2004
DOI: 10.1002/elps.200305861
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Comparison of two glutaraldehyde immobilization techniques for solid‐phase tryptic peptide mapping of human hemoglobin by capillary zone electrophoresis and mass spectrometry

Abstract: Stabilization of proteolytic enzymes, especially by immobilization, is of considerable interest because of their potential applications in medicine and the chemical and pharmaceutical industries. We report here a detailed comparison of two procedures for trypsin immobilization using the same homobifunctional agent, glutaraldehyde, for the purpose of peptide mapping. These methods include covalent coupling either to controlled pore glass (solid support) or via a cross-linking reaction (without any solid support… Show more

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Cited by 35 publications
(24 citation statements)
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“…Photopolymerized sol-gel monoliths (PSG) with pepsin encapsulated in the gel matrix enlarged the surface and facilitated the accessibility of enzymatic sites for large proteins [253]. Moreover, supportless immobilization by enzyme cross-linking through glutaraldehyde was used [251]. Enhanced enzymatic activity in combination with reaction chambers of minute volume and elevated substrate concentrations considerably reduces incubation time [252].…”
Section: Enzymatic Microreaction Devices In Ce-msmentioning
confidence: 99%
See 1 more Smart Citation
“…Photopolymerized sol-gel monoliths (PSG) with pepsin encapsulated in the gel matrix enlarged the surface and facilitated the accessibility of enzymatic sites for large proteins [253]. Moreover, supportless immobilization by enzyme cross-linking through glutaraldehyde was used [251]. Enhanced enzymatic activity in combination with reaction chambers of minute volume and elevated substrate concentrations considerably reduces incubation time [252].…”
Section: Enzymatic Microreaction Devices In Ce-msmentioning
confidence: 99%
“…When executed in solution, long incubation times, single use, and rapid loss of catalytic activity are frequently encountered [251]. As an alternative, digestion can also take place in enzymatic microreactors, with the enzymes immobilized on a solid support, such as CPG or monolithic phases [251][252][253].…”
Section: Enzymatic Microreaction Devices In Ce-msmentioning
confidence: 99%
“…Okafo et al [53] then separated tryptic peptides of globin chains by using phytic acid as an additive in the buffer. Migneault et al [54] separated the Hb digests by CZE using three given batches of immobilized method: (i) glutaraldehydetrypsin, (ii) glutaraldehyde-cross-linked trypsin, and (iii) free trypsin. Recently, Lin et al [55] developed a simple and rapid procedure for mapping of Hb D-Ouled Rabah, Hb Marseille, Hb G-Philadelphia, and Hb Ube-2 from globin chains of total a-and b-or the individual a-or b-chains, as shown in Fig.…”
Section: Globin Chains and Peptides Mappingmentioning
confidence: 99%
“…Glutaraldehyde has been used for many years for enzyme immobilization (27). It reacts with several functional protein groups, such as amine, thiol, phenol, and imidazole, since nucleophilic amino acid residues are the most reactive ones.…”
Section: Fig 3 Fduv Of Standard Solutions Of N-acetylglucosamine (Amentioning
confidence: 99%