Hg(II) sequestration and protection by the MerR metal-binding domain (MBD)

Author:

Qin Jie1,Song Lingyun1,Brim Hassan2,Daly Michael J.2,Summers Anne O.1

Affiliation:

1. Department of Microbiology and the Center for Metalloenzyme Studies, University of Georgia, Athens, GA 30602-2605, USA

2. Department of Pathology, Uniformed Services University of the Health Sciences, Bethesda, MD 20814-4799, USA

Abstract

MerR, the metalloregulator of the bacterial mercury resistance (mer) operon, binds Hg(II) with high affinity. To study the mechanism of metal-induced activation, a small protein was previously engineered embodying in a single polypeptide the metal-binding domain (MBD) ordinarily formed between two monomers of MerR. Here the physiological and biochemical properties of MBD expressed on the cell surface or in the cytosol were examined, to better understand the environments in which specific metal binding can occur with this small derivative. Over 20 000 surface copies of MBD were expressed perEscherichia colicell, with metal stoichiometries of ∼1·0 Hg(II) per MBD monomer. Cells expressing MBD on their surface in rich medium bound 6·1-fold more Hg(II) than those not expressing MBD. Although in nature cells use the entiremeroperon to detoxify mercury, it was interesting to note that cells expressing only MBD survived Hg(II) challenge and recovered more quickly than cells without MBD. Cell-surface-expressed MBD bound Hg(II) preferentially even in the presence of a 22-fold molar excess of Zn(II) and when exposed to equimolar Cd(II) in addition. MBD expressed in the cystosol also afforded improved survival from Hg(II) exposure forE. coliand for the completely unrelated bacteriumDeinococcus radiodurans.

Publisher

Microbiology Society

Subject

Microbiology

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