Preparation of Metal-Immobilized Methacrylate-Based Monolithic Columns for Flow-Through Cross-Coupling Reactions

Sabarudin, Akhmad; Shu, Shin; Yamamoto, Kazuhiro; Umemura, Tomonari

doi:10.3390/molecules26237346

Cited by 4 publications

(5 citation statements)

References 50 publications

(54 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Higher sequence coverage results were obtained for the smaller of the studied proteins (18 307.55 Da) βLG (oxidation and phosphorylation, respectively -49% and 0% (classical digestion in solution), 60% and 79% (classical digestion in solution and ZipTip pipette tips), 65% and 0% (µ-IMER), 80% and 89% (µ-IMER and ZipTip pipette tips). However, taking into account the results of βLG phosphorylation, which itself is not a phosphorylated protein and phosphorylation products should not occur (a commercial protein was used), the use of ZipTip was successful for the bigger protein (23,885.90 Da) βCN (oxidation and phosphorylation, respectively -20% and 0% (classical digestion in solution), 26% and 27% (classical digestion in solution and ZipTip pipette tips), 33% and 30% (µ-IMER), 41% and 33% (µ-IMER and ZipTip pipette tips). As the post-translational modi cations affect the structure and biological functions of proteins and peptides by modifying the side chains of amino acids after their biosynthesis the knowledge on their presence might be of particular importance in preparation of functional food preparations or diet additives like protein hydrolysates.…”

Section: Discussionmentioning

confidence: 99%

“…To the best of our knowledge, there are many studies in which monolith-based enzyme microreactors are obtained to exploit both monolithic bed advantages or digestion performance to detect and identi y digestion products by mass spectrometry [22], [23]. Villegas et al used the IMER-CE-MS method for enzymatic digestion, separation, and on-line characterization of proteins [24].…”

Section: Introductionmentioning

confidence: 99%

“…The more commonly used bottom-up strategy involves the classical tryptic in-gel digestion or enzymatic digestion of proteins into peptides, which are then identi ed on the mass spectrometer. While numerous studies have focused on monolith-based enzyme microreactors for the detection and identi cation of digestion products using mass spectrometry, to our knowledge, no literature has reported a comparison between the classical in-solution digestion method and μ-IMER, in conjunction with the use of ZipTips pipette tips for peptide enrichment [12], [13].…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Identification of post-translational modifications of milk and whey proteins with different structures

Rodzik

Railean-Plugaru

Pomastowski³

et al. 2023

Preprint

View full text Add to dashboard Cite

Post-translational modifications (PTMs) regulate cellular processes, and any disruption of PTMs leads to abnormal activity of biological processes, and therefore diseases. The main goal of the present research was focused on developing a rapid analytical method for identifying PTMs in milk (β-casein) and whey (β-lactoglobulin) proteins that differ by structure and composition; the chosen proteins are considered the richest source of nutrients and functional components. The classical in-gel protein digestion method and protein digestion in a microreactor (μ-IMER) method has been performed. In addition, ZipTip pipette tipscontaining C18 reverse phase media were used for both methods to concentrate and purify peptide samples; they also aimed to determine the effect of such a prepared sample on the improvement or deterioration of the sequence coverage result. As support for the preparation of the microreactor, a monolithic copolymer synthesized from GMA and EDMA was used. Subsequently, surface modifications were carried out to attach the enzyme with the highest efficiency. The efficiency of the prepared microreactor was evaluated under HPLC chromatographic conditions using a small-molecule trypsin substrate (BAEE). The obtained hydrolysates from the microreactor and the classical digestion in solution method in the presence of ZipTip pipette tips and without were analyzed by MALDI-TOF MS.

show abstract

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Identification of post-translational modifications of milk and whey proteins with different structures

Rodzik

Railean-Plugaru

Pomastowski³

et al. 2023

Preprint

View full text Add to dashboard Cite

show abstract

“…Subsequent MS and MS/MS analysis of peptides will increase sensitivity and specificity, reveal the identity of proteins, and allow specific assignment of modifications sites 15 . While numerous studies have focused on monolith-based enzyme microreactors for the detection and identification of digestion products using mass spectrometry, to our knowledge, no literature has reported a comparison between the classical in-gel digestion method and μ-IMER, in conjunction with the use of ZipTips for peptide enrichment 16 , 17 .…”

Section: Introductionmentioning

confidence: 99%

Immobilized enzyme microreactors for analysis of tryptic peptides in β-casein and β-lactoglobulin

Rodzik,

Railean,

Pomastowski

et al. 2023

Sci Rep

View full text Add to dashboard Cite

In this study, our primary objective was to develop an effective analytical method for studying trypsin-digested peptides of two proteins commonly found in cow's milk: β-casein (βCN) and β-lactoglobulin (βLG). To achieve this, we employed two distinct approaches: traditional in-gel protein digestion and protein digestion using immobilized enzyme microreactors (μ-IMER). Both methods utilized ZipTip pipette tips filled with C18 reverse phase media for sample concentration. The μ-IMER was fabricated through a multi-step process that included preconditioning the capillary, modifying its surface, synthesizing a monolithic support, and further surface modification. Its performance was evaluated under HPLC chromatography conditions using a small-molecule trypsin substrate (BAEE). Hydrolysates from both digestion methods were analyzed using MALDI-TOF MS. Our findings indicate that the μ-IMER method demonstrated superior sequence coverage for oxidized molecules in βCN (33 ± 1.5%) and βLG (65 ± 3%) compared to classical in-gel digestion (20 ± 2% for βCN; 49 ± 2% for βLG). The use of ZipTips further improved sequence coverage in both classical in-gel digestion (26 ± 1% for βCN; 60 ± 4% for βLG) and μ-IMER (41 ± 3% for βCN; 80 ± 5% for βLG). Additionally, phosphorylations were identified. For βCN, no phosphorylation was detected using classical digestion, but the use of ZipTips showed a value of 27 ± 4%. With μ-IMER and μ-IMER–ZipTip, the values increased to 30 ± 2% and 33 ± 1%, respectively. For βLG, the use of ZipTip enabled the detection of a higher percentage of modified peptides in both classical (79 ± 2%) and μ-IMER (79 ± 4%) digestions. By providing a comprehensive comparison of traditional in-gel digestion and μ-IMER methods, this study offers valuable insights into the advantages and limitations of each approach, particularly in the context of complex biological samples. The findings set a new benchmark in protein digestion and analysis, highlighting the potential of μ-IMER systems for enhanced sequence coverage and post-translational modification detection.

show abstract

“…Taking the above into account, the modification of polymeric materials by means of organic ligands is efficient if there is a large surface area for the chemical or physical modification process. Polymeric materials with these characteristics are known as monoliths [ 7 , 8 , 9 ], which are polymers or copolymers obtained through a polymerization processes in the presence of a porogenic agent [ 10 , 11 ]; in this way, a highly porous material can be obtained that confers a large surface area to the polymer, which is convenient for the modification processes and also for the adsorption processes of heavy metal cations or other types of substances.…”

Section: Introductionmentioning

confidence: 99%

Removal of Toxic Metal Ions Using Poly(BuMA–co–EDMA) Modified with C-Tetra(nonyl)calix[4]resorcinarene

Castillo-Aguirre

Maldonado

Esteso

2022

Toxics

View full text Add to dashboard Cite

A copolymer of poly(BuMA–co–EDMA) modified with C-tetra(nonyl)calix[4]resorcinarene was obtained via the impregnation method. The formation of the modified copolymer was confirmed and investigated using various techniques; in this way, the presence of calix[4]resorcinarene was confirmed by FT-IR spectroscopy and by high resolution transmission electron microscopy. The modified copolymer was used for the removal of highly toxic cations (Pb2+, Hg2+, and Cd2+) from aqueous solutions. To perform the removal, we used the batch sorption technique and the effects of time of contact, pH, and volume of sample on the effective sorption were determined. The best results were observed for Pb2+ extraction, which was comparatively more efficient. Adsorption–desorption experiments revealed that the modified copolymer could be used for several cycles without significant loss of adsorption capacity. Finally, the results showed that the modified copolymer application is highly efficient for the removal of lead ions from aqueous solutions.

show abstract

Preparation of Metal-Immobilized Methacrylate-Based Monolithic Columns for Flow-Through Cross-Coupling Reactions

Cited by 4 publications

References 50 publications

Identification of post-translational modifications of milk and whey proteins with different structures

Identification of post-translational modifications of milk and whey proteins with different structures

Immobilized enzyme microreactors for analysis of tryptic peptides in β-casein and β-lactoglobulin

Removal of Toxic Metal Ions Using Poly(BuMA–co–EDMA) Modified with C-Tetra(nonyl)calix[4]resorcinarene

Contact Info

Product

Resources

About