Binding and accumulation of hemin in Porphyromonas gingivalis are induced by hemin.

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Infection and Immunity, July 1994, p. 2885-2892, Vol. 62, No. 7
0019-9567/1994/$04.00+0 DOI:

research-article

Binding and accumulation of hemin in Porphyromonas gingivalis are induced by hemin.

C A Genco, B M Odusanya, and G Brown

Department of Microbiology and Immunology, Morehouse School of Medicine, Atlanta, Georgia 30310.

ABSTRACT

Although hemin is an essential nutrient for the black-pigmentedoral bacterium Porphyromonas gingivalis, the mechanisms involvedin hemin binding and uptake are poorly defined. In this study,we have examined the binding of hemin and Congo red (CR) toP. gingivalis whole cells and have defined the conditions formaximal binding. Additionally, the accumulation of hemin byP. gingivalis under growing conditions has been characterized.P. gingivalis A7436 was grown under hemin- or iron-deplete conditions(basal medium [BM] or Schaedler broth with dipyridyl [SBD])or under hemin- or iron-replete conditions (BM with hemin [BMH]or Schaedler broth [SB]), and hemin and CR binding were assessedspectrophotometrically. Binding of hemin by P. gingivalis wholecells was rapid and was observed in samples obtained from cellsgrown under hemin- and iron-replete and hemin-deplete conditionsbut was not observed in cells grown under iron limitation. Wealso found that P. gingivalis whole cells bound more hemin whengrown in BMH or SB than cells grown in BM or SBD. Binding ofCR by P. gingivalis A7436 was also enhanced when cells weregrown in the presence of hemin or when cells were incubatedwith hemin prior to CR binding. Hemin binding and accumulationwere also assessed using [14C]hemin and [59Fe]hemin under growingconditions. Both [14C]hemin and [59Fe]hemin were accumulatedby P. gingivalis, indicating that iron and the porphyrin ringwere taken into the cell. Binding and accumulation of heminunder growing conditions were also induced by growth of P. gingivalisin hemin-replete media. Hemin accumulation was inhibited bythe addition of KCN to P. gingivalis cultures, indicating thatactive transport was required for hemin uptake. [14C]hemin bindingand accumulation were also inhibited by the addition of eithercold hemin or protoporphyrin IX. Taken together, these resultsindicate that P. gingivalis transports the entire hemin moietyinto the cell and that the binding and accumulation of heminare induced by growth of cultures in the presence of hemin.

Infection and Immunity, July 1994, p. 2885-2892, Vol. 62, No. 7
0019-9567/1994/$04.00+0 DOI:

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