experiments suggest that short DNA strands associate by end-to-end stacking. Here, we report interactions between DNAs with modified ends. DNA duplexes, 20 bp long, were capped with short T(4) loops at 2, 1 or 0 ends, and were placed in solutions containing 20 mM Mg(2+). Association was observed only in constructs with one or more uncapped ends. DNA-DNA interactions were characterized by measuring variations in small angle x-ray scattering (SAXS) curves at the lowest scattering angles. Second virial coefficients were computed from the SAXS data. Our results confirm that end-to-end stacking plays an important role in short strand DNA-DNA interactions.


Journal of Applied Crystallography | 2007

Focusing capillary optics for use in solution small-angle X-ray scattering

Jessica S. Lamb; Sterling Cornaby; Kurt Andresen; Lisa W. Kwok; Hye Yoon Park; Xiangyun Qiu; Detlef-M. Smilgies; Donald H. Bilderback; Lois Pollack

Measurements of the global conformation of macromolecules can be carried out using small-angle X-ray scattering (SAXS). Glass focusing capillaries, manufactured at the Cornell High Energy Synchrotron Source (CHESS), have been successfully employed for SAXS measurements on the heme protein cytochrome c. These capillaries provide high X-ray flux into a spot size of tens of micrometres, permitting short exposures of small-volume samples. Such a capability is ideal for use in conjunction with microfluidic mixers, where time resolution may be determined by beam size and sample volumes are kept small to facilitate mixing and conserve material.


Physical Review Letters | 2007

Inter-DNA attraction mediated by divalent counterions.

Xiangyun Qiu; Kurt Andresen; Lisa W. Kwok; Jessica S. Lamb; Hye Yoon Park; Lois Pollack


Physical Review Letters | 2004

Spatial Distribution of Competing Ions around DNA in Solution

Kurt Andresen; Rhiju Das; Hye Yoon Park; Heather Smith; Lisa W. Kwok; Jessica S. Lamb; E. J. Kirkland; Daniel Herschlag; K. D. Finkelstein; Lois Pollack

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Hye Yoon Park

Seoul National University

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Xiangyun Qiu

George Washington University

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Li Li

Cornell University

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Brian D. Zoltowski

Southern Methodist University

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