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1.
J Lipid Res ; 65(6): 100560, 2024 06.
Artigo em Inglês | MEDLINE | ID: mdl-38750995

RESUMO

Zinc is required for virtually all biological processes. In plasma, Zn2+ is predominantly transported by human serum albumin (HSA), which possesses two Zn2+-binding sites of differing affinities (sites A and B). Fatty acids (FAs) are also transported by HSA, with seven structurally characterized FA-binding sites (named FA1-FA7) known. FA binding inhibits Zn2+-HSA interactions, in a manner that can impact upon hemostasis and cellular zinc uptake, but the degree to which binding at specific FA sites contributes to this inhibition is unclear. Wild-type HSA and H9A, H67A, H247A, and Y150F/R257A/S287A (FA2-KO) mutant albumins were expressed in Pichia pastoris. Isothermal titration calorimetry studies revealed that the Zn2+-binding capacity at the high-affinity Zn2+ site (site A) was reduced in H67A and H247A mutants, with site B less affected. The H9A mutation decreased Zn2+ binding at the lower-affinity site, establishing His9 as a site B ligand. Zn2+ binding to HSA and H9A was compromised by palmitate, consistent with FA binding affecting site A. 13C-NMR experiments confirmed that the FA2-KO mutations prohibited FA binding at site FA2. Zn2+ binding to the FA2-KO mutant was unaffected by myristate, suggesting binding at FA2 is solely responsible for inhibition. Molecular dynamics studies identified the steric obstruction exerted by bound FA in site FA2, which impedes the conformational change from open (FA-loaded) to closed (FA-free) states, required for Zn2+ to bind at site A. The successful targeting of the FA2 site will aid functional studies exploring the interplay between circulating FA levels and plasma Zn2+ speciation in health and disease.


Assuntos
Ácidos Graxos , Albumina Sérica Humana , Zinco , Zinco/metabolismo , Humanos , Sítios de Ligação , Ácidos Graxos/metabolismo , Albumina Sérica Humana/metabolismo , Albumina Sérica Humana/química , Ligação Proteica
2.
Biomolecules ; 14(1)2024 Jan 13.
Artigo em Inglês | MEDLINE | ID: mdl-38254704

RESUMO

Interactions between proteins and metal ions and their complexes are important in many areas of the life sciences, including physiology, medicine, and toxicology. Despite the involvement of essential elements in all major processes necessary for sustaining life, metalloproteomes remain ill-defined. This is not only owing to the complexity of metalloproteomes, but also to the non-covalent character of the complexes that most essential metals form, which complicates analysis. Similar issues may also be encountered for some toxic metals. The review discusses recently developed approaches and current challenges for the study of interactions involving entire (sub-)proteomes with such labile metal ions. In the second part, transition metals from the fourth and fifth periods are examined, most of which are xenobiotic and also tend to form more stable and/or inert complexes. A large research area in this respect concerns metallodrug-protein interactions. Particular attention is paid to separation approaches, as these need to be adapted to the reactivity of the metal under consideration.


Assuntos
Proteoma , Íons
3.
Int J Biol Macromol ; 222(Pt B): 1925-1935, 2022 Dec 01.
Artigo em Inglês | MEDLINE | ID: mdl-36206839

RESUMO

Biomimetic mineralization of enzymes for enhanced stability and activity is an important area of research due to its potential applications. Inorganic materials with enzymes coated and or embedded in them, viz., protein-inorganic hybrid nanomaterials with distinctive morphology and surface characteristics are promising candidates for exploring their elevated enzymatic activity. In this work, we have developed two different types of protein inorganic nanohybrid materials using a 120 kDa lectin purified from bitter gourd seeds (Momordica charantia lectin, MCL), and (i) copper phosphate nanoflowers to result in a protein - inorganic nano hybrid material CuPNF_MCL and (ii) encapsulating the protein in zeolitic imidazole framework, ZIF8_MCL. While CuPNF_MCL showed floral morphology, the ZIF8_MCL mostly showed hexapod morphology as noticed from the microscopy data. Both the nanomaterials showed a distinctive trend of decrease in size with increase in the protein concentration used during the preparation. The nanoflowers also showed an increase in the tightness of the packing of petals with increase in the protein concentration. Powder X-Ray diffraction studies confirmed the crystallinity of the inorganic frameworks. The Fourier Transform infrared spectroscopy studies coupled with confocal imaging of the fluorophore tagged MCL embedded hybrids confirmed the presence of the protein. The MCL protein was examined for its ability to cleave DNA, i.e., nuclease activity using pBR322, wherein the form I plasmid is completely transformed into the form II / III at 2 mg/mL concentration of the protein. However, both the hybrids showed a superior nuclease activity as compared to the protein, wherein the CuPNF_MCL showed a threefold greater nuclease activity as compared to the ZIF8_MCL. The greater nuclease activity of CuPNF_MCL is attributable to its mesoporous nature with higher pore size and pore volume as compared to that in case of ZIF8_MCL, which is microporous in nature. Thus, in this paper, we have purified a nuclease like lectin from bitter gourd seeds and improved its nuclease property by converting it into inorganic hybrid nanomaterial of two types wherein higher activity was observed in the material having better porosity and surface area characteristics.


Assuntos
Momordica charantia , Zeolitas , Momordica charantia/química , Lectinas/química , Cobre/metabolismo , Fosfatos/metabolismo , Biomimética , Imidazóis/metabolismo , Desoxirribonucleases/metabolismo
4.
ACS Omega ; 4(8): 13231-13240, 2019 Aug 20.
Artigo em Inglês | MEDLINE | ID: mdl-31460450

RESUMO

A triazole-derivatized, spiro-indoline-linked, 1,3-di-derivative of calix[4]arene (L) has been synthesized to take advantage of its ion-binding capability in the ring-open form. Indeed, the spiro-indoline moiety is well known for its photochromic, acidochromic, and metallochromic properties. Therefore, the L has been explored for Cu2+ binding, cell imaging, and anticancer activity of the corresponding complex since Cu2+ complexes are known for such activity. The conversion from the closed to open form of L is expedited by light or proton, while the metal ion can open as well as stabilize it. The open form of L showed binding of Cu2+ ratiometrically as demonstrated by absorption and fluorescence spectroscopy. This leads to the formation of 1:1 complex with a binding constant of (6.9 ± 2.3) × 105 M-1, with the lowest detection limit being 1.9 nM. In the complex, the Cu2+ is bound by two triazole-N and two phenolic-O groups resulting in a distorted tetrahedral coordination core of CuN2O2 as demonstrated based on density functional theory studies. To form such coordination core, the arms underwent considerable changes in some of the dihedral angles. The binding of Cu2+ to L induces self-assembly of L by varying from simple particles to rodlike structures when bound to Cu2+. The on-off fluorescence intensity of L and its Cu2+-bound species are responsible for imaging cancer cells. The L shows red fluorescence in MDA-MB-231 cancer cells by targeting mitochondria as proved based on the colocalization study carried out using MitoTracker Green. While the L alone is nontoxic to cancer cells, the presence of Cu2+ brings cell death to an extent of 90% with an IC50 value of 165 nM by bringing a substantial quench in the fluorescence of L. A shift of population from G0/G1 and G2M phases to the Sub-G1 phase was observed as the concentration of the complex was increased, indicating cell death as studied by fluorescence-activated cell sorting. Thus, the present work clearly proved that a calix[4]arene functionalized at the lower rim with spiro-indoline moieities when complexed with Cu2+ acts as an efficient anticancer agent and is capable of imaging cancer cells.

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