ABSTRACT
The double Mn2+ complex of concanavalin A with bound saccharide (SMMPL) was examined by electron paramagnetic resonance (EPR) spectroscopy and magnetic susceptibility measurements. A room temperature X-band (9 GHz) EPR spectrum of SMMPL revealed a relatively weak, broad resonance in contrast to the spectrum with a six-line hyperfine-split pattern observed for the mononuclear, high-spin Mn2+ complex found in Ca2+-Mn2+-concanavalin A with saccharide present (SCMPL). The EPR spectrum of SMMPL at 77 K, however, consisted of a series of overlapping patterns of 11 hyperfine-split lines near g = 2.0 with members of each pattern separated by 47 G, half the value of the hyperfine splitting of SCMPL. These 11-line patterns are preserved at Q-band (35 GHz), indicating that the manganese ions in SMMPL form a spin-coupled, binuclear center. As expected for an exchange-coupled system, the EPR signal of SMMPL at 77 K saturates at a higher microwave power than those for SCMPL or Mn2+ aquoion. There is also a marked loss of EPR signal intensity for SMMPL between 4.2 and 1.4 K, which supports the view that the pair of manganese ions is exchanged-coupled. The temperature dependence of both the magnetic susceptibility and the low-temperature EPR spectral intensity can be explained by a model in which the two high-spin Mn2+ ions of SMMPL are antierromagnetically exchanged-coupled with an isotropic coupling constant J = 1.8 cm-1 (for the spin Hamiltonian Hex = JS1.S2). Zero-field splitting D' was estimated to be 375 G from the EPR spectrum.(ABSTRACT TRUNCATED AT 250 WORDS)
Subject(s)
Concanavalin A , Manganese , Metalloproteins , Electron Spin Resonance Spectroscopy , Kinetics , Magnetics , Protein Binding , Protein Conformation , ThermodynamicsABSTRACT
Low temperature (T less than or equal to 20 K) EPR measurements have revealed the presence of a heretofore undetected signal in uteroferrin, a purple protein bearing a single iron atom per molecule. All three of its principal g values (1.923, 1.738, and 1.583) lie well below the free electron value of 2.0023. Magnetic susceptibility data from 2-77 K confirm that the novel EPR spectrum arises from a paramagnetic center with a single unpaired electron spin. Quantitative correlation of the EPR, susceptibility, and optical data point to chromophoric iron as the source of the rhombic EPR spectrum. Furthermore, close agreement between the concentration of iron and the integrated intensity of the rhombic EPR signal show that the iron in the paramagnetic center is mononuclear. Reduction of the protein to its pink form leaves the rhombic signal essentially unaltered. The previously reported g' = 4.3 EPR signal accounts for only a small fraction of the total iron in the protein and undoubtedly arises from adventitious iron. Collectively, these results strongly suggest that uteroferrin represents a new class of low spin iron proteins.
Subject(s)
Glycoproteins/analysis , Metalloproteins/analysis , Acid Phosphatase , Animals , Electron Spin Resonance Spectroscopy , Iron/analysis , Isoenzymes , Protein Binding , Swine , Tartrate-Resistant Acid PhosphataseABSTRACT
Magnetic and spectroscopic properties of mu-oxo-bis-hemins from natural and structurally related porphyrins were investigated as probes for ascertaining the presence or absence of FeIII-O-FeIII linkages between hemin moieties of hemeproteins. Magnetic susceptibilities of solids from 2.2 to 293 degrees K were investigated. The data fit the temperature variations expected for a pair of antiferromagnetically coupled S = 5/2, iron (III) porphyrins with J values of 175, 190, 195, 205, and 210 degrees K for deuterohemins with hydrogen, vinyl, 2'-ethoxycarbonylcyclopropyl, acetyl, propionyl, and ethyl 2,4-substituents, respectively. This magnetic character is reflected in PMR spectra that exhibit resonances with far less broadening and paramagnetic shift than is the case for monomeric high-spin hemins. Only impurities are seen in EPR spectra, which serve effectively in monitoring the magnetic purity of preparations. An infrared active asymmetric stretching frequency characteristic of the FeOFe linkage can be identified by substitution of 160 by 180. Electronic spectra are highly characteristic with poorly resolved absorption bands. The substituents on the porphyrin ring exert significant, but usually not large, electronic and steric effects on these properties. Solvent effects were relatively small and no firm evidence for binding of ligands trans to bridging oxygen was found. The uniqueness of these physical properties and their low sensitivity to changes in porphyrin structure or medium facilitates the identification of mu-oxo linkage in hemins or oxidized hemeproteins.
