苹果酸脱氢酶的结构及功能

苹果酸脱氢酶（MDH）可以催化苹果酸与草酰乙酸间的可逆转换,主要参与TCA循环、光合作用、C4循环等代谢途径。苹果酸脱氢酶可分为NAD-依赖性的MDFI（NAD—MDH）和NADP-依赖性的MDH（NADP—MDH）。在所有真核生物和大部分细菌中,MDH通常形成同源二聚体,在少数细菌中为四聚体。不同来源的MDH催化机制和它们的动力学性质十分类似,显示了它们具有高度的结构相似性。MDH的功能多样,包括线粒体中的能量提供和植物的活性氧代谢等。回顾了苹果酸脱氢酶在生理学、医学、农学领域的研究进展,并针对其生化特性、空间结构特点、催化机理等生物学功能的分子生物学进展进行了综述。     

番茄苹果酸脱氢酶同工酶分析

植物细胞内存在着苹果酸脱氢酶(MDH)的同工酶,催化苹果酶草酰乙酸反应。目前认为,MDH同工酶存在于不同的亚细胞结构中,参与不同的代谢途径。细胞质中的可溶性MDH与丙酮酸羧化支路相联系,与非自养性的二氧化碳固定有关;线粒体中的MDH催化三羧酸循环的一个步骤;微体中的MDH则与光呼吸或乙醛酸循环有关;而叶绿体中的MDH(其辅酶是NADP)和光合作用有关。可见MDH与植物生理代谢的多条重要途径密切相关。因此,分析MDH同工酶对于探讨植物的正常生理和病理是必要的。菠菜、玉米、小麦等植     

CO2／盐冲击对小麦幼苗呼吸酶活性的影响

以不同抗盐小麦 (Triticum aestivum L.)为材料 ,研究了 CO2 /盐冲击对幼苗生长状况、叶绿素含量、光呼吸和三羧酸循环 (TCAC)关键酶活性的影响。结果表明 :Na Cl抑制小麦生长 ,而 CO2 促进生长 ,这种效应盐处理植株比非盐处理植株明显 ;Na Cl降低叶绿素含量 ,CO2 可使其轻微提高 ;盐对普通小麦TCAC中的异柠檬酸脱氢酶 (IDH)、琥珀酸脱氢酶 (SDH)、苹果酸脱氢酶 (MDH)和光呼吸中的乙醇酸氧化酶 (GO)、羟基丙酮酸还原酶 (HPR)有刺激作用 ,CO2 则抑制它们的活性。抗盐小麦对 CO2 /盐冲击的反应与普通小麦有差别。结果可以说明 ,CO2 能够减轻 Na Cl对植物的毒害效应     

偶联法测定PEPCase活性时OAA非酶催化脱羧引起的误差及其在一定范围内的校正

PEPCase(EC4.1.1.31)广泛存在于植物与微生物中。自1953年被发现以来,尤其是近10年,作为C_4双羧酸途径和景天科植物酸代谢途径的关键酶,PEPCase得到了广泛的研究。在这些研究中人们主要应用了4种活性测定方法:1.苹果酸脱氢酶(EC1.1.1.37,简称MDH)偶联测定法;2.H~(14)CO_3~-放射化学测定法;3.草酰乙酸检     

深黄被孢霉苹果酸脱氢酶基因的克隆和表达

目的通过对深黄被孢霉(Mortierella isabellina)M6-22中MDH基因的分离鉴定,为深入了解苹果酸脱氢酶(MDH)的生理特性、结构和功能奠定基础,并进一步探讨生物体中MDH的代谢作用。方法通过基因克隆的方法以深黄被孢霉的cDNA为模板,PCR扩增获得苹果酸脱氢酶基因MIMDH1。结果测序结果显示该序列长990bp,分别编码329个氨基酸。序列分析表明该序列与瓜笄霉菌(Choanephora cucurbitarum)MDH的相同性高达77%。将MIMDH1片段连接到表达载体pET32a(+)中构建重组表达质粒pET32aMIMDH1并转化至大肠埃希菌BL21中诱导表达,SDS-PAGE电泳检测在50kD左右有一条蛋白表达条带,经镍柱亲和层析纯化和酶活分析结果显示所纯化的重组蛋白酶活高达379.28U/mg。结论克隆的cDNA序列MIMDH1是一个新的苹果酸脱氢酶基因,所编码的蛋白具有MDH的活性。     

GA3处理对低温胁迫条件下玉米种子呼吸代谢的影响

以低温敏感型的"丰禾1号"和耐低温型的"郑单958"两个玉米品种为实验材料,采用GA3浸种的处理方式("丰禾1号"为20 mg·L-1、"郑单958"为5 mg·L-1),探究了GA3对低温胁迫条件下玉米种子萌发过程中种胚中可溶性糖和可溶性蛋白含量及淀粉酶活性和呼吸途径关键酶活性的影响。结果表明:低温胁迫条件下,GA3浸种处理显著提升了玉米种胚中可溶性糖含量及可溶性蛋白的积累,增强了低温胁迫下细胞的渗透势;α-淀粉酶、β-淀粉酶和总淀粉酶活性显著提高;提高了苹果酸脱氢酶(MDH)、丙酮酸激酶(PK)、联合酶(G-6-PDH和6-PGDH)的活性,提高了糖酵解(EMP)、三羧酸循环(TCA)、磷酸戊糖途径(PPP)途径的运转效率,保证了细胞的物质代谢和能量供应;GA3浸种处理可以显著提高种子对低温的抵抗能力,从而在低温胁迫条件下促进其萌发。     

细胞质雄性不育水稻幼穗和花药的呼吸酶活性研究

研究珍汕97A和珍汕97B的雌雄蕊原基形成期、花粉母细胞形成期和花粉母细胞减数分裂期的幼穗及单核期、二核期和三核期的花药中呼吸代谢三羧酸循环（TCA）的苹果酸脱氢酶（MDH）和异柠檬酸脱氢酶（IDH）及戊糖途径（PPP）的磷酸葡萄糖脱氢酶（G6PDH）、磷酸葡萄糖酸脱氢酶（6PGDH）和5一磷酸核糖异构酶（RSPI）的活性。结果表明：可育花药的5种酶活性皆高于同期不育花药;而幼穗中,TCA途径中的MDH和IDH在不育系与保持系之间无差异,PPP途径的G6PDH和6PGDH及R5PI则保持系高于不育系。这说明不育系中PPP发生的变化早于TCA途径,PPP途径的改变可能与小孢子败育有着更为直接的关系。     

藏羚羊骨骼肌肌红蛋白含量及乳酸脱氢酶、苹果酸脱氢酶活力的研究

目的:探讨藏羚羊骨骼肌对低氧环境的适应机制。方法:以生活在同海拔高度(4 300 m)的藏绵羊和低海拔绵羊(1 800 m)为对照,用分光光度法测定三种动物骨骼肌中肌红蛋白(Mb)含量、乳酸(LA)含量,酶活力法测定三种动物骨骼肌中乳酸脱氢酶(LDH)和苹果酸脱氢酶(MDH)活力。结果:藏羚羊骨骼肌中Mb含量明显高于藏绵羊和低海拔绵羊(P<0.05),而藏绵羊和低海拔绵羊间无明显差异。LA含量和LDH活力明显低于藏绵羊和低海拔绵羊(P<0.05),而MDH活力及MDH/LDH比值显著高于藏绵羊和低海拔绵羊(P<0.05),藏绵羊和低海拔绵羊间无明显差异。结论:藏羚羊可能通过增加骨骼肌中Mb的含量,提高其在低氧环境获取氧的能力,且藏羚羊骨骼肌组织中有氧代谢比例高,这可能与肌肉中Mb含量较高有关,推测藏羚羊较高的Mb含量可能是其适应高原缺氧条件的分子基础之一。     

油菜素内酯对低氧胁迫黄瓜幼苗根系有氧呼吸同工酶表达的影响

探讨了24-表油菜素内酯(EBR)对低氧胁迫黄瓜幼苗根系有氧呼吸同工酶表达的影响.结果表明:低氧胁迫增强了异柠檬酸脱氢酶(IDH)、琥珀酸脱氢酶(SDH)、苹果酸脱氢酶(MDH)及苹果酸酶(ME)同工酶的表达,并产生了一些新的条带;低氧下施用10-3 mg·L-1的外源EBR处理后6、9d时IDH、MDH同工酶的表达分别比单纯低氧处理提高了52.8％、13.6％及39.1％、11.3％,ME同工酶的表达在处理3d时比单纯低氧处理提高了11.6％,SDH同工酶表达6、9d时则分别比单纯低氧处理下降了42.9％和36.1％.可见,低氧胁迫下营养液添加EBR可调节黄瓜根系IDH、SDH、MDH及ME同工酶的表达,进而有利于缓解低氧胁迫对黄瓜幼苗根系的伤害.     

过量表达苹果酸脱氢酶对大肠杆菌NZN111产丁二酸的影响

大肠杆菌NZN111是敲除了乳酸脱氢酶的编码基因 (ldhA) 和丙酮酸-甲酸裂解酶的编码基因 (pflB) 的工程菌,厌氧条件下由于辅酶NAD(H) 的不平衡导致其丧失了代谢葡萄糖的能力。构建了苹果酸脱氢酶的重组菌大肠杆菌NZN111/pTrc99a-mdh,在厌氧摇瓶发酵过程中通过0.3 mmol/L的IPTG诱导后重组菌的苹果酸脱氢酶 (Malate dehydrogenase,MDH) 酶活较出发菌株提高了14.8倍,NADH/NAD+的比例从0.64下降到0.26,同时NAD+和NADH浓度分别     

Malate plays a central role in plant nutrition

Malate occupies a central role in plant metabolism. Its importance in plant mineral nutrition is reflected by the role it plays in symbiotic nitrogen fixation, phosphorus acquisition, and aluminum tolerance. In nitrogen-fixing root nodules, malate is the primary substrate for bacteroid respiration, thus fueling nitrogenase. Malate also provides the carbon skeletons for assimilation of fixed nitrogen into amino acids. During phosphorus deficiency, malate is frequently secreted from roots to release unavailable forms of phosphorus. Malate is also involved with plant adaptation to aluminum toxicity. To define the genetic and biochemical regulation of malate formation in plant nutrition we have isolated and characterized genes involved in malate metabolism from nitrogen-fixing root nodules of alfalfa and those involved in organic acid excretion from phosphorus-deficient proteoid roots of white lupin. Moreover, we have overexpressed malate dehydrogenase in alfalfa in attempts to improve nutrient acquisition. This report is an overview of our efforts to understand and modify malate metabolism, particularly in the legumes alfalfa and white lupin.     

Malate Dehydrogenase Isoenzymes in Cotton Leaves of Different Ages

Malate dehydrogenase isoenzymes from the blades of different aged leaves of the cotton plant have been investigated. The total extractable malate dehydrogenase activity varied widely between leaves of different ages and different locations on the plant. Malate dehydrogenase zymograms developed from the extracts which contained significantly different levels of enzyme activity appear to indicate the presence of different groups of malate dehydrogenase isoenzymes in leaves of different ages. However, under appropriate conditions of polyacrylamide gel electrophoresis, the same number of malate dehydrogenase isoenzymes with the same relative mobilities were detected in all the leaves studied. These findings are discussed in relation to reports that malate dehydrogenase isoenzymes change with plant development or that they have different roles in the plant.     

Malate dehydrogenase in phototrophic purple bacteria: purification, molecular weight, and quaternary structure.

The citric acid cycle enzyme malate dehydrogenase was purified to homogeneity from the nonsulfur purple bacteria Rhodobacter capsulatus, Rhodospirillum rubrum, Rhodomicrobium vannielii, and Rhodocyclus purpureus. Malate dehydrogenase was purified from each species by either a single- or a two-step protocol: triazine dye affinity chromatography was the key step in purification of malate dehydrogenase in all cases. Purification of malate dehydrogenase resulted in a 130- to 240-fold increase in malate dehydrogenase specific activity, depending on the species, with recoveries ranging from 30 to 70%. Homogeneity of malate dehydrogenase preparations from the four organisms was determined by sodium dodecyl sulfate and nondenaturing polyacrylamide gel electrophoresis; a single protein band was observed in purified preparations by both techniques. The molecular weight of native malate dehydrogenases was determined by four independent methods and estimated to be in the range of 130,000 to 140,000 for the enzyme from R. capsulatus, R. rubrum, and R. vannielii and 57,000 for that from R. purpureus. It is concluded that malate dehydrogenase from R. capsulatus, R. rubrum, and R. vannielii is a tetramer composed of four identical subunits, while the enzyme from R. purpureus is a dimer composed of two identical subunits.     

Resistance of tropoelastin and elastin peptides to degradation by alpha 2-macroglobulin-protease complexes

When α-ketoglutarate is the substrate, malate is a considerably more effective inhibitor of glutamate dehydrogenase than glutamate, oxalacetate, aspartate, or glutarate. Malate is a considerably poorer inhibitor when glutamate is the substrate. Malate is competitive with α-ketoglutarate, uncompetitive with TPNH, and noncompetitive with glutamate. The above, plus the fact that malate is a considerably more potent inhibitor when TPNH rather than TPN is the coenzyme, indicates that malate is predominantly bound to the α-ketoglutarate site of the enzyme-TPNH complex and has a considerably lower affinity for the enzyme-TPN complex. Ligands which decrease binding of TPNH to the enzyme such as ADP and leucine markedly decrease inhibition by malate. Conversely, GTP, which increases binding of TPNH to the enzyme also enhances inhibition by malate. Malate also decreases interaction between mitochondrial aspartate aminotransferase and glutamate dehydrogenase. This effect of malate on enzyme-enzyme interaction is enhanced by DPNH and GTP which also increase inhibition of glutamate dehydrogenase by malate and is decreased by TPN, ADP, ATP, α-ketoglutarate, and leucine which decrease inhibition of glutamate dehydrogenase by malate. These results indicate that malate could decrease α-ketoglutarate utilization by inhibiting glutamate dehydrogenase and retarding transfer of α-ketoglutarate from the aminotransferase to glutamate dehydrogenase. These effects of malate would be most pronounced when the mitochondrial level of α-ketoglutarate is low and the level of malate and reduced pyridine nucleotide is high.     

Malate dehydrogenases from actinomycetes: structural comparison of Thermoactinomyces enzyme with other actinomycete and Bacillus enzymes.

Malate dehydrogenases from bacteria belonging to the genus Thermoactinomyces are tetrameric, like those from Bacillus spp., and exhibit a high degree of structural homology to Bacillus malate dehydrogenase as judged by immunological cross-reactivity. Malate dehydrogenases from other actinomycetes are dimers and do not cross-react with antibodies to Bacillus malate dehydrogenase.     

Identification of cytoplasmic nodule-associated forms of malate dehydrogenase involved in the symbiosis between Rhizobium leguminosarum and Pisum sativum

The malate dehydrogenase activity (EC 1.1.1.37), present in the cytoplasm of Pisum sativum root nodules, can be separated by ion-exchange chromatography into four different fractions. Malate dehydrogenase activity present in the cytoplasm of roots elutes mainly as a single peak. During nodule development an increase in malate dehydrogenase activity per gram of material was observed. This increase occurred concomitantly with the increase in nitrogenase activity. The kinetic properties of the separated malate dehydrogenases of root nodule cytoplasm and root cytoplasm were studied. The Km values for malate (2.6 mM), NAD+ (27 microM), oxaloacetate (18 microM) and NADH (13 microM) of the dominant form of the root nodule cytoplasm are much lower than those of the dominant malate dehydrogenase root form (64 mM, 4.4 mM, 89 microM and 70 microM respectively). Binding of malate by the enzyme-NADH complex from root nodules results in an abortive complex, thereby blocking the further reduction of oxaloacetate by NADH. The dominant root malate dehydrogenase does not form the abortive complex. From the kinetic data it is concluded, first, that the root nodule forms of the enzyme are capable of catalysing at a high rate the reduction of oxaloacetate, to meet the demands for malate governed by the bacteroid and the infected plant cell. The second conclusion, drawn from the kinetic data, is that under physiological conditions the conversion of oxaloacetate can be controlled just by the malate concentration. Consequently the major root nodule forms of malate dehydrogenase are able to allow a high flux of malate production from oxaloacetate but also to establish a sufficient oxaloacetate concentration necessary for the assimilation and transport of fixed nitrogen.     

Malate dehydrogenase isoenzymes from cotton leaves: molecular weights

Malate dehydrogenase isolated from leaves of the cotton plant (Gossypium hirsutum L.) appears in the form of several isoenzymes. Four of the isoenzymes found in cotton leaf extracts appear to be charge isomers with a molecular weight of approximately 60,000. A fifth malate dehydrogenase isoenzyme found in leaf extracts has a molecular weight of approximately 500,000. Under appropriate conditions it is possible to form this high molecular weight isoenzyme from at least one of the smaller isoenzymes. In addition, malate dehydrogenase isoenzymes of approximately 700,000 and 130,000 molecular weight have been observed under some conditions, although these isoenzymes do not appear in the crude cotton leaf preparations. The relationship of this heterogeneity with respect to size and to the discrepancies in the number and size of malate dehydrogenase isoenzymes reported from plant tissues may be significant.     

Malate dehydrogenase: a model for structure, evolution, and catalysis.

Malate dehydrogenases are widely distributed and alignment of the amino acid sequences show that the enzyme has diverged into 2 main phylogenetic groups. Multiple amino acid sequence alignments of malate dehydrogenases also show that there is a low degree of primary structural similarity, apart from in several positions crucial for nucleotide binding, catalysis, and the subunit interface. The 3-dimensional structures of several malate dehydrogenases are similar, despite their low amino acid sequence identity. The coenzyme specificity of malate dehydrogenase may be modulated by substitution of a single residue, as can the substrate specificity. The mechanism of catalysis of malate dehydrogenase is similar to that of lactate dehydrogenase, an enzyme with which it shares a similar 3-dimensional structure. Substitution of a single amino acid residue of a lactate dehydrogenase changes the enzyme specificity to that of a malate dehydrogenase, but a similar substitution in a malate dehydrogenase resulted in relaxation of the high degree of specificity for oxaloacetate. Knowledge of the 3-dimensional structures of malate and lactate dehydrogenases allows the redesign of enzymes by rational rather than random mutation and may have important commercial implications.     

Malate Dehydrogenase Mutants in Escherichia coli K-12

Mutants devoid of malate dehydrogenase activity have been isolated in Escherichia coli K-12. They do not possess detectable malate dehydrogenase when grown aerobically or anaerobically on glucose as sole carbon source. All mutants revert spontaneously; a few partial revertants have been found with a malate dehydrogenase exhibiting altered electrophoretic mobility. Therefore, only one such enzyme appears to exist in the strains examined. No evidence could be obtained for the presence of a malate dehydrogenase not linked to nicotinamide adenine dinucleotide. Mutants deficient in both malate dehydrogenase and phosphoenol pyruvate carboxylase activities will grow anaerobically on minimal glucose plus succinate medium; also, malate dehydrogenase mutants do not require succinate for anaerobic growth on glucose. The anaerobic pathway oxaloacetate to succinate or succinate to aspartate appears to be accomplished by aspartase. Malate dehydrogenase is coded for by a locus somewhere relatively near the histidine operon, i.e., a different chromosomal location than that known for other citric acid cycle enzymes.