渗透胁迫对杜氏盐藻胞内甘油含量及相关酶活性影响

杜氏盐藻（Dunaliella salina）是一种抗渗透能力强的单细胞绿藻,甘油在其渗透调节过程中发挥重要作用。本实验对5种不同NaCl浓度条件下,盐藻的生长、细胞内甘油含量及甘油代谢相关酶的活性变化进行了测定。结果表明,NaCl浓度过高或过低均影响盐藻的生长;高渗胁迫条件下甘油含量迅速增加,3-磷酸甘油磷酸酶的活性和二羟丙酮还原酶催化二羟丙酮转化为甘油的活性明显增加;而低渗胁迫条件下的甘油含量会迅速降低,3-磷酸甘油磷酸酶的活性丧失,二羟丙酮还原酶催化甘油转化为二羟丙酮的活性增加。基于此实验结果,我们对盐藻渗透胁迫条件下细胞内的甘油代谢过程与其抗渗透胁迫能力的相关性进行了探讨。     

二羟丙酮还原酶在杜氏盐藻渗透调节过程中的特性

从杜氏盐藻分离得到的二羟丙酮还原酶能专一性地催化二羟丙酮和甘油之间的可逆反应。酶催化二羟丙酮还原及甘油氧化的最适 PH分别为7.5和9.0;藻细胞经高渗处理,其甘油含量增加,酶催化甘油合成的活性比处理前提高120％,且大于其催化甘油转化的活性;藻细胞经低渗处理,其甘油含量减少,酶催化甘油转化的速率比处理前提高32％,暗示二羟丙酮还原酶在杜氏盐藻渗透调节过程中是甘油合成或转化的一个关键酶。     

培养液NaCl浓度对杜氏盐藻3-磷酸甘油脱氢酶同工酶的影响

目的：探讨在不同NaCl浓度下,杜氏盐藻（Dunaliella salina）的3-磷酸甘油脱氢酶（Glycerol 3-phosphate dehydrogen-ase,GPDH）同工酶的活性与其渗透调节相关性。方法：采用聚丙烯酰胺凝胶电泳（polyacrylamide gel electrophoresis,PAGE）技术对在不同NaCl浓度生长的杜氏盐藻的GPDH进行同工酶电泳检测。结果：在0.5mol/LNaCl低盐的条件下,杜氏盐藻具有4种NAD＋-GPDH同工酶,分别为GPDH1、GPDH2、GPDH3、GPDH4。当NaCl逐渐分别增高为2.0、3.0、4.0、5.0mol/L时,只有1种NAD＋-GPDH同工酶即GPDH1。结论：GPDH1具有较高活性,这与高盐胁迫时细胞大量合成甘油进行渗透调节密切相关。     

杜氏盐藻质膜ATPase在渗透调节中的可能作用

杜氏盐藻是一种以甘油为渗透调节物质的单细胞海藻,能够在0.08～5.0mol/L NaGl的培养液中生长。当外界NaGl浓度从0.5mol/L上升到4.0mol/L时,藻细胞内的Na~+和K~+含量变化不大,甘油含量则从6.20Pg/cell上升到51.50pg/cell。当藻细胞承受2.0mol/L到3.0mol/L NaCl的高渗胁迫时,能通过增加细胞内甘油含量来恢复原有形态;同时,藻细胞的H~+分泌增加,ATP含量下降;20μmol/L Na_3VO_4抑制了这些变化。KGN处理虽降低藻细胞内的ATP含量,却增加K~+外流和Na~+内渗。     

外源海藻糖对小麦幼苗耐盐性的影响

以盐敏感小麦品种鲁麦15为材料,分别用完全Hoagland营养液、150mmol／L NaCl和150mmol／L NaCl 10mmol／L海藻糖处理小麦幼苗,测定小麦幼苗生长、离子含量、根系质膜H^ -ATPase、SOD活性、MDA含量等指标,旨在探讨外源海藻糖在抗盐性中的作用。结果表明：外源海藻糖可明显缓解盐胁迫对小麦幼苗生长的抑制作用;明显提高NaCl胁迫条件下小麦幼苗叶片中K^ 的含量,降低Na^ 的含量,降低其Na^ ／K^ ;提高NaCl胁迫条件下小麦幼苗SOD活性,降低MDA的含量,降低细胞质膜透性,缓解根系质膜H^ -ATPase活性抑制。以上结果表叫外源海藻糖可能通过增加活性氧清除能力、缓解质膜伤害、维持胞质离子稳态提高植物抗盐性。     

发状念珠藻对盐胁迫的响应

探讨了发状念珠藻(NostocflagelliformeBornetFlah)对盐胁迫的耐受适应机制,采用含不同浓度NaCl(0、01、02、04、06、08、10mol/L)的BG110培养液处理具有正常生理活性的丝状体,25±05℃,40μmol/m2/s下照光培养12h,测定藻体光合作用、呼吸作用等生理活性以及体内一些物质的含量,结果表明:随培养液中NaCl浓度的升高藻体光合作用、呼吸作用以及PSⅡ活性(Fv/Fm)降低;质膜透性不断增大,丙二醛含量升高,自由水含量、自由水/束缚水比值下降,类胡萝卜素、可溶性糖含量增加,脯氨酸含量变化不大。由此可知,盐胁迫下发状念珠藻正常生理活性受到抑制而表现出一定的抗逆能力;该藻对盐胁迫具有一定的耐受能力,类胡萝卜素的增加有助于清除藻体内的氧自由基,可溶性糖可能是其主要渗透调节物质之一,脯氨酸在盐胁迫中的渗透调节作用不大。       

NaCl胁迫对超大甜椒种子萌发及幼苗生长的影响

以超大甜椒种子和幼苗为材料,采用水培法研究低、中、高浓度(50、150、250 mmol·L-1)NaCl胁迫对其种子萌发和幼苗生长的影响.结果显示:(1)低浓度NaCl处理促进种子萌发,而中、高浓度NaCl处理抑制种子萌发;NaCl处理第18天时,高浓度NaCl处理植株全部死亡,其余各处理植株苗高、叶面积、地上部鲜重和干重均随处理浓度升高而下降,但低浓度NaCl能刺激超大甜椒的根系生长.(2)低、中浓度NaCl处理时,植株叶绿素含量未受到大的影响,类胡萝卜素含量却随胁迫时间延长微量升高;在盐胁迫7 d的周期内,低、中浓度NaCl处理植株MDA含量、SOD活性和可溶性糖含量均随浓度升高及时间延长显著增加,脯氨酸含量在低浓度下变化不明显而中浓度下显著升高;在高浓度NaCl处理3 d中,MDA含量急剧升高,SOD活性先升高后下降,脯氨酸和可溶性糖含量显著增加.研究发现,NaCl胁迫浓度越高对超大甜椒种子萌发和幼苗生长的抑制效应越明显;低中浓度NaCl处理幼苗能通过自身的抗氧化酶清除系统和渗透调节物质来抵抗胁迫引起伤害,类胡萝卜素可能也有一定的抗胁迫作用,而高浓度NaCl处理增加了膜脂过氧化程度,严重影响了活性氧和渗透调节物质的正常代谢.     

共表达甘油脱氢酶和二羟丙酮激酶对大肠杆菌生长及甘油代谢的影响

考察共表达甘油脱氢酶(GldA)和二羟丙酮激酶(DhaKLM)对大肠杆菌生长及甘油代谢的影响。结果表明:在好氧条件下,共表达甘油脱氢酶及二羟丙酮激酶可以提高大肠杆菌利用甘油合成菌体的效率,利用等量的甘油,重组菌最高菌密度比对照菌提高了70%,细胞干质量为3.54 g(以每升发酵液计)。在厌氧条件下,仅共表达甘油脱氢酶并不能促进大肠杆菌的甘油代谢,而同时共表达甘油脱氢酶和二羟丙酮激酶可以明显提高大肠杆菌代谢甘油的能力,每克菌体消耗的甘油量提高了42%,每克干细胞中达11.08 g,代谢产物组成也发生显著变化,乙酸成为主要产物。这说明共表达gldA及dhaKLM基因能有效促进大肠杆菌好氧利用甘油生长及厌氧甘油代谢的能力。     

一氧化氮对盐胁迫下烟草细胞渗透调节能力的影响

一氧化氮(NO)作为信号分子广泛参与植物的生长发育、逆境胁迫响应过程。为了明确NO对细胞渗透调节作用,该研究以NaCl为盐胁迫因子,以烟草悬浮细胞为材料,研究了NO对盐胁迫下细胞渗透调节能力的影响。结果显示:(1)NaCl胁迫能诱发烟草细胞内源NO的生成,且100mmol·L-1 NaCl诱发了细胞内源NO的快速产生,在1h达到峰值,NO产生量约为对照的2倍,之后NO产生量快速下降,直至3h才逐渐回升,并在48h内维持在较高水平。(2)外源NO显著增强了烟草细胞的抗渗透胁迫能力,且150μmol·L-1 NO供体硝普钠(SNP)处理显著提高了NaCl胁迫下细胞的活力和再生能力(提高幅度分别为78.6%和63.2%),降低了细胞死亡率(降幅约为48.5%);SNP处理下的NaCl胁迫细胞能更大程度降低渗透势,延缓水势的降低,维持细胞压力势。(3)外源NO显著促进了NaCl胁迫细胞中脯氨酸的合成和积累,且150μmol·L-1 SNP处理将NaCl胁迫细胞中的脯氨酸含量提高25.9%;SNP处理也影响了脯氨酸代谢关键酶的活性和基因表达水平,即提高了谷氨酸脱氢酶(GDH)、精氨酸酶和鸟氨酸转氨酶(OAT)的活性,降低了脯氨酸脱氢酶(PDH)的活性,同时使GDH、OAT和PDH基因的表达表现出与酶活性相似的变化趋势。研究表明,NO参与了盐胁迫下烟草细胞的渗透调节,通过调控脯氨酸代谢可能是NO参与渗透调节的重要机制。     

盐胁迫下宁夏枸杞苯丙烷代谢相关基因差异表达分析北大核心CSCD

为探究盐胁迫条件下宁夏枸杞苯丙烷代谢相关基因差异表达规律,以不同浓度NaCl(0,100,200,300 mmol/L)处理的水培宁夏枸杞幼苗为研究材料,利用高通量测序技术和qRT-PCR对盐胁迫下宁夏枸杞苯丙烷代谢相关基因差异表达进行分析,同时对该途径中关键酶活性及产物含量进行测定。结果表明,(1)宁夏枸杞在不同浓度NaCl处理下共有58个苯丙烷代谢相关基因差异表达,且随着盐胁迫程度的增加大部分基因表达水平上调或不变;(2)随着NaCl浓度的增加,宁夏枸杞叶片抗氧化酶SOD、POD、CAT的活性均下降,而酚类物质、类黄酮和木质素的含量在100 mmol/L NaCl处理下均显著积累。研究发现,宁夏枸杞可能通过调控苯丙烷代谢相关基因上调表达,增加酚类物质、类黄酮和木质素的合成,来清除过多活性氧和提升细胞壁强度以适应盐胁迫;宁夏枸杞可耐受的NaCl浓度在100~200 mmol/L之间。     

Comparative analysis on the key enzymes of the glycerol cycle metabolic pathway in Dunaliella salina under osmotic stresses

The glycerol metabolic pathway is a special cycle way; glycerol-3-phosphate dehydrogenase (G3pdh), glycerol-3-phosphate phosphatase (G3pp), dihydroxyacetone reductase (Dhar), and dihydroxyacetone kinase (Dhak) are the key enzymes around the pathway. Glycerol is an important osmolyte for Dunaliella salina to resist osmotic stress. In this study, comparative activities of the four enzymes in D. salina and their activity changes under various salt stresses were investigated, from which glycerol metabolic flow direction in the glycerol metabolic pathway was estimated. Results showed that the salinity changes had different effects on the enzymes activities. NaCl could stimulate the activities of all the four enzymes in various degrees when D. salina was grown under continuous salt stress. When treated by hyperosmotic or hypoosmotic shock, only the activity of G3pdh in D. salina was significantly stimulated. It was speculated that, under osmotic stresses, the emergency response of the cycle pathway in D. salina was driven by G3pdh via its response to the osmotic stress. Subsequently, with the changes of salinity, other three enzymes started to respond to osmotic stress. Dhar played a role of balancing the cycle metabolic pathway by its forward and backward reactions. Through synergy, the four enzymes worked together for the effective flow of the cycle metabolic pathways to maintain the glycerol requirements of cells in order to adapt to osmotic stress environments.     

Regulation of glycerol metabolism in Zygosaccharomyces rouxii in response to osmotic stress

Summary Enzyme analyses indicated that the metabolism of glycerol by Zygosaccharomyces rouxii occurred via either glycerol-3-phosphate (G3P) or dihydroxyacetone (DHA). The route via DHA is significant in osmoregulation. The specific activities of glycerol dehydrogenase (GDHG) and DHA kinase, which metabolize glycerol via DHA, increased nine- and fourfold respectively during osmotic stress [0.960 water activity (a_w) adjusted with NaCl] when compared to non-stressed conditions (0.998 a_w). Both pathways are under metabolic regulation. Glycerol kinase, mitochondrial G3P dehydrogenase and DHA kinase are induced by glycerol while the latter is also repressed by glucose. Cells treated with cycloheximide prior to osmotic upshock showed significantly lower DHA kinase and GDHG levels and lower intracellular glycerol concentrations when compared to untreated control cells. Thus protein synthesis is essential for osmotic adaptation. Offprint requests to: B. A. Prior     

Cloning and characterization of a plastidic glycerol 3-phosphate dehydrogenase cDNA from Dunaliella salina

A cDNA encoding a nicotinamide adenine dinucleotide (NAD+) -dependent glycerol 3-phosphate dehydrogenase (GPDH) has been cloned by rapid amplification of cDNA ends from Dunaliella salina. The cDNA is 3032 base pairs long with an open reading frame encoding a polypeptide of 701 amino acids. The polypeptide shows high homology with published NAD+ -dependent GPDHs and has at its N-terminal a chloroplast targeting sequence. RNA gel blot analysis was performed to study GPDH gene expression under different conditions, and changes of the glycerol content were monitored. The results indicate that the cDNA may encode an osmoregulated isoform primarily involved in glycerol synthesis. The 701-amino-acid polypeptide is about 300 amino acids longer than previously reported plant NAD+ -dependent GPDHs. This 300-amino-acid fragment has a phosphoserine phosphatase domain. We suggest that the phosphoserine phosphatase domain functions as glycerol 3-phosphatase and that, consequently, NAD+ -dependent GPDH from D. salina can catalyze the step from dihydroxyacetone phosphate to glycerol directly. This is unique and a possible explanation for the fast glycerol synthesis found in D. salina.     

Enzymes involved in the formation of glycerol 3-phosphate and the by-products dihydroxyacetone and glycerol in Zymomonas mobilis

Abstract In Zymomonas mobilis a novel pathway for the formation of glycerol 3-phosphate was identified by enzymatic studies and nuclear magnetic resonance spectroscopy. This pathway branches off from the Entner-Doudoroff pathway at the intermediate glyceraldehyde 3-phosphate and proceedes via dihydroxyacetone phosphate, dihydroxyacetone, glycerol to glycerol 3-phosphate. The reaction sequence is catalyzed by the enzymes triosephosphate isomerase (0.4 U (mg protein)⁻¹), dihydroxyacetone phosphatase (0.31 U (mg protein)⁻¹), dihydroxyacetone reductase (0.25 U (mg protein)⁻¹), and glycerokinase (0.08 mU (mg protein)⁻¹), respectively. The action of a postulated aldolase catalyzing the cleavage of fructose 6-phosphate to dihydroxyacetone and glyceraldehyde 3-phosphate could be excluded.     

杜氏盐藻渗透调节过程中的甘油代谢途径

杜氏盐藻在适应外界盐浓度变化的过程中,甘油是其主要的渗透调节物质。低渗处理提高藻细胞的呼吸速率６０％以上;高渗处理对呼吸无明显影响,但大大刺激光合放氧速率。呼吸链的细胞色素电子传递链抑制剂ＫＣＮ和交替氧化酶抑制剂ＳＨＡＭ对杜氏藻渗透调节过程中的呼吸．胞内甘油、ＡＴＰ、淀粉会量的变化有不同的抑制效果。低渗情况下,胞内甘油转化为淀粉,所需能量由正常呼吸链和交替氧化酶途径同时提供;高渗情况下．淀粉则降解为甘油,光下甘油合成的能量主要由光合电子链提供,暗中则由正常呼吸链提供。     

甘油代谢对杜氏盐藻盐耐受性的调节

杜氏盐藻是迄今发现的世界上最耐盐的单细胞真核生物,能在0.05 mol/L至饱和NaCl浓度下正常生长,因此其耐盐机制倍受人们关注。研究发现,杜氏盐藻盐耐受性与甘油代谢密切相关。为此,我们综述其耐盐机制、甘油代谢调控、甘油代谢与盐耐受性关联性、甘油代谢重要酶的分子生物学研究等进展,希望对深入研究植物耐盐机制、培育耐盐作物新品种及开发甘油等高附加值次生代谢产物等研究提供有益帮助。     

Two Isoforms of Dihydroxyacetone Phosphate Reductase from the Chloroplasts of Dunaliella tertiolecta

Three isoforms of dihydroxyacetone phosphate reductase in extracts from Dunaliella tertiolecta have been separated by a diethylaminoethyl cellulose column chromatography with a shallow NaCl gradient. The chloroplasts contained the two major isoforms, and the third, minor form was in the cytosol. The isoforms are unstable in the absence of glycerol and they are cold labile, but they may be partially reactivated at 35[deg]C. The first chloroplast form to elute from the DEAE cellulose column was the major form when the cells were grown on high NaCl and it has been referred to as the form for glycerol production for osmoregulation or "osmoregulator form." The second form increased in specific activity when inorganic phosphate was increased in the growth media to stimulate growth, and it has been given the designation for the form for glyceride synthesis, "glyceride form." The osmoregulator form was stimulated by NaCl added to the enzyme assay, but not by reduced Escherichia coli thioredoxin. The glyceride form had properties similar to the enzyme in leaf chloroplast, such as inhibition by NaCl and by fatty acyl-coenzyme A derivatives and some stimulation by dithiothreitol, uridine diphosphate galactose, cyti-dine diphosphate dipalmatoyl diglyceride, and reduced E. coli thioredoxin. Thus, Dunaliella chloroplasts have a salt-stimulated osmoregulatory form of dihydroxyacetone phosphate reductase, which seems to have a role in glycerol production, and an isoform, which may be involved in glyceride synthesis and which has properties similar to the enzyme in chloroplasts of higher plants.