细胞色素C的电化学行为研究

本文评述了细胞色素Ｃ电化学研究的发展概况，重点介绍了细胞色素Ｃ在促进剂作用下的电化学行为，促进剂种类，影响促进作用的因素及促进机理。     

水溶性壳聚糖的制备与应用

水溶性壳聚糖的制备与应用赵文伟，于黎，钟晓光，张月芳，孙家珍（中国科学院长春应用化学研究所，长春１３００２２）壳聚糖（ｃｈｉｔｏｓａｎ，（１，４）－２－胺基－２－脱氧－β－Ｄ－葡聚糖）是由甲壳素（ｃｈｉｔｉｎ，（１，４）－２－乙酰胺基－２－２脱氧－β...     

细胞色素P－450单加氧酶的模拟──轴向配体在锰卟啉／亚碘酰苯催化环己烷加氧反应中的作用

细胞色素Ｐ－４５０单加氧酶的模拟──轴向配体在锰卟啉／亚碘酰苯催化环己烷加氧反应中的作用江淑萍，叶兴凯，吴越（中国科学院长春应用化学研究所，长春１３００２２）关键词环己烷，锰卟啉，轴向配体，氧化，单加氧酶目前，细胞色素Ｐ－４５０单加氧酶的模拟有两个途...     

细胞色素C在吡啶,聚吡啶修饰的金电极上的直接电化学

研究了细胞色素Ｃ在吡啶修饰的金电极上的电化学反应，结果表明，只具有一个功能团的吡啶分子和它的聚合物对细胞色素Ｃ电化学反应也有促进作用，讨论了影响促进剂促进作用的主要因素。     

维生素B1对细胞色素C电化学反应的影响

本文探讨了细胞色素Ｃ在维生素Ｂ１修饰金电极上的电化学反应，结果表明维生素Ｂ１是细胞色素Ｃ电化学反应很好的促进剂而且它的促进作用与金电极表面维生素Ｂ１分子数量相关。     

微多相聚氨酯大孔树脂吸附细胞色素c的研究

微多相聚氨酯大孔树脂吸附细胞色素ｃ的研究史林启＊何炳林（南开大学吸附分离功能高分子材料国家重点实验室、高分子化学研究所天津３０００７１）关键词微多相聚氨脂大孔树脂，细胞色素ｃ，吸附选择性１９９６－０７－１５收稿，１９９６－１０－２４修回国家自然科学基...     

促进剂分子中共轭π键对细胞色素电化学的影响

比较了具有单功能基团的共轭有机小分子噻吩和四氢噻吩对细胞色素ｃ直接电化学反应的促进作用，发现四氢噻吩不能加速细胞色素ｃ的直接电化学反应。而噻吩是一种很好的促进剂，表明噻吩分子中的共轭π键在加速细胞色素ｃ的电子传递过程中起着重要作用。     

细胞色素C电化学反应的静电作用模型

首次发现,简单的阴离子Ⅰ~-是细胞色素c电化学反应的良好促进剂。在碘离子修饰的金电极上能观察到细胞色素c的准可逆电化学反应。根据细胞色素c的结构特点和碘离子的吸附特性,提出了一个以静电作用为基础的细胞色素c的电化学反应的模型。     

几种促进剂存在下细胞色素C电子迁移过程的研究

报道了应用近年来发展的薄层光谱电化学技术,对几种促进剂（４,４＇－二硫基联吡啶、腺嘌呤、Ｌ－半胱氨酸）存在下细胞色素Ｃ电子迁移过程进行了探讨。     

含二羟基二苯酮的系列热致液晶共聚酯的合成和表征──Ⅲ．含4，4＇－二羟基二苯砜结构的共聚酯

含二羟基二苯酮的系列热致液晶共聚酯的合成和表征──Ⅲ．含４，４＇－二羟基二苯砜结构的共聚酯董德文，池振国，倪玉山，丁孟贤（中国科学院长春应用化学研究所长春１３００２２）陈玉（东北师范大学分析测试中心长春１３００２４）关键词４，４＇－二羟基二苯酮，热致...     

Determination of iodide in seawater and edible salt by microcolumn liquid chromatography with poly(ethylene glycol) stationary phase

An ion chromatography method for rapid and direct determination of iodide in seawater and edible salt is reported. Separation was achieved using a laboratory-made C30 packed column (100 mm x 0.32 mm i.d.) modified with poly(ethylene glycol) (PEG). Effects of eluent composition on retention behavior of inorganic anions have been investigated. Both cation and anion of the eluent affected the retention of analyte anions. The retention time of anions increased with increasing eluent concentration when lithium chloride, sodium chloride, potassium chloride, sodium sulfate, magnesium sulfate were used as the eluent, while it decreased with increasing eluent concentration when ammonium sulfate was used as the eluent. The detection limit for iodide obtained by injecting 0.2 microl of sample was 9 microg/l (S/N = 3). The present method was successfully applied to the rapid and direct determination of iodide in seawater and edible salt samples. Partition may be involved in the present separation mode.     

Modulation of direct electron transfer of cytochrome c by use of a molecularly imprinted thin film

We describe the preparation of a molecularly imprinted polymer film (MIP) on top of a self-assembled monolayer (SAM) of mercaptoundecanoic acid (MUA) on gold, where the template cytochrome c (cyt c) participates in direct electron transfer (DET) with the underlying electrode. To enable DET, a non-conductive polymer film is electrodeposited from an aqueous solution of scopoletin and cyt c on to the surface of a gold electrode previously modified with MUA. The electroactive surface concentration of cyt c was 0.5 pmol cm^?2. In the absence of the MUA layer, no cyt c DET was observed and the pseudo-peroxidatic activity of the scopoletin-entrapped protein, assessed via oxidation of Ampliflu red in the presence of hydrogen peroxide, was only 30 % of that for the MIP on MUA. This result indicates that electrostatic adsorption of cyt c by the MUA–SAM substantially increases the surface concentration of cyt c during the electrodeposition step, and is a prerequisite for the productive orientation required for DET. After template removal by treatment with sulfuric acid, rebinding of cyt c to the MUA–MIP-modified electrode occurred with an affinity constant of 100,000 mol^?1 L, a value three times higher than that determined by use of fluorescence titration for the interaction between scopoletin and cyt c in solution. The DET of cyt c in the presence of myoglobin, lysozyme, and bovine serum albumin (BSA) reveals that the MIP layer suppresses the effect of competing proteins.     

Determination of iodide in seawater samples by ion chromatography with chemically-bonded poly(ethylene glycol) stationary phase

An ion chromatographic method for the rapid and direct determination of iodide in seawater is reported. Poly(ethylene glycol) (PEG) groups were chemically bonded onto silica gel or C30-bonded silica gel via diol groups. PEG-bonded C30 binary phases allowed determination of iodide in seawater samples without any interference. Effects of eluent composition on retention behavior of inorganic anions have been investigated. Both cation and anion of the eluent affected the retention of analyte anions. The retention time of anions increased with increasing eluent concentration. The detection limit for iodide obtained by injecting 0.2 microl of sample was 13 microg l(-1) (S/N=3) while the limit of quantitation was 43 microg l(-1) (S/N=10). The present method was successfully applied to the rapid and direct determination of iodide in seawater with long-term durability.     

Characterization of protein-attached conducting polymer monolayer

Cytochrome c (cyt c)-immobilized monolayers and multiple monolayers of a conducting polymer [poly(terthiophene-3-carboxylic acid) polymer (poly-TTCA)] were prepared, where the monolayer of monomer precursor was fabricated with the Langmuir-Blogett technique. Covalent immobilization of cyt c was achieved by the formation of an amide bond between the carboxylic groups of the conducting polymer and amines groups of lysine in cyt c. The monolayer of poly-TTCA and poly-TTCA/cyt c was characterized by cyclic voltammetry, XPS, EQCM, Auger electron spectra (AES), and atomic force microscopy (AFM). The immobilization of cyt c on the polymer layer reveals the direct electron-transfer processes of cyt c. Cyclic voltammetry of the poly-TTCA/cyt c-modified electrode showed a pair of reversible peaks at approximately +212/+201 mV (Epa/Epc) versus Ag/AgCl in a 0.2 M phosphate buffer solution (pH 7.0). The peak separation and the redox peak current of the poly-TTCA/cyt c-modified electrodes were gradually increased by increasing the number of poly-TTCA/cyt c layers on the electrode. The heterogeneous electron-transfer rate constant (ks) of cyt c at the poly-TTCA/cyt c-monolayer-modified electrode was estimated to be 0.874 s(-1). The method provides a novel route for the fabrication of protein (cyt c)-immobilized and/or lipid (palmitoyloleoylphosphatidic acid)-immobilized monolayers and multiple monolayers of a conducting polymer. Cyt c bonded on the conductive polymer layers was applied for bioelectronic devices with unique functionality.     

Weak interactions and molecular recognition in systems involving electron transfer proteins

Electrostatic interactions and other weak interactions between amino acid side chains on protein surfaces play important roles in molecular recognition, and the mechanism of their intermolecular interactions has gained much interest. We established that charged peptides are useful for investigating the molecular recognition character of proteins and their molecular interaction induced structural changes. Positively charged lysine peptides competitively inhibited electron transfer from reduced cytochrome f (cyt f or cytochrome c (cyt c) to oxidized plastocyanin (PC), due to neutralization of the negatively charged site of PC by formation of PC-lysine peptide complexes. Lysine peptides also inhibited electron transfer from cyt c to cytochrome c peroxidase. Likewise, negatively charged aspartic acid peptides interacted with the positively charged sites of cytfand cyt c, and competitively inhibited electron transfer from reduced cytfor cyt c to oxidized PC and from [Fe(CN)6]4- to oxidized cyt c. Changes in the geometry and a shift to a higher redox potential of the active site Cu of PC on oligolysine binding were detected by spectroscopic and electrochemical measurements, owing to the absence of absorption in the visible region for lysine peptides. Structural and redox potential changes were also observed for cyt f and cyt c by interaction with aspartic acid peptides.     

Studies on the electrochemical behavior of cytochrome c and its interaction with DNA at a Co/GC ion implantation modified electrode

The electrochemical behavior of cytochrome c (cyt c) and its interaction with DNA at a Co/glassy carbon (GC) ion implantation modified electrode were studied by linear sweep and cyclic voltammetry. In 0.005 mol dm(-3) Tris-0.05 mol dm(-3) NaCl buffer solution (pH = 7.10), a sensitive reduction derivative peak of cyt c was obtained by linear sweep voltammetry. The peak potential was 0.032 V (SCE). The peak current was proportional to the concentration of cyt c. The electrode process was quasi-reversible with adsorption. The electrode reaction rate constant k and the electron transfer coefficient a of cyt c were 4.42 s(-1) and 0.47, respectively. AES and XPS experiments showed that Co was implanted into the surface of the GC electrode (GCE). The implanted Co formed Co-C, which catalyzed the reduction of cyt c. The reaction of DNA with cyt c led to an electrochemically active complex, which resulted in an increase in the reduction current of cyt c. After adding DNA into the solution containing cyt c, the electrode process was still quasi-reversible with adsorption.     

Cytochrome c–dimyristoylphosphatidylglycerol interactions studied by asymmetrical flow field-flow fractionation

Lipid membranes are well recognized ligands that bind peripheral and integral proteins in a specific manner and regulate their function. Cytochrome c (cyt c) is one of the partner peripheral protein that binds to the lipid membranes via electrostatic and hydrophobic interactions. In this study, asymmetrical flow field-flow fractionation (AsFlFFF) was used to compare the interactions of cyt c with the acidic phospholipid 1,2-dimyristoyl-sn-glycero-3-phospho-rac-glycerol (DMPG), oleic acid (OA), and sodium dodecyl sulfate (SDS). The influence of pH and the cyt c–lipid molar mass ratios were evaluated by monitoring the diffusion coefficients and particle diameter distributions obtained for the free and lipid-bound protein. The hydrodynamic particle diameter of cyt c (pI 10) was 4.1 nm at pH 11.4 and around 4.2 nm at pH 7.0 and 8.0. Standard molar mass marker proteins were used for calibration to obtain the molar masses of free cyt c and its complexes with lipids. AsFlFFF revealed the binding of cyt c to DMPG and to OA to be mainly electrostatic. In the absence of electrostatic interactions, minor complex formation occurred, possibly due to the extended lipid anchorage involving the hydrophobic cavity of cyt c and the hydrocarbon chains of DMPG or SDS. The possibility of the formation of the molten globule state of cyt c, induced by the interaction between cyt c and lipids, is discussed.Electronic Supplementary Material Supplementary material is available for this article at     

Simultaneous determination of bromide and iodide ions by capillary isotachophoresis using quaternary ammonium salts

Bromide and iodide ions were determined simultaneously by capillary isotachophoresis using an aqueous electrolyte system; the separation principle was based on the ion-pairing equilibria between tetradecyldimethylbenzylammonium ion and these anions in the leading electrolyte. The interaction between iodide ion and tetradecyldimethylbenzylammonium ion was stronger than that for bromide ion. Thus complete separation of bromide and iodide ions could be obtained by using a leading electrolyte containing 1.5 mM tetradecyldimethylbenzylammonium ion. The pH of the leading electrolyte was adjusted to 5.0. The relative standard deviations of the zone length for bromide and iodide ions were 1.1 and 1.2%, respectively, when mixture of 3.0 mM of these ions was analysed. A 150-μl volume could be injected for the simultaneous determination of low concentrations of bromide and iodide ions.     

Direct electrochemistry of cytochrome c on nanotextured diamond surface

Nanotextured diamond surfaces with geometrical properties close to protein dimensions were used for the realization of direct electron transfer of cytochrome c (cyt c) without any covalent bonding. The peroxidase activity of native and denatured cyt c was also investigated. Cyclic voltammograms of native cyt c show quasi-reversible electron transfer reactions, while no heme redox activity is detected for denatured cyt c. Unfolding (denaturation) of cyt c can be achieved in the presence of hydrogen peroxide. Partially or fully denatured cyt c showed higher peroxidase activity than native cyt c. This is because denatured cyt c loses its tertiary structure and hydrogen peroxide is easier to access the heme redox center. The apparent Michaelis–Menten constant K_m for native and denatured cyt c has been determined to be 0.23 mM and 0.08 mM.     

Interactions of apo cytochrome C with alternating copolymers of maleic acid and alkene

Apo cytochrome c (apo cyt c) tends to aggregate at alkali pH. Poly(isobutylene-alt-maleic acid) (PIMA) is soluble molecularly, whereas poly(1-tetradecene-alt-maleic acid) (PTMA) forms particles that tend to dissociate by increasing pH and decreasing concentration. Dynamic light scattering and surface plasmon resonance are used to investigate the interactions of PIMA and PTMA with apo cyt c at different pH values to understand the mechanism of the interactions. When the positive or negative charges are in excess, the copolymer-protein complex particles can be stabilized by the charges on the surface. When the ratio of the positive to negative charges is close to the stoichiometric value, precipitation occurs. At pH 11.8, both PTMA and apo cyt c carry negative charges, but the hydrophobic interaction makes them form complexes. A competition exists between the interaction of the copolymer with apo cyt c and the self-aggregation of PTMA or apo cyt c alone. The interaction of PIMA or PTMA with apo cyt c at neutral and alkali pH destroys the aggregation of PTMA or apo cyt c and forms new complex particles.