Potentiation by sulfide of hydrogen peroxide-induced killing of Escherichia coli.

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Infect Immun. 1985 September; 49(3): 538-543

Potentiation by sulfide of hydrogen peroxide-induced killing of Escherichia coli.

E H Berglin and J Carlsson

ABSTRACT

L-Cysteine potentiates 100-fold the hydrogen peroxide-inducedkilling of a growing culture of Escherichia coli K-12 (Berglinet al., J. Bacteriol. 152:81-88). In the present study it isshown that hydrogen sulfide is formed from L-cysteine and thatsodium sulfide could substitute for L-cysteine in the potentiationof hydrogen peroxide-induced killing of E. coli K-12. Additionof an amino acid, L-leucine, L-valine, or L-alanine, to an L-cysteine-containingmedium with a growing culture of E. coli K-12 inhibited hydrogensulfide formation and the potentiation of hydrogen peroxide-inducedkilling. These amino acids did not inhibit hydrogen sulfideformation from L-cysteine by a cell extract, and they did notinhibit the potentiation by sulfide of hydrogen peroxide-inducedkilling. This indicated that the amino acids protected the culturefrom L-cysteine-potentiated, hydrogen peroxide-induced killingby inhibiting the transport of L-cysteine into the cell. Thepotentiation by sodium sulfide of hydrogen peroxide-inducedkilling was abolished by the metal ion chelator 2,2'-bipyridyl.This indicated that metal ions, in addition to sulfide, wereinvolved in the killing. Toxic effects of hydrogen peroxideare often presumed to be mediated by hydroxyl radicals formedin iron-catalyzed reactions. It was demonstrated that iron sulfidewas more efficient than ferrous iron in catalyzing the formationof hydroxyl radicals from hydrogen peroxide. It was suggestedthat hydrogen sulfide formed in polymicrobial infections mayplay an important role in the host defense by potentiating theantimicrobial effect of hydrogen peroxide produced by phagocyticcells.

Infect Immun. 1985 September; 49(3): 538-543

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