嗜盐细菌中四氢嘧啶和羟基四氢嘧啶的生物合成及其生物学功能

在嗜盐细菌盐适应中,四氢嘧啶(1,4,5,6-四氢-2-甲基-4-嘧啶羧酸)和羟基四氢嘧啶(1,4,5,6-四氢-2-甲基-5-羟基-4-嘧啶羧酸)发挥着十分重要的作用。四氢嘧啶的生物合成以L-天冬氨酸-β-半醛(ASA)为底物,依次由2,4-二氨基丁酸转氨酶(EctB),2,4-二氨基丁酸乙酰基转移酶(EctA)和四氢嘧啶合成酶(EctC)催化反应,分别生成L-2,4-二氨基丁酸(DABA),N-乙酰-L-2,4-二氨基丁酸(ADABA)和四氢嘧啶。羟基四氢嘧啶则由四氢嘧啶羟化酶(EctD)将四氢嘧啶羟基化产生。通常,四氢嘧啶合成基因以ectABC基因簇的形式存在,而羟基四氢嘧啶合成基因ectD单独存在。四氢嘧啶生物合成基因在微生物菌株和转基因经济作物中的表达可以提高其耐盐碱旱等抗逆能力,羟基四氢嘧啶合成基因的表达可以增强宿主耐热和耐干燥的能力。四氢嘧啶类相容性溶质的生物学功能及其潜在应用已成为前沿性研究热点。     

渗透压冲击下中度嗜盐菌Halomonas sp. Y四氢嘧啶类相容性溶质的合成与释放

【背景】四氢嘧啶类物质在高温、冷冻和干燥等逆境条件下,对酶、蛋白质、核酸及整个细胞具有良好的保护作用,已经应用于酶制剂、生物医药及护肤品等相关领域。目前此类物质只能依赖中度嗜盐菌采用细菌泌乳工艺进行商业化生产,因此四氢嘧啶类高产菌株及其发酵技术的研究日益受到国内外研究者关注。【目的】分离获得高产合成四氢嘧啶类相容性溶质的中度嗜盐细菌,研究渗透压冲击对其胞内四氢嘧啶合成与释放的影响,探索细菌泌乳法制备四氢嘧啶的可行性。【方法】采用涂布平板法分离中度嗜盐菌,对分离菌株进行形态、生理生化和16S rRNA基因序列分析,鉴定其种属;采用高效液相色谱法(HPLC)和质谱法(MS)分析四氢嘧啶类物质,细菌泌乳法制备四氢嘧啶类物质。【结果】从盐池土样中分离到一株以四氢嘧啶类物质为主要相容性溶质的中度嗜盐菌Y,鉴定为盐单胞菌(Halomonas sp.)Y。盐单胞菌Y能在NaCl质量浓度为10-250 g/L的培养基中生长,最适生长的NaCl浓度为100 g/L;HPLC-MS测试结果证明盐单胞菌Y可同时合成四氢嘧啶和羟基四氢嘧啶2种相容性溶质,在最适生长的盐浓度下其合成量分别达175.5 mg/g和47.9 mg/g;在NaCl质量浓度为0-30 g/L的低渗溶液中胞内四氢嘧啶类物质经5 min即可达到最大释放率,而细菌泌乳工艺中最适合诱导四氢嘧啶释放的低渗溶液为质量浓度为10 g/L的NaCl溶液;采用细菌泌乳工艺制备四氢嘧啶,经连续11轮的高渗/低渗冲击,四氢嘧啶总合成量为6.0 g/L,总释放量为5.7 g/L,平均释放率为64.5%,底物转化率为128.9 mg/g。【结论】盐单胞菌Y是一株较高产合成四氢嘧啶类的中度嗜盐菌,能够耐受反复的渗透压冲击,采用细菌泌乳工艺显著提高了四氢嘧啶的制备效率。     

中度嗜盐菌四氢嘧啶合成基因的克隆与功能分析

中度嗜盐菌Bacillus alcalophilus DTY1分离自晋西北黄土高原盐碱土壤, 能够产生耐盐相关的相容性溶质四氢嘧啶。为了研究四氢嘧啶的功能, 克隆了DTY1菌株四氢嘧啶合成基因簇ectABC。ectA、ectB和ectC分别编码169、428和132个氨基酸的肽链, 分别与B. halodurans C-125中的二氨基丁酸乙酰基转移酶(EctA)、二氨基丁酸氨基转移酶(EctB)、四氢嘧啶合成酶(EctC)同源性达59%、81%和81%。将携带该基因簇的4.0 kb片段转入蜡质芽孢杆菌B. cereus Z后, 芽孢杆菌的耐盐度显著提高。HPLC检测发现, 在1.0% NaCl浓度下, 转化菌B. cereus Z-E菌株生成70.1 mg/g四氢嘧啶, 而在5.0%的NaCl浓度下四氢嘧啶的产量高达118.6 mg/g, 显著高于B. alcalophilus DTY1的四氢嘧啶产量。而且随着盐浓度的提高, 四氢嘧啶的合成量也随之提高。由此证明四氢嘧啶参与中度嗜盐菌重要的渗透调节, ectABC的表达受盐诱导。     

中度嗜盐菌四氢嘧啶合成基因的克隆与功能分析

中度嗜盐菌Bacillus alcalophilus DTY1分离自晋西北黄土高原盐碱土壤, 能够产生耐盐相关的相容性溶质四氢嘧啶。为了研究四氢嘧啶的功能, 克隆了DTY1菌株四氢嘧啶合成基因簇ectABC。ectA、ectB和ectC分别编码169、428和132个氨基酸的肽链, 分别与B. halodurans C-125中的二氨基丁酸乙酰基转移酶(EctA)、二氨基丁酸氨基转移酶(EctB)、四氢嘧啶合成酶(EctC)同源性达59%、81%和81%。将携带该基因簇的4.0 kb片段转入蜡质芽孢杆菌B. cereus Z后, 芽孢杆菌的耐盐度显著提高。HPLC检测发现, 在1.0% NaCl浓度下, 转化菌B. cereus Z-E菌株生成70.1 mg/g四氢嘧啶, 而在5.0%的NaCl浓度下四氢嘧啶的产量高达118.6 mg/g, 显著高于B. alcalophilus DTY1的四氢嘧啶产量。而且随着盐浓度的提高, 四氢嘧啶的合成量也随之提高。由此证明四氢嘧啶参与中度嗜盐菌重要的渗透调节, ectABC的表达受盐诱导。     

新喀里多尼亚弧菌CGJ02-2中四氢嘧啶合成基因簇ectABC的克隆及其功能鉴定

研究旨在克隆新的四氢嘧啶合成基因簇,并对其功能进行鉴定,为应用于四氢嘧啶的生产奠定基础。从新喀里多尼亚弧菌CGJ02-2中克隆获得四氢嘧啶合成基因簇ectABC,ectABC与表达载体pBAD连接后转化至大肠杆菌BW25113中,通过L-阿拉伯糖诱导表达。采用SDS-PAGE和液质联用鉴定重组表达蛋白,利用全细胞催化合成四氢嘧啶,通过高分辨质谱鉴定四氢嘧啶,并从天冬氨酸浓度、KCl浓度、温度和pH 4个方面优化催化条件。结果表明,来自新喀里多尼亚弧菌CGJ02-2 基因组的ectABC大小为2 235 bp。SDS-PAGE显示表达产物中有3个重组蛋白产生, 液质联用鉴定表明其分子量分别与ectA、ectB、ectC的理论分子量一致。高分辨质谱分析发现全细胞催化上清中有四氢嘧啶产生。优化后的最适全细胞催化条件为：天冬氨酸浓度100 mmol·L^-1,KCl浓度100 mmol·L^-1,温度30 ℃,pH 7.0,最优条件下产量为1.11 mg·mL^-1。研究从弧菌中克隆了四氢嘧啶合成基因簇ectABC,并在大肠杆菌BW25113中实现了异源表达和低盐环境下的四氢嘧啶合成,为大规模发酵生产四氢嘧啶奠定了基础。     

Halomonas venusta DSM4743渗透压冲击下四氢嘧啶合成与释放

选择耐受较高NaCl浓度,而且四氢嘧啶胞内浓度阈值较高的菌株,研究其四氢嘧啶发酵条件和工艺,对于提高四氢嘧啶的制备效率具有实际意义。考察了碳源、NaCl浓度、酵母膏添加量对Halomonas venustaDSM4743四氢嘧啶合成的影响,考察了优化条件下的四氢嘧啶分批发酵进程,并利用"细菌挤奶"工艺制备四氢嘧啶。结果表明:谷氨酸单钠为唯一碳氮源、NaCl浓度为1.5mol/L、酵母膏添加量为0.5%的条件有利于四氢嘧啶合成。在优化条件下10L发酵罐分批发酵,四氢嘧啶最大合成量为3.2g/L,合成效率为2.7g/(L.d)。通过"细菌挤奶"工艺制备四氢嘧啶,6个渗透压冲击循环后,四氢嘧啶总合成量为14.7g/L,总释放量为14.3g/L,平均释放率为97%,合成效率2.1g/(L.d)。中度嗜盐菌Halomonas venusta DSM4743耐受较高浓度的NaCl,而且四氢嘧啶胞内浓度阈值较高,优化的发酵条件及"细菌挤奶"工艺,获得了较高的四氢嘧啶制备效率。     

古盐井中嗜盐菌的分离及四氢嘧啶的制备

[目的]分离鉴定古盐井中的嗜盐菌,确定相容性溶质,增加相容性溶质的合成。[方法]从盐井卤水中分离嗜盐菌,对菌株进行形态、生理生化和16S rRNA分析,用高效液相色谱法(HPLC)和质谱法(MS)确定相容性溶质,以谷氨酸钠为唯一碳氮源来制备四氢嘧啶。[结果]菌株S2为色盐杆菌属;相容性溶质为四氢嘧啶; 1. 5 mol/L Na Cl时四氢嘧啶达到最适合成浓度,为0. 168 3 mg/mL,单位质量合成量为238. 201 mg/g;以谷氨酸钠为唯一碳氮源时,相同体积发酵液中四氢嘧啶的总合成量与单位质量合成量均增加,四氢嘧啶合成量为0. 184 8 mg/mL,单位质量合成量为390. 389 mg/g。[结论]成功分离出了产四氢嘧啶的嗜盐菌,并且以谷氨酸钠为唯一碳氮源时四氢嘧啶合成量大大增加。     

四氢嘧啶羟化酶的研究进展

作为相容性物质,5-羟化四氢嘧啶不仅可以调节渗透压,还可以稳定蛋白结构,在医药、生物制造和化工行业具有广阔的发展前景。四氢嘧啶羟化酶属于Fe2+与2-酮戊二酸依赖型双加氧酶超家族,主要催化四氢嘧啶生成5-羟化四氢嘧啶。我们简要介绍了四氢嘧啶羟化酶的基因来源、活性检测、蛋白结构、催化机理及活性中心等方面的研究进展。     

一株可用于四氢嘧啶制备的中度嗜盐菌

<正>四氢嘧啶(1,4,5,6-四氢-2-甲基-4-嘧啶羧酸)是中度嗜盐细菌的一种渗透压补偿性溶质[1],可以平衡细胞的渗透压,并且在高温、冷冻和干燥等逆境下,对酶、DNA、细胞膜和整个细胞提供保护作用,因此四氢嘧     

四氢嘧啶微生物合成与应用研究进展

极端环境微生物定义了生命的边界。为了适应各种极端环境,极端环境微生物通过合成许多独特的活性化合物来保护自己。四氢嘧啶就是其中一种代表性的保护性物质。它最早是从极端嗜盐菌中发现的,作为调节细胞渗透压的一类相容性溶质,可以帮助微生物适应高盐等恶劣环境。研究发现四氢嘧啶不仅是一种重要的渗透压调节剂,还是一种高效的生物保护剂,可以帮助蛋白、核酸、生物膜乃至整个细胞对抗高温、干燥、冷冻和辐射等多种逆境。因此,四氢嘧啶在生物保护、生物医药和生物科技等众多领域展现出广阔的商业化应用前景。随着合成生物学和代谢工程技术的快速发展,传统的嗜盐菌四氢嘧啶生产方法已逐步被产率更高、环境更友好的生物工程菌及技术所取代。本文围绕四氢嘧啶的微生物合成及其应用研究进行综述,为后续四氢嘧啶的开发和应用提供重要参考。     

高盐盐湖可分离嗜盐耐盐菌的种群多样性及四氢嘧啶产量评价

为了解柴达木盆地茶卡盐湖、柯柯盐湖和小柴旦盐湖等三大硫酸镁亚型高盐盐湖可分离嗜盐耐盐菌的种群多样性,采用RM中、高盐培养基筛选分离可培养的嗜盐菌和耐盐菌,扩增16S rRNA基因序列进行种属鉴定和环境因子典范对应分析(CCA),选取优势菌属构建系统发育树,并采用高效液相色谱法(HPLC)检测次级代谢产物四氢嘧啶(Ect...     

Comparison of ectoine synthesis regulation in secreting and non-secreting strains of Halomonas

Ectoine is an osmotic pressure compatible solute. It is synthesized by Halomonas and other microorganisms in a hypertonic environment. As a stabilizing agent of cells proteins, nucleic acids and other biological products, ectoine has wide applications. Therefore, an efficient production method for ectoine is in great demand. Ectoine is overproduced by Halomonas salina DSM 5928, an ectoine-secreting strain, in which the synthesis of ectoine is not limited by its intracellular threshold concentration. In order to explain the mechanism of secretion of ectoine, the response to NaCl stress, and the release and uptake kinetics of ectoine were compared between H. salina DSM 5928 and Halomonas elongata DSM 2581, a non-ectoine-secreting strain. Moreover, the ectoine binding protein TeaA from each of these two strains was cloned and expressed, and binding abilities were examined in vitro. The results indicated that H. salina DSM 5928 and H. elongata DSM 2581 respond to NaCl in the medium in different ways. Compared with H. elongata DSM 2581, the amount of ectoine released was higher and the uptake of ectoine under NaCl stress was lower in H. salina DSM 5928. In addition, the binding ability of TeaA to ectoine in H. salina DSM 5928 was also lower. These results reveal the secretion mechanism of ectoine as well as critical regulation and control factors involved in ectoine synthesis.     

Ectoines as compatible solutes and carbon and energy sources for the halophilic bacterium Chromohalobacter salexigens

AIMS: To investigate the catabolism of ectoine and hydroxyectoine, which are the major compatible solutes synthesized by Chromohalobacter salexigens. METHODS AND RESULTS: Growth curves performed in M63 minimal medium with low (0.75 mol l(-1) NaCl), optimal (1.5 mol l(-1) NaCl) or high (2.5 mol l(-1) NaCl) salinity revealed that betaine and ectoines were used as substrate for growth at optimal and high salt. Ectoine transport was maximal at optimal salinity, and showed 3- and 1.5-fold lower values at low and high salinity respectively. The salt-sensitive ectA mutant CHR62 showed an ectoine transport rate 6.8-fold higher than that of the wild type. Incubation of C. salexigens in a mixture of glucose and ectoine resulted in a biphasic growth pattern. However, CO(2) production due to ectoine catabolism was lower, but not completely abolished, in the presence of glucose. When used as the sole carbon source, glycine betaine effectively inhibited ectoine and hydroxyectoine synthesis at any salinity. CONCLUSIONS: The catabolic pathways for ectoine and hydroxyectoine in C. salexigens operate at optimal and high (although less efficiently) salinity. Endogenous ectoine(s) may repress its own transport. Ectoine utilization was only partially repressed by glucose. Betaine, when used as carbon source, suppresses synthesis of ectoines even under high osmolarity conditions. SIGNIFICANCE AND IMPACT OF THE STUDY: This study is a previous step to the subsequent isolation and manipulation of the catabolic genes, so as to generate strains with enhanced production of ectoine and hydroxyectoine.     

Contribution of chemical changes in membrane lipids to the osmoadaptation of the halophilic bacterium Chromohalobacter salexigens

The long-term response of the broad-salt growing halophile Chromohalobacter salexigens DSM 3043T to salt stress has been investigated with respect to adaptive changes in membrane lipid composition. This study included the wild-type and three salt-sensitive, ectoine-deficient strains: CHR62 (ectA::Tn1732, unable to grow above 0.75 M NaCl), CHR63 (ectC::Tn1732, unable to grow above 1.5 M NaCl), and CHR64, which was able to grow in minimal medium M63 up to 2.5 M NaCl, but its growth was slower than the wild-type strain at salinities above 1.5 M NaCl. This mutant accumulated ectoine and hydroxyectoine as major compatible solutes, but also the ectoine precursor, N-gamma-acetyldiaminobutyric acid, and was found to be affected in the ectoine synthase gene ectC. The main phospholipids of the wild-type strain were phosphatidylethanolamine, phosphatidylglycerol (PG), and cardiolipin (CL). Major fatty acids were detected as 16:0, 18:1, and 16:1, including significant amounts of cyc-19:0, and cyc-17:0. CL and cyclopropane fatty acids (CFA) levels were elevated when the wild-type strain was grown at high salinity (2.5 M NaCl). Membranes of the most salt-sensitive trains CHR62 and CHR63, but not of the less salt-sensitive strain CHR64, contained lower levels of CL. The proportion of cyc-19:0 in CHR64 was three-fold (at 2.0M NaCl) and 2.5-fold (at 2.5 M NaCl) lower than that of the wild type, suggesting that this mutant has a limited capacity to incorporate CFA into phospholipids at high salt. The addition of 1 mM ectoine to cultures of the wild-type strain increased the ratio PG/CL from 1.8 to 3.3 at 0.75 M NaCl, and from 1 to 6.5 at 2.5 M NaCl, and led to a slight decrease in CFA content. Addition of 1 mM ectoine to the mutants restored the steady-state levels of CL and CFA found in the wild-type strain supplemented with ectoine. These findings suggest that exogenous ectoine might attenuate the osmostress response involving changes in membrane lipids.