鱼肝铁蛋白铁核表层接受电子能力的研究

采用直接电化学技术研究Hong鱼肝铁蛋白（Liver Ferritin of Dasyatis akajei,DALF）铁核表层接受还原电子的快慢速率和释放铁的动力学级数及规律。实验结果表明,在有氧环境下,DALF铁核表层以两相行为的方式快速地从铂金电极上获得还原电子且用于释放铁反应,其释放铁的还原电们分别为－125mV－375mV(vs.NHE,下同）。在控制还原电位为－200mV和－500mV的条件下,DALF铁核表层解放铁的速率分别为11．1Fe^3 /(DALF.min)和33．3Fe^3 (DALF.min）,因而认为DALF从铂金电极接受电子和解放铁的速率快慢与还原电位高低有关。血红素不仅能络合于DALF蛋白壳（DALFh）上,而且还能加速DALFh释放铁的速率,但无法增加DALFh释放铁的总量。DALF铁核结构中的磷铁组成存在着非均匀性。DALF铁核表层磷铁结构具有接受来自于蛋白壳电子隧道提供的还原电子能力。     

氧化HDL_2在大鼠肝窦状隙细胞内代谢

大鼠肝窦状隙细胞培养结果显示：氧化高密度脂蛋白２（ｏｘ－ＨＤＬ２）对异硫氰酸荧光素（ＦＩＴＣ）荧光标记ｏｘ－ＨＤＬ２的细胞结合有竞争抑制作用,而ＨＤＬ２则无。细胞内吞ＦＩＴＣ－ｏｘ－ＨＤＬ２的荧光强度（ＦＳ）和［３Ｈ］ＣＥ－ｏｘ－ＨＤＬ２（ｒ－ｏｘ－ＨＤＬ２）的放射强度分别是内吞ＦＩＴＣ－ＨＤＬ２的４５．５％和ｒＨＤＬ２的６１．４％。内吞ＦＳ主要存在于三氯醋酸（ＴＣＡ）沉淀部分,而放射强度主要存在于ＴＣＡ上清液部分。细胞释放的ＦＳ和放射活性分别是内吞量的６７．７％和１０．９％,且主要存在于ＴＣＡ可沉淀部分。结果提示：（１）大鼠肝窦状隙细胞可能存在着ｏｘ－ＨＤＬ受体,该受体不同于ＨＤＬ受体。（２）ｏｘ－ＨＤＬ２在细胞内代谢方式与ＨＤＬ２相似,均没有经历溶酶体分解途径。在细胞内载脂蛋白与胆固醇酯（ＣＥ）组分经历一个解离过程。细胞截留大部分ＣＥ后,将载脂蛋白（Ａｐｏ）与剩余ＣＥ重组成脂蛋白并以逆向胞饮方式释放到胞外。（３）氧化修饰减弱ＨＤＬ２逆向转运胆固醇能力     

杜氏盐藻细胞质膜氧化还原系统

杜氏盐藻细胞质膜具的氧化ＮＡＤ（Ｐ）Ｈ,还原Ｆｅ（ＣＮ）＾３－６和Ｏ２的氧化还原系统。当Ｆｅ（ＣＮ）＾３－６浓度为０．６ｍｍｏｌ／Ｌ,氧化ＮＡＤＨ的Ｋｍ为９６μｍｏｌ／Ｌ,Ｖｍａｘ为１５９ｎｍｏｌ１０＾－８ｃｅｌｌｓｍｉｎ＾－１,最适ｐＨ为８．５。ＴｒｉｔｏｎＸ－１００可促进ＮＡＤＨ和Ｆｅ（ＣＮ）＾３－６的氧化还原活性。ＮＡＤＨ能促进藻细胞的氧吸收,最适ｐＨ为８．５。在无外源电子供体存在时,细胞质     

杜氏盐藻细胞质膜氧化还原系统

杜氏盐藻细胞质膜具有氧化ＮＡＤ（Ｐ）Ｈ、还原Ｆｅ（ＣＮ）和Ｏ２的氧化还原系统。当Ｆｅ（ＣＮ）浓度为０．６ｍｍｏｌ／Ｌ时,氧化ＮＡＤＨ的Ｋｍ为９６μｍｏｌ／Ｌ,Ｔｍａｘ为１５９ｎｍｏｌ１０－８ｃｅｌｌｓｍｉｎ－１,最适ｐＨ为８．５。ＴｒｉｔｏｎＸ－１００可促进ＮＡＤＨ和Ｆｅ（ＣＮ）的氧化还原活性。ＮＡＤＨ能促进藻细胞的氧吸收,最适ＰＨ为８．５。在无外源电子供体存在时,细胞质电子供体提供的电子使Ｆｅ（ＣＮ）还原。培养液ＰＨ影响正常呼吸链、交替氧化酶途径和质膜电子传递链的耗氧比例;当有外源ＮＡＤＨ存在时,ＳＨＡＭ明显促进细胞的氧吸收,并且质膜电子传递链的耗氧比例增加。     

中国伞滑刃线虫属─新纪录（真滑刃目：寄生滑刃科）

中国伞滑刃线虫属─新纪录（真滑刃目：寄生滑刃科）ＴＨＥＮＥＷＲＥＣＯＲＤＯＦＢＵＲＳＡＰＨＥＬＥＮＣＨＵＳＦＲＯＭＣＨＩＮＡ（ＡＰＨＥＬＥＮＣＨＩＤＡ：ＰＡＲＡＳＩＴＡＰＨＥＬＥＮＣＨＩＤＡＥ）￥ＹＩＮＧａｎ－ｌｉｕ;ＦＡＮＧＹｕ－ｓｈｅｎｇ（Ｄｅｐ...     

水分胁迫对小麦根细胞质膜氧化还原系统的影响

水分胁迫使小麦根质膜ＮＡＤＨ和ＮＡＤＰＨ的氧化速率及Ｆｅ（ＣＮ）６＾３－和ＥＤＴＡ－Ｆｅ＾３＋的还原速率明显降低。对照与胁迫处理的质膜氧化还原系统活性均不受鱼藤酮、抗霉素Ａ和ＤＣＮ等呼吸链抑制剂的影响。在不加Ｆｅ（ＣＮ）６＾－３作为电子受体时,水杨基羟肟酸（ＳＨＡＭ）可明显刺激质膜ＮＡＤＨ的氧化和Ｏ２吸收速率。水分胁迫促使ＳＨＡＭ刺激的ＮＡＤＨ氧化明显降低,但却使Ｏ２吸收略有上升。     

L—山梨糖脱氢酶的纯化及性质的研究

从５Ｌ罐发酵Ｌ－山梨糖的Ｇｌｕｃｏｎｉｂａｃｔｅｒ ｏｘｙｄａｎｓ ＳＣＢ３２９和Ｂａｃｉｌｌｕｓ ｔｈｕｒｉｎｇｉｅｎｓｉｓ ＳＣＢ９３３混合菌株中差速离心收集ＳＣＢ３２９菌体,破碎,离心获得无细胞抽提液,硫酸铵分级沉淀蛋白后依次经ＤＥＡＥ Ｃｅｌｌｕｌｏｓｅ ５２和Ｑ Ｓｅｐｈａｒｏｓｅ ＦＦ柱层析分得到了Ｌ－册梨糖脱氢酶（ＳＤＨ）,它能将Ｌ－册梨糖脱氢氧化为Ｌ－册梨酮,ＳＤＳ－ＰＡＧＥ电泳测     

NMR法研究天花粉蛋白TDK肽片段的溶液构象

用ＨＮＭＲ法测定ＴＤＫ肽在Ｈ２Ｏ（ＨＯＤＫ）,５０％六氟丙醇（ＦＰＤＫ）和２ｍｏｌ／ＬＧｕ．ＨＣｌ（ＧＵＤＫ）溶液构象。在ＨＯＤＫ和ＦＰＤＫ中,ＴＤＫ肽的两段序列Ａｓｐ０－Ｉｌｅ４,Ｓｅｒ９－Ｉｌｉ１７分别具有较稳定的α－螺旋含量;而ＧＵＤＫ的ＳＡＬＳ序列仍能检测到有序残存结构。并假设ＳＡＬＳ序列是肽链形成二级结构的原始核心。     

水分胁迫对小麦根细胞质膜氧化还原系统的影响

水分胁迫使小麦根质膜ＮＡＤＨ和ＮＡＤＰＨ的氧化速率及Ｆｅ（ＣＮ）６３－和ＥＤＴＡ－Ｆｅ３＋的还原速率明显降低。对照与胁迫处理的质膜氧化还原系统活性均不受鱼藤酮抗霉素Ａ和ＫＣＮ等呼吸链抑制剂的影响。在不加Ｆｅ（ＣＮ）６３－作为电子受体时,水杨基羟肘酸（ＳＨＷ）可明显刺激质膜ＮＡＤＨ的氧化和Ｏ２吸收速率。水分胁迫促使ＳＨＡＭ刺激的ＮＡＤＨ氧化明显降低,但却使Ｏ２吸收略有上升。     

猕猴桃果实的生理生化特征

猕猴桃果实的生理生化特征魏玉凝,李曜东（中国科学院植物所,北京１０００４４）ＴＨＥＰＨＹＳＩＯＬＯＧＩＣＡＬＡＮＤＢＩＬＣＨＥＭＩＣＡＬＣＨＡＲＩＣＴＥＲＩＳＴＩＣＳＯＦＫＩＷＩＦＲＵＩＴ￥ＷｅｉＹｕ－ｎｉｎｇ;ＬｉＹａｏ－ｄｏｎｇ（Ｉｎｓｔｉｔｕｔ...     

Characteristics and Kinetics of Iron Releasefrom the Ferritin under the EGCG reduction

The mechanism of iron release from ferritin in vivo is still unclear even though it represents a key step of the metabolism of iron in vivo. Here, both interaction intensity and binding stability between epigallocatechin gallate (EGCG) from tea and liver ferritin of Dasyatis akajei (DALF) were investigated using UV–visible, fluorescence and circular dichroism (CD) spectrometry, respectively. The results indicated that EGCG could reduce the iron within the ferritin shell directly in the absence of chemical reducers such as Na₂S₂O₄, but this process was strictly pH-dependent, and the rate of iron release is faster at low pH than at high pH. The kinetic study of iron release showed that this process fitted the law of zero order reaction, which differed from that of first order reaction by various chemical reducers such as Vitamin C. In addition, Both fluorescence and CD spectrometry were further used to study the reduction mechanism of iron release in vitro, showing that there was a slight conformation change of the ferritin shell during EGCG reduction because of a complex formation of DALF–EGCG. It appears that chemical reducers with large molecular sizes reduce the iron across the protein shell by the way of an electron transfer pathway (ETP). A novel pathway for iron release from DALF with EGCG reduction is suggested to explain for a reductive route of iron metabolism by biological reducers in vivo.     

混合蛋白质体系中魟鱼和海兔肝铁蛋白释放铁的动力学研究

分别制备含有魟鱼肝铁蛋白(1iver ferritin of Dasyatis akajei,DALF)和海兔肝铁蛋白(Liver ferritin of Aplysia,ALF)的混合蛋白质体系。选用电子光谱技术和不同电子供体,研究在混合蛋白质体系中,DALF和ALF释放铁的动力学过程和规律。实验结果表明,采用Na2S2O4作为还原剂时,DALF以两相行为进行释放铁的反应;而选用抗坏血酸作为还原剂时,DALF却以一级反应动力学方式进行释放铁的反应,简化释放铁的过程。在混合蛋白质体系中且以抗坏血酸和Na2S2O4为电子供体时,ALF均以一级反应动力学过程进行释放铁的反应,认为某些蛋白质参与协助ALF释放铁反应,从而简化释放铁的过程。     

猪脾铁蛋白电子隧道特性及释放铁途径的研究

维生素Ｃ和连二亚硫酸钠混合后只能加速猪脾铁蛋白释放铁的速率,并不能使铁蛋白释放铁的动力学途径由复杂转化为简单．而单独维生素Ｃ却能利用蛋白壳上的电子隧道传递电子,迫使铁蛋白以二分之一的反应级数方式释放整体铁核的铁并起着抗磷酸盐阻遏释放铁速率的作用,简化释放铁的途径．对维生素Ｃ参与铁蛋白释放铁的机理进行了讨论．     

Purification,electrophoretic behavior,and kinetics of iron release of liver ferritin of Dasyatis akajei

From the liver of fish Dasyatis akajei, ferritin has been isolated by thermal denaturation and ammonium sulfate fractionation and then further purified by anion exchange chromatography and gel exclusion chromatography. The molecular weight of the liver ferritin of D. akajei (DALF) was measured to be 400 kDa by PAGE. Moreover, SDS-PAGE experimentation indicates that protein shell of DALF consists of the H and L subunits with molecular weight of 18 and 13 kDa, respectively. Using isoelectric focusing with pH ranging from 5.0 to 6.0, the ferritin purified by the PAGE exhibited three bands with different pI values in the gel slab. Diameters of the protein shell and iron core were also investigated by transmission electron microscope and determined to be 10–12 nm and 5–8 nm, respectively. A kinetic study of DALF reveals that the rate of self-regulation of the protein shell rather than the complex surface of the iron core plays an important role in forming a process for iron release with mixed orders.     

MALDI-TOF质谱技术研究铁蛋白蛋白壳表层的电荷分布

采用Sephacryl S-300排阻层析和DEAE－纤维素层析技术分离纯化Hong鱼肝铁蛋白（Liver ferritin of Dasyatis Akajei,DALF）。纯化后的DALF经梯度聚丙烯酰胺凝胶再次分离后,显示出两条凝胶事,即单分子DALF和双聚态DALF。选用基质辅助激光解吸离子化飞行时间质谱技术（MALDI－TOF MS）研究DALF的电荷分布时,发现DALF蛋白壳表层上显示出三种不同质荷比的分子离子峰,其质荷比为10369.41m/z、20710.33m/z和41809.43m/z。当DALF亚基被解离后,这三个分子离子峰随之消失,因而推测DALF蛋白壳表层存在着高密度正电荷区域,并与该蛋白形成非电惰性有着密切联系。通过拟出DALF蛋白壳表面电荷分布模型,进一步阐明DALF从铂电极上接受电子的机理。     

细菌铁蛋白氧化还原特性及电极活性的研究

棕色固氮菌细菌铁蛋白能直接快速地从金属铂电极上得到电子或提供电子给铂电极。经－６００ｍＶ（相对于ＮＨＥ）还原电位处理后,还原态细菌铁蛋白在可见光谱区中（３８０－５８０ｎｍ）所呈现的整体吸收光谱强度明显高于氧化态细菌铁蛋白的吸收光谱强度。经氯化钴处理后的细菌铁蛋白表现出较弱的电极活性及释放铁的速率明显下降。此外,细菌铁蛋白在体外模拟棕色固氮菌整体细胞内的微量氧环境体系中仍有氢还原现象,因而推测细菌铁蛋白在该菌体内也能进行吸氢反应。细菌铁蛋白是一种类似有吸氢氢酶功能的蛋白质     

Kinetics of iron release from pig spleen ferritin with bare platinum electrode reduction

Several anaerobic electrochemical cells were employed to study the kinetics of iron release from pig spleen ferritin (PSF) at a bare platinum electrode. Controlled potential microcoulometry (CPM) is the principal technology used to investigate the kinetics in the absence of a mediator. A kinetic study of iron release by microcoulometry has revealed that ferritin undergoes direct electron transfer at the electrode in the absence of a mediator, indicating that ferritin is an electroactive protein. Several experiments failed to show that alpha'alpha-bipyridyl has the capacity to reduce hydrolyzed Fe(3+) within the ferritin core after it has been reduced by the electrode at -600 mV vs. NHE in the absence of mediator. PSF is known to bind heme to generate a hemeoprotein, named pig spleen hemeoferritin (PSF(ho)). The rate of iron release is accelerated by the heme binding to PSF(ho) without the need for small mediators. Under similar conditions, two kinetic processes for iron release from PSF and bacterial ferritin of Azoaobacter vinelandii (AvBF) were studied and both fit a zero-order law. In addition, the rate of iron release in PSF can be accelerated two-fold by a specific reduction system consisting of ascorbic acid (AA) and the bare platinum electrode at -600 mV. However, this kinetic process does not follow zero-, half-, first, or second-order rate laws. A model is proposed to explain a mechanism of direct electron transfer between ferritin and the electrode is derived to describe the kinetics of iron release.     

马脾铁蛋白释放铁的反应级数和速率相数的转换

采用差示法研究铁蛋白释放铁的动力学规律和反应级数的转换。结果表明：马脾铁蛋白释放铁的速率及相数与还原剂Ｎａ２Ｓ２Ｏ４浓度及铁还原速率无关,与该蛋白蛋白壳的调节速率有关。在ｐＨ５．０￣６．０范围内,马脾铁蛋白以三相不同速率方式释放占原铁核总铁量８０％的铁。但在ｐＨ９．０介质中,ＯＨ＾－不仅能参与铁蛋白铁核组成,减缓释放铁的速率,而且使原混合级反应转换为一级反应,从而使铁蛋白释放铁的动力学过程由复杂转     

Reductive release of iron from ferritin by cation free radicals of paraquat and other bipyridyls

NADPH-cytochrome P-450 reductase-catalyzed reduction of paraquat promoted the release of iron from ferritin. Aerobically, iron release was inhibited approximately 60% by superoxide dismutase, whereas xanthine oxidase-dependent iron release was inhibited nearly 100%. This suggests that both superoxide and the paraquat cation radical can catalyze the release of iron from ferritin. Accordingly, under anaerobic conditions, the paraquat radical mediated a very rapid, complete release of iron from ferritin. Similarly, the cation free radicals of the closely related chemicals, diquat and benzyl viologen, also promoted iron release. ESR studies demonstrated that electron transfer from the paraquat cation radical to ferritin accounts for the reductive release of iron. The ferritin structure was not altered by exposure to the paraquat radical and also retained its ability to re-incorporate iron. These studies indicate that release of iron from ferritin may be a common feature contributing to free radical-mediated toxicities.