Tiffany Derrick scite author profile

Two copper-binding compounds/cofactors (CBCs) were isolated from the spent media of both the wild type and a constitutive soluble methane monooxygenase (sMMOC) mutant, PP319 (P. A. Phelps et al., Appl. Environ. Microbiol. 58:3701–3708, 1992), of Methylosinus trichosporium OB3b. Both CBCs are small polypeptides with molecular masses of 1,218 and 779 Da for CBC-L1 and CBC-L2, respectively. The amino acid sequence of CBC-L1 is S?MYPGS?M, and that of CBC-L2 is SPMP?S. Copper-free CBCs showed absorption maxima at 204, 275, 333, and 356 with shoulders at 222 and 400 nm. Copper-containing CBCs showed a broad absorption maximum at 245 nm. The low-temperature electron paramagnetic resonance (EPR) spectra of copper-containing CBC-L1 showed the presence of a copper center with an EPR splitting constant between those of type 1 and type 2 copper centers (g⊥ = 2.087, g∥︀ = 2.42 G, ‖A∥︀‖ = 128 G). The EPR spectrum of CBC-L2was more complex and showed two spectrally distinct copper centers. One signal can be attributed to a type 2 Cu2+ center (g⊥ = 2.073, g∥︀ = 2.324 G, ‖A∥︀‖ = 144 G) which could be saturated at higher powers, while the second shows a broad, nearly isotropic signal near g⊥ = 2.063. In wild-type strains, the concentrations of CBCs in the spent media were highest in cells expressing the pMMO and stressed for copper. In contrast to wild-type strains, high concentrations of CBCs were observed in the extracellular fraction of the sMMOC mutants PP319 and PP359 regardless of the copper concentration in the culture medium.

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Safety, uptake, and use of a dapivirine vaginal ring for HIV-1 prevention in African women (HOPE): an open-label, extension study

Mirembe

Hunidzarira

Hillier

et al. 2021

The Lancet HIV

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Separation and Analysis of Peptides and Proteins

et al. 1999

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This review focuses on selected applications of the separation and analysis of peptides and proteins published during the period of 1997-1998. Specific topic areas covered include high-performance liquid chromatography (HPLC), ultrafiltration, capillary electrophoresis (CE), affinity-based methods for protein isolation and separation, mass spectrometry (MS), detection of nonenzymatic posttranslational modifications, nuclear magnetic resonance spectroscopy (NMR), infrared (IR) and Raman spectroscopy, circular dichroism (CD), UV-visible absorption spectroscopy, dynamic light scattering, and calorimetry. The quantification and identification of peptides and proteins by chromatographic methods and MS have become fairly routine, as has the conformational analysis of peptides and small proteins in solution by CD, IR, and NMR. Therefore, these topics are not reviewed in detail here. In this review, we have attempted to highlight new technological developments or unique applications of analytical methods that impact the analysis of peptides and proteins.

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Analysis of Protein/Ligand Interactions with NMR Diffusion Measurements: The Importance of Eliminating the Protein Background

Derrick

McCord

Larive

2002

Journal of Magnetic Resonance

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¹⁹F diffusion NMR analysis of enzyme–inhibitor binding

Derrick

Lucas

Dimicoli

et al. 2002

Magnetic Reson in Chemistry

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Tiffany Derrick

Copper-Binding Compounds from Methylosinus trichosporium OB3b

Safety, uptake, and use of a dapivirine vaginal ring for HIV-1 prevention in African women (HOPE): an open-label, extension study

Separation and Analysis of Peptides and Proteins

Analysis of Protein/Ligand Interactions with NMR Diffusion Measurements: The Importance of Eliminating the Protein Background

¹⁹F diffusion NMR analysis of enzyme–inhibitor binding

Contact Info

Product

Resources

About

Tiffany Derrick

Copper-Binding Compounds from Methylosinus trichosporium OB3b

Safety, uptake, and use of a dapivirine vaginal ring for HIV-1 prevention in African women (HOPE): an open-label, extension study

Separation and Analysis of Peptides and Proteins

Analysis of Protein/Ligand Interactions with NMR Diffusion Measurements: The Importance of Eliminating the Protein Background

19F diffusion NMR analysis of enzyme–inhibitor binding

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Product

Resources

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¹⁹F diffusion NMR analysis of enzyme–inhibitor binding