97 research outputs found
Ptychographic hyperspectral spectromicroscopy with an extreme ultraviolet high harmonic comb
We demonstrate a new scheme of spectromicroscopy in the extreme ultraviolet
(EUV) spectral range, where the spectral response of the sample at different
wavelengths is imaged simultaneously. It is enabled by applying ptychographical
information multiplexing (PIM) to a tabletop EUV source based on high harmonic
generation, where four spectrally narrow harmonics near 30 nm form a spectral
comb structure. Extending PIM from previously demonstrated visible wavelengths
to the EUV/X-ray wavelengths promises much higher spatial resolution and more
powerful spectral contrast mechanism, making PIM an attractive
spectromicroscopy method in both the microscopy and the spectroscopy aspects.
Besides the sample, the multicolor EUV beam is also imaged in situ, making our
method a powerful beam characterization technique. No hardware is used to
separate or narrow down the wavelengths, leading to efficient use of the EUV
radiation
Quantitative Chemically-Specific Coherent Diffractive Imaging of Buried Interfaces using a Tabletop EUV Nanoscope
Characterizing buried layers and interfaces is critical for a host of
applications in nanoscience and nano-manufacturing. Here we demonstrate
non-invasive, non-destructive imaging of buried interfaces using a tabletop,
extreme ultraviolet (EUV), coherent diffractive imaging (CDI) nanoscope. Copper
nanostructures inlaid in SiO2 are coated with 100 nm of aluminum, which is
opaque to visible light and thick enough that neither optical microscopy nor
atomic force microscopy can image the buried interfaces. Short wavelength (29
nm) high harmonic light can penetrate the aluminum layer, yielding
high-contrast images of the buried structures. Moreover, differences in the
absolute reflectivity of the interfaces before and after coating reveal the
formation of interstitial diffusion and oxidation layers at the Al-Cu and
Al-SiO2 boundaries. Finally, we show that EUV CDI provides a unique capability
for quantitative, chemically-specific imaging of buried structures, and the
material evolution that occurs at these buried interfaces, compared with all
other approaches.Comment: 12 pages, 8 figure
Oxidation of a single active site suffices for the functional inactivation of the dimeric Bacillus subtilis OhrR repressor in vitro
Bacillus subtilis OhrR is a dimeric repressor that senses organic peroxides and regulates the expression of the OhrA peroxiredoxin. Derepression results from oxidation of an active site cysteine which ultimately results in formation of a mixed disulfide with a low molecular weight thiol, a cyclic sulfenamide, or overoxidation to the sulfinic or sulfonic acids. We expressed a single-chain OhrR (scOhrR) in which the two monomers were connected by a short amino-acid linker. scOhrR variants containing only one active site cysteine were fully functional as repressors and still responded, albeit with reduced efficacy, to organic peroxides in vivo. Biochemical analyses indicate that oxidation at a single active site is sufficient for derepression regardless of the fate of the active site cysteine. scOhrR with only one active site cysteine in the amino-terminal domain is inactivated at rates comparable to wild-type whereas when the active site is in the carboxyl-terminal domain the protein is inactivated much more slowly. The incomplete derepression noted for single active site variants of scOhrR in vivo is consistent with the hypothesis that protein reduction regenerates active repressor and that, in the cell, oxidation of the second active site may also contribute to derepression
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High-Resolution, Quantitative, and Three-Dimensional Coherent Diffractive Imaging with a Tabletop Euv Source
Imaging is a critical tool used across a broad range of applications in science, technology, medicine, and manufacturing. Microscopy, the type of imaging which allows us to access the elusive yet rich world of what is smaller than we can naturally see-- makes it possible to observe and design the nano-world of biological, material, and nanofabricated systems.
In this thesis, I describe the development of a new type of microscopy that combines two powerful tools: coherent extreme ultraviolet (EUV) light sources produced by high harmonic generation, and ptychographic coherent diffractive imaging. This microscope produces high-resolution, chemically-specific, phase- and amplitude- contrast images with large fields of view on the order of hundreds of microns, while preserving a high spatial resolution on the scale of tens of nanometers.
Recently, we extended this new tabletop microscopy technique to image reflective samples, periodic samples, and to image dynamic nano-scale elastic and thermal processes. I will discuss these advances and in particular demonstrate two new capabilities: first, a new imaging technique with high compositionally- and morphologically-sensitive quantitative information, capable of imaging reactions and diffusion at a buried interface. This capability will open up a new, exquisitely sensitive layer-by-layer imaging that has many applications in nanoscience and nanotechnology, including surface and materials science and metrology. Secondly, I will demonstrate imaging of a thick sample in three dimensions. By accounting for diffraction within a thick sample, it is possible to obtain high-resolution three-dimensional images of biological and meta-material samples non-invasively, and without the use of staining or labeling
Kinetics of RNA polymerase-promoter complex formation: effects of nonspecific DNA-protein interactions.
The rates of formation of RNA polymerase-promoter open complexes at the galactose P2 and lactose UV5 promoters of E. coli were studied using polyacrylamide gels to separate the heparin-resistant complexes from unbound DNA. Both the apparent rate and extent of reaction at these promoters are inhibited at excess RNA polymerase. This inhibition, which can be relieved by the addition of non-promoter DNA, is interpreted to be the result of occlusion of the promoter site by nonspecifically bound polymerase. Additionally, biphasic kinetics are observed at both gal P2 and lac UV5, but not at the PR promoter of phage lambda. This behavior disappears when the concentration of RNA polymerase in the binding reaction is less than that of the promoter fragment. It is proposed that at excess enzyme nonspecifically bound polymerase molecules sliding along the DNA may "bump" closed complexes from the promoter site thereby reducing the rate of open complex formation. Kinetics mechanisms quantifying both the occlusion and bumping phenomena are presented
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