酵母羧甲基化及光照甘油醛-3-磷酸脱氢酶在碘化钾溶液中荧光发色团的形成

CM-GAPDH在碘化钾溶液中,NAD~+的存在下,形成发射波长为383nm的荧光物。对照的NAD~+与碘化钾溶液混合不产生荧光物。全位及半位修饰光照酶的内源荧光在碘化钾溶液中的变化与天然酶的有明显不同。两者在碘化钾中都形成383nm的荧光,但全位修饰光照酶形成383nm荧光的最适碘化钾浓度为1.0M;半位修饰的为0.8M。以上结果暗示:383nm荧光物的形成需要GAPDH和NAD~+同时存在,并且与活性部位巯基修饰的多少有关,该荧光物可能位于GAPDH的活性部位。     

酵母GAPDH在碘化钾溶液中荧光发色团的形成

酵母GAPDH的剩余活力在碘化钾为0.1M溶液中趋近于零,内源荧光在碘化钾为0.1—0.4M时迅速被淬灭,在0.5—2.0M时基本不变,3.0M时达到最低。并在一定浓度的碘化钾溶液中形成新的荧光发色性质(Ex336nm;Em383nm),量子产率大约为0.2,但形成该荧光发色团较为缓慢。与NAD荧光衍生物(Chen-LuTsou,etal.(1983)Biochem.Soc.Trans.11,425—429)不同的是,GAPDH在碘化钾溶液中形成荧光发色团时不需要光的激发。肌酸激酶及胰岛素不形成这种荧光衍生物。     

3-磷酸甘油醛脱氢酶的胍变性——全位与半位修饰酶的比较

酵母3-磷酸甘油醛脱氢酶在盐酸胍溶液中内源荧光及NAD荧光衍生物的410nm特征荧光发射光谱的变化结果提示,全位及半位修饰羧甲基酶活性部位与NAD共价连接的荧光衍生物的形成,明显受到盐酸胍的干扰,并且前者比后者更为显著.全位及半位修饰光照酶的特征荧光在低胍浓度下较内源荧光降低更为显著,同时伴有最大发射峰先红移后兰移的现象.NAD荧光衍生物的特征荧光在胍溶液中减弱的动力学过程分为快相和慢相,快相一级动力学常数比慢相的大两个数量级,全位及半位修饰酶的特征荧光的减弱快慢相速度常数分别属于同一个数量级.以上结果提示:酶活性部位的构象较整个分子来说更易被变性剂扰乱,柔性强于整个分子;NAD荧光衍生物的形成需要活性部位具有正确的空间几何结构.     

蛇肌甘油醛-3-磷酸脱氢酶的研究 Ⅲ.萤光衍生物的生成

蛇肌CM-Apo-GAPDH在NAD~ 存在的条件下,经紫外光照产生萤光衍生物。其校正发射光谱峰值在420nm,校正激发光谱呈三峰形,峰值在240nm、285nm、325nm。蛇肌GAPDH萤光衍生物生成的最适条件为:在pH7.6～8.0的缓冲液中光照8分钟,NAD~ 与酶克分子浓度的比值为60。用325nm激发、410nm发射的萤光滴定测NAD~ 与CM-GAPDH的结合,表明由于蛇肌GAPDH羧甲基化使NAD~ 与酶的结合所表现的负协同性变得弱得多。萤光衍生物A_(280)/A_(260)为1.61～1.63,相当于蛇肌GAPDH萤光衍生物每分子中的四个亚基含有二分子NAD~ ,蛇肌GAPDH萤光衍生物的生成也属于半位反应。     

蛇肌甘油醛-3-磷酸脱氢酶的研究——Ⅲ.萤光衍生物的生成

蛇肌CM-Apo-GAPDH在NAD~ 存在的条件下,经紫外光照产生萤光衍生物。其校正发射光谱峰值在420 nm,校正激发光谱呈三峰形,峰值在240 nm、285nm、325nm。蛇肌GAPDH 萤光衍生物生成的最适条件为:在pH7.6～8.0的缓冲液中光照8分钟,NAD~ 与酶克分子浓度的比值为60。用325nm 激发、410nm 发射的萤光滴定测NAD~ 与CM-GAPDH 的结合,表明由于蛇肌GAPDH 羧甲基化使NAD 与酶的结合所表现的负协同性变得弱得多。萤光衍生物A_(280)/A260为1.61～1.63,相当于蛇肌GAPDH 萤光衍生物每分子中的四个亚基含有二分子NAD~ ,蛇肌GAPDH 萤光衍生物的生成也属于半位反应。     

龙虾肌羧甲基甘油醛-3-磷酸脱氢酶NAD~+荧光衍生物的生成与性质

龙虾肌甘油醛-3-磷酸脱氢酶与兔肌酶一样,用碘代乙酸修饰后,在NAD~+存在下经紫外光照射也能形成荧光衍生物。 pH对荧光衍生物的生成和稳定性有很大影响,同时,异类离子的不同影响也很明显。 定磷分析法测定荧光衍生物上的NAD~+含量,同位素示踪法观察衍生物生成过程的脱羧,都证明此光化学反应为半位反应。     

邻苯二甲醛对糖基化3－磷酸甘油醛脱氢酶的修饰及荧光性质的研究

ＯＰＴ修饰ＧＡＰＤＨ及ｇＧＡＰＤＨ的荧光衍生物与Ｔｒｐ残基之间存在非辐射的能量传递。在不同浓度的ＧｕＨＣｌ溶液中,糖基化和非糖基化酶ＯＰＴ衍生物的荧光的变化具有一定的差异。特别是两者的荧光在碘化钾溶液中的淬来有明显的不同。ＯＰＴ修饰动力学研究表明,ｇＧＡＰＤＨ的修饰速度快于ＧＡＰＤＨ的修饰速度。以上结果提示：糖基化的位点可能在赖氨酸残基上,并且被糖基化的残基可能位于或靠近活性部位。     

龙虾肌甘油醛-3-磷酸脱氢酶及其衍生物与NAD~+的结合

平衡柱层析法测得每分子龙虾肌羧甲基化甘油醛-3磷酸脱氢酶能结合3.9分子NAD~+,而每分子光照酶则只能结合2分子NAD~+。 由蛋白荧光淬灭法得到,在25℃、pH7.0的磷酸盐缓冲液中,全酶、羧甲基酶及光照酶与NAD~+结合时均呈负协同性。     

蛇肌甘油醛-3-磷酸脱氢酶的研究 Ⅰ.纯化和一些基本性质

用硫酸铵分级、DEAE-纤维素柱层析、羧甲基纤维素柱层析分离和纯化了蛇肌GAPDH。聚丙烯酰胺凝胶电泳和醋酸纤维素薄膜电泳均为一条带。用此法提纯的蛇肌GAPDH A_(280)/A_(260)为2.1,是Apo-GAPDH。在纯化的Apo-GAPDH中加入NAD~ 能够得到结晶。Sephadex G-150凝胶过滤法测得蛇肌GAPDH的分子量约为150,000。十二烷基硫酸钠凝胶电泳也为一条带,亚基分子量约为38,000。表明蛇肌GAPDH是由相同的四个亚基组成的。用Ferdinand法测得比活为100。蛇肌GAPDH的N-末端氨基酸为缬氨酸。每分子含巯基数、色氨酸和酪氨酸残基数分别为12、12和36。重量法测得蛇肌Apo-GAPDH消光系数E_(280)~(0.1%)为0.775;Holo-GAPDH的消光系数E_(280)~(0.1%)为1.02。蛇肌GAPDH对甘油醛-3-磷酸的米氏常数为1.67×10~(-3)M,对NAD~ 的米氏常数为1.11×10~(-4)M。NAD~ 与蛇肌Apo-GAPDH结合后有Racker带,每分子蛇肌GAPDH可结合4分子NAD~ ,酶与NAD~ 的结合表现为负协同性。蛇肌GAPDH的圆二色谱,近紫外区Apo-GAPDH在285nm处有一负峰,292nm、270nm处有肩。加入NAD~ 后负峰变大并且蓝移。NAD~ 的加入似乎影响了酪氨酸所处的微环境。远紫外区Apo-GAPDH在220nm处有一负峰,208nm处有一个肩;加入NAD~ 后,负峰值稍稍变大,但峰的位置和形状未变。表明蛇肌GAPDH中,含较多的β-折迭,较少的α-螺旋。NAD~ 的加入对二级结构影响不大。     

邻苯二甲醛对糖基化3－磷酸甘油醛脱氢酶的修饰及荧光性质的研究

ＯＰＴ修饰ＧＡＰＤＨ及ｇＧＡＰＤＨ的荧光衍生物与Ｔｒｐ残基之间存在非辐射的能量传递。在不同浓度的ＧｕＨＣｌ溶液中,糖基化和非糖基化酶ＯＰＴ衍生物的荧光的变化具有一定的差异。特别是两者的荧先在碘化钾溶液中的淬灭有明显的不同。ＯＰＴ修饰动力学研究表明,ｇＧＡＰＤＨ的修饰速度快于ＧＡＰＤＨ的修饰速度。以上结果提示：糖基化的位点可能在赖氨酸残基上,并且被糖基化的残基可能位于或靠近活性部位。     

Subunit interactions in rabbit-muscle glyceraldehyde-phosphate dehydrogenase, as measured by NAD+ and NADH binding.

1. The binding parameters for NADH and NAD+ to rabbit-muscle glyceraldehyde-phosphate dehydrogenase (D-glyceraldehyde-3-phosphate:NAD+ oxidoreductase (phosphorylating), EC 1.2.1.12) have been measured by quenching of the flourescence of the protein and the NADH. 2. The fact that the degree of protein fluorescence quenching by bound NAD+ or NADH, excited at 285 nm and measured at 340 nm ('blue' tryptophans), is not linearly related to the saturation functions of these nucleotides, leads to a slight overestimation of the interaction energy and an underestimation of the concentration of sites, if linearity is assumed. 3. This is also the case for NADH, but not for NAD+, when the protein fluorescence is excited at 305 nm and measured at 390 nm ('red' tryptophans). 4. The binding of NAD+ can be described by a model in which the binding of NAD+, via negative interactions within the dimer, induces weaker binding sites, with the result that the microscopic dissociation constant is 0.08 microM at low saturation and 0.18 microM for the holoenzyme. 5. The binding of NADH can be described on the basis of the same model, the dissociation constant at low saturation being 0.5 microM and of the holoenzyme 1.0 microM. 6. The fluorescence of bound NADH is not sensitive to the conformational changes that cause the decrease in affinity of bound NAD+ or NADH. 7. The binding of NAD+ to the 3-phosphoglyceroyl enzyme can be described by a dissociation constant that is at least two orders of magnitude greater than the dissociation constants of the unacylated enzyme. The affinity of NAD+ to this form of the enzyme is in agreement with the Ki calculated from product inhibition by NAD+ of the reductive dephosphorylation of 1,3-diphosphoglycerate.     

肽链及蛋白质N-末端羰酰荧光衍生物的形成

短肽及胰岛素的N-末端经Dixpn转氨后具有荧光发色性质,其激发与发射波长随肽链氨基酸残基的种类和数量的不同而有差异,其范围大约为Ex 312—333nm;Em 398—408nm;量子产率为0.020—0.03.荧光发色团的基本化学结构可能是N-末端α-羰酰基及其相连的酰胺基,并且N-末端第二及第三位氨基酸残基对其荧光性质有影响.在碱性溶液中(pH>9.0)它的荧光强度降低,但在NaCl溶液中随盐浓度的增加而增强.在不同浓度的CuHCl溶液中,羰酰三肽的荧光强度变化随其氨基酸残基的种类和构型的不同而有差异.以上结果提示;α-羰酰荧光衍生物可能作为蛋白及肽N-末端的荧光探剂,可能成为研究蛋白和肽结构与功能的一种手段.     

Specific interactions of 3-phosphoglyceroyl-glyceraldehyde-3-phosphate dehydrogenase with coenzymes.

The binding of oxidized and reduced coenzyme (NAD+ and NADH) to 3-phosphoglyceroyl-glyceraldehyde-3-phosphate dehydrogenase has been studied spectrophotometrically and fluorimetrically. The binding of NAD+ to the acylated sturgeon enzyme is characterized by a significant quenching of the enzyme fluorescence (about 25%) and the induction of a difference spectrum in the ultraviolet absorbance region of the enzyme. Both of these spectroscopic properties are quantitatively distinguishable from those of the corresponding binary enzyme-NAD+ complex. Binding isotherms estimated by gel filtration of the acylated enzyme are in close agreement to those obtained by spectrophotometric and fluorimetric titrations. Up to four NAD+ molecules are bound to the enzyme tetramer. No anticooperativity can be detected in the binding of oxidized coenzyme, which is well described on the basis of a single class of four binding sites with a dissociation constant of 25 muM at 10 degrees C, pH 7.0. The binding of NADH to the acylenzyme has been characterized spectrophotometrically. The absorption band of the dihydronicotinamide moiety of the coenzyme is blue-shifted to 335 nm with respect to free NADH. In addition, a large hypochromicity (23%) is observed together with a significant increase of the bandwidth at half height of this absorption band. This last property is specific to the acylenzyme-DADH complex, since it disappears upon arsenolysis of the acylenzyme. The binding affinity of NADH to the acylated enzyme has been estimated by performing simultaneous spectrophotometric and fluorimetric titrations of the NADH appearance upon addition of NAD+ to a mixture of enzyme and excess glyceraldehyde 3-phosphate. In contrast to NAD+, the reduced coenzyme NADH appears to be relatively strongly bound to the acylated enzyme, the dissociation constant of the acylenzyme-NADH complex being estimated as 2.0 muM at 25 degrees C. In addition a large quenching of the NADH fluorescence (about 83%) is observed. The comparison of the dissociation constants of the coenzyme-acylenzyme complexes and the corresponding Michaelis constants suggests a reaction mechanism of the enzyme in which significant formation and dissociation of NAD+-acylenzyme and NADH-acylenzyme complexes occur. Under physiological conditions the activity of the enzyme can be regulated by the ratio of oxidized and reduced coenzymes. Possible reasons for the lack of anticooperativity in coenzyme binding to the acylated form of the enzyme are discussed.     

The role of nicotinamide adenine dinucleotide in the inhibition of bovine liver S-adenosylhomocysteine hydrolase by neplanocin A

Neoplanocin A, a cyclopentenyl analog of adenosine, has been shown recently to be a tight binding inhibitor of S-adenosylhomocysteine (AdoHcy) hydrolase (EC 3.3.1.1), exhibiting a stoichiometry of one molecule of inhibitor per molecule of the enzyme tetramer (Borchardt, R. T., Keller, B. T., and Patel-Thombre, U. (1984) J. Biol. Chem. 259, 4353-4358). In the present study a detailed analysis was performed of the possible role of the enzyme-bound NAD+ in the inactivation of AdoHcy hydrolase by neplanocin A. The NAD+/NADH content was quantitated using a fluorescence technique. The native enzyme showed intrinsic fluorescence with an emission maximum at 460 nm when excited at 340 nm, partially due to NADH bound to the enzyme. It was found that the content of NAD+ and NADH in freshly prepared, native enzyme is equal, having a stoichiometry of two nucleotides per enzyme molecule (tetramer). In addition, it was observed that the enzymatic activity of the native enzyme can be increased by about 30% following preincubation with NAD+. Furthermore, it was demonstrated that the mechanism of inhibition of AdoHcy hydrolase by neplanocin A involves the reduction of enzymatically bound NAD+ to NADH. Catalytic activity of the inactivated enzyme could be fully recovered in a time-dependent manner by further incubation with NAD+ (but not NADH). It was also found that inhibition by neplanocin A does not involve dissociation of the bound NAD+ or NADH from the enzyme, but simply reduction of the NAD+ to NADH.     

肽链及蛋白质N-末端喹喔啉类荧光衍生物的形成

蛋白质及肽链N-末端经Dixon转氨后的羰酰基与邻苯二胺作用可形成喹喔啉类荧光衍生物.形成这一发色团的过程较为缓慢;喹喔啉短肽的激发(Ex 293-305nm)与发射(Em 360-365nm)波长随肽链氨基酸残基组成不同而有一定变化;喹喔啉胰岛素荧光衍生物的激发光波长为Ex318nm,发射波长为Em 353nm.喹喔啉三肽的荧光在乙二醇溶液中的变化因其氨基酸残基组成的不同而有差异.以上结果提示:喹喔啉类荧光衍生物可能作为研究蛋白和肽结构与功能的一种手段.     

Demonstration and possible function of NADH:NAD+ transhydrogenase from ascaris muscle mitochondria.

Mitochondria from the muscle of Ascaris lumbricoides var. suis function anaerobically. NADH is generated in the intermembrane space as a consequence of the "malic" enzyme reaction. It has been suggested that this reducing equivalent in the form of hydride ion, would be translocated across the inner membrane in order to mediate ATP generation via the fumarate reductase reaction. In accord with this suggestion, intact Ascaris mitochondria showed appreciable NADH oxidase activity. Sonication resulted in an approximately 2-fold increase in NADH oxidase activity, whereas "malic" enzyme, fumarase, and NADH:NAD+ transhydrogenase activities increased approximately 7- to 14-fold, respectively. Phosphorylation capabilities and permeability toward pyridine nucleotides also indicated the intactness of the mitochondria. Ascaris mitochondria incubated anaerobically in the presence of fumarate, and [14C]NADH catalyzed a rapid reduction of the fumarate to succinate with the concomitant formation of equivalent quantities of extramitochondrial NAD+. However, very little isotope was recovered from the washed mitochondria, indicating the possibility of hydride ion translocation in the absence of nucleotide translocation. NADH:NAD+ transhydrogenase has been isolated from the muscle mitochondria of the intestinal nematode, Ascaris lumbricoides var. suis. The enzyme seems to have been solubilized from the mitochondrial membrane fraction by treatment with sodium deoxycholate followed by dialysis and subsequent adsorption by and elution from alumina C gamma. No NADPH:NAD+ transhydrogenase activity was detectable, making the Ascaris system unique over others reported. Activity was protected by L-cysteine, reduced glutathione and dithioerythritol, but strongly inhibited by low concentrations of p-chloromercuribenzoate or silver nitrate. The thionicotinamide derivative of NAD+ (thioNAD+) was employed to accept hydride ions from NADH in order to assay spectrophotometrically at 398 nm. Apparent Km values for thioNAD+ and NADH were 1 X 10(-4) M and 8 X 10(-6) M, respectively. That the physiological nucleotide, could act as hydride ion acceptor from NADH was indicated by the findings that NAD+ competitively inhibited the reduction of thioNAD+ when assayed at 398 nm. The additional finding of a noncompetitive inhibition between NAD+ and NADH suggested at least two binding sites on the enzyme, one for NADH and another common site for NAD+ and thioNAD+. More conclusive evidence indicating the participation of NAD+ as acceptor was obtained by incubation of the enzyme with NADH and [14C]NAD+ and demonstrating a rapid formation of [14C]NADH. These findings, in conjunction with those discussed above, suggest a physiological function of this enzyme in hydride ion translocation.