一株耐碱变形假单胞菌ZY-3的鉴定及其脱氮特性

【背景】目前缺少具有高效脱氮能力、较高生物安全性、能处理高碱含氮污水的好氧反硝化菌株,难以使用生物方法处理高碱性的工业、养殖废水。【目的】对前期于佛山市一水产养殖池塘底泥中分离得到的耐碱高效好氧反硝化细菌ZY-3进行研究,期望获得一株能用于不同酸碱环境脱氮的高效、安全的好氧反硝化细菌。【方法】通过形态学、生理生化试验及16S rRNA基因序列分析方法对菌株种属进行鉴定,采用抗生素试验及斑马鱼攻毒试验进行菌株的环境生物安全性评估,利用3种含不同氮素的含氮模拟废水进行脱氮能力的测定。【结果】确定ZY-3为假单胞菌属变形假单胞菌（Pseudomonas plecoglossicida）,其对多种临床常用抗生素敏感,对水生生物的毒性低,该菌株在高浓度含氮模拟废水中以28℃、180 r/min振荡培养时,其对数期出现在4—12 h,在12 h时NH₄⁺-N、NO₃^--N和NO₂^--N的去除率分别达到94.87%、81.44%和98.02%,其pH耐受范围为6.0—10.0。【结论】得到一株安全、高效、具有广泛pH适应范围的耐碱好氧反硝化细菌P. plecoglossicida ZY-3,其在有氧条件下对3种氮素（NH₄⁺-N、NO₃^–-N、NO₂^–-N）具有快速去除能力。     

不同来源的尿卟啉原Ⅲ转甲基酶在脱氮假单胞菌中的表达及其对生产维生素B_(12)的影响

S-腺苷-L-甲硫氨酸依赖型尿卟啉原Ⅲ转甲基酶(S-adenosy-L-methionine uroprophyrinogen Ⅲ methyltransferase,SUMT)催化尿卟啉原Ⅲ(uroprophyrinogen Ⅲ,urogen Ⅲ)中心碳原子C-2和C-7甲基化生成前咕啉-2,是维生素B_(12)生物合成途径中的一步关键酶。本文分别克隆了荚膜红细菌来源的RCcob A1,RCcob A2和脱氮假单胞菌来源的PDcob A,并在VB_(12)生产菌株脱氮假单胞菌中过表达和发酵。通过对三株重组菌维生素B_(12)发酵结果分析可知,SUMT(PDcob A),SUMT1(RCcob A1)和SUMT2(RCcob A2)的表达有利于维生素B_(12)产量的提高,与对照菌株相比分别提高了16.48%,10.2%和31.86%。根据摇瓶发酵的结果在5 L发酵罐上进行了放大实验,p BBR122-PblaRCcob A2的产量为144.5 mg/L,相比对照菌p BBR122-Pbla(111.3 mg/L)产量提高了29.83%左右。结论:SUMT的表达可以在一定程度上解除维生素B_(12)合成途径中的瓶颈,提高维生素B_(12)产量。     

脱氮除磷假单胞菌的筛选及定量检测

【目的】筛选具有较强脱氮除磷能力的细菌,建立结合S1酶保护分析的分子探针技术,以分析该菌在发酵过程中的数量变化情况。【方法】采用缺磷培养基厌氧培养、富磷培养基好氧培养和硝酸盐还原产气实验进行脱氮除磷菌筛选。通过16S rRNA基因序列分析及同源性比对,结合菌株的生理生化鉴定试验,鉴定筛选株。设计相应的16S rRNA探针组,建立结合S1酶保护分析的分子探针技术。【结果】筛选的菌株被鉴定为假单胞菌Pseudomonas sp.,命名为LY10。菌株LY10在富磷培养基中好氧培养24 h,总磷去除率达90.01%。在反硝化聚磷培养基中培养48 h,总氮和总磷去除率分别为84.71%和89.37%。针对假单胞菌16S rRNA基因序列设计了一组用于结合S1酶保护分析的分子探针Probe-P.sp,该探针具有很高的甄别灵敏度,能够将LY10与丛毛单胞属(Commonas)等5种细菌区分开;分子探针定量分析假单胞菌LY10,其细胞量与吸光值呈线性关系,检测的线性范围为103~106 cells/mL,线性方程为:y=-0.967 87+0.372 99x(R2=0.996 7,n=5)。【结论】新筛的假单胞菌LY10的脱氮除磷能力较强,具有生物脱氮除磷的工业化应用潜质。所建立的结合S1酶保护分析的分子探针技术的特异性和灵敏度良好,有望应用于混菌体系中的假单胞菌的定性定量分析。     

透明颤菌vgb基因在脱氮假单胞菌中的表达及对维生素B12合成的碳中心代谢流分析

在为维生素B₁₂生产菌株脱氮假单胞菌确立合适的接合转移操作条件的基础上,通过单交换的方式,将vgb基因整合到脱氮假单胞菌染色体上,获得了vgb重组菌株Pvgb-16,并通过¹³C同位素标记实验,探索VHb蛋白对脱氮假单胞菌碳中心代谢流变化和维生素B₁₂合成的影响。研究结果表明,在相同的供氧条件下,vgb重组菌株Pvgb-16拥有更高的比生长速率和比产物合成速率,与出发菌株相比分别提升了22%和52%。碳代谢通量分布分析表明,vgb重组菌株Pvgb-16的PP途径改善,提升了NADPH合成通量;甘氨酸由甜菜碱合成的通量上升,促进了前体物质氨基乙酰丙酸的合成,进一步加速维生素B₁₂的合成。总体来看,含vgb基因的重组菌株与出发菌株相比在促进菌体的生长、维生素B₁₂的合成速率及得率上都有显著效果,对进一步的发酵生产应用研究具有重要意义。     

假单胞菌胞外多糖发酵条件的研究

研究了假单胞菌（Ｐｓｅｕｄｏｍｏｎａｓｓｐ．６）利用木糖产胞外多糖的发酵条件。实验表明ＫＨ２ＰＯ４,Ｏ２和高碳氮比对多糖合成有促进作用,在发酵后期补加木糖有助于多糖产量的提高     

假单胞菌发酵液提高原油采收率的研究

筛选得到了一株假单胞菌D-1,其发酵液具有很高的表面活性,浓度为10%的发酵液的表面张力为45mN/m左右,则将其发酵液作为一种生物表面活性剂.经实验确定了发酵培养基的最适配方。在室内条件下,D-1的发酵液不仅能提高实验岩芯内原油的采收率10%左右,而且对原油2的防蜡率可以达到60%左右,因此,D-1在油田应用中会有很大的潜力。     

假单胞菌属的一个新种

从桔汁矿化水饮料中分离到一株编号为9191的革兰氏阴性短杆菌,其形态、生理生化特性与假单胞菌属已报道的种均不相同.该菌株具极生单鞭毛,氧化酶和触酶均阳性;O-F葡萄糖为非发酵型,不产生荧光色素,不产生脓菌素,不产生类胡萝卜色素,对葡萄糖呈碱反应.经类脂粒染色后细胞内可见PHB颗粒积聚.脲酶阳性,硝酸盐还原阳性,反硝化阴性;不水解淀粉和明胶,精氨酸双水解酶阴性;41℃下不生长,在麦康凯和SS平板上不生长.在0.85%CaCl_2的牛肉汤中不生长;利用β-羟基丁酸作为唯一碳源;DNA中G+C含量为65.15mol%.因此定为假单胞菌属中的一个新种.根据其对生理盐水敏感的特性,命名为盐敏假单胞菌(Pseudomonas halosensibilis Zou ＆ Cai nov.sp.).     

Effects of air pressure oscillation amplitude on oxygen transfer rate and biomass productivity in a solid-state fermenter

The modified sulfite oxidation method was adapted for estimation of the overall oxygen transfer rate in a pressure oscillating, solid-state fermenter. At 4.5 atm and 30 °C, the oxygen transfer rate reached 717 mmol kg^–1 initial dry matter h^–1 in this system against 37 mmol kg^–1 initial dry matter h^–1 in a static tray fermenter. At 30 °C and 3 atm, Azotobacter vinelandii grew on wheat straw and reached 4.7×10¹⁰ c.f.u. g^–1 substrate dry matter after 36 h, while only 8.2×10⁹ c.f.u. g^–1 substrate dry matter was obtained in a static tray system.     

Improved large-scale production of vitamin B12 by Pseudomonas denitrificans with betaine feeding

The strategy of betaine control for vitamin B(12) large-scale fermentation by Pseudomonas denitrificans was investigated in this paper. The results obtained in shake-flask experiments demonstrated that betaine could greatly stimulate vitamin B(12) biosynthesis but had an inhibition to cell growth. Based on the influence of betaine on the fermentation of P. denitrificans, betaine feeding was a beneficial strategy to solve the inconsistency between cell growth and vitamin B(12) production. As a result, an effective and economical strategy of betaine feeding was established for vitamin B(12) fermentation in 120-m(3) fermenter, in which betaine was continuously fed to maintain betaine concentration of the broth at the range of 5-7g/l during 50-140h of fermentation.     

An effective and simplified pH-stat control strategy for the industrial fermentation of vitamin B12 by Pseudomonas denitrificans

In order to improve the productivity of vitamin B(12) by Pseudomonas denitrificans carried out in a 120-m(3) fermenter, the effect of pH on vitamin B(12) biosynthesis was investigated. Results obtained from shake flask experiments showed that the feeding of carbon source (beet molasses or glucose) and methyl-group donor (betaine or choline chloride) significantly influenced the pH and the biosynthesis of vitamin B(12). In contrast to beet molasses or choline chloride, using glucose as a feed medium and betaine as a methyl-group donor, pH could be maintained at a stable range. As a result, higher vitamin B(12) production was achieved. Accordingly, an effective and simplified pH-stat control strategy was established for the fermentation of vitamin B(12) in a 120-m(3) industrial fermenter. When the new pH control strategy was applied, pH was stably kept in the range of 7.15-7.30 during fermentation. Thus, 214.3 mug/mL of vitamin B(12) was achieved.     

L－丙氨酸生产菌种培养条件的研究

本文从培养基组成、通气量、培养温度及培养时间四个方面研究并提出了Ｌ－丙氨酸生产菌种ＰｓｅｕｄｏｍｏｎａｓＩＡＭ１１５２－Ａ的最佳培养条件。     

铜绿假单胞菌产蛋白酶的发酵条件优化

【目的】鉴定一株来源于酱油曲能够分泌蛋白酶的铜绿假单胞菌CAU342A,优化其产蛋白酶的发酵条件。【方法】采用形态学观察、16S r RNA基因序列比对和生理生化方法鉴定菌株CAU342A;通过碳源、氮源、初始pH、温度、表面活性剂及发酵时间的单因素优化和正交试验获得最适发酵条件。【结果】菌株CAU342A被鉴定为铜绿假单胞菌(Pseudomonas aeruginosa),其最适发酵产酶条件为(质量体积比):3%酒糟,1.5%酵母浸提物,0.05%吐温-80,0.5%NaCl,0.7%K_2HPO_4,0.3%KH_2PO_4,0.04%MnSO_4,培养基初始pH 7.5,30°C培养72 h。在最适发酵条件下,该菌株最大产酶水平达到2 653.5 U/m L。蛋白酶酶谱分析表明该菌株能够产生至少4种具有蛋白酶活性的同工酶,其中两个主要酶谱带对应分子量分别为32 k D和50 k D。【结论】铜绿假单胞菌CAU342A高产蛋白酶,具有很大的工业应用潜力。     

Alginate production by <Emphasis Type="Italic">Pseudomonas mendocina</Emphasis> in a stirred draft fermenter

In this study alginate production by Pseudomonas mendocina in a laboratory-scale fermenter was investigated. In the experiments the effect of temperature (25–31°C) and agitation (500–620 rev min⁻¹) at a constant air flow of 10 v/v/h were evaluated in relation to the rate of glucose bioconversion to alginate using response surface methodology (RSM). The fermenter configuration was also adapted to a system with a screw mixer and draft tube, due to the change in rheological characteristics of the fermentation broth. The adjusted model indicates a temperature of 29.1°C and agitation of 553 rev min⁻¹ for optimum alginate synthesis. In this fermentation system a Y _p/s of 44.8% was achieved. The alginate synthesized by P. mendocina showed a partially acetylated pattern as previously reported for alginates obtained from other Pseudomonas spp and Azotobacter vinelandii.