Coupling factor activity of the purified pea mitochondrial F1-ATPase

The pea cotyledon mitochondrial F₁-ATPase was released from the submitochondrial particles by a washing procedure using 300 mM sucrose /2 mM Tricine (pH 7.4). The enzyme was purified by DEAE-cellulose chromatography and subsequent sucrose density gradient centrifugation. Using polyacrylamide gel electrophoresis under non-denaturing conditions, the purified protein exhibited a single sharp band with slightly lower mobility than the purified pea chloroplast CF₁-ATPase. The molecular weights of pea mitochondrial F₁-ATPase and pea chloroplast CF₁-ATPase were found to be 409 000 and 378 000, respectively. The purified pea mitochondrial F₁-ATPase dissociated into six types of subunits on polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulfate. Most of these subunits had mobilities different from the subunits of the pea chloroplast CF₁-ATPase. The purified mitochondrial F₁-ATPase exhibited coupling factor activity. In spite of the observed differences between CF₁ and F₁, the mitochondrial enzyme stimulated ATP formation in CF₁-depleted pea chloroplast membranes. Thus, the mitochondrial F₁ was able to substitute functionally for the chloroplast CF₁ in reconstituting photophosphorylation.     

The activation and inactivation of the Dunaliella salina chloroplast coupling factor 1 (CF1) in vivo and in situ

Preillumination of intact cells of the eukaryotic, halotolerant, cell-wall-less green alga Dunaliella salina induces a dark ATPase activity the magnitude of which is about 3–5-fold higher than the ATPase activity observed in dark-adapted cells. The light-induced activity arises from the activation and stabilization in vivo of chloroplast coupling factor 1 (CF₁). This activity, 150–300 μmol ATP hydrolyzed/mg Chl per h, rapidly decays (with a half-time of about 6 min at room temperature) in intact cells but only slowly decays (with a half-time of about 45 min at room temperature) if the cells are lysed by osmotic shock immediately after illumination. The activated form of the ATPase in lysed cells is inhibited if the membranes are treated with ferri- but not ferrocyanide, suggesting that the stabilization of the activated form of CF₁ is due to the reduction of the enzyme in vivo in the light.     

N-Ethylmaleimide inhibition of the catalytic activities of the Dunaliella salina coupling factor 1 (CF1) and the restoration of the inhibition of the CF1 ATPase activity by N-ethylmaleimide

The sensitivity of the catalytic activities of the D. salina chloroplast coupling factor 1 (CF₁) to chemical modification by N-ethylmaleimide has been investigated. (i) When D. salina thylakoid membranes are treated with N-ethylmaleimide, both photophosphorylation and the inducible CF₁ ATPase activity are partially (approx. 60%) inhibited. The inhibition of both activities does not require the presence of a proton-motive force, and the inhibition of photophosphorylation is directly related to the N-ethylmaleimide-covalent modification of CF₁ as shown by (a) the time-course for the inhibition and (b) the maximal extent of inhibition. (ii) Treatment of the purified, latent, D. salina CF₁ with low concentrations of N-ethylmaleimide also results in the partial (approx. 60%) inhibition of the inducible ATPase activity (I₅₀ ≈ 50 μM). The inhibition does not require the presence of the chemical modifier during the activation of the enzyme. (iii) N-ethylmaleimide-induced inhibition of the ATPase activity of either membrane-bound or solubilized CF₁ is partially reversed by either (a) prolonged incubation at low concentrations of N-ethylmaleimide or (b) short incubation times at high concentrations of N-ethylmaleimide. The results are interpreted as indicating multiple binding sites on the D. salina CF₁ that have different rates of reactivity with N-ethylmaleimide. Those sites (or site) that react rapidly with N-ethylmaleimide cause(s) an inhibition of both ATP synthase and ATPase activities, whereas those sites (or site) that react more slowly partially restore(s) the original-ATPase activity. The effects of N-ethylmaleimide on the catalytic activity of D. salina CF₁ are probably mediated by N-ethylmaleimide-induced conformational changes of the enzyme.     

Disposition of water in chloroplast coupling factor 1 (CF1) A neutron scattering analysis

Small-angle neutron scattering experiments were performed in dilute aqueous solutions of chloroplast F₁-ATPase. By contrast variation in ¹H₂O/²H₂O mixtures and when using different concentrations of glycerol in ²H₂O, structural information on the spatial distribution of dry protein and water was obtained. The maximum distance within latent and active CF₁ was 12 nm. the shape of CF₁ was globular. The total volume of CF₁ was 900 nm³, and its dry volume (excluding the volume of one water molecule per two exchangeable hydrogen atoms) was 400 nm³. A volume of 670 nm³ was inaccessible to glycerol at low glycerol concentrations (less than 25%). At higher concentrations (up to 50%) a volume of 460 nm³ was excluded to glycerol. Within the resolution of our experiment (1.6 nm) there was no evidence for particular water-rich regions or of secluded water spaces or any particular places for glycerol exchange. Upon thiol activation of the latent enzyme only small changes in structure were detectable just at the limits of the experimental error. They suggest an enhancement of the surface roughness.     

The binding of eosin-labeled subunit δ to the isolated chloroplast ATPase, CF1, as revealed by rotational diffusion in solution

We investigated the binding of subunit δ to solubilized chloroplast ATPase. Purified δ was covalently labeled with eosin 5-isothiocyanate and its rotational correlation time was determined by a photoselection technique as a function of added CF₁ (containing δ) and of CF₁(−δ) (lacking δ). In aqueous buffer the rotational correlation time of labeled δ was 33 ns. This is compatible with a rather elongated shape with the dimensions 2b = 100 Å/2a = 28 Å. Binding of δ to CF₁ decreased the rotational correlation time about 10-fold. The result was a biphasic decay of the laser flash-induced absorption anisotropy which was analyzed to yield the proportion of δ (bound to CF₁) relative to δ (free). CF₁(−δ), which completely lacked the δ-subunit, bound one δ (mol/mol) with high affinity (K_d ≈ 100 nM) and at least another δ with about 20-fold lower affinity. The δ-containing CF₁, revealed only the low-affinity site(s) for δ. This was compatible with a 1:1 stoichiometry of δ in isolated CF₁.     

Guanosine and formycin triphosphates bind at non-catalytic nucleotide binding sites of CF1 ATPase and inhibit ATP hydrolysis

Guanosine triphosphate and formycin triphosphate (FTP) in the presence of excess Mg²⁺ can bind to empty non-catalytic sites of spinach chloroplast ATPase (CF₁). This results in a greatly reduced capacity for ATP hydrolysis compared to the enzyme with non-catalytic sites filled with ATP. With two GTP bound at non-catalytic sites the inhibition is about 90%; with two FTP bound about 80% inhibition is obtained. Binding and release of the nucleotides from the non-catalytic sites are relatively slow processes. Exposure of CF₁ with one or two empty non-catalytic sites to 5–10 μM FTP or GTP for 15 min suffices for about 50% of the maximum inhibition. Reactivation of CF₁ after exposure to higher FTP or GTP concentrations requires long exposure to 2 μM EDTA. The findings show that, contrary to previous assumptions, GTP can bind tightly to non-catalytic sites of CF₁. They suggest that the presence of adenine nucleotides at non-catalytic sites might be essential for high catalytic capacity of the F₁ ATPases.     

The synthesis of the tripodal phosphine CH3C{CH2P(m-CF3C6H4)2}3 and its rhodium coordination chemistry

The new tripodal phosphine CH₃C{CH₂P(m-CF₃C₆H₄)₂}₃, CF₃PPP, was prepared by reacting CH₃C(CH₂Br)₃ with Li⁺P(m-CF₃C₆H₄)₂⁻, the latter being best obtained by adding Li⁺NⁱPr₂⁻ to PH(m-CF₃C₆H₄)₂. The rhodium complexes [RhCl(CO)(CF₃PPP)], [Rh(LL)(CF₃PPP)](CF₃SO₃) (LL = 2 CO or NBD), [RhX₃(CF₃PPP)], [RhX(MeCN)₃(CF₃PPP)](CF₃SO₃)₂ (X = H and Cl), [RhCl₂(MeCN)(CF₃PPP)](CF₃SO₃) and [Rh(MeCN)₃(CF₃PPP)](CF₃SO₃)₃ were prepared and characterized. The X-ray crystal structure of [Rh(NBD)(CF₃PPP)](CF₃SO₃) is reported. The lower oxygen sensitivity of the CF₃PPP rhodium(I) complexes, relative to the corresponding species with the parent ligand CH₃C(CH₂PPh₂)₃, is attributed to the higher effective nuclear charge on the metal centers caused by the presence of the six CF₃ substituents on the terdentate phosphine. A similar effect may be responsible for the easier hydrolysis of the CF₃PPP-containing, cationic rhodium(III) complexes relative to the corresponding compounds of the parent ligand.     

Photoaffinity cross-linking of F1ATPase from spinach chloroplasts by 3''-arylazido-β-alanyl-8-azido ATP

UV irradiation of the ATPase (CF₁) from spinach chloroplasts in the presence of 3'-arylazido-β-alanyl-8-azido ATP (8,3'-DiN₃ATP) results in a nucleotide-dependent inactivation of the enzyme and in a nucleotide-dependent formation of -β cross-links. The results demonstrate an interfacial localization of the nucleotide binding sites on CF₁.     

肥沃耕层构建对东北黑土区旱地土壤肥力和玉米产量的影响

有机物料还田是提高土壤肥力、改善土壤结构和增加作物产量的重要农艺措施之一。本研究通过分析有机物料深混还田构建肥沃耕层后土壤的有机质、速效养分含量和玉米产量,明确了黑土区不同土壤类型旱地土壤肥力指标和玉米产量对肥沃耕层构建方式的响应特征,以期为实现东北黑土区旱地保护性利用和农业可持续发展提供科学依据。采用小区试验与大区示范相结合的方式,在黑龙江省、吉林省和辽宁省选取9个生态类型区作为试验点,土壤类型包括黑土(中厚黑土和薄层黑土)、草甸土、黑钙土、白浆土、棕壤、暗棕壤和褐土。每个试验点均设置了玉米秸秆深混构建肥沃耕层(CF_Ⅰ)、秸秆配合有机肥深混构建肥沃耕层(CF_Ⅱ)和无有机物料还田(CK)3个处理。其中,CF_Ⅰ、CF_Ⅱ处理的小区试验和大区示范的秸秆还田量分别为10000 kg·hm^-2和全量还田,CF_Ⅱ处理的有机肥施用量为30000 t·hm^-2;CF_Ⅰ和CF_Ⅱ处理中有机物料的还田深度均为0~35 cm。结果表明: 不同土壤类型旱地的土壤肥力差异较大,不同土层表现为亚耕层土壤肥力小于耕层土壤,其中暗棕壤和白浆土尤为突出;棕壤、褐土耕层和亚耕层的土壤肥力均偏低;黑土和草甸土的质地比较黏重和犁底层较厚。在试验时间为两年以上的5个试验点中,与CK相比,CF_Ⅰ和CF_Ⅱ处理耕层的土壤有机质、碱解氮、速效磷和速效钾含量平均增加1.85 g·kg^-1、20.16 mg·kg^-1、1.56 mg·kg^-1和17.2 mg·kg^-1,亚耕层较耕层增加了2.09 g·kg^-1、12.06 mg·kg^-1、2.18 mg·kg^-1和3.84 mg·kg^-1。与CK相比,CF_Ⅰ处理显著增加了耕作层和亚耕层土壤有机质和速效磷含量,CF_Ⅱ处理显著增加了耕作层和亚耕层的全部土壤肥力指标,说明肥沃耕层构建是提高土壤肥力的重要途径,其中玉米秸秆配施有机肥是快速提升土壤肥力的有效方法。受不同地区水热条件和土壤类型等的影响,不同试验区的玉米产量差异较大;不同处理间差异显著,表现为CF_Ⅱ>CF_Ⅰ>CK,说明肥沃耕层构建方式在不同生态类型区均能有效提高玉米产量。采用玉米秸秆或者玉米秸秆配合有机肥深混的肥沃耕层构建方式能够同步培肥耕层和亚耕层土壤,提高玉米产量。不同生态类型区应根据土壤类型、有机物料来源等采取相应的肥沃耕层构建方式,建议在有机肥源充足的区域,优先采用秸秆配合有机肥深混构建肥沃耕层。     

Ligand induced P---H bond formation and a comparison of the reactivity of two isomers of the carbonyl hydride [Pt2(μ-PBu2)2(H)(CO)(PBu2H)]CF3SO3

The Pt₂ ^(II) isomeric terminal hydrides [(CO)(H)Pt(μ-PBu^t ₂)₂Pt(PBu^t ₂H)]CF₃SO₃ (1a), and [(CO)Pt(μ-PBu^t ₂)₂Pt(PBu^t ₂H)(H)]CF₃SO₃ (1b), react rapidly with 1 atm of carbon monoxide to give the same mixture of two isomers of the Pt₂ ^(I) dicarbonyl [Pt₂(μ-PBu^t ₂)(CO)₂(PBu^t ₂H)₂]CF₃SO₃ (3-Pt); the solid state structure of the isomer bearing the carbonyl ligands pseudo-trans to the bridging phosphide was solved by X-ray diffraction. A remarkable difference was instead found between the reactivity of 1a and 1b towards carbon disulfide or isoprene. In both cases 1b reacts slowly to afford [Pt₂(μ-PBu^t ₂)(μ,η²,η²-CS₂)(PBu^t ₂H)₂]CF₃SO₃ (4-Pt), and [Pt₂(μ-PBu^t ₂)(μ,η²,η²-isoprene) (PBu^t ₂H)₂]CF₃SO₃ (6-Pt), respectively. In the same experimental conditions, 1a is totally inert. A common mechanism, proceeding through the preassociation of the incoming ligand followed by the P---H bond formation between one of the bridging P atoms and the hydride ligand, has been suggested for these reactions.     

Dioxo-molybdenum(VI) and -tungsten(VI) BINOL and alkoxide complexes: Synthesis and catalysis in sulfoxidation, olefin epoxidation and hydrosilylation of carbonyl groups

The reaction of MoO₂(mes)₂ with S-H₂BINOL (mes = 2,4,6-Me₃C₆H₂; H₂BINOL = 1,1′-bi-2-naphthol) and (CF₃)₂MeCOH in THF yielded the novel dioxo-molybdenum(VI) complexes MoO₂(S-BINOL)(THF)₂ and MoO₂[OCMe(CF₃)₂]₂(THF), respectively. Similar tungsten derivatives WO₂(S-BINOL)(THF) and WO₂[OCMe(CF₃)₂]₂(THF) have been prepared by the reaction of WO₂Cl₂(DME) with the corresponding lithium salts of BINOL and 1,1,1,3,3,3-hexafluoro-2-methyl-2-propanol, respectively. Catalytic experiments have shown that MoO₂(S-BINOL)(THF)₂ is an active catalyst in the sulfoxidation of methyl phenyl sulfide and in the epoxidation of cis-cyclooctene with tert-butylhydroperoxide, under mild conditions. The BINOL complex was, however, not found to be enantioselective. In addition, the catalytic activity of the molybdenum species MoO₂(S-BINOL)(THF)₂ and MoO₂[OCMe(CF₃)₂]₂(THF) in the hydrosilylation of carbonyl groups has been explored.     

An ab initio MO-LCAO investigation of the electronic structure of organic hydroperoxides and platinum(II) hydroperoxo complexes: A contribution to the knowledge of the mechanism of olefin epoxidation

A possible new process of activation of the OOH group in the mechanism of ethylene epoxidation catalysed by Pt(II) diphosphine complexes has been investigated by ab initio MO-LCAO calculations. The electronic and geometric features of YOOH species (Y = H, CH₃, t-But, CF₃, CH₃CO, (PH₃)₂Pt(CF₃), (PH₃)₃PtCl) have been evaluated and compared. Coordination of the OOH group to platinum induces an inversion of the polarity of the O-O bond when compared to any organic hydroperoxide; parallelly it favours the isomerisation of the OOH group from a hydroperoxo to an oxywater-like structure. This latter effect could be an important factor in favouring the reaction of the platinum coordinated OOH group with ethylene to form ethylene oxide. In fact, calculations on the energetics of the interaction between H₂O₂ and C₂H₄ have shown that isomerisation of HOOH to H₂OO oxywater structure is the rate determining step for the epoxidation process.     

基于微卫星分析的长丰鲢种质资源遗传监测

长丰鲢(CF)为我国人工培育的鱼类新品种, 自推广应用以来取得了良好的效果。开展长丰鲢种质资源遗传监测, 对其优良性状保持具重要作用。研究采用18对微卫星引物分析了鲢(L)和长丰鲢世代间(CF₁、CF₂和CF₃)的遗传多样性和遗传结构。结果表明: 鲢遗传多样性指数高于长丰鲢, 遗传多样性也较长丰鲢丰富。而长丰鲢子代间CF₁到CF₃平均等位基因数(N_a)从5.7222下降到5.0556; 平均有效等位基因数(N_e)从3.2551下降到3.1461; 平均观测杂合度(H_o)从0.6975下降到0.5407; 平均期望杂合度(H_e)从0.6422下降到0.6235; 多态信息含量(PIC)从0.5784下降到0.5609。CF₁到CF₃的遗传参数是逐渐下降, 遗传多样性逐渐降低, 但群体间遗传多样性仍较高。长丰鲢子代间F_st在0.0160—0.0315, 表明其群体已出现了遗传分化, 但分化程度较低。长丰鲢各世代间遗传距离逐渐增加, 遗传相似度逐渐减小。研究表明经过连续3代利用, 长丰鲢CF₁到CF₃的遗传结构发生了改变, 遗传多样性呈下降趋势, 但遗传多样性水平仍较高。研究结果为长丰鲢进一步优良性状的维持提供了依据。     

ADP binding and ATP synthesis by reconstituted H-ATPase from chloroplasts

The H⁺-ATPase from chloroplasts, CF₀F₁, was isolated, purified and reconstituted into asolectin liposomes. The enzyme was brought either into the oxidized state or into the reduced state, and the rate of ATP synthesis was measured after energisation of the proteoliposomes with an acid—base transition ΔpH (pH_in = 5.0, pH_out = 8.5) and a K⁺/valinomycin diffusion potential, Δφ (K⁺_in = 0.6 mM, K⁺_out = 60 mM). A rate of 250 s⁻¹ was observed with the reduced enzyme (85 s⁻¹ in the absence of Δφ). A rate of 50 s⁻¹ was observed with the oxidized enzyme under the same conditions (15 s⁻¹ in the absence of Δφ). The reconstituted enzyme contained 2 ATP_bound per CF₀F₁ and 1 ADP_bound per CF₀F₁. Upon energisation the enzyme was activated and 0.9 ADP per CF₀F₁, was released. Binding of ADP to the active reduced enzyme was observed under different conditions. In the absence of phosphate the rate constant for ADP binding was 10⁵ M⁻¹·s⁻¹ under energized and de-energized conditions. In the presence of phosphate the rate of ADP binding drastically increased under energized conditions, and strongly decreased under de-energized conditions.     

The synthesis and reactivity of electrophilic iridium (III) complexes containing bis (diphenylphosphino) ethane

The complex Ir(CH₃) (CO) (CF₃SO₃)₂ (dppe) (1) has been synthesized from the reaction of Ir(CH₃)I₂(CO) (dppe) and silver triflate. Methane and IrH(CO) (CF₃SO₃)₂ (dppe) (2) are formed when a methylene chloride solution of 1 is placed under 760 torr dihydrogen. Conductivity studies indicate that methylene chloride solutions of complexes 1 and 2 are weak electrolytes and only partially ionized at concentrations above 1 mM. Complex 2 is an effective hydrogenation catalyst for ethylene and 1-hexene while acetone hydrogenation is inhibited by the formation of [IrH₂(HOCH(CH₃)₂) (CO) (dppe)] (OTf) (3). Linear dimerization and polymerization of styrene occurs via a carbocationic mechanism initiated by triflic acid elimination from 2. Treatment of an acetonitrile solution of Ir(CH₃)I₂(CO) (dppe) with silver hexafluorophosphate produces the solvent promoted carbonyl insertion product [Ir(C(O)CH₃) (NCCH₃)₃ (dppe)] [PF₆]₂ (7) which readily undergoes deinsertion in methylene chloride to form [Ir(CH₃) (CO) (NCCH₃)₂ (dppe)] [PF₆]₂ (8) and acetonitrile.     

Ruthenium(III) maltolato-nitroimidazole complexes: synthesis and biological activity

The Ru(III) metronidazole-maltolato and -ethylmaltolato complexes, trans-[RuL₂(metro)₂]CF₃SO₃ (L = ma (1a) or etma (1b)), have been synthesized and tested for potential anti-tumour activity against the human breast cancer cell line MDA-MB-435S using a so-called MTT assay in phosphate-buffered saline; ma = 3-hydroxy-2-methylpyran-4-onato, etma = 2-ethyl-3-hydroxypyran-4-onato, metro = 2-methyl-5-nitro-1H-imidazole-1-ethanol (metronidazole); MTT = 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide. The complexes exhibit lower IC₅₀ values than our previously reported Ru(III) tris-maltolato and -ethylmaltolato complexes [D.C. Kennedy, A. Wu, B.O. Patrick, B.R. James, Inorg. Chem. 44 (2005) 6529–6535]. An improved synthetic route to the 2-nitroimidazole EF5 (2-(2-nitro-1-H-imidazol-1-yl)-N-(2,2,3,3,3-pentafluoropropyl)acetamide) is reported, as well as a related synthesis of a 3-nitro-1,2,4-triazole derivative of EF5, triF5 (2-(3-nitro-1-H-triazol-1-yl)-N-(2,2,3,3,3- pentafluoropropyl)acetamide). The complexes [RuL₂(EF5)₂]CF₃SO₃ (4a and 4b) and [Ru(ma)₂(triF5)₂]CF₃SO₃ (5) were prepared from the [RuL₂(EtOH)₂]CF₃SO₃ complexes (3a and 3b); IC₅₀ values for 3–5 are high. Data on the uptake of Ru by the cells are also reported. The complexes were characterized generally by all or some of the following methods: elemental analyses, NMR, IR and mass spectroscopies, conductivity, and cyclic voltammetry; complexes 1a and 1b were also analyzed by X-ray crystallography.     

The rate of ATP synthesis catalyzed by reconstituted CF0F1-liposomes: Dependence on ΔpH and Δψ

The kinetics of proton-transport coupled ATP synthesis in CF₀F₁ reconstituted into asolectin liposomes was investigated upon energization of the membrane by an artificially generated ΔpH and Δψ. With a rapid mixing system the rate of ATP synthesis was measured at short reaction times (under 200 ms) where all parameters (ΔpH, Δψ, substrate and product concentrations) remain practically constant at their initial values. The rate of ATP synthesis depends, in a sigmoidal way, on ΔpH, the maximal rate being 200 ATP per CF₀F₁ per s. At constant ΔpH, an additional diffusion potential increases the rate until the maximal rate is reached.     

Mono-η complexes of chromium(II) and chromium(0). Electron demanding substituents, structural and spectroscopic data comparisons

Using thermal and photochemical methods a series of new chromium complexes has been prepared: (ν⁶-p-C₆H₄F₂)Cr(CO)₃; (ν⁶-C₆H₅CF₃)Cr(CO)₃; [m-C₆H₄(CF₃)₂]Cr(CO)₃; (ν⁶-C₆H₅F)Cr(CO)₂H(SiCl₃); (ν⁶-C₆H₅F)Cr(CO)₂(SiCl₃)₂; (p-C₆H₄F₂)Cr(CO)₂-H(SiCl₃); (C₆H₅CF₃)Cr(CO)₂H(SiCl₃(p-C₆H₄F₂)Cr(CO)₂(SiCl₃)₂; C₆H₅CF₃)Cr(CO)₂(SiCl₃)₂; [m-C₆H₄(CF₃)₂]Cr(CO)₂-H(SiCl₃); [m-C₆H₄(CF₃)₂]Cr(CO)₂(SiCl₃)₂. Two compounds were structurally characterized by X-ray diffraction. These data combined with IR and ¹H NMR have allowed assessment of some of the electronic and steric effects. The Cr-arene bond is considerably longer in the Cr(II) derivatives than in the Cr(0) species. Also the Cr center, as might be expected, is less electron rich in the Cr(II) dicarbonyl disilyl derivatives. The ν⁶-p-C₆H₄F₂ ligands are slightly folded so that the C---F carbons are moved further away from the Cr center. Comparison of structural and electronic effects is made with a series of similar chromium compounds reported in the literature. These new (arene)Cr(II) derivatives possess more labile ν⁶-arene ligands, which promise a rich chemistry at the chromium center.     

Synthesis, spectroscopic properties and X-ray crystal structures of two dinuclear alkoxo-bridged copper(II) compounds with the ligand bis(1-methyl-2-benzimidazolyl) propane. A unique alkoxo-bridged Cu(II) dinuclear compound with an additional bidentate bridging triflate anion

Based on the new ligand bis(1-methyl-2-benzimidazolyl) propane (abbreviated as mtbz) several new copper(II) coordination compounds have been prepared and characterized structurally and spectroscopically. Two representative compounds, i.e. [Cu₂(mtbz)₂(CH₃)₂- (CF₃SO₃)](CF₃SO₃) (1) and [Cu₂(mtbz)₂(CH₃O)₂](ClO₄)₂ (4) were characterized structurally by X-ray diffraction. Crystal data for 1: monoclinic, space group P2₁/c, a=13.6585(5), B=39.981(3), C=20.919(1) Å, β=125.98(1)°, Z=8. Crystal data for 4: monoclinic, space group P2₁/c, a=13.115(2), B=9.523(2), C=17.908(4) Å, β=111.71(1)°, Z=2. Structures 1 and 4 each consist of a dinuclear unit with bridging methoxo groups and one ligand linked to each copper via an N atom. Structure 1 (which consists of two dinuclear, crystallographically independent, but chemically identical units) has the two copper atoms bridged by a triflate anion, providing each copper atom a square-pyramidal coordination, while the copper atoms in structure 4 have an almost a square-planar geometry. The Cu---Cu distances (Å) within the dinuclear units are: 1, 2.9775(13), 2.9751(13); 4, 2.9872(16); the Cu---O---Cu bridging angles (°) are: 1, 101.7(3), 101.7(3), 100.9(3), 102.1(3); 4, 103.2(2). The mid-IR section focused on the vibrations of the triflate anion reveals interesting results concerning the assignments of that anion related to the v_as(S---O) band. Characteristic Cu---O vibrations in the far-IR section were found at 386 and 230 cm⁻¹ for the methoxo-bridged and 454 and 332 cm⁻¹ for the ethoxo-bridged compounds. These dinuclear species are EPR silent, and only a weak signal of monomeric impurities is observed. They also show a diamagnetic behavior below room temperature.     

Hetero-polynuclear complexes containing bridging diphenylphosphino-alkenes and -alkynes. The crystal structure of an Rh2{μ−ν:ν−P(Ph2) (CH2)3C≡CR}Co2 complex

The phosphinoalkenes Ph₂P(CH₂)_nCH=CH₂ (n= 1, 2, 3) and phosphinoalkynes Ph₂P(CH₂)_n C≡CR (R = H, N = 2, 3; R = CH₃, N = 1) have been prepared and reacted with the dirhodium complex (η−C₅H₅)₂Rh₂(μ−CO) (μ−η²−CF₃C₂CF₃). Six new complexes of the type (ν−C₅H₅)₂(Rh₂(CO) (μ−η¹:η¹−CF₃C₂CF₃)L, where L is a P-coordinated phosphinoalkene, or phosphinoalkyne have been isolated and fully characterized; the carbonyl and phosphine ligands are predominantly trans on the Rh---Rh bond, but there is spectroscopic evidence that a small amount of the cis-isomer is formed also. Treatment of the dirhodium-phosphinoalkene complexes with (η−CH₃C₅H₄)Mn(CO)₂thf resulted in coordination of the manganese to the alkene function. The Rh₂---Mn complex [(η−C₅H₅)₂Rh₂(CO) (μ−η¹:η¹−CF₃C₂CF₃) {Ph₂P(CH₂)₃CH=CH₂} (η−CH₃C₅H₄)Mn(CO)₂] was fully characterized. Simi treatment of the dirhodium-phosphinoalkyne complexes with Co₂(CO)₈ resulted in the coordination of Co₂(CO)₆ to the alkyne function. The Rh₂---Co₂ complex [(η−C₅H₅)₂Rh₂(CO) (μ−η¹:η¹−CF₃C₂CF₃) {Ph₂PCH₂C≡CCH₃}Co₂(CO)₂], C₃₇H₂₅Co₂F₆O₇PRh₂, was fully characteriz spectroscopically, and the molecular structure of this complex was determined by a single crystal X-ray diffraction study. It is triclinic, space group (C_i¹, No. 2) with a = 18.454(6), B = 11.418(3), C = 10.124(3) Å, = 112.16(2), β = 102.34(3), γ = 91.62(3)°, Z = 2. Conventional R on |F| was 0.052 fo observed (I > 3σ(I)) reflections. The Rh₂ and Co₂ parts of the molecule are distinct, the carbonyl and phosphine are mutually trans on the Rh---Rh bond, and the orientations of the alkynes are parallel for Rh₂ and perpendicular for Co₂. Attempts to induce Rh₂Co₂ cluster formation were unsuccessful.