The activation mechanism of human porphobilinogen synthase by 2-mercaptoethanol: intrasubunit transfer of a reserve zinc ion and coordination with three cysteines in the active center

Nori Sawada; Noriyuki Nagahara; Tadashi Sakai; Yoshiaki Nakajima; Masayasu Minami; Tomoyuki Kawada

doi:10.1007/s00775-005-0629-5

The activation mechanism of human porphobilinogen synthase by 2-mercaptoethanol: intrasubunit transfer of a reserve zinc ion and coordination with three cysteines in the active center

J Biol Inorg Chem. 2005 Mar;10(2):199-207. doi: 10.1007/s00775-005-0629-5. Epub 2005 Mar 4.

Authors

Nori Sawada¹, Noriyuki Nagahara, Tadashi Sakai, Yoshiaki Nakajima, Masayasu Minami, Tomoyuki Kawada

Affiliation

¹ Environmental Medicine, Graduate School of Medicine, Nippon Medical School, Bunkyo-ku, Tokyo, Japan.

PMID: 15747133
DOI: 10.1007/s00775-005-0629-5

Abstract

Human porphobilinogen synthase [EC.4.2.1.24] is a homo-octamer enzyme. In the active center of each subunit, four cysteines are titrated with 5,5'-dithiobis(2-nitrobenzoic acid). Cys(122), Cys(124) and Cys(132) are placed near two catalytic sites, Lys(199) and Lys(252), and coordinate a zinc ion, referred to as "a proximal zinc ion", and Cys(223) is placed at the orifice of the catalytic cavity and coordinates a zinc ion, referred to as "a distal zinc ion", with His(131) . When the wild-type enzymes C122A (Cys(122)-->Ala), C124A (Cys(124)-->Ala), C132A (Cys(132)-->Ala) and C223A (Cys(223)-->Ala) were oxidized by hydrogen peroxide, the levels of activity were decreased. Two cysteines were titrated with 5,5'-dithiobis(2-nitrobenzoic acid) in the wild-type enzyme, while on the other hand, one cysteine was titrated in the mutant enzymes. When wild-type and mutant enzymes were reduced by 2-mercaptoethanol, the levels of activity were increased: four and three cysteines were titrated, respectively, suggesting that a disulfide bond was formed among Cys(122), Cys(124) and Cys(132) under oxidizing conditions. We analyzed the enzyme-bound zinc ion of these enzymes using inductively coupled plasma mass spectrometry with gel-filtration chromatography. The results for C223A showed that the number of proximal zinc ions correlated to the level of enzymatic activity. Furthermore, zinc-ion-free 2-mercaptoethanol increased the activity of the wild-type enzyme without a change in the total number of zinc ions, but C223A was not activated. These findings suggest that a distal zinc ion moved to the proximal binding site when a disulfide bond among Cys(122), Cys(124) and Cys(132) was reduced by reductants. Thus, in the catalytic functioning of the enzyme, the distal zinc ion does not directly contribute but serves rather as a reserve as the next proximal one that catalyzes the enzyme reaction. A redox change of the three cysteines in the active center accommodates the catch and release of the reserve distal zinc ion placed at the orifice of the catalytic cavity.

MeSH terms

Binding Sites
Cysteine / chemistry*
Enzyme Activation
Gene Expression
Humans
Kinetics
Mercaptoethanol / metabolism*
Mutagenesis, Site-Directed
Mutation
Porphobilinogen Synthase / chemistry*
Porphobilinogen Synthase / genetics
Porphobilinogen Synthase / metabolism*
Protein Binding
Zinc / chemistry*

Substances

Mercaptoethanol
Porphobilinogen Synthase
Zinc
Cysteine