Mössbauer studies of ferrihemequinidine complexes

The system ferriprotoporphyrin IX-(+)-quinidine (FPQd) was investigated by Mössbauer spectroscopy at both 4.1 and 90 K. FPQd complexes were prepared by interaction of 10⁻² to 10⁻³ M aqueous solutions of the components at pH 11–12 and 26 °C. Previous investigations of analogous complexes showed characteristic and unusually large circular dichroism bands near 400 nm at alkaline pH values. The present Mössbauer data obtained for FP either in the presence or absence of Qd at both pH 11–12 and 9 indicate identical isomeric shifts in all cases. Both free and complexed FP iron is in a high-spin state. The temperature dependence of the FPQd complex indicates slow spin-spin relaxation at 90 K and fast relaxation at 4.1 K. Qd appears to increase the iron-iron distance of FP in the complexes with references to FP alone, in agreement with previous suggestions on the structure of the complex.     

Heme iron state in various oxyhemoglobins probed using Mössbauer spectroscopy with a high velocity resolution

A comparative study of oxyhemoglobins from pig, rabbit, normal human and patients with blood system malignant diseases was performed using Mössbauer spectroscopy with a high velocity resolution at 90 K. Mössbauer spectra were fitted with the help of two models: using one quadrupole doublet (model of equivalent iron electronic structure in α- and β-subunits of hemoglobins) and superposition of two quadrupole doublets (model of non-equivalent iron electronic structure in α- and β-subunits of hemoglobins). The results obtained using both models demonstrated small variations of hyperfine parameters that were related to the heme iron state variation in different hemoglobins. These results were compared with structural and functional differences of the hemoglobins investigated.     

Towards an understanding of the quadrupole splittings found in the Mössbauer spectroscopic data of a number of substituted tetraphenylporphyriniron(III) halides

Mononuclear and μ-oxo-dimers of a series of unsymmetrical substituted tetraphenylporphyriniron(III) complexes have been prepared and studied using Mössbauer spectroscopy. The Mössbauer data are discussed and compared to the other known data for similar high spin Fe(III) porphyrinsA good correlation between Hammet σ_R° (the mesomeric values) of the porphyrin substituent and the Mössbauer quadrupole splitting (Δ) has been found.     

Freeze-quench 57Fe-Mössbauer spectroscopy: trapping reactive intermediates

⁵⁷Fe-Mössbauer spectroscopy is a method that probes transitions between the nuclear ground state (I = 1/2) and the first nuclear excited state (I = 3/2). This technique provides detailed information about the chemical environment and electronic structure of iron. Therefore, it has played an important role in studies of the numerous iron-containing proteins and enzymes. In conjunction with the freeze-quench method, ⁵⁷Fe-Mössbauer spectroscopy allows for monitoring changes of the iron site(s) during a biochemical reaction. This approach is particularly powerful for detection and characterization of reactive intermediates. Comparison of experimentally determined Mössbauer parameters to those predicted by density functional theory for hypothetical model structures can then provide detailed insight into the structures of reactive intermediates. We have recently used this methodology to study the reactions of various mononuclear non-heme-iron enzymes by trapping and characterizing several Fe(IV)-oxo reaction intermediates. In this article, we summarize these findings and demonstrate the potential of the method.     

119Sn Mössbauer spectroscopic studies of the products of the reaction of triorganotin(IV) derivatives with 6-thiopurine

A structural study of the products of the reaction of R₃Sn^IV derivatives (R = Me, Buⁿ, Ph) with 6-thiopurine, 6-TPH₂, and its sodium salt, 6-TPHNa, has been undertaken using Mössbauer spectroscopy and the point-charge model rationalization of the Mössbauer parameter nuclear quadrupole splitting. The synthetic reactions have been carried out at ca. 0 °C, 20 °C and 50 °C. The Mössbauer spectra of the complexes AlK₃Sn(6-TPH) are consistent with the occurrence of two distinct tin(IV) sites in samples prepared at the lower temperature, while one only site appears by increasing the temperature of the reaction. Two tin sites constantly occur in the products of the reactions involving the Ph₃Sn^IV moiety; the stoichiometry is assumed to be (Ph₃Sn)₃(6-TPH)(6-TP) for the uniquely-formed complex. Solid state polymeric structures with trigonal bipyramidal environments of the tin atoms and planar SnC₃ skeletons have been proposed. The apical ligand atoms have been assumed to be N, S and N, N in the samples showing two individual tin(IV) sites, and N, N when a single site was present.     

Study of storage iron in cultured chick embryo fibroblasts and rat glioma cells,using Mössbauer spectroscopy

⁵⁷Fe Mössbauer spectra of normal and Rous sarcoma virus-infected cultured chick embryo fibroblasts and rat glioma cells have been measured between 0.08 and 318 K. Ferritin-like iron and bacterio-ferritin-like iron have been found in these cells, in various relative amounts, indicating a close relationship between the two storage materials. The bacterio-ferritin-like iron was found to be predominantly membrane-bound. Above 260 K very wide lines were observed in the Mössbauer spectra, yielding an effective viscosity of about 1 poise in the normal chick embryo fibroblasts and about 0.5 poise in the virus-infected chick embryo fibroblasts.     

Comparative Mössbauer and infrared analysis of iron-containing melanins

A Mössbauer study was carried out on some types of melanin. ⁵⁷Fe³⁺ was bound to melanin from sepia ink and to that obtained by autooxidation of l-DOPA and dopamine. Mössbauer spectra, performed in parallel with infrared measurements, indicated that paracrystalline subunits are present, showing a superparamagnetic behaviour. The preferential binding sites for iron are different in melanins having l-DOPA as precursor from those obtained starting from dopamine. In particular, the linkage to carboxylic groups in predominant in the former, and linkage to phenolic, aminic and/or indolic groups can be observed in the latter. The results also confirm the close similarity between natural sepia melanin and that obtained from an l-DOPA precursor.     

Solution studies on tetra(p-carboxyphenyl)porphyrin iron(II) using Mössbauer spectroscopy and electronic absorption spectroscopies

Mössbauer (78 K) and electronic absorption spectra (298 K) of tetra(p-carboxyphenyl)porphyrin iron(II) solutions are reported and discussed. Evidence for only two iron(II) complexes, the first an intermediate spin and the second a high spin complex, is found in the Mössbauer spectra. Electronic absorption spectra show a low spin complex is present at very low concentrations. It is observed from these results that the carboxy groups on the phenyl rings of this porphyrin greatly influence the chemistry. From the difference in the quadrupole splitting for the intermediate spin complex compared to that found in the tetra(p-sulphophenyl)porphyrin iron(II) system, the substituent on the phenyl ring clearly changes the electron density on the pyrrole nitrogen atoms.     

Investigation of iron pools in cucumber roots by Mössbauer spectroscopy: direct evidence for the Strategy I iron uptake mechanism

Distinct chemical species of iron were investigated by Mössbauer spectroscopy during iron uptake into cucumber roots grown in unbuffered nutrient solution with or without ⁵⁷Fe-citrate. Mössbauer spectra of iron deficient roots supplied with 10–500 μM ⁵⁷Fe-citrate for 30–180 min and 24 h and iron-sufficient ones, were recorded. The roots were analysed for Fe concentration and Fe reductase activity. The Mössbauer parameters in the case of iron-sufficient roots revealed high-spin iron(III) components suggesting the presence of Fe^III-carboxylate complexes, hydrous ferric oxides and sulfate–hydroxide containing species. No Fe^II was detected in these roots. However, iron-deficient roots supplied with 0.5 mM ⁵⁷Fe^III-citrate for 30 min contained significant amount of Fe^II in a hexaaqua complex form. This is a direct evidence for the Strategy I iron uptake mechanism. Correlation was found between the decrease in Fe reductase activity and the ratio of Fe^II–Fe^III components as the time of iron supply was increased. The data may refer to a higher iron reduction rate as compared to its uptake/reoxidation in the cytoplasm in accordance with the increased reduction rate in iron deficient Strategy I plants.     

125Te Mössbauer spectra of the intercalation compound (Te2)2(I2)

The quadrupole split asymmetric ¹²⁵Te Mössbauer spectrum recorded from the compound (Te₂)₂(I₂), in which monomolecular planar layers of iodine molecules are intercalated between layers of tellurium, is a reflection of the distorted environment of tellurium atoms in a two-dimensional layered compound in which the elongated flat crystals are preferentially orientated. The differences between the Mössbauer parameters recorded from (Te₂)₂(I₂) and those recorded from elemental tellurium and the tellurium(0) species in the compound Te₃Cl₂ are associated with small differences between the environments of tellurium in the three compounds. The Mössbauer spectra recorded from (Te₂)₂(I₂) are consistent with a recently proposed model on which the electronic band structure of (Te₂)₂(I₂) has been derived.     

Protein dynamics of a β-sheet protein

Rhodnius prolixus Nitrophorin 4 (abbreviated NP4) is an almost pure β-sheet heme protein. Its dynamics is investigated by X-ray structure determination at eight different temperatures from 122 to 304 K and by means of Mössbauer spectroscopy. A comparison of this β-sheet protein with the pure α-helical protein myoglobin (abbreviated Mbmet) is performed. The mean square displacement derived from the Mössbauer spectra increases linearly with temperature below a characteristic temperature T _c. It is about 10 K larger than that of myoglobin. Above T _c the mean square displacements increase dramatically. The Mössbauer spectra are analyzed by a two state model. The increased mean square displacements are caused by very slow motions occurring on a time scale faster than 140 ns. With respect to these motions NP4 shows the same protein specific modes as Mbmet. There is, however, a difference in the fast vibration regime. The B values found in the X-ray structures vary linearly over the entire temperature range. The mean square displacements in NP4 increase with slopes which are 60% larger than those observed for Mbmet. This indicates that nitrophorin has a larger structural distribution which makes it more flexible than myoglobin.     

Studies of the reactions of iron(II) ascorbate mixtures with molecular oxygen in solution

Mössbauer and electronic absorbance spectroscopic studies on the reactions of iron(II): ascorbic acid with molecular oxygen in aqueous and methanolic solutions are reported. Both spectroscopic techniques show that in the starting mixtures there are no iron(II): ascorbate complexes. On mixing the iron(II)/ascorbate solution with solutions containing molecular oxygen at pH 6–7 high spin iron(III) is observed in the Mössbauer spectrum. Coloured intermediates, the lifetimes of which are solvent dependent, are seen by stopped-flow spectrophotometry. We assign these coloured intermediates as iron(III) ascorbate complexes. The stoichiometry of the initial reaction between iron(II) and oxygen is shown to be 2Fe(II):O₂ by stopped-flow methods. A scheme for the overall reactions is discussed.     

Iron coordination geometry in full-length, truncated, and dehydrated forms of human tyrosine hydroxylase studied by Mössbauer and X-ray absorption spectroscopy

Full-length human tyrosine hydroxylase 1 (hTH1) and a truncated enzyme lacking the 150 N-terminal amino acids were expressed in Escherichia coli and purified either with or without (6×histidine) N-terminal tags. After reconstitution with ⁵⁷Fe(II), the Mössbauer and X-ray absorption spectra of the enzymes were compared before and after dehydration by lyophilization. Before dehydration, >90% of the iron in hTH1 had Mössbauer parameters typical for high-spin Fe(II) in a six-coordinate environment [isomer shift δ(1.8–77?K)=1.26–1.24?mm s^–1 and quadrupole splitting ΔE _Q=2.68?mm s^–1]. After dehydration, the Mössbauer spectrum changed and 63% of the area could be attributed to five-coordinate high-spin Fe(II) (δ=1.07?mm s^–1 and ΔE _Q=2.89?mm s^–1 at 77?K), whereas 28% of the iron remained as six-coordinate high-spin Fe(II) (δ=1.24?mm s^–1 and ΔE _Q=2.87?mm s^–1 at 77?K). Similar changes upon dehydration were observed for truncated TH either with or without the histidine tag. After rehydration of hTH1 the spectroscopic changes were completely reversed. The X-ray absorption spectra of hTH1 in solution and in lyophilized form, and for the truncated protein in solution, corroborate the findings derived from the Mössbauer spectra. The pre-edge peak intensity of the protein in solution indicates six-coordination of the iron, while that of the dehydrated protein is typical for a five-coordinate iron center. Thus, the active-site iron can exist in different coordination states, which can be interconverted depending on the hydration state of the protein, indicating the presence or absence of a water molecule as a coordinating ligand to the iron. The present study explains the difference in iron coordination determined by X-ray crystallography, which has shown a five-coordinate iron center in rat TH, and by our recent spectroscopic study of human TH in solution, which showed a six-coordinated iron center.     

Mössbauer spectroscopy of iron metabolism and iron intracellular distribution in liver of rats

Mössbauer spectroscopy was used to investigate the distribution of iron in rat organs and its localisation in liver subcellular fractions. A ⁵⁷Fe-sucrose complex solution was injected by 0.5 ml doses into tail veins of anmals every day, during a 6-day period. Mössbauer spectra were measured in spleen, blood, liver and liver subcellular fractions. The Mössbauer spectrum of a spleen sample has two symmetrical doublets, one with δ=0.6 mm/s and Δ=0.7 mm/s, and the other with δ=1.0 mm/s and Δ=2.35 mm/s. The Mössbauer spectrum of blood has parameters which are close to those for carboxyhemoglobin and oxyhemoglobin complexes. After the addition of sodium citrate, the proportion of the carboxyhemoglobin complexes increases. The Mössbauer spectrum of liver has a two-component pattern with two symmetrical doublets, the first with δ=0.6 mm/s and Δ=0.63 mm/s and the second with δ=1.4 mm/s and Δ=3.45 mm/s. The first component, which was identified as ferritin, is present in all subcellular fractions (800 × g_av sediment fraction, mitochondrial/lysosomal, microsomal and supernatant fractions), with its content in microsomal fraction. After the addition of NaBH₄ to mitochondrial/lysosomal fraction, about 20 % of the iron contained in ferritin was reduced. In the Mössbauer spectrum this is reflected by an appearance of a doublet with δ=0.85 mm/s and Δ=3.7 mm/s.     

Dynamics of Hemoglobin Investigated by Mössbauer Spectroscopy

Abstract

Mössbauer Spectra of ⁵⁷Fe enriched horse hemoglobin and sperm whale myoglobin were measured in the temperature range from 80 K to 260 K. An analysis of the temperature dependence of the recoiless fraction (the Lamb-Mössbauer factor) shows it to be sensitive to conformational fluctuations which affect the mean square displacement of the iron. We have found that the protein conformation has a dramatic effect on these measurements. For hemoglobin greater conformational fluctuations at lower temperatures are observed for carbonmonoxyhemoglobin in the liganded conformation than for deoxyhemoglobin in the unliganded conformation. On the other hand, the Lamb-Mössbauer factor is insensitive to the binding of ligands to myoglobin and shows conformational fluctuations similar to deoxyhemoglobin even in the liganded state. It is also shown that a reversible complex with the distal histidine is formed in frozen deoxyhemoglobin solutions above 200 K where the Lamb-Mössbauer factor shows the excitation of new modes of conformational fluctuations. This complex is not formed with carbonmonoxyhemoglobin which already has a sixth ligand and with deoxymyoglobin which appears to undergo much more limited conformational fluctuations. A possible relationship between the formation of the distal histidine complex and the cooperative ligand binding reaction is suggested by results with partially liganded hemoglobin which indicate increased formation of the distal histidine complex.     

4-Piperidinylpyridinium tetrachloroferrate(III): structure and low-temperature magnetic ordering

4-Piperidinylpyridine and FeCl₃ in CH₃CN/conc. HCl yield the title compound, whose crystal structure shows almost tetrahedral [FeCl₄]⁻ anions, and cations exhibiting the pyridinium tautomer. The temperature dependence of the Mössbauer spectra and AC susceptibility confirm a Néel temperature of approximately 2.5 K and an uncanted three-dimensional antiferromagnetic ground state.     

Mössbauer spectroscopic studies of hemoglobin and its isolated subunits.

Samples of 90% enriched 57Fe hemoglobin and its isolated subunits have been prepared. M?ssbauer spectroscopic measurements have been made on three such samples. Sample one contained contributions of oxyhemoglobin, deoxyhemoglobin, and carbonmonoxyhemoglobin. This sample was studied from a temperature of 90 K down to 230 mK. Measurements were also made at 4.2 K using a small applied magnetic field of 1.0 T. In general, the measured quadrupole splittings and isomer shifts for each component agreed with previous measurements on single component samples in the literature, and thus demonstrated that chemically enriched hemoglobin has not been altered. The second and third samples were isolated alpha and beta subunits, respectively. We have found measurable M?ssbauer spectral differences between the HbO2 sites in the alpha subunit sample and the beta subunit sample. The measured M?ssbauer spectral areas indicate that the iron ion has the largest mean-square displacement at the deoxy Hb sites as compared to that at the oxy- and carbonmonoxy Hb sites. The mean-square displacement at the HbO2 sites is the smallest.     

Nature of iron deposits on the cardiac walls in β-thalassemia by Mössbauer spectroscopy

An identification of the nature and an estimation of the particle size distribution of the iron deposits on thalassemic heart tissue is carried out by variable temperature Mössbauer spectroscopy. Comparison of Mössbauer spectra obtained for the thalassemic heart tissue (I) with those of normal heart tissue (II) and of horse spleen ferritin (III) identifies the iron deposits to be small, superparamagnetic particles of ferritin and/or hemosiderin, two closely related iron storage proteins containing an iron core of (FeOOH)₈(FeO · OPO₃H₂). The dependence of the superparamagnetic relaxation time, τ₂, of magnetically ordered fine particles on their volume V via the magnetic anisotropy constant K of the material and the condition τ > τ_L, the Larmor precession time of the nuclear magnetic moment of ⁵⁷Fe about an effective magnetic field, for observation of hyperfine structure are used in analyzing the Mössbauer data to yield the particle size distribution. Particle diameters are estimated to be $\text{74 ± 12}\text{A}\text{?}$.