Jack of all trades: versatile catechol crosslinking mechanisms

Yang, Juan; Stuart, Martien A. Cohen; Kamperman, Marleen

doi:10.1039/c4cs00185k

Cited by 593 publications

(632 citation statements)

References 150 publications

(229 reference statements)

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“…However, many of the crosslinking mechanisms for catechol-containing polymers that have been proposed involve the reaction between a quinone-intermediate and another amino acid. Amino acids that have been variously proposed to be involved in Table III. intermolecular and intramolecular crosslinking reactions include lysine, histidine, cysteine and DOPA; the results from the present work indicate that cross-linking the protein resulted in an increase of the corrosion inhibition of the HY80 substrate, therefore the protein may not require a large amount of DOPA in its composition to crosslink effectively; 15 the observations from the present work support those findings.…”

Section: Resultssupporting

confidence: 82%

Investigations of Mussel Adhesive Proteins as Flash Rust Inhibitors

Nelson

Hansen

2016

J. Electrochem. Soc.

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Several proteins found in the adhesive system of the common blue mussel Mytilus edulis have chemical properties which may enable them to inhibit the flash rusting of steels. In this work, Mytilus edulis foot proteins (MAPs) 1, 3, and 5 were isolated and applied to a high strength low alloy steel in a number of buffer systems containing varying amounts of borate, acetate, and phosphate at pH 5.5-7.0. Treated steel samples were then monitored in an exposure chamber at 40 • C and 100% relative humidity for 7 days. The MAP treatments were also evaluated using electrochemical impedance spectroscopy (EIS). The effect of enzymatic crosslinking of the applied proteins using mushroom tyrosinase was also investigated. Steel samples treated with MAP-1 did not inhibit corrosion when the protein was dissolved in deionized water, and the effect of MAP-1 dissolved in buffers containing acetate was not significantly different from control samples. However, when dissolved in 0.05 M phosphate buffer solution at pH 5.5, MAP-3 and MAP-5 were capable of significantly increasing the time to corrosion and significantly reducing the mass loss of the steel coupons in the exposure chamber compared with controls when treated with enzyme. The performance of the crosslinked MAP-5 was similar to a commercial flash rust inhibitor applied at the same mass concentration as the protein, suggesting that MAP-5 and similar proteins or polymers may be capable of inhibiting corrosion. In the past two decades, mussel adhesive proteins (MAPs) from the common blue mussel Mytilus edulis (L) have been the subject of a few investigations into their potential use as corrosion inhibitors, with the hope being that the properties of these biomolecules could be replicated in new formulations of environmentally-friendly corrosion inhibitors. [1][2][3][4] MAPs have a number of unique properties, most of which rely to some extent on the presence of the catecholic amino acid L-3, 4 dihydroxyphenylalanine (DOPA). Like other catechols, DOPA can form strong complexes with many metals, particularly Fe(III).5 These metal-catechol complexes can form either in solution, or on a metal oxide surface.6 It has been shown that in some cases the formation of stable organometallic complexes on a metal surface can inhibit corrosion by preventing the dissolution of the oxide layer to which it is adsorbed.7 Previous investigations have indicated that DOPA-containing proteins are capable of inhibiting corrosion to various degrees on some metals. 1,[8][9][10][11][12][13] In addition to this, DOPA can participate in crosslinking reactions as a result of chemical or enzymatic oxidation. When oxidized, DOPA forms a quinone-intermediate, which can in turn react further with catechol groups or nucleophiles present elsewhere in the protein to form a crosslinked protein.14,15 Previous findings by Hansen et al. 16 demonstrated that enzymatic cross-linking of adsorbed MAP-1 protein resulted in thickening of the protein film, whereas others have reported a compression of the adsorbed prot...

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Section: Resultssupporting

confidence: 82%

Investigations of Mussel Adhesive Proteins as Flash Rust Inhibitors

Nelson

Hansen

2016

J. Electrochem. Soc.

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“…Consistent with the suggestion of oxidative crosslinking at the developing interface, recent studies of adult barnacle interfaces using in situ cyclic voltammetry have revealed electrochemical behavior consistent with the presence of redox active compounds (Golden et al, 2016), as well as spectroscopic evidence for the presence of phenolic compounds in interfacial barnacle fluids (Burden et al, 2012). Quinone tanning can be driven by free radicals or enzymes and mediates crosslinking in diverse systems and contexts, including sclerotized insect cuticle and mussel byssal threads (Korytowski et al, 1987;Waite, 1995;Suderman et al, 2006;Yang et al, 2014). Surprisingly, antimicrobial properties of barnacle secretions have not been deeply explored, even after the identification of a barnacle cement protein with homology to the antibacterial enzyme lysozyme (Kamino and Shizuri, 1998).…”

Section: Discussionmentioning

confidence: 55%

Barnacle biology before, during and after settlement and metamorphosis: a study of the interface

Essock‐Burns

Gohad

Orihuela

et al. 2016

Journal of Experimental Biology

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Mobile barnacle cypris larvae settle and metamorphose, transitioning to sessile juveniles with morphology and growth similar to that of adults. Because biofilms exist on immersed surfaces on which they attach, barnacles must interact with bacteria during initial attachment and subsequent growth. The objective of this study was to characterize the developing interface of the barnacle and substratum during this key developmental transition to inform potential mechanisms that promote attachment. The interface was characterized using confocal microscopy and fluorescent dyes to identify morphological and chemical changes to the interface and the status of bacteria present as a function of barnacle developmental stage. Staining revealed patchy material containing proteins and nucleic acids, reactive oxygen species amidst developing cuticle, and changes in bacteria viability at the developing interface. We found that as barnacles metamorphose from the cyprid to juvenile stage, proteinaceous materials with the appearance of coagulated liquid were released into and remained at the interface. It stained positive for proteins, including phosphoprotein, as well as nucleic acids. Regions of the developing cuticle and the patchy material itself stained for reactive oxygen species. Bacteria were absent until the cyprid was firmly attached, but populations died as barnacle development progressed. The oxidative environment may contribute to the cytotoxicity observed for bacteria and has the potential for oxidative crosslinking of cuticle and proteinaceous materials at the interface.

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“…We suggestt hat the coupling reactiono ft hiols catalyzed by PDA should follow am echanism similar to that of mussel adhesion [4,5] and that of disulfide bond formation in DsbB [23,24] in nature.S cheme 1s hows that the proposed mechanism consists of three steps:o ne, nucleophilic attack of the quinone groups on the PDA particles (state 1) by the first thiolate anion to form at hiol-dopamine adduct (state 2), as illustrated by previousw ork; [38] two, attack of the thioether adduct by as econd thiolate anion to form ad isulfide and phenol-state dopamine (state 3);t hree, oxidization of phenol-state dopamine into quinone-state dopamine by oxygen dissolved in the solution.The quinone groups on the PDA particles were identified by X-ray photoelectrons pectroscopy (XPS) (FigureS4), which is in accordance with the previousr eport. [39] To further understand this mechanism, PDA particlesw ereu sed to sequentially catalyzet he individual oxidative couplings of sodium 3-mercapto-1-propanesulfonate (MPS), MGL, and sodium 3-mercapto-1-propanesulfonate (shown in Figure 1).…”

mentioning

confidence: 88%

“…[1][2][3][4][5][6] They playacrucial role in maintaining the conformationals tability and biological activity of proteins [1,2] and participate in the adhesion process of mussel foot protein. [4,5] Over the past decades, these chemicals have received much attentiona saresult of their artificial applicationsi ns ynthesizing pharmaceutical molecules, [7,8] constructing functional materials, [9][10][11] building dynamic combinatorial libraries, [12,13] and preparing sulfur-containing organic compounds. [14,15] Numerous methods have been developed to form disulfide bonds in both scientific laboratories and industrial factories.…”

mentioning

confidence: 99%

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Polydopamine as a Catalyst for Thiol Coupling

Yang

et al. 2015

ChemCatChem

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In biological systems, disulfide bonds are formed efficiently under mild conditions without the release of harmful byproducts. Inspired by nature, we report a biomimetic polydopamine (PDA) catalyst for oxidative thiol coupling. This reaction was accelerated with only a small amount of PDA particles in neutral, weakly alkaline, and even weakly acidic aqueous media at room temperature under an air atmosphere. The catalytic particles were facilely separated and were reused without a decrease in activity. The entire process is totally biofriendly, including the synthesis of the PDA particles. This route is especially useful for the synthesis of pharmaceutical molecules.

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Jack of all trades: versatile catechol crosslinking mechanisms

Cited by 593 publications

References 150 publications

Investigations of Mussel Adhesive Proteins as Flash Rust Inhibitors

Investigations of Mussel Adhesive Proteins as Flash Rust Inhibitors

Barnacle biology before, during and after settlement and metamorphosis: a study of the interface

Polydopamine as a Catalyst for Thiol Coupling

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