高等植物果聚糖研究进展

果聚糖是高等植物重要的贮藏碳水化合物 ,因植物种类和发育阶段而异 ,主要存在 5种类型的结构 :线型菊糖型果聚糖、菊糖型果聚糖新生系列、线型梯牧草糖型果聚糖、混合型梯牧草糖型果聚糖和梯牧草糖型果聚糖新生系列。果聚糖的代谢模型随着代谢酶—蔗糖 :蔗糖果糖基转移酶、蔗糖 :果聚糖_6_果糖基转移酶、果聚糖 :果聚糖果糖基转移酶、果聚糖 :果聚糖_6_果糖基转移酶、果聚糖外水解酶等的发现、纯化和克隆日趋清晰。此外 ,果聚糖分子生物学研究也取得了一定的进展     

蔗糖:蔗糖-1-果糖基转移酶的表面展示及酶学性质分析

【目的】蔗糖:蔗糖-1-果糖基转移酶催化1分子蔗糖上的果糖基转移到另一个蔗糖分子上,形成1-蔗果三糖和葡萄糖。在低聚果糖中,1-蔗果三糖益生素活性最高。本研究将该酶展示在酵母菌细胞表面上,并用于1-蔗果三糖的制备。【方法】将来自莴苣的蔗糖:蔗糖-1-果糖基转移酶基因克隆到用于酵母细胞表面展示的表达载体上,并在解脂亚罗酵母菌中进行异源表达,表达的酶展示在该细胞表面上,然后以蔗糖为底物,研究表面展示的蔗糖:蔗糖-1-果糖基转移酶的性质。【结果】免疫荧光实验结果表明蔗糖:蔗糖-1-果糖基转移酶已展示在酵母菌的细胞表面上,高效液相色谱结果表明酵母表面展示的该酶具有转移酶的催化活性。该酶的最适作用温度、最适作用p H分别为45°C和7.5;该酶的催化活性受Zn2+和Cu2+的抑制,受Ca2+激活;该酶重复使用7次后,酶活下降50%。表面展示的蔗糖:蔗糖-1-果糖基转移酶和3%蔗糖混合后在40°C条件下孵育30 min后,所产1-蔗果三糖含量最高为20.8 mmol/L。【结论】蔗糖:蔗糖-1-果糖基转移酶在解脂亚罗酵母菌中得到成功表达,并展示在其细胞表面上,生化研究表明该重组蛋白具有果糖基转移酶活性,且催化蔗果三糖的生成。表面展示的蔗糖:蔗糖-1-果糖基转移酶作为一种全细胞催化剂能够用于1-蔗果三糖的制备。     

青春双岐杆菌中β-呋喃果糖苷酶的提纯和一些性质

双岐杆菌是革兰氏阳性、不产芽孢的厌氧菌,主要存在于人和一些动物的肠道中,具有阻止有害细菌滋生和感染的作用。双岐杆菌能选择性水解低聚果糖,而哺乳动物的消化酶不能水解低聚果糖。 微生物中的β—呋喃果糖苷酶可分为两类,一类为蔗糖酶,它能水解蔗糖但不水解菊糖;另一类为外菊糖酶(β-果糖苷酶),它不仅水解蔗糖也能水解菊糖,它们对蔗糖和菊糖的活性比相差甚大。有些青春双岐杆菌提取物水解1-蔗果三糖的速度比蔗糖和菊糖快,并能从1-蔗果三糖产生果糖和蔗糖。青春双岐杆菌G-1菌株的提取物对1-蔗果三糖的活性很高,当底物浓度各为5mM时,它对1-蔗果三     

黑曲霉QU10果糖基转移酶的克隆表达

微生物果糖基转移酶能够以蔗糖为底物产生低聚果糖。为获得更多新酶资源,通过PCR法成功地克隆出黑曲霉QU10的果糖基转移酶基因(Gen Bank Accession No.KF699529),基因片段长度为1 941 bp,包含一个54 bp的内含子。进一步利用RT-PCR法克隆了果糖基转移酶的c DNA,其编码628个氨基酸。将所得片段定向克隆到p ET-22b、p GAPZA及p GAPZαA载体,并转化至大肠杆菌或毕赤酵母中,通过筛选获得果糖基转移酶表达活力高的转化子。利用α信号肽的毕赤酵母转化子获得最高果糖基转移酶胞外酶活力为431 U/m L,是原始菌株酶活力的35倍。此毕赤酵母重组酶为同源二聚体,半天然PAGE表观分子量约200 k Da。以蔗糖为底物,果糖基转移酶在p H 5.0、45℃下反应4 h,酶解产物中主要是蔗果三糖和四糖,蔗果寡糖最高可占总质量的58%。结果表明,果糖基转移酶酵母工程菌具有很高的转果糖基的能力,而且表达活力高,具有潜在的工业应用价值。     

黑曲霉QU10果糖基转移酶的克隆表达（英文）

微生物果糖基转移酶能够以蔗糖为底物产生低聚果糖。为获得更多新酶资源,通过PCR法成功地克隆出黑曲霉QU10的果糖基转移酶基因(Gen Bank Accession No.KF699529),基因片段长度为1 941 bp,包含一个54 bp的内含子。进一步利用RT-PCR法克隆了果糖基转移酶的c DNA,其编码628个氨基酸。将所得片段定向克隆到p ET-22b、p GAPZA及p GAPZαA载体,并转化至大肠杆菌或毕赤酵母中,通过筛选获得果糖基转移酶表达活力高的转化子。利用α信号肽的毕赤酵母转化子获得最高果糖基转移酶胞外酶活力为431 U/m L,是原始菌株酶活力的35倍。此毕赤酵母重组酶为同源二聚体,半天然PAGE表观分子量约200 k Da。以蔗糖为底物,果糖基转移酶在p H 5.0、45℃下反应4 h,酶解产物中主要是蔗果三糖和四糖,蔗果寡糖最高可占总质量的58%。结果表明,果糖基转移酶酵母工程菌具有很高的转果糖基的能力,而且表达活力高,具有潜在的工业应用价值。     

小麦植株中可溶性糖纸层析定量方法

小麦、大麦、黑麦等作物以及某些单子叶和菊科植物的营养器官或貯藏器官中的可溶性糖类,除一般单糖(葡萄糖、果糖)双糖(蔗糖)外,还有大量果聚糖类存在,而且有时作为貯藏形式。它们的分子结构一端是蔗糖,蔗糖的果糖基通过2,1或2,6糖甙链连接着若干果糖基,形成一系列结构相似的寡糖或多糖,不具还原性。一般的分析方法不能分类测定。我们     

微生物菊糖酶及其在菊糖转化成果糖中的应用潜力

在自然界中,菊糖(inulin)是作为菊科和某些禾本科作物的贮藏物质而存在的。菊芋(Helianthus tuberosus L.)蒲公英(Taraxacum officinathus)、菊苣(Cichorium intybus)、大丽花(Dahlia pinnata)和牛蒡属植物(Arctium)等都是重要的菊糖来源。菊糖的化学本质是通过线性的β-2.1糖苷键连接的果聚糖。--菊糖分子的每一链长约25-30个果糖单位,末端连接一葡萄糖残基,分子量大约为3000-5000。菊糖的链长与分子量的大小因不同的植物、收获季节及作物的成熟程度等有关。     

Levan果聚糖的应用与生产研究进展

Levan是一类果聚糖,由大量的果糖单元以β-（2,6）果糖苷键连接构成聚糖主链并含有少量β-（2,1）果糖苷键连接的支链组成。部分微生物来源的Levan具有抗肿瘤、抗病毒、降血糖、降血脂、免疫增强等重要的生物活性,在医药和功能性食品方面具有巨大的应用潜能。微生物发酵液提取和酶法合成是目前大量获得Levan果聚糖的两种方法,其中微生物发酵液提取的Levan果聚糖产量和蔗糖转化率一般较低,且发酵液中同时存在的其他高聚物不利于Levan的规模化纯化;而利用Levan蔗糖酶以蔗糖为底物转果糖基合成的Levan果聚糖产量已经高达200g/L、蔗糖转化率高达50%,并且Levan蔗糖酶合成Levan过程中酶的活性受到pH值、温度、螯合剂、金属离子等多种因素的影响,可以通过控制反应条件促进多糖合成反应的进行。因此,酶法合成将是工业化获得Levan果聚糖的主要方式。     

果糖基转移酶及其固定化研究进展

果糖基转移酶能够催化蔗糖水解并通过转果糖基作用产生低聚果糖。本文综述了十几年来国内外对果糖基转移酶及其固定化研究的若干结果和进展。对该领域的发展趋势作了扼要的展望。     

低聚果糖及其制备的研究进展

果糖基转移酶能够催化蔗糖水解并通过转果糖基作用产生低聚果糖。本文综述了十几年来国内外对果糖基转移酶及其固定化研究的若干结果和进展。对该领域的发展趋势作扼要的展望。     

Fructan of the inulin neoseries is synthesized in transgenic chicory plants (Cichorium intybus L.) harbouring onion (Allium cepa L.) fructan:fructan 6G-fructosyltransferase

Fructan (polyfructosylsucrose) is an important storage carbohydrate in many plant families. fructan:fructan 6G-fructosyltransferase (6G-FFT) is a key enzyme in the formation of the inulin neoseries, a type of fructan accumulated by members of the Liliales. We have cloned the 6G-FFT from onion by screening a cDNA library using barley sucrose:fructan 6-fructosyltransferase (6-SFT) as a probe. The deduced amino acid sequence showed a high homology with plant invertases and 6-SFT. Incubation of protein extracts from transgenic tobacco plants with the trisaccharide 1-kestose and sucrose resulted in the formation of neokestose and fructans of the inulin neoseries with a degree of polymerization up to six. Introduction of the onion 6G-FFT into chicory resulted in the synthesis of fructan of the inulin neoseries, in addition to the synthesis of linear inulin.     

Kinetic behaviour and specificity of β-fructosidases in the hydrolysis of plant and microbial fructans

Fructosidases, in particular exo-β-fructosidases, may act on fructans such as inulins and levans of plant and bacterial origin to produce fructose. In this paper, the kinetic properties of a commercial preparation (Fructozyme L) and a recombinant exoinulinase (BfrA) from Thermotoga maritima, were studied using fructan polymer substrates from various sources. Both enzymatic preparations preferentially hydrolyzed β2-1 linkages and low molecular weight fructans. We show that chicory inulin is degraded most efficiently by both preparations, followed by bacterial inulin, in spite of its high molecular weight and branching in β2-6 positions. All bacterial levans were more slowly hydrolyzed. Michaelis–Menten kinetics describe the hydrolysis of sucrose and low molecular weight fructans (≤8.3 kDa) by both enzyme preparations, while first order kinetics were observed with respect to bacterial fructans due to the high molecular weight and, therefore, low molar concentrations. Comparison of second order rate constants indicates that bacterial inulin (Leuconostoc citreum CW28) is hydrolyzed more slowly with both enzyme preparations than chicory inulin by approximately one order of magnitude. For Leuconostoc mesenteroides NRRL B-512F levan, the second order rate constant for Fructozyme L is 200-fold lower than for chicory inulin. However, the second order rate constant for BfrA is only 22-fold lower than for chicory inulin. Taken together, our studies characterize the kinetics of fructan hydrolysis and also suggest that the kinetic parameters may be used to differentiate between fructan structures.     

Comparative studies of the degradation of grass fructan and inulin by strains of Lactobacillus paracasei subsp. paracasei and Lactobacillus plantarum

Four strains of Lactobacillus paracasei subsp. paracasei and Lact. plantarum are investigated within 16 d in order to determine the formation of metabolites during the degradation of grass fructan and inulin as well as the subsequent fermentation to lactic acid. The decrease of the total content of fructans throughout the entire time of investigation shows differences specific for strains as for either fructan substrate. The strain Lact. plantarum V 54/6 completely degrades the grass fructan and inulin within no longer than 13 d. The utilization of fructan by the other strains is temporally delayed, and in a smaller degree of degradation, especially remarkable for inulin cleavage. The structural modifications of decomposed fructans are characterized by a noticeable shift of the mean DP from approximately 80 to the oligomeric range analysed by anion exchange chromatography. Additionally, a newly formed series of peaks of oligomeric saccharides was detected during the degradation of grass fructan and inulin. Part of the fructose that is derived from cleavage of fructans is fermented immediately by the LAB strains into differently high amounts of lactic acid. The abundance of formed fructose is enriched in the medium to a varying extent, depending on the strain as well as the substrate used. From these results a number of fructan degradative enzymes in lactobacilli have been concluded to possibly vary their modes of regulation: strain specific exo- and endohydrolases with different activities against β-2,1 and β-2,6 linked fructan.     

Molecular characterization and expression of a cDNA encoding fructan:fructan 6G-fructosyltransferase from asparagus (Asparagus officinalis)

* Fructan:fructan 6G-fructosyltransferase (6G-FFT) catalyses a transfructosylation from fructooligosaccharides to C6 of the glucose residue of sucrose or fructooligosacchrides. In asparagus (Asparagus officinalis), 6G-FFT is important for the synthesis of inulin neoseries fructan. Here, we report the isolation and functional analysis of the gene encoding asparagus 6G-FFT. * A cDNA clone was isolated from asparagus cDNA library. Recombinant protein was produced by expression system of Pichia pastoris. To measure enzymatic activity, recombinant protein was incubated with sucrose, 1-kestose, 1-kestose and sucrose, or neokestose. The reaction products were detected by high performance anion-exchange chromatography. * The deduced amino acid sequence of isolated cDNA was similar to that of fructosyltransferases and vacuolar type invertases from plants. Recombinant protein mainly produced inulin neoseries fructan, such as 1F, 6G-di-beta-D-fructofuranosylsucrose and neokestose. * Recombinant protein demonstrates 6G-FFT activity, and slight fructan:fructan 1-fructosyltransferase (1-FFT) activity. The ratio of 6G-FFT activity to 1-FFT activity was calculated to be 13. The characteristics of the recombinant protein closely resemble those of the 6G-FFT from asparagus roots, except for a difference in accompanying 1-FFT activity.     

Fructan synthesis in transgenic tobacco and chicory plants expressing barley sucrose:fructan 6-fructosyltransferase

We have recently cloned a cDNA encoding sucrose:fructan 6-fructosyltransferase (6-SFT), a key enzyme of fructan synthesis forming the β-2,6 linkages typical of the grass fructans, graminans and phleins [Sprenger et al. (1995) Proc. Natl. Acad. Sci. USA 92, 11652–11656]. Here we report functional expression of 6-SFT from barley in transgenic tobacco and chicory. Transformants of tobacco, a plant naturally unable to form fructans, synthesized the trisaccharide kestose and a series of unbranched fructans of the phlein type (β-2,6 linkages). Transformants of chicory, a plant naturally producing only unbranched fructans of the inulin type (β-2,1 linkages), synthesized in addition branched fructans of the graminan type, particularly the tetrasaccharide bifurcose which is also a main fructan in barley leaves.     

Determination of the structure and degree of polymerisation of fructans from Echinacea purpurea roots

Highly water soluble fructans have been isolated from Echinacea purpurea (L.) Moench. roots by hot water extraction and precipitation at three different ethanol concentrations (80% v/v, 60% v/v and 40% v/v). The structure of the fructans has been characterised by three analytical methods: GC of silylated oxime derivatives and partially methylated alditol acetates, respectively, as well as 13C NMR analysis. The mean degree of polymerisation (mean DP) of each fructan has been determined by the glucose/fructose ratio. E. purpurea fructans represent linear inulin-type fructans with almost exclusively beta-(2-->1)-linked fructosyl units, terminal glucose and terminal fructose. Small proportions of beta-(2-->1,2-->6)-linked branch point residues were detected. The mean DP of the fructan fractions depends on the ethanol concentration used for precipitation: the lower the ethanol concentration the higher the mean DP. Corresponding results were found with all of the three analytical methods: 80% ethanol-insoluble fructan from E. purpurea shows an average mean DP of 35, 60% ethanol-insoluble fructan of 44 and 40% ethanol-insoluble fructan of 55. The applied methods provide sufficient sensitivity to determine not only the composition and structure but also the mean degree of polymerisation of fructans.     

Properties of fructan:fructan 1-fructosyltransferases from chicory and globe thistle,two Asteracean plants storing greatly different types of inulin

Remarkably, within the Asteraceae, a species-specific fructan pattern can be observed. Some species such as artichoke (Cynara scolymus) and globe thistle (Echinops ritro) store fructans with a considerably higher degree of polymerization than the one observed in chicory (Cichorium intybus) and Jerusalem artichoke (Helianthus tuberosus). Fructan:fructan 1-fructosyltransferase (1-FFT) is the enzyme responsible for chain elongation of inulin-type fructans. 1-FFTs were purified from chicory and globe thistle. A comparison revealed that chicory 1-FFT has a high affinity for sucrose (Suc), fructose (Fru), and 1-kestose as acceptor substrate. This makes redistribution of Fru moieties from large to small fructans very likely during the period of active fructan synthesis in the root when import and concentration of Suc can be expected to be high. In globe thistle, this problem is avoided by the very low affinity of 1-FFT for Suc, Fru, and 1-kestose and the higher affinity for inulin as acceptor substrate. Therefore, the 1-kestose formed by Suc:Suc 1-fructosyltransferase is preferentially used for elongation of inulin molecules, explaining why inulins with a much higher degree of polymerization accumulate in roots of globe thistle. Inulin patterns obtained in vitro from 1-kestose and the purified 1-FFTs from both species closely resemble the in vivo inulin patterns. Therefore, we conclude that the species-specific fructan pattern within the Asteraceae can be explained by the different characteristics of their respective 1-FFTs. Although 1-FFT and bacterial levansucrases clearly differ in their ability to use Suc as a donor substrate, a kinetic analysis suggests that 1-FFT also works via a ping-pong mechanism.     

Cloning and functional analysis of a high DP fructan:fructan 1-fructosyl transferase from Echinops ritro (Asteraceae): comparison of the native and recombinant enzymes

Inulin-type fructans are the simplest and most studied fructans and have become increasingly popular as prebiotic health-improving compounds. A natural variation in the degree of polymerization (DP) of inulins is observed within the family of the Asteraceae. Globe thistle (Echinops ritro), artichoke (Cynara scolymus), and Viguiera discolor biosynthesize fructans with a considerably higher DP than Cichorium intybus (chicory), Helianthus tuberosus (Jerusalem artichoke), and Dahlia variabilis. The higher DP in some species can be explained by the presence of special fructan:fructan 1-fructosyl transferases (high DP 1-FFTs), different from the classical low DP 1-FFTs. Here, the RT-PCR-based cloning of a high DP 1-FFT cDNA from Echinops ritro is described, starting from peptide sequence information derived from the purified native high DP 1-FFT enzyme. The cDNA was successfully expressed in Pichia pastoris. A comparison is made between the mass fingerprints of the native, heterodimeric enzyme and its recombinant, monomeric counterpart (mass fingerprints and kinetical analysis) showing that they have very similar properties. The recombinant enzyme is a functional 1-FFT lacking invertase and 1-SST activities, but shows a small intrinsic 1-FEH activity. The enzyme is capable of producing a high DP inulin pattern in vitro, similar to the one observed in vivo. Depending on conditions, the enzyme is able to produce fructo-oligosaccharides (FOS) as well. Therefore, the enzyme might be suitable for both FOS and high DP inulin production in bioreactors. Alternatively, introduction of the high DP 1-FFT gene in chicory, a crop widely used for inulin extraction, could lead to an increase in DP which is useful for a number of specific industrial applications. 1-FFT expression analysis correlates well with high DP fructan accumulation in vivo, suggesting that the enzyme is responsible for high DP fructan formation in planta.