Mario A. Barón-Rodríguez scite author profile

Abstractβ-2-microglobulin (β2m) self-associates into fibrillar amyloid deposits in the musculoskeletal system of patients undergoing hemodialysis treatment. Previous studies have shown that stoichiometric amounts of Cu(II) at near physiological conditions can cause β2m to organize into native-like dimers prior to forming amyloid fibrils. Here, we report the results from selective covalent labeling reactions combined with mass spectrometry that provide insight into the amino acid residues that mediate dimer formation in the wild-type protein. Using three complementary covalent labeling reagents, we find that the dimer interface is formed by the anti-parallel stacking of ABED β-sheets from two β2m monomers. In addition, our data clearly indicate that a dimer interface involving the interactions of D-D strands from separate protein units as seen in the recent crystal structures of two mutant β2m oligomers is unlikely.β-2-microglobulin (β2m) is the non-covalently bound light chain of the class I major histocompatibility complex (MHC-I) (1). It is a monomeric protein with 99 residues (~12 kDa). It adopts a seven-stranded β-sandwich fold with one β sheet formed by four strands and the other by three strands. A disulfide bond between Cys25 and Cys80 links strands the two sheets in the folded state of the protein. β2m is vital for the correct folding, assembly, and cell-surface expression of the MHC-I complex. As part of normal cell turnover, β2m is released from the MHC-I complex and carried to the kidney where it is degraded. Upon renal failure, serum levels of β2m increase up to ~60 times above the normal level of 0.1 µM, and the protein aggregates into insoluble amyloid fibrils in the joints (2,3). Elevated β2m concentrations alone, however, are not sufficient to trigger fibrillogenesis (4,5). β2m amyloid formation must therefore result from features unique to hemodialysis, but the exact cause in vivo is not known. ®2m amyloid fibrils can be generated in vitro, though, under acidic conditions (pH < 3.6) (6), by removing the first six N-terminal amino acids (7), by mixing the protein with collagen at pH = 6.4 (8), by sonicating the protein in the presence of sodium dodecyl sulfate at pH = *Corresponding author Department of Chemistry, University of Massachusetts, Amherst, rwvachet@chem.umass.edu, Telephone: (413) 545-2733, Fax: (413) . † Department of Chemistry, Universidad Industrial de Santander, AA 678, Bucaramanga, Colombia SUPPORTING INFORMATION AVAILABLEAdditional data can be found in the Supporting Information. These data include (i) plots showing the intensities of unmodified and modified forms of fragment Ile1-Tyr10 for three trials in the absence of Cu; (ii) tables presenting the intensities of unmodified and modified forms of peptide fragments containing residues Asn83, Lys94, and Lys6; (iii) plots illustrating the intensities of unmodified and modified forms of fragment Ile1-Tyr10 in the absence of Cu and 2 hours after addition of Cu; (iv) plots illustrating the extent of NHSA modification of β2m res...

show abstract

Structural Insights into the Pre-Amyloid Tetramer of β-2-Microglobulin from Covalent Labeling and Mass Spectrometry

Mendoza

Barón-Rodríguez

Blanco

et al. 2011

Biochemistry

View full text Add to dashboard Cite

The main pathogenic process underlying dialysis-related amyloidosis (DRA) is the accumulation of β-2-microglobulin (β2m) as amyloid fibrils in the musculoskeletal system, and some evidence suggests that Cu(II) may play a role in β2m amyloid formation. Cu(II)-induced β2m fibril formation is preceded by the formation of discrete, oligomeric intermediates, including dimers, tetramers, and hexamers. In this work, we use selective covalent labeling reactions combined with mass spectrometry to investigate the amino acids responsible for mediating tetramer formation in wild-type β2m. By comparing the labeling patterns of the monomer, dimer, and tetramer, we find evidence that the tetramer interface is formed by the interaction of D strands from one dimer unit and G strands from another dimer unit. This covalent labeling data along with molecular dynamics calculations enable the construction of a tetramer model that indicates how the protein might proceed to form even higher order oligomers.

show abstract

Synthesis, Biological Evaluation and In Silico Computational Studies of 7-Chloro-4-(1H-1,2,3-triazol-1-yl)quinoline Derivatives: Search for New Controlling Agents against Spodoptera frugiperda (Lepidoptera: Noctuidae) Larvae

Rosado-Solano

Barón-Rodríguez

Florez

et al. 2019

J. Agric. Food Chem.

View full text Add to dashboard Cite

The insecticidal and antifeedant activities of five 7-chloro-4-(1H-1,2,3-triazol-1-yl)quinoline derivatives were evaluated against the maize armyworm, Spodoptera frugiperda (J.E. Smith). These hybrids were prepared through a copper-catalyzed azide alkyne cycloaddition (CuAAC, known as a click reaction) and displayed larvicidal properties with LD50 values below 3 mg/g insect, and triazolyl-quinoline hybrid 6 showed an LD50 of 0.65 mg/g insect, making it 2-fold less potent than methomyl, which was used as a reference insecticide (LD50 = 0.34 mg/g insect). Compound 4 was the most active antifeedant derivative (CE50 = 162.1 μg/mL) with a good antifeedant index (56–79%) at concentrations of 250–1000 μg/mL. Additionally, triazolyl-quinoline hybrids 4–8 exhibited weak inhibitory activity against commercial acetylcholinesterase from Electrophorus electricus (electric-eel AChE) (IC50 = 27.7 μg/mL) as well as low anti-ChE activity on S. frugiperda larvae homogenate (IC50 = 68.4 μg/mL). Finally, molecular docking simulations suggested that hybrid 7 binds to the catalytic active site (CAS) of this enzyme and around the rim of the enzyme cavity, acting as a mixed (competitive and noncompetitive) inhibitor like methomyl. Triazolyl-quinolines 4–6 and 8 inhibit AChE by binding over the perimeter of the enzyme cavity, functioning as noncompetitive inhibitors. The results described in this work can help to identify lead triazole structures from click chemistry for the development of insecticide and deterrent products against S. frugiperda and related insect pests.

show abstract

Design of a Repellent Against Aedes aegypti (Diptera: Culicidae) Using in silico Simulations With AaegOBP1 Protein

Portilla-Pulido

Castillo-Morales

Barón-Rodríguez³

et al. 2019

View full text Add to dashboard Cite

Skin irritation has been reported to be the main adverse effect of excessive use of N,N-diethyl-m-toluamide (DEET) and ethyl 3-acetyl(butyl)amino (IR3535) commercial repellents. Therefore, there is an interest in alternatives of natural origin such as essential oils (EOs) and major compounds, which have repellent effects but have no contraindications. The main purpose of the present study was to identify the repellent effect of selected terpenes on Aedes aegypti Linnaeus, 1762 (Diptera: Culicidae) by in silico analysis based on their affinity with the odorant protein AaegOBP1. The protein-metabolite interactions in 20 terpenes were analyzed using the SwissDock tool. Terpenes presenting the highest affinity compared with commercial repellents were selected to evaluate repellent activity at concentrations 0.1, 10, and 25% against Ae. aegypti. Different periods (0–2, 2–15, 15–60 min) were evaluated with DEET as a positive control. The toxicity of terpenes was verified through Osiris and Molinspiration Cheminformatics Software, and cytotoxicity assays in Vero and HepaRG cells were performed using the MTT method. Two formulations were prepared with polyethylene glycol to evaluate skin long-lasting in vivo assay. The results showed four terpenes: geranyl acetate, nerolidol, α-bisabolol, and nerol, with affinity to AaegOBP1 comparable with DEET and IR3535. Geranyl acetate, nerolidol, and their mixtures showed no cytotoxicity and protection percentages close to 100% during the test at concentrations 10 and 25%. Long-lasting assays with geranyl acetate and nerolidol formulate showed 3 h as maximum protection time with 100% protection percentage. These metabolites and their mixtures are candidates to repellent formulations with times and protection percentages similar to DEET.

show abstract

Evaluación del potencial antioxidante en extracto de espinaca por voltamperometría cíclica

Pérez-Cabeza

Angarita

Cervantes

et al. 2018

rev.ion

View full text Add to dashboard Cite

Resumen La capacidad antioxidante de extractos de plantas ha sido estudiada por técnicas voltamperométricas gracias a su sensibilidad, selectividad, bajo costo, simplicidad y rapidez. En esta investigación se utilizó la Voltamperometría Cíclica para estudiar el potencial antioxidante en la preservación de extractos etanólicos de hojas de espinaca (Spinacia oleracea). Los extractos se obtuvieron luego de macerar hojas de espinaca con etanol industrial y llevar a ultrasonido. Los barridos potenciométricos de los extractos a 0, 7 y 15 días de preparación se realizaron en una solución amortiguadora Sørensen. Se utilizaron electrodos de Au (trabajo), Ag/AgCl (referencia) y Pt (auxiliar) desde-1,2 hasta 1,2V. Los resultados mostraron una alta capacidad antioxidante de los extractos (potenciales de oxidación por debajo de los 600mV) y una disminución en la corriente durante el aumento de la preservación de los extractos (0, 7 y 15 días); lo cual permitió concluir que su potencial antioxidante disminuye a través del tiempo gobernada por una cinética de primer orden. Además, los resultados de la capacidad antioxidante fueron correlacionados con la cuantificación de polifenoles totales, mediante en método de Folin Ciocalteu.

show abstract

scite is a Brooklyn-based organization that helps researchers better discover and understand research articles through Smart Citations–citations that display the context of the citation and describe whether the article provides supporting or contrasting evidence. scite is used by students and researchers from around the world and is funded in part by the National Science Foundation and the National Institute on Drug Abuse of the National Institutes of Health.

Contact Info

customersupport@researchsolutions.com

10624 S. Eastern Ave., Ste. A-614

Henderson, NV 89052, USA

This site is protected by reCAPTCHA and the Google Privacy Policy and Terms of Service apply.

Blog Terms and Conditions API Terms Privacy Policy Contact Cookie Preferences Do Not Sell or Share My Personal Information

Made with 💙 for researchers

Part of the Research Solutions Family.