Control of Listeria spp. by Competitive-Exclusion Bacteria in Floor Drains of a Poultry Processing Plant

In previous studies workers determined that two lactic acid bacterium isolates, Lactococcus lactis subsp. lactis C-1-92 and Enterococcus durans 152 (competitive-exclusion bacteria [CE]), which were originally obtained from biofilms in floor drains, are bactericidal to Listeria monocytogenes or inhibit the growth of L. monocytogenes both in vitro and in biofilms at 4 to 37°C. We evaluated the efficacy of these isolates for reducing Listeria spp. contamination of floor drains of a plant in which fresh poultry is processed. Baseline assays revealed that the mean numbers of Listeria sp. cells in floor drains sampled on six different dates (at approximately biweekly intervals) were 7.5 log₁₀ CFU/100 cm² for drain 8, 4.9 log₁₀ CFU/100 cm² for drain 3, 4.4 log₁₀ CFU/100 cm² for drain 2, 4.1 log₁₀ CFU/100 cm² for drain 4, 3.7 log₁₀ CFU/100 cm² for drain 1, and 3.6 log₁₀ CFU/100 cm² for drain 6. The drains were then treated with 10⁷ CE/ml in an enzyme-foam-based cleaning agent four times in 1 week and twice a week for the following 3 weeks. In samples collected 1 week after CE treatments were applied Listeria sp. cells were not detectable (samples were negative as determined by selective enrichment culture) for drains 4 and 6 (reductions of 4.1 and 3.6 log₁₀ CFU/100 cm², respectively), and the mean numbers of Listeria sp. cells were 3.7 log₁₀ CFU/100 cm² for drain 8 (a reduction of 3.8 log₁₀ CFU/100 cm²), <1.7 log₁₀ CFU/100 cm² for drain 1 (detectable only by selective enrichment culture; a reduction of 3.3 log₁₀ CFU/100 cm²), and 2.6 log₁₀ CFU/100 cm² for drain 3 (a reduction of 2.3 log₁₀ CFU/100 cm²). However, the aerobic plate counts for samples collected from floor drains before, during, and after CE treatment remained approximately the same. The results indicate that application of the two CE can greatly reduce the number of Listeria sp. cells in floor drains at 3 to 26°C in a facility in which fresh poultry is processed.     

Cell association and degradation of α2-macroglobulin-trypsin complexes in hepatocytes and adipocytes

¹²⁵I-labelled α₂-macroglobulin-typrin complex (¹²⁵I-labelled α₂-macroglobulin·trypsin) was associated to isolated rat adipocytes and hepatocytes with a half-time of about 60 min at 37°C. The association of 0.5 μg/ml ¹²⁵I-labelled α₂-macroglobulin·trypsin was inhibited by unlabelled α₂-macroglobulin·trypsin with a half-inhibition constant of about 8 μg/ml (11 nM). ¹²⁵I-Labelled α₂-macrioglubulin became cell-associated to a smaller extent (10–40% of that of α₂-macroglobulin·trypsin) and the half-inhibition constant was about 35 μg/ml in adipocytes. The cell associated of ¹²⁵I-labelled α-macroglobulin·trypsin was markedly inhibited by dansylcadaverin, bacitracin, omission of Ca²⁺ from the medium or pretreatment of the cell with trypsin. After incubation for 180 min more than 60% of the cell-associated ¹²⁵-Ilabelled α₂-macroglobulin·trypsin was not removed by treatment of the cells with trypsin-EDTA and represented probably internalized marterial. ¹²⁵I-Labelled α₂-macroglobulin·trypsin was degraded to trichloroacetic acid-soluble fragments by suspensions of both cell types but only to a negligible extent by incubation media preincubated with these cells. The rate of degradation of 0.5 μg/ml ¹²⁵I-labelled α₂-macroglobulin was approx. 40% of that of ¹²⁵I-labelled α₂-macroglobulin·trypsin. Degradation of ¹²⁵I-labelled α₂-macroglobulin·trypsin was abolished by a high concentration (0.5 mg/ml) and α₂-macroglobulin·trypsin. It is concluded that α₂-macroglobulin·trypsin by a specific and saturable mechanism is bound to, internalized and degraded by isolated rat adipocytes and hepatocytes.     

Plastoquinol generates and scavenges reactive oxygen species in organic solvent: Potential relevance for thylakoids

The present work reports reactions of plastoquinol (PQH₂-9) and plastoquinone (PQ-9) in organic solvents and summarizes the literature to understand similar reactions in thylakoids. In thylakoids, PQH₂-9 is oxidized by the cytochrome b₆/f complex (Cyt b₆/f) but some PQH₂-9 is also oxidized by reactions in which oxygen acts as an electron acceptor and is converted to reactive oxygen species (ROS). Furthermore, PQH₂-9 reacts with ROS. Light enhances oxygen-dependent oxidation of PQH₂-9. We examined the oxidation of PQH₂-9 via dismutation of PQH₂-9 and PQ-9 and scavenging of the superoxide anion radical (O₂^?) and hydrogen peroxide (H₂O₂) by PQH₂-9. Oxidation of PQH₂-9 via dismutation to semiquinone was slow and independent of pH in organic solvents and in solvent/buffer systems, suggesting that intramembraneous oxidation of PQH₂-9 in darkness mainly proceeds via reactions catalyzed by the plastid terminal oxidase and cytochrome b₅₅₉. In the light, oxidation of PQH₂-9 by singlet oxygen and by O₂^? formed in PSI contribute significantly. In addition, Cyt b_6/f forms H₂O₂ with a PQH₂-9 dependent mechanism. Measurements of the reaction of O₂^? with PQH₂-9 and PQ-9 in acetonitrile showed that O₂^? oxidizes PQH₂-9, forming PQ-9 and several PQ-9-derived products. The rate constant of the reaction between PQH₂-9 and O₂^? was found to be 10⁴?M^?1?s^?1. H₂O₂ was found to oxidize PQH₂-9 to PQ-9, but failed to oxidize all PQH₂-9, suggesting that the oxidation of PQH₂-9 by H₂O₂ proceeds via deprotonation mechanisms producing PQH^?-9, PQ^2?-9 and the protonated hydrogen peroxide cation, H₃O₂⁺.     

The interaction between water and the polar head in inverted phosphatidylcholine micelles A 2H and 31P relaxation study

²H and ³¹P spin-lattice relaxation times (T₁) were studied for invented egg phosphatidylcholine micelles in CCl₄ as functions of ²H₂O concentration. When the ²H₂O/phosphatidylcholine mole ratio changed from 1.0 to 18.0, T₁ of ³¹P increased by about 2.6 fold, whereas T₁ of ²H increased by about 50 fold. A quantitative analysis of the deuterium T₁ data showed that there is only one water molecule tightly bound to the polar head, and it is in rapid exchange with the rest of the water molecules. The activation energy for the deuterium T₁ was 7.1 ± 0.8 kcal/mol (30 ± 3 kJ/mol), and was independent of the ²H₂O concentration.     

D2O-induced ion channel activation in Characeae at low ionic strength

Effects of D₂O were studied on internodal cells of the freshwater alga Nitellopsis obtusa under plasmalemma perfusion (tonoplast-free cells) with voltage clamp, and on Ca²⁺ channels isolated from the alga and reconstituted in bilayer lipid membranes (BLM). External application of artificial pond water (APW) with D₂O as the solvent to the perfused plasmalemma preparation led to an abrupt drop of membrane resistance (R _m = 0.12 ±0.03 kΩ · cm²), thus preventing further voltage clamping. APW with 25% D₂O caused a two-step reduction of R _m : first, down to 2.0 ± 0.8 kΩ · cm², and then further to 200 Ω · cm², in 2 min. It was shown that in the first stage, Ca²⁺ channels are activated, and then, Ca²⁺ ions entering through them activate the Cl^? channels. The Ca²⁺ channels are activated irreversibly. If 100 mm CsCl was substituted for 200 mm sucrose (introduced for isoosmoticity), no effect of D₂O on R _m was observed. Intracellular H₂O/D₂O substitution also did not change R _m . In experiments on single Ca²⁺ channels in BLM H₂O/ D₂O substitution in a solution containing 100 mm KCl (trans side) produced no effect on channel activity, while in 10 mm KCl, at negative voltage, the open channel probability sharply increased. This effect was irreversible. The single channel conductance was not altered after the H₂O/D₂O substitution. The discussion of the possible mechanism of D₂O action on Ca²⁺ and Cl^? channels was based on an osmotic-like stress effect and the phenomenon of higher D-bond energy compared to the H-bond.     

A Transmural Gradient in the Cardiac Na/K Pump Generates a Transmural Gradient in Na/Ca Exchange

We previously demonstrated a transmural gradient in Na/K pump current (I _P) and [Na⁺] _i , with the highest maximum I _P and lowest [Na⁺] _i in epicardium. The present study examines the relationship between the transmural gradient in I _P and Na/Ca exchange (NCX). Myocytes were isolated from canine left ventricle. Whole-cell patch clamp was used to measure current generated by NCX (I _NCX) and inward background calcium current (I _ibCa), defined as inward current through Ca²⁺ channels less outward current through Ca²⁺-ATPase. When resting myocytes from endocardium (Endo), midmyocardium (Mid) or epicardium (Epi) were studied in the same conditions, I _NCX was the same and I _ibCa was zero. Moreover, Western blots were consistent with NCX protein being uniform across the wall. However, the gradient in [Na⁺] _i , with I _ibCa = 0, should create a gradient in [Ca²⁺] _i . To test this hypothesis, we measured resting [Ca²⁺] _i using two methods, based on either transport or the Ca²⁺-sensitive dye Fura2. Both methods demonstrated a significant transmural gradient in resting [Ca²⁺] _i , with Endo > Mid > Epi. This gradient was eliminated by exposing Epi to sufficient ouabain to partially inhibit Na/K pumps, thus increasing [Na⁺] _i to values similar to those in Endo. These data support the existence of a transmural gradient for Ca²⁺ removal by NCX. This gradient is not due to differences in expression of NCX; rather, it is generated by a transmural gradient in [Na⁺] _i , which is due to a transmural gradient in plasma membrane expression of the Na/K pump.     

Kinetics of the decomposition of hydrogen peroxide in the presence of ethylenediaminetetraacetatocerium(IV) complex

The rate of reaction of [Ce(EDTA)(OH)_nⁿ⁻] with H₂O₂ in 0.10 M KNO₃ solution was investigated at various temperatures. The presence of a peroxy intermediate is inferred from spectrophotometric measurements. The general rate equation,

is valid for pH 7-9 with n= 1 and 2 complexes involved. The rate constants k_l and k₂ were determined at 25 °C to be 0.054 and 0.171 M⁻¹ s⁻¹ respectively. The corresponding activation enthalpies, as calculated from Arrhenius plots, were δH₁^#= 51.3 ± 14.8 and δH₂^#= 41.8 ± 5.3 kJ m⁻¹ and the activation entropies were δS₁^#=-97 ± 47 and ΔS₂^#=−119±17 J K⁻¹ m⁻¹.     

Different coordination modes of an aryl-substituted hydrotris(pyrazolyl)borate ligand in rhodium and iridium complexes

Complexes Tp^tolRh(C₂H₄)₂ (1a) and Tp^tolRh(CH₂C(Me)C(Me)CH₂) (1b) have been prepared by reaction of KTp^tol with the appropriate [RhCl(olefin)₂]₂ dimer (Tp^tol means hydrotris(3-p-tolylpyrazol-1-yl)borate). The two complexes show a dynamic behaviour that involves exchange between κ² and κ³ coordination modes of the Tp^tol ligand. The iridium analogue, Tp^tolIr(CH₂C(Me)CHCH₂) (2) has also been synthesized, and has been converted into the Ir(III) dinitrogen complex [(κ⁴-N,N’,N’’,C-Tp^tol)Ir(Ph)(N₂) (3) by irradiation with UV light under a dinitrogen atmosphere. Compound 3 constitutes a rare example of Ir(III)-N₂ complex structurally characterized by X-ray crystallography. Its N₂ ligand can be easily substituted by acetonitrile or ethylene upon heating and denticity changes in the Tp^tol ligand, from κ⁴-N,N’,N’’,C (monometallated Tp^tol, from now on represented as Tp^tol′) to κ⁵-N,N′,N″,C,C″ (dimetallated Tp^tol ligand, represented as Tp^tol″) have been observed. When complex 3 is heated in the presence of acetylene, dimerization of the alkyne takes place to yield the enyne complex [(κ⁵-N,N′,N′′,C,C′-Tp^tol)Ir(CH₂CHCCH), 7¸ in which the unsaturated organic moiety is bonded to iridium through the carbon-carbon double bond.     

Relationship of respiration to body weight in the tilapia Oreochromis niloticus under resting and normoxic conditions

• 1.1. The relationships of oxygen consumption (V_o2, ml/min/fish), ventilation volume (V_g, ml/min/fish), stroke volume (V_s, ml/stroke/fish), respiration frequency (RF, stroke/min) and oxygen utilization (U, %) to body weight (W, g) in the tilapia under resting and normoxic conditions were V_o2 = 0.002835W^0.754193, V_g = 0.688965W^0.722786, V_s = 0.002790W^1.017188, RF = 248.58210W^−0.296139, U = 0.000935W + 87.394288, respectively.

     

Group V Secretory Phospholipase A2 Is Involved in Tubular Integrity and Sodium Handling in the Kidney

Group V (GV) phospholipase A₂ (PLA₂) is a member of the family of secreted PLA₂ (sPLA2) enzymes_. This enzyme has been identified in several organs, including the kidney. However, the physiologic role of GV sPLA₂ in the maintenance of renal function remains unclear. We used mice lacking the gene encoding GV sPLA₂ (Pla2g5^−/−) and wild-type breeding pairs in the experiments. Mice were individually housed in metabolic cages and 48-h urine was collected for biochemical assays. Kidney samples were evaluated for glomerular morphology, renal fibrosis, and expression/activity of the (Na⁺ + K⁺)-ATPase α1 subunit. We observed that plasma creatinine levels were increased in Pla2g5^−/− mice following by a decrease in creatinine clearance. The levels of urinary protein were higher in Pla2g5^−/− mice than in the control group. Markers of tubular integrity and function such as γ-glutamyl transpeptidase, lactate dehydrogenase, and sodium excretion fraction (FE_Na⁺) were also increased in Pla2g5^−/− mice. The increased FE_Na⁺ observed in Pla2g5^−/− mice was correlated to alterations in cortical (Na⁺ + K⁺) ATPase activity/ expression. In addition, the kidney from Pla2g5^−/− mice showed accumulation of matrix in corticomedullary glomeruli and tubulointerstitial fibrosis. These data suggest GV sPLA₂ is involved in the maintenance of tubular cell function and integrity, promoting sodium retention through increased cortical (Na⁺ + K⁺)-ATPase expression and activity.     

Ceramide-1-Phosphate, in Contrast to Ceramide, Is Not Segregated into Lateral Lipid Domains in Phosphatidylcholine Bilayers

Sphingolipids are key lipid regulators of cell viability: ceramide is one of the key molecules in inducing programmed cell death (apoptosis), whereas other sphingolipids, such as ceramide 1-phosphate, are mitogenic. The thermotropic and structural behavior of binary systems of N-hexadecanoyl-D-erythro-ceramide (C₁₆-ceramide) or N-hexadecanoyl-D-erythro-ceramide-1-phosphate (C₁₆-ceramide-1-phosphate; C₁₆-C1P) with 1,2-dipalmitoyl-sn-glycero-3-phosphocholine (DPPC) was studied with DSC and deuterium nuclear magnetic resonance (²H-NMR). Partial-phase diagrams (up to a mole fraction of sphingolipids X = 0.40) for both mixtures were constructed based on DSC and ²H-NMR observations. For C₁₆-ceramide-containing bilayers DSC heating scans showed already at X_cer = 0.025 a complex structure of the main-phase transition peak suggestive of lateral-phase separation. The transition width increased significantly upon increasing X_cer, and the upper-phase boundary temperature of the mixture shifted to ∼65°C at X_cer = 0.40. The temperature range over which ²H-NMR spectra of C₁₆-ceramide/DPPC-d₆₂ mixtures displayed coexistence of gel and liquid crystalline domains increased from ∼10° for X_cer = 0.1 to ∼21° for X_cer = 0.4. For C16-C1P/DPPC mixtures, DSC and ²H-NMR observations indicated that two-phase coexistence was limited to significantly narrower temperature ranges for corresponding C1P concentrations. To complement these findings, C₁₆-ceramide/1-palmitoyl-2-oleoyl-sn-glycero-3-phosphocholine (POPC) and C16-C1P/POPC mixtures were also studied by ²H-NMR and fluorescence techniques. These observations indicate that DPPC and POPC bilayers are significantly less perturbed by C₁₆-C1P than by C₁₆-ceramide and that C₁₆-C1P is miscible within DPPC bilayers at least up to X_C1P = 0.30.     

Stepwise reactions of two N-CH2CN or two N-CH2C(NH)OMe groups attached to macrocyclic copper(II) complexes: Preparation of homo- and hetero-di-N-functionalized macrocyclic complexes

The hetero-functionalized macrocyclic complex [CuL²](ClO₄)₂ bearing one N-CH₂C(NH)OMe and one N-CH₂CN groups as well as [CuL³](ClO₄)₂ bearing two N-CH₂C(NH)OMe groups have been prepared selectively by the reaction of [CuL¹](ClO₄)₂ (L² = 2,13-bis(cyanomethyl)-5,16-dimethyl-2,6,13,17-tetraazatricyclo[16.4.0.^1.180^7.12]docosane) with methanol. The N-CH₂C(NH)OCH₃ group in [CuL²](ClO₄)₂ is quite inert against acid hydrolysis. On the other hand, the functional pendant arms in [CuL³](ClO₄)₂ readily undergo acid hydrolysis. Both [CuL⁴](ClO₄)₂ bearing one N-CH₂COOCH₃ and one N-CH₂C(NH)OCH₃ groups and [CuL⁵](ClO₄)₂ bearing two N-CH₂OOCH₃ groups have been prepared by the stepwise hydrolysis of [CuL³](ClO₄)₂. The reactivity of the functional pendant arms in [CuL¹](ClO₄)₂ or [CuL³](ClO₄)₂ is quite different from that in [NiL¹](ClO₄)₂ or [NiL³](ClO₄)₂. The crystal structure of [CuL²](ClO₄)₂ shows that the complex has a slightly distorted square-pyramidal coordination polyhedron with an apical Cu-N (N-CH₂C(NH)OCH₃ group) bond. The N-CH₂C(NH)OCH₃ and/or N-CH₂COOCH₃ groups in [CuL³](ClO₄)₂, [CuL⁴](ClO₄)₂, and [CuL⁵](ClO₄)₂ are involved in coordination, and the complexes have distorted trans-octahedral coordination polyhedron. The axial Cu-N (N-CH₂C(NH)OCH₃ group) distance (2.396(7) Å) of [CuL⁴](ClO₄)₂ is considerably longer than the Cu-N (N-CH₂C(NH)OCH₃ group) distance (2.169(3) Å) of [CuL²](ClO₄)₂.     

Kinetics of ligand substitution in platinum(II) complexes: A study on the concept of nucleophilic discrimination

Several platinum(II) complexes of the general type [Pt(OND)X] have been prepared and characterized, the ligand (OND) representing the phenolate anion of the tridentate Schiff bases N-(2- diethylaminoethyl)-salicylaldimine (D = NEt₂), N-(2- ethylaminoethyl)-salicylaldimine (D = NHEt) and N- (3-thia-n-pentyl)-salicylaldimine (D= SEt) and X= Cl, NO₃. As shown by conductimetric studies the nitrato complexes [Pt(OND)NO₃] dissociate completely in methanol according to:

Spectrophotometry (normal and stopped-flow) has been used to study the kinetics of solvent substitution according to

with a variety of neutral and anionic nucleophiles Y in methanol at 20 °C and constant ionic strength, I= 0.2 M (NaClO₄). The substitution follows a one- term rate law, v = k_obs[Pt(OND)(H₂O)⁺] = k_Y[Y]- [Pt(OND)(H₂O)⁺]. The k_Y data obtained for 13 (D = NEt₂) and 7 (D = NHEt; SEt) different nucleophiles Y cannot be adequately correlated with their n_pt⁰ values according to the well-known relationship log k_Y = sn_pt⁰ + log k_s. The deviations are strongest for large and bulky nucleophiles such as Y=Ph₃P, Bu₃P, Ph₃As, I^- and for D = NEt₂, from which it is concluded that steric crowding hinders the formation of the 5-coordinate transition state. The rate reducing steric cis-effect observed is of the order k_Y(D = NEt₂):k_Y(D = NHEt):k_Y(D = SEt) = 1:35:63 for small nucleophiles Y and as large as 1:192:2640 for Y = Ph₃P. The introduction of substituents X in the salicylaldehyde ring in ortho (X³), meta (X⁴) and para position (X⁵) to the phenolic oxygen proves the existence of rather small electronic effects (X⁴, X⁵) and much stronger steric effects of bulky substituents X³, neighboring the donor oxygen.With the standard substrate trans-[Ptpy₂Cl₂] some new n_pt⁰ values were determined, namely for N, N′- dimethylthiourea (n_pt⁰ = 7.02), N, N′ -diphenylthlourea (n_pt⁰ = 7.19), N, N, N′, N′-tetramethylthiourea (n_pt⁰ = 6.05) and for the pseudo-halide dicyanoamide ion, N(CN)₂^- (n_pt⁰= 3.05). The n_pt⁰ value for the pseudo-halide tricyanomethanide, ion, C(CN)₃^-, was estimated to be 3.03.     

Barium inhibition of sodium ion transport in toad bladder

The effect of Ba²⁺ on Na⁺ transport and electrical characteristics of toad bladder was determined from change produced in short circuit current (I_sc, epithelial, apical and basal-lateral potentials (ψ_t, ψ_a, ψ_b), epithelial and membrane resistances (R_t, R_a, R_b) and shunt resistance (R_s). Mucosal Ba²⁺ had no effect. Serosal Ba²⁺ reduced I_sc, ψ_t, ψ_a, and ψ_b, but had no effect on R_t, R_a, R_b and R_s. Minimal effective Ba²⁺ concentration was 5 · 10^?5 M. The phenomenon was reversed by Ba²⁺ removal, but not by 86 mM serosal K⁺. Ba²⁺ inhibition of I_sc did not impair the response to vasopressin which was quantitatively the same as controls. ψ_a with Ba²⁺ equalled ψ_b. After Ba²⁺ inhibition, ouabain produced no further decrease in ψ_t and I_sc. Ba²⁺ exposure after ouabain did not decrease ψ_t and I_sc. The results suggest that Ba²⁺ inhibits the basal-lateral electrogenic Na⁺ pump.     

Synthesis and solid-state structures of (triphos)iridacyclopentadiene complexes as models for vinylidene intermediates in the [2 + 2 + 1] cyclotrimerization of alkynes

The iridium 1,1,1-tris(diphenylphosphinomethyl)ethane (triphos) complexes [{κ²(C¹,C⁴)-CRCRCRCR}{CH₃C(CH₂PPh₂)₃}Ir(NCMe)]BF₄ (2-NCMe, R = CO₂Me) and [{κ²(C¹,C⁴)-CRCRCRCR}{CH₃C(CH₂PPh₂)₃}Ir(CO)]BF₄ (2-CO, R = CO₂Me) serve as models for proposed iridium-vinylidene intermediates of relevance to the [2 + 2 + 1] cyclotrimerization of alkynes. The solid-state structures of 2-NCMe, 2-CO, and [κ²(C¹,C⁴)-CRCRCRCR]{CH₃C(CH₂PPh₂)₃}Ir(Cl) (2-Cl), were determined by X-ray crystallography.     

Manganese(II) complexes of di-2-pyridinylmethylene-1,2-diimine di-Schiff base ligands: Structures and reactivity

Manganese(II) complexes [Mn(L)X₂] were prepared and characterized, where L is a neutral di-Schiff base ligand incorporating pyridylimine donor arms, including (1R,2R)-N,N′-bis(2-pyridylmethylidene)-1,2-diphenylethylenediimine (L¹), (1R,2R)-N,N′-bis(6-methyl-2-pyridylmethylidene)-1,2-cyclohexyldiimine (L²), or (1R,2R)-, (1S,2S)- or racemic N,N′-bis(2-pyridylmethylidene)-1,2-cyclohexyldiimine (L³), and X⁻ =  or Cl⁻. Product complexes were structurally characterized, specifically including [Mn(R,R-L¹)(NCCH₃)₃](ClO₄)₂, [Mn(R,R-L²)(OH₂)₂](ClO₄)₂ and racemic [Mn(L³)Cl₂]. The first of these complexes features a heptacoordinate ligand field in a distorted pentagonal bipyramid, and the latter two are hexacoordinate, but retain equatorially monovacant pentagonal bipyramidal structures. Complexes [Mn(L³)X₂] (X⁻ = Cl⁻, ) were reacted with the primary phosphine FcCH₂PH₂ (Fc = -C₅H₄FeC₅H₅), H₂O and ethyldiazoacetate (EDA). The first two substrates prompted reactivity at a single ligand imine bond, resulting in hydrophosphination and hydrolysis, respectively. Complexes of the derivative ligands were also structurally characterized. Evidence for EDA activation was obtained by electrospray ionization mass spectrometry, but catalytic carbene transfer was not obtained.     

Copper(II)-mediated oxime-nitrile coupling in non-aqueous solutions: Synthetic, structural and magnetic studies of the copper(II)-salicylaldehyde oxime reaction system

The reactions of salicylaldehyde oxime (H₂salox) with Cu^II precursors yielded the known complexes [Cu(Hsalox)₂] (1) and [Cu(Hsalox)₂]_n (2), as well as complexes [Cu₃(salox)(L₁)(L₂)]·MeCN (3·MeCN), [CuCl(L₁)] (4) and [Cu₂Na(O₂CMe)₅(HO₂CMe)]_n (5), where L₁⁻ = o-O-C₆H₄-CHNO-C(CH₃)NH and L₂³⁻ = o-O-C₆H₄-CHNO-C(o-O-C₆H₄)N. L₁⁻ was formed in situ via the nucleophilic addition of the oximato O-atom of salox²⁻ to the unsaturated nitrile group of the MeCN reaction solvent. L₂³⁻ is also formed in situ probably through the nucleophilic attack of the oximato O-atom to the unsaturated nitrile group of salicylnitrile; the latter, although not directly added to the reaction mixture, can be produced via the dehydration of salox²⁻. Compounds 1 and 2 contain Hsalox⁻ bound to the metal center in two different coordination modes; they both contain the same mononuclear unit, however a 2D network is generated in 2 due to a relatively long Cu-O_oximato bond. Compound 3 contains three different ligands, i.e. salox²⁻, L₁⁻ and L₂³⁻, which act as μ₃-κ²O:κO′:κN, κO:κN:κN′ and μ₃-κ²O:κ²N:κO′:κN′, respectively, whereas 4 consists of a square planar Cu^II atom bound to a κO:κN:κN′ L₁⁻ and a chloride ion. Compound 5 consists of dinuclear [Cu₂(O₂CMe)₅(HO₂CMe)]⁻ units and Na⁺ ions assembled into an overall 3D network structure. Magnetic susceptibility measurements from polycrystalline samples of 2 and 5 gave best-fit parameters J = +0.36 cm⁻¹ (H = −J?_i?_j) and J = −360 cm⁻¹, zj = +20 cm⁻¹ (H = −J?_i?_j − zJ〈S_z〉?_z), respectively.     

A gene locus affecting tolerance to BGG in mice.

A genetic analysis was made of the ease of tolerance induction to bovine γ-globulin (BGG) in DBA/2, BALB/c, F₁ and backcross generation mice. Like parental DBA/2 mice, the F₁ generation of BALB/c × DBA/2 becomes tolerant when treated with 2 mg BGG. A backcross of this F₁ to DBA/2 parents produced mice that all became tolerant to this dose of BGG. A backcross of F₁ mice to BALB/c parents produced 50% offspring tolerized by the same dose of BGG and 50% resistant to tolerance induction.The data suggest a single autosomal locus affecting tolerance induction. Data presented elsewhere suggest that the locus affects macrophage function. We propose that this locus be called tolerance (symbol Tol-l) and the two alleles be (Tol-l^a (DBA/2 type) and Tol-l^b (BALB/c type) with Tol-l^a being dominant.     

The low spin - high spin equilibrium in the S2-state of the water oxidizing enzyme

In Photosystem II (PSII), the Mn₄CaO₅-cluster of the active site advances through five sequential oxidation states (S₀ to S₄) before water is oxidized and O₂ is generated. Here, we have studied the transition between the low spin (LS) and high spin (HS) configurations of S₂ using EPR spectroscopy, quantum chemical calculations using Density Functional Theory (DFT), and time-resolved UV-visible absorption spectroscopy. The EPR experiments show that the equilibrium between S₂^LS and S₂^HS is pH dependent, with a pK_a?≈?8.3 (n?≈?4) for the native Mn₄CaO₅ and pK_a?≈?7.5 (n?≈?1) for Mn₄SrO₅. The DFT results suggest that exchanging Ca with Sr modifies the electronic structure of several titratable groups within the active site, including groups that are not direct ligands to Ca/Sr, e.g., W1/W2, Asp61, His332 and His337. This is consistent with the complex modification of the pK_a upon the Ca/Sr exchange. EPR also showed that NH₃ addition reversed the effect of high pH, NH₃-S₂^LS being present at all pH values studied. Absorption spectroscopy indicates that NH₃ is no longer bound in the S₃Tyr_Z state, consistent with EPR data showing minor or no NH₃-induced modification of S₃ and S₀. In both Ca-PSII and Sr-PSII, S₂^HS was capable of advancing to S₃ at low temperature (198?K). This is an experimental demonstration that the S₂^LS is formed first and advances to S₃via the S₂^HS state without detectable intermediates. We discuss the nature of the changes occurring in the S₂^LS to S₂^HS transition which allow the S₂^HS to S₃ transition to occur below 200?K. This work also provides a protocol for generating S₃ in concentrated samples without the need for saturating flashes.