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Cysteines β93 and β112 as Probes of Conformational and Functional Events at the Human Hemoglobin Subunit Interfaces
Three variants of tetrameric human hemoglobin, with changes at the α 1 β 2/ α 2 β 1-interface, at the α 1 β 1/ α 2 β 2-interface, and at both interfaces, have been constructed. At α 1 β 2/ α 2 β 1-interface the β93 cysteine was replaced by alanine ( βC93A), and at the α 1 β 1/ α 2 β 2-interface the...
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| Published in: | Biophysical journal 1999, Vol.76 (1), p.88-97 |
|---|---|
| Main Authors: | , , , , , , |
| Format: | Article |
| Language: | English |
| Citations: | Items that this one cites Items that cite this one |
| Online Access: | Get full text |
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| Summary: | Three variants of tetrameric human hemoglobin, with changes at the
α
1
β
2/
α
2
β
1-interface, at the
α
1
β
1/
α
2
β
2-interface, and at both interfaces, have been constructed. At
α
1
β
2/
α
2
β
1-interface the
β93 cysteine was replaced by alanine (
βC93A), and at the
α
1
β
1/
α
2
β
2-interface the
β112 cysteine was replaced by glycine (
βC112G). The
α
1
β
2 interface variant,
βC93A, and the
α
1
β
1/
α
1
β
2 double mutant,
β(C93A+C112G), were crystallized in the T-state, and the structures determined at 2.0 and 1.8
Å resolution, respectively. A comparison of the structures with that of natural hemoglobin A shows the absence of detectable changes in the tertiary folding of the protein or in the T-state quaternary assembly. At the
β112 site, the void left by the removal of the cysteine side chain is filled by a water molecule, and the functional characteristics of
βC112G are essentially those of human hemoglobin A. At the
β93 site, water molecules do not replace the cysteine side chain, and the alanine substitution increases the conformational freedom of
β146His, weakening the important interaction of this residue with
β94Asp. As a result, when Cl
− is present in the solution, at a concentration 100
mM, the Bohr effect of the two mutants carrying the
β93Cys→Ala substitution,
βC93A and
β(C93A+C112G), is significantly modified being practically absent below pH 7.4. Based on the crystallographic data, we attribute these effects to the competition between
β94Asp and Cl
− in the salt link with
β146His in T-state hemoglobin. These results point to an interplay between the
βHis146-
βAsp94 salt bridge and the Cl
− in solution regulated by the Cys present at position
β93, indicating yet another role of
β93 Cys in the regulation of hemoglobin function. |
|---|---|
| ISSN: | 0006-3495 1542-0086 |
| DOI: | 10.1016/S0006-3495(99)77180-8 |