Stability, unfolding mechanism, spectroscopic, densimetric, and structural characteristics of the oxidatively stable C69S variant (HodC) of 1H-3-hydroxy-4-oxoquinaldine 2,4-dioxygenase (Hod) have been determined by classical and pressure modulation scanning calorimetry (DSC and PMDSC, respectively), circular dichroism (CD) spectroscopy, differential scanning densimetry (DSD), and dynamic light scattering measurements. At 25 degrees C, hexahistidine-tagged HodC has a hydrodynamic radius of 2.3 nm and is characterized by an unusually high degree of alpha-helical structure of approximately 60%, based on deconvolution of CD spectra. The percentage of beta-sheets and -turns is expected to be relatively low in view of its sequence similarity to proteins of the alpha/beta-hydrolase fold superfamily. His6HodC exhibits three-state unfolding (N <--> I <--> D) with an intermediate state I that exhibits at the transition temperature a volume larger than that of the native or denatured state. The intermediate state I is also associated with the highest isothermal expansion coefficient, alphaP, of the three states and exhibits a significantly lower percentage of alpha-helical structure than the native state. The stability difference between the native and intermediate state is rather small which makes I a potential candidate for reactions with various ligands, particularly those having a preference for the apparently preserved beta-type motifs.
Hollow polymeric capsules prepared from Layer-by-Layer coating of colloidal templates with polyelectrolyte multilayers are promising materials for drug delivery and release applications. Details of the wall structure arising from the core dissolution process are investigated by high resolution scanning electron microscopy (SEM), using both secondary (SE) and backscattered electron (BSE) imaging modes. Atomic force microscopy (AFM) of the capsules in liquid was used as an independent technique. BSE images of the coated templates may be used for a rough estimation of the wall thickness. A freeze-drying procedure allows for the first time the investigation of dried multilayer capsules with an intact shape by SEM. Details of the nanostructure of the capsule walls are obtained, the topography shows structures on the scale of several 10 nm, corresponding to single chains. These structures are confirmed by AFM in liquid. In addition, after core dissolution single holes with sizes above 10 nm can be identified in the capsule wall. These holes are the structural property controlling the permeation and release and are here visualized for the first time. The number of holes per capsule as well as their distribution and size are analysed and discussed in their relevance for release applications.Scheme 1 Graphical illustration of the composition of the capsules.
Thermodynamic stability parameters and the equilibrium unfolding mechanism of His 6HodC69S, a mutant of 1 H-3-hydroxy-4-oxoquinaldine 2,4-dioxygenase (Hod) having a Cys to Ser exchange at position 69 and an N-terminal hexahistidine tag (His 6HodC69S), have been derived from isothermal unfolding studies using guanidine hydrochloride (GdnHCl) or urea as denaturants. The conformational changes were monitored by following changes in circular dichroism (CD), fluorescence, and dynamic light scattering (DLS), and the resulting transition curves were analyzed on the basis of a sequential three-state model N = I = D. The structural changes have been correlated to catalytic activity, and the contribution to stability of the disulfide bond between residues C37 and C184 in the native protein has been established. A prominent result of the present study is the finding that, independent of the method used for denaturing the protein, the unfolding mechanism always comprises three states which can be characterized by, within error limits, identical sets of thermodynamic parameters. Apparent deviations from three-state unfolding can be rationalized by the inability of a spectroscopic probe to discriminate clearly between native, intermediate, and unfolded ensembles. This was the case for the CD-monitored urea unfolding curve.
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