Resonance Raman studies of the peroxotitanate(IV) complexes K2(Ti(O2)(SO4)2)·5H2O and K2(Ti(O2)(C2O4)2)·3H2O

The resonance Raman spectra of K₂(Ti(O₂)(SO₄)₂)·5H₂O and K₂(Ti(O₂)(C₂O₄)₂)·3H₂O are recorded. The results are consistent with the triangular structure of the peroxotitanium unit, Ti(O₂), with C_2ν symmetry. The ν(OO), ν_s(TiO) and ν_as(TiO) are observed around 890, 610 and 535 cm⁻¹, respectively. The resonance effects are shown to be associated with the 425 nm absorption band. This band is assigned to the O₂²⁻ → Ti(IV) charge-transfer transition. The calculated force constant values for the O₂²⁻ and TiO bonds are 320 and 275 N m⁻¹, respectively.     

The Effect of Cyclopropane on Ion Uptake and Protoplasmic Streaming in Barley Roots

Increasing concentrations of cyclopropane up to about 95 % C₃H₆—5 % O₂ caused an increasing inhibition of uptake by excised barley roots from KC1 solution, much more so for Cl than K. No inhibition of K uptake from K₂SO₄ occurred under similar conditions. It is suggested that the small decrease in K uptake from KC1 is related to the large decrease in Cl uptake and that C₃H₆ primarily inhibits Cl uptake with little or no effect on K uptake. Time curves of uptake in 80 % C₃H₆ 20 % O₂ revealed no indication of cumulative injury in either KC1 or K₂SO₄ for periods up to 3 hours. The amount of organic acid production associated with K uptake from K₂SO₄ was about the same in 80 % C₃H_g— 20 % O₂ as in air. Oxygen consumption in K₂SO₄ was unaffected by the gas mixture and only slightly affected in KC1. Protoplasmic streaming in epidermal cells was rapidly stopped at C₃H₆ concentrations of 20 % or higher. In 80 % C₃H₆–20 % O₂ the effect on streaming was confined mostly to the outer two or three layers of root cells. A connection between the cessation of streaming and the inhibition of Cl uptake appeared to exist but very little if any relationship between streaming and K uptake was observed.     

Total nitrogen determining for plant material containing nitrate

A nonfoaming method for semimicro Kieldahl determination of total nitrogen in plant samples containing appreciable amounts of nitrate was developed for use with a digestion block utilizing test tubes for digestion flasks. The sample (30 to 200 mg) is treated with 5 ml of a sulfuric acid:salicylie acid (30:1 $\text{v}\text{w}$) mixture at room temperature for 1 hr. Catalyst [K₂SO₄:CuSeO₃·2H₂O:pumice 970:19:11 w/w/w)] is added and the mixture is digested at 360 to 380°C for 1 hr after the mixture clears. Ammonium in the digest is determined by a suitable method. This semimicro Kjeldahl procedure results in a 95% or better recovery of nitrate, either from KNO₃ or from KNO₃ added to plant material.     

Structural and vibrational characteristics of the tetrasulfatodimolybdenum ions with MoMo bond orders of 3.5 and 4.0

The compound K₄[Mo₂(SO₄)₄]Br·4H₂O has been made and its crystal structure determined. Space group P4/mnc; unit cell dimensions, a = 11.903(2), c = 8.021(1) Å, V = 1136(1) ų. The compound is isomorphous with the analogous chloride whose structure has been reported. The MoMo and MoBr distances are 2.169(2) and 2.926(1) Å, respectively and the [Mo₂(SO₄)₄] ³⁻ ions reside on crystallographic special positions with 4/m symmetry. The Raman spectra of both the bromo and chloro compounds have been measured and the MoMo stretching frequency is 370 ± 1.5 cm⁻¹ in each, for the compounds containing the natural isotopic distribution of molybdenum. The chloro compound has been prepared containing the pure isotope ⁹²Mo as well, and the Raman spectra recorded. The v(MoMo) band is shifted by 6.8 ± 0.5 cm⁻¹. The compound K₄[Mo₂(SO₄)₄]·2H₂O has also been prepared with Mo at natural abundance and with the pure isotope ¹⁰⁰Mo, whereby a shift of 8.5 ± 0.5 cm⁻¹ was found. These and other results will be discussed with regard to the similarity of the Raman spectra of the Mo₂(S0₄)₄³⁻ and M0₂(S0₄)₄⁴⁻ species.     

Evaluation of methods for total selenium determination in yeast

The selenium determination in biological materials by the classical fluorometric method (FM) is time-consuming and also hazardous, as it requires the destruction of the organic matrix samples with hot HNO₃/HClO₄ mixtures prior to analysis. Accordingly, commercial analytical laboratories are increasingly using faster instrumental methods; for sample digestion, avoid using HClO₄. Because of these procedural changes, the results obtained by commercial laboratories may be unreliable, especially for samples containing Se in organic forms. One such “difficult” substrate is Se yeast, which contains most of its Se as selenomethionine. To establish which methods for Se analysis and sample digestion are applicable, samples of Se yeast and of selenomethionine standards were sent to laboratories employing either flame atomic absorption spectrometry (FAAS), inductively coupled plasma-mass spectrometry (ICP-MS), or hydride generation atomic absorption spectrometry (HGAAS). The result were compared with those obtained by FM and non-destructive instrumental neutron activation analysis (INAA). ICP-MS, after microwave digestion of sample with HNO₃/H₂O₂, produced results within 5% of the expected values, as did those obtained by FM and INAA. With FAAS, acceptable results were obtained after digestion with HNO₃/HCl. With HGAAS, sample digestion with HNO₃/H₂O₂ produced values that were systematically elevated by about 10% and exhibited standard deviations of ≥10%. Thus, current methods of sample digestion are applicable for Se yeast analysis by ICP-MS and FAAS, but not by HGAAS.     

Treatment of cotton seeds for germination

Summary Effects of H₂SO₄, H₂O₂, C₂H₅OH and of acetone on germination of cotton seeds and on the growth of seedling root were studied under laboratory conditions. H₂SO₄ or H₂O₂ hastened germination but decreased the ultimate number of seeds germinated. Higher temperature (27°C) hastened germination and increased the number of seeds germinated. Root length remained unaffected by treatments at room temperature while H₂SO₄ or H₂SO₄/H₂O₂ substantially decreased it at 27°C.     

Synthesis and spectroscopic properties of Co(salen) derivatives containing pendant thioether groups and their dioxygen adducts

Two Co(salen) derivatives, Co(sal-ipsen) and Co(sal-bsen), containing pendant (CH₂)₂S(i-C₃H₇) and (CH₂)₂SC₆H₅ groups were synthesized. Electronic and ESR spectra in methylene chloride show that the former is five-coordinate with pendant thioether coordination at 198 K or below whereas the latter is four-coordinate at 198 K and becomes a mixture of the four- and five-coordinate species at liquid nitrogen temperature. Upon oxygenation at low temperatures, both complexes form dioxygen adducts in which the pendant thioether groups are coordinated to the trans position to dioxygen. Resonance Raman spectra show that Co(sal-ipsen) yields an equilibrium mixture of the 1:1 and 1:2(O₂/ Co) adducts at 190 K while Co(sal-bsen) forms only the 1:1 adduct under similar conditions. These differences between Co(sal-ipsen) and Co(sal-bsen) can be attributed to the variance in basicity of their pendant sulfur atoms.     

The structure and properties of tetrakis(tironato)cerate(IV), Na12[Ce(C6H2O2(SO3)2)4]·9H2O·6C3H7NO

The title complex, prepared in 1 M NaOH, was crystallized from hot N,N-dimethylformamide/ ethanol solutions to give Na₁₂[Ce(C₆H₂O₂(SO₃)₂)₄]· 9H₂O·6DMF. The purple—brown crystals were examined by X-ray diffraction while inside quartz capillaries filled with DMF, (λ_max 425 nm, ϵ 3664; λ_sh 520 nm, ϵ 2240) and belong to space group Pbca, Z=8 with a=21.846(4), b=17.348(2), c=43.103- (6) Å, V=16.335(7) ų, D_c=1.693 gcm^t−3, D_o=1.725 g cm^t−3. Diffractometer data were collected using Mo Kα radiation to 2θ=43^o. For 7331 independent data with F_o²>3σ(F_o²) full matrix least squares refinement converged to unweighted and weighted R factors of 0.072 and 0.110, respectively, with a mixture of anisotropic and isotropic thermal parameters. The disordered DMF atom parameters were not refined. The structure consists of discrete monomeric Ce(C₆H₂S₂O₈)₄¹²⁻ units with 12 Na⁺ counter cations and 10 H₂O molecules (two with half occupancy), and 6 DMF molecules of solvation filling up spaces between cations and anions. Cerium(IV) is in a general position with a coordination polyhedron close to the trigonal-faced dodecahedron, D_2d, with the angles between the two BAAB trapezoids of 2.3^o and 3.7^o. The average CeO(A) distance, 2.363(9) Å is longer than the average CeO(B) distance, 2.326(15)Å, with the reverse being true for one of the four tironato ligands. The average ring OCeO angle is 67.9(1)^o. The cerium (IV) complex is found by cyclic voltammetry to undergo a quasi-reversible one-electron reduction (in strongly basic solution with excess tiron) with Ef=−497 mV vs. SCE, hence the ratio of the formation constants for tetrakis(tironato)cerate(IV) to that for tetrakis(tironato)cerate(III), K_IV/K_III, is 10³³. Characterization of other tiron salts is reported.     

Comparison of two methods for the isolation of phytolith occluded carbon from plant material

Background and aims

Phytolith occluded carbon (PhytOC) is of interest for isotope studies, dating of sediments and the capture and storage of carbon. Many methodologies have been used for the isolation of phytoliths from plant material; however, there are wide disparities in the PhytOC contents when determined by different methodologies. In this study we examine the utility of the two main methods used for quantifying PhytOC.

Methods

These methods are: (1) a microwave digestion followed by a Walkley-Black digestion, and (2) H₂SO₄/H₂O₂.

Results

Method (1) produced PhytOC values over 50 times higher than those acquired by method (2). SEM examination indicated that the differences were likely due to shattering of the phytoliths by method (2) allowing consumption by the acid and peroxide of PhytOC .

Conclusion

These results indicate that for the samples analysed here: 1] the modified microwave method allowed the total PhytOC to be measured, 2] the H₂SO₄/H₂O₂ method allowed the PhytOC within the tightly packed silica matrix to be measured, and 3] the PhytOC retained within the phytolith cavities could possibly be calculated by subtracting 2] from 1]. For the samples analysed here most of the PhytOC resided in the phytolith cavities.     

Reactions of VCl3, VCl4 and TiX4 (XCl,Br) with benzofuroxan and its 5-methyl-, 5-chloro- and 5-methoxi-derivatives. I.

By means of the reaction between VCl₃ and benzofuroxan the compound VCl₃·2C₆H₄N₂O₂ was obtained, while in reaction with TiX₄ (XCl, Br) the compounds with stoichiometry TiX₄·C₆H₄N₂O₂ (X Cl, Br) were obtained.Furthermore, with some benzofuroxan derivatives (5-methyl, 5-chloro and 5-methoxi) the complexes MCl₄·2YC₆H₃N₂O₂ (MTi, V; YCH₃O, Cl, CH₃), TiCl₄·YC₆H₃N₂O₂ (YCH₃O, CH₃) and TiBr₄·YC₆H₃N₂O₂ (YCH₃O, Cl, CH₃) have been isolated.The compounds were characterized by elementary analysis, cryoscopic molecular weight determination in nitrobenzene, magnetic measurements and IR, Vis and EPR spectroscopy.     

The New Basic Triple Salt Containing Magnesium Hydroxide

The quaternary system K₂SO₄–MgSO₄–Mg(OH)₂–H₂O and the associated systems (a) K₂SO₄–Mg(OH)₂–H₂O and (b) MgSO₄–Mg(OH)₂–H₂O were investigated at 100° Though isotherm (a) exhibited nothing new, isotherm (b) exhibited basic magnesium sulfate, MgSO₄ · 5Mg(OH)₂·3H₂O, as the solid phase. The solid phases of quaternary isotherm were the new basic triple salt K₂SO₄ · 2MgSO₄ · Mg(OH)₂ · 2H₂O, langbeinite, basic magnesium sulfate, kieserite and potassium sulfate.     

Effects of Some Environmental Factors on Growth Characteristics of Candida utilis on Peat Hydrolysates

Samples of peat from Pine Island and Brookston bogs in Minnesota were hydrolyzed with various concentrations of HCl or H₂SO₄ solutions, before or after debituminization (an extraction process used to remove waxy materials, bitumens, from peat), to produce peak hydrolysates as growth substrates for Candida utilis. Hydrolysates were neutralized with concentrated NaOH solution to pH 3.5, 4.5, 5.0, 5.5, 6.0, and 7.0. The precipitated humates were removed by filtration. The resulting peat hydrolysates were amended with reagent-grade K₂HPO₄, K₂SO₄, and MgSO₄, 200, 100, and 50 mg per liter of peat hydrolysate, respectively. The debituminized peat produced more total nitrogen (TN) and reducing substances (RS) than the nondebituminized peat. Peat hydrolysates produced by HCl solutions contained slightly higher RS and TN than those produced by H₂SO₄ solutions; however, the latter were better growth substrates than the former. The yield coefficients in both H₂SO₄ and HCl hydrolysates initially decreased at 12 to 24 h and then increased gradually over the remaining incubation period (24 to 96 h). As TN and RS were increased, an increase in cell density, biomass, and productivity was observed. In contrast, a decrease in specific growth rate occurred as the RS and TN were increased. The generation time of C. utilis was affected by the concentrations of RS and TN. A peak substrate yield coefficient was found at pH 5.0 in HCl hydrolysates and at pH 6.0 to 6.5 in H₂SO₄ hydrolysates. Good linear correlation coefficients were found between RS and biomass of C. utilis. The coefficients of correlation increased as the TN level in hydrolysates was increased.     

Synthesis and spectroscopic studies of platinum(II) complexes of N,N′-dicyclohexylethylenediamine

The platinum(II) complexes of the formula [Pt(DCHEDA)X₂], where DCHEDA is N,N′-dicyclohexylethylenediamine and X⁻ is CL⁻, Br⁻, I⁻, 0.5C₂O₄²⁻ (oxalate), 0.5C₃H₂O₄²⁻ (malonate), 0.5C₉H₄O₆²⁻ (4-carboxyphthalate), 0.5S₂O₃²⁻ or 0.5SO₄²⁻, have been synthesized and characterized by UVVis, IR, and ¹H NMR spectral techniques. All the above complexes are non-electrolytes in DMF/H₂O, except the sulphate complex which becomes a 1:1 electrolyte after incubation for 24 h at 28 °C. The halide complexes were also studied by X-ray photoelectron spectroscopy and these data suggest that there is π-bonding from platinum to halide in these complexes. The oxalate, malonate and sulphate bind in their complexes as bidentate ligands to platinum through two oxygen atoms whereas the thiosulphate in its complex binds as a bidentate ligand to platinum through one oxygen atom and one sulphur atom.     

Purification and characterization of a glycolic acid (GA) oxidase active toward diglycolic acid (DGA) produced by DGA-utilizing Rhodococcus sp. No. 432

Diglycolic acid (DGA) oxidizing activity was found in crude extracts of Rhodococcus sp. no. 432 grown in DGA. Glycolic acid (GA) oxidase was purified approximately 80 times by treatment with streptomycin sulfate, precipitation with (NH₄)₂SO₄, chromatographies with DEAE-cellulose, DEAE-Toyopearl and Butyl-Toyopearl, and gel filtration on Toyopearl HW-55. The purified GA oxidase was almost homogeneous on sodium dodecyl sulfate (SDS) polyacrylamide gel electrophoresis. The purity was calculated to be more than 95%. The molecular weight of the enzyme, which appeared to consist of three identical units, was 158,000. Each subunit of GA oxidase included one molecule of FAD as a cofactor. The isoelectric point of the enzyme was around 5.3. GA oxidase was stable below 30°C and at the pH range of 6.0–8.5. The optimum pH and temperature were around 7.5 and 40°C, respectively. Oxygen, cytochrome c, ferricyanide and 2,6-dichlorophenol indophenol (DCIP) acted as an electron acceptor. The activity of GA oxidase was strongly inhibited by potassium cyanide, quinine, quinacrine, monoiodoacetate, 1,4-benzoquinone and some heavy metal ions. GA oxidase also had activity in DGA, GA, glyoxylic acid (GOA), methoxy acetate, ethoxy acetate and l-malate. Alcohols and other organic acids were not oxidized by the enzyme. The apparent K_m values for DGA, GA and GOA were about 26.7, 0.5 and 4.4 mM, respectively. The reaction products from DGA were supposed to be GOA and GA by the enzymatic assays. The reaction mechanism of GA oxidase in oxidation of DGA was supposed to be as follows: HOOCH₂COCH₂COOH+H₂O+acceptor→HOOCCHO+HOOCCH₂OH+ reduced acceptor.     

Thermodynamics and coordination characteristics of the hydronium-uranium(VI)-dicyclohexano-24-crown-8 extraction complex

The extraction equilibrium of the hydronium-uranium(VI)-dicyclohexano-24-crown-8 complex was carried out in the crown ether1,2-dichloroethaneHCl aqueous solution system at different temperatures. The extraction complex has the overall composition (L)₂·(H₃O⁺·χH₂O)₂·UO₂Cl₄²⁻ (L = dicyclohexano-24-crown-8). The values of the extraction equilibrium constants (K_ex) increase steadily with a decrease in temperature: 13.5 (298 K), 7.96 (301 K), 4.20 (303 K) and 2.07 (305 K). A plot of log K_ex against 1/T shows a straight line. The value of the enthalpy change, ΔH°, was calculated from the slope and equals −212 kJ mol⁻¹. The value of the entropy change, ΔS°, was calculated from ΔH° and K_ex and equals −690 J K⁻¹ mol⁻¹, whereas ΔG° = −6.45 kJ mol⁻¹. Comparing these thermodynamic parameters with those of the dicyclohexano-18-crown-6 isomer A [1] (ΔS° = −314 J K⁻¹ mol⁻¹, ΔH° = −101 kJ mol⁻¹ and ΔG° = −8.37 kJ mol⁻¹), it can be seen that ΔH° and ΔS° are more negative for the former than for the latter, and both are enthalpy-stabilized complexes. The molecular structure of the complex has the feature that there are two H₅O₂⁺ ions in it, in contrast to the H₃O⁺ ions in the dicyclohexano-18-crown-6 isomer A complex [1]. Each of the H₅O₂⁺ ions is held in the crown ether cavity by four hydrogen bonds. The H₅O₂⁺ ion has a central bond. The uranium atom forms UO₂Cl₄²⁻ as a counterion away from the crown ether. The formation of this complex is in good agreement with more negative entropy change and less negative free energy change, as mentioned above.     

On the mechanism of hydrogen peroxide-, superoxide-, and ultraviolet light-induced DNA cleavages of inactive bleomycin-iron (III) complex

The ³²P-labeled DNA cleavage experiments showed that the biological activity of the bleomycin(BLM)-Fe(III)OH^? complex is evidently induced by addition of H₂O₂ and KO₂, or by irradiation of UV light. Hydrogen peroxide contributes to the conversion from the inactive BLM-Fe(III)OH^? complex to the active BLM-Fe(III)O₂H^? complex, and UV light to the reduction of the BLM-Fe(III)OH^? complex to the BLM-Fe(II) complex. The proposed hypothetical mechanism for cyclic function of BLM-iron complex is similar to that of certain heme-oxygenases and heme-oxidases.     

Peroxidation of lysozyme treated with Cu(II) and hydrogen peroxide

When lysozyme was treated with Cu(II) and H₂O₂ at pH 7.4, the protein underwent polymerization as well as changes in its fluorescent characteristics. Upon prolonged incubation, most of the protein aggregates were degraded into smaller peptides. Amino acid analysis indicated that the basic amino acid residues were most susceptible to the oxidation. Tryptophan residues were converted to N-formylkynurenine and kynurenine, and lysine residues were deaminated to form α-aminoadipic acid δ-semi- aldehyde. During Cu(II)H₂O₂ treatment, the formation of carbonyl groups was accompanied by the loss of free amino groups in the protein. Succinylation of free amino groups protected lysine residues from oxidation by Cu(II)H₂O₂, but failed to prevent polymerization. The studies with the modified lysozyme suggest that Cu(II)H₂O₂ can oxidize various amino acid residues in addition to lysine to generate different types of carbonyl compounds and these carbonyl compounds may be responsible for the formation of crosslinks in the polymerization process.     

Infrared and raman study of matrix isolated M(SO2) molecules. The structure of the molecular ion SO2−

The IR and Raman spectra of Cs(SO₂), K(SO₂) and Na(SO₂) molecules were studied by ³²S/³⁴S and ¹⁶O/¹⁸O isotopic substitution technique. These molecules have a planar ring configuration of C_2v symmetry with the OSO angle equal to 109°±5° and the SO bond length of 0.149±0.001 nm. The alkali metal atom interacts symmetrically with the oxygen atoms of the SO₂⁻ group. The doubling observed for the vibrations of Cs(S¹⁶O¹⁸O) was attributed to a matrix effect.     

A differential pulse polarographic assay for O-methylation of catechols by catechol-O-methyltransferase

A new method is described for monitoring the enzyme-eatalyzed O-methylation of norepinephrine (or other catechol substrate) by catechol-O-methyltransferase. Norepinephrine and normetanephrine combine with bis-2-(ethylhexyl)hydrogen phosphate at pH 7.4 to form an ion pair which is quantitatively extracted with an immiscible organic solvent by an application of partition chromatography. The mixture of catechol substrate and O-methylated products are then simultaneously determined in 0.5 m H₂SO₄ solution by monitoring their oxidation at a carbon paste electrode by a differential pulse polarographic technique.     

H2O2-Induced Oxidative Stress Affects SO4= Transport in Human Erythrocytes

The aim of the present investigation was to verify the effect of H₂O₂-induced oxidative stress on SO₄⁼ uptake through Band 3 protein, responsible for Cl^-/HCO₃^- as well as for cell membrane deformability, due to its cross link with cytoskeletal proteins. The role of cytoplasmic proteins binding to Band 3 protein has been also considered by assaying H₂O₂ effects on hemoglobin-free resealed ghosts of erythrocytes. Oxidative conditions were induced by 30 min exposure of human erythrocytes to different H₂O₂ concentrations (10 to 300 μM), with or without GSH (glutathione, 2 mM) or curcumin (10 μM), compounds with proved antioxidant properties. Since SO₄⁼ influx through Band 3 protein is slower and better controllable than Cl^- or HCO₃^- exchange, the rate constant for SO₄⁼ uptake was measured to prove anion transport efficiency, while MDA (malondialdehyde) levels and –SH groups were estimated to quantify the effect of oxidative stress. H₂O₂ induced a significant decrease in rate constant for SO₄⁼ uptake at both 100 and 300 μM H₂O₂. This reduction, observed in erythrocytes but not in resealed ghosts and associated to increase in neither MDA levels nor in –SH groups, was impaired by both curcumin and GSH, whereas only curcumin effectively restored H₂O₂-induced changes in erythrocytes shape. Our results show that: i) 30 min exposure to 300 μM H₂O₂ reduced SO₄⁼ uptake in human erythrocytes; ii) oxidative damage was revealed by the reduction in rate constant for SO₄⁼ uptake, but not by MDA or –SH groups levels; iii) the damage was produced via cytoplasmic components which cross link with Band 3 protein; iv) the natural antioxidant curcumin may be useful in protecting erythrocytes from oxidative injury; v) SO₄⁼ uptake through Band 3 protein may be reasonably suggested as a tool to monitor erythrocytes function under oxidative conditions possibly deriving from alcohol consumption, use of drugs, radiographic contrast media administration, hyperglicemia or neurodegenerative diseases.