Hydrogen Production with High Evolution Rate and High Yield by Immobilized Cells of Hydrogen-producing Bacteria Strain B49 in a Column Reactor

To improve the hydrogen evolution rate in continuous hydrogen production of a fermentative hydrogen-producing bacteria strain B49 (AF481148 in EMBL), 4% immobilized cells by polyvinyl alcohol-boric acid method, with the addition of a small amount of calcium alginate in a column reactor obtain hydrogen yield of 2.31 mol H2/mol glucose and hydrogen evolution rate of 1435.4 ml/L culture&middoth respectively at medium retention time of 2 h with a medium containing l0 g glucose/L. As the cell density in gel beads is increased to 8%, hydrogen yield and hydrogen evolution rate for l0 g glucose/L are 2.34 mol H2/mol glucose and 2912.4 ml/L culture &middot h respectively at medium retention time of 1 h, and for molasses wastewater COD of 7505.9 mg/L hydrogen production potential of 205.6 ml/g COD and hydrogen evolution rate of 2057.7 ml/L culture&middoth at hydraulic retention time of 0.75 h are observed. In the continuous culture pH value keeps around 3.9 by self regulation.

Partial Characteristics of Hydrogen Production by Fermentative Hydrogen-producing Bacterial Strain B49

To investigate the characteristics of hydrogen production by a novel fermentative hydrogen-producing bacterial strain B49 (AF481148 in EMBL), batch experiments are conducted under different conditions. Hydrogen production has a correlation with cell growth and the consumption of glucose and soluble protein. The optimum pH for cell growth is 4.5±0.15. At acidic pH 4.0±0.15, the bacteria has the maximum accumulated hydrogen volume of 2382 ml/L culture and the maximum hydrogen evolution rate of 339.9 ml/L culture·h with 1% glucose. The optimum temperature for cell growth and hydrogen production is 35℃. In addition, fermentative hydrogen-producing bacterial strain B49 can generate hydrogen from the decomposition of other organic substrates such as wheat, soybean, corn, and potato. Moreover, it can also produce hydrogen from molasses wastewater and brewage wastewater, and hydrogen yields are 137.9 ml H 2/g COD and 49.9 ml H 2/g COD, respectively.

The start-up of biohydrogen-producing process by bioaugmentation in the EGSB reactor

Expanded granular sludge bed （EGSB） reactor and bioaugmentation were employed to investigate biohydrogen production with molasses wastewater. The start-up experiments consisted of two stages. In the first stage （0 - 24d） seeded with activated sludge, the butyric acid type-fermentation formed when the initial expanding rate, organic loading rate （OLR）, the initial redox potential （ORP） and hydraulic retention time （HRT） were 10%, 10.0 kg COD/（m^3·d）, -215 mV and 6.7 h, respectively. At the beginning of the second stage on day 25, the novel hydrogen-producing fermentative bacterial strain B49 （AF481148 in EMBL） were inoculated into the reactor under the condition of OLR 16. 0 kg COD/（m^3·d）, ORP and HRT about - 139 mV and 6.7 h, respectively, and then the reaction system transformed to ethanol-type fermentation gradually with the increase in OLR. When OLR, ORP and HRT were about 94.3 kg COD/（m^3·d）, -250 mV and 1.7 h, respectively, the system achieved the maximum hydrogen-producing rate of 282.6 mL H2/L reactor·h and hydrogen percentage of 51% -53% in the biogas.

Magnesium improves hydrogen production by a novel fermentative hydrogen-producing bacterial strain B49

Batch experiments were conducted to investigate the effects of magnesium on glucose metabolism, including growth and hydrogen-producing capacity of fermentative hydrogen-producing bacterial strain B49. These abilities were enhanced with an increase in magnesium concentration. At the end of fermentation from （10 g/L） glucose, for 10 mg/L MgCl2·6H2O the cell growth in terms of optical density （OD） at 600nm was 0.46, the ratio of ethanol amount （mg/L） to acetate amount （mg/L） was 1.1, and the accumulated hydrogen volume was 934.9 mL H2/L culture; for 200 mg/L of MgCl2·6H2O OD600 nm was increased to 1.34. The accumulated hydrogen volume was increased to 2 360.5 mL H2/L culture, the ratio of ethanol amount （mg/L） to acetate amount （mg/L） was increased to 1.3 and polysaccharide was decreased to 2.5 mg/L. Moreover, the magnesium solution addition to the medium at different fermentation times affected hydrogen-producing ability. However, the later the addition time was postponed, the less the effect was on hydrogen evolution. Further experiments confirmed the enhancement was dependent on magnesium ions and not on the other inorganic ions such as SO42- or Cl-, which constituted the magnesium salts.

Length polymorphisms for intergenic spacer regions of 16S-23S rDNA in members of the new hydrogen-producing bacteria

A method based on PCR amplification of the 16S rRNA gene (rDNA)-23S rDNA intergenic spacer regions (ISR) was developed for the identification of species within the novel group hydrogen-producing anaerobes. The sizes of the PCR products varied from 1264 to 398 bp. Strain of isolate Rennanqilyf 3 was characterized as having products of 1262,398,638,437 and 436 bp. The isolate Rennanqilyf 1 had product of 1264 bp. The isolate Rennanqilyf 13 had products of 1261,579 and 485 bp. Of the 3 species of the novel group hydrogen-producing anaerobes examined, no one was indistinguishable. Two environmental isolates were identified as hydrogen-producing bacteria, which were new species in present taxon. Rennanqilyf 3 could not be associated with any Clostridium sp. studied. Rennanqilyf 1 could be classified into Clostridium genus. The combination between 16S rDNA equencing and length polymorphisms of IRS in 16S-23S rDNA is a better method for determining species of the hydrogen-producing bacteria.

化能驱动的产乙酸菌转化利用CO_(2)研究进展

利用微生物发酵一碳气体生产燃料和高值化学品,是实现碳资源回收利用和绿色生物制造的重要途径之一。产乙酸菌可利用CO或H_(2)为能量来源,通过伍德-永达尔(Wood-Ljungdahl)途径固定CO_(2),维持自身代谢,并生产乙酸、乙醇等高附加值产品。相较于化学催化而言,该生物催化过程对原料气体比例要求不高、反应条件温和、产物选择性高。在气体发酵中,CO和H_(2)均可作为菌株生长和代谢的能量来源,二者具有不同的能量代谢模式。同时,不同的产乙酸菌代谢产物也不相同。发酵过程中气体溶解度低限制了能量供给,导致微生物生长速率慢、原料利用率低以及目标产物产量低等问题。提高气体利用效率和扩大产乙酸菌的产物谱,是面向产业化应用的必然要求。本文简述了产乙酸菌的伍德-永达尔途径、产乙酸途径和产乙醇途径等天然代谢途径,从分子改造的角度总结了产乙酸菌利用一碳气体发酵生产高附加值产品如乙醇、2,3-丁二醇、丙酮、异丙醇等的相关研究进展,并从提高能量供给和产物选择性的角度进行了总结。最后,本文以能量代谢为切入点对产乙酸菌转化一碳气体进行了展望,以期为未来的生物制造提供参考。

厌氧生境体系中产氢产乙酸细菌的FISH定量解析

产氢产乙酸细菌是一类在有机物厌氧降解过程中起重要作用的细菌。以基于16S rRNA序列设计的特异性寡核苷酸探针为基础,优化FISH实验条件,确定该技术检测产氢产乙酸细菌的实验条件为样品固定19h、乙醇脱水5min,杂交缓冲液中甲酰胺浓度55%。运用建立的FISH技术检测了几种厌氧消化体系中产氢产乙酸细菌的数量,并与用传统MPN方法的结果进行了比较。结果表明,产氢产乙酸细菌分布广泛,废水处理UASB反应器和动物消化道,特别是反刍动物瘤胃中的产氢产乙酸细菌数量较高,其丰度分别为1.70×109 cells/mL样品,6.50×108 cells/mL样品。湖底沉积物中产氢产乙酸细菌数量较少,仅占整个微生物群落的0.4%,含量为1.20×108 cells/mL样品。

一个产氢产乙酸菌互营共培养体的培养基优化

营养生态位位于产酸发酵菌和产甲烷菌之间的产氢产乙酸菌,其分离培养困难,种子资源匮乏,限制了基于强化产氢产乙酸功能作用的高效厌氧生物处理技术的开发.在前期获得对丙酸具有较强降解能力的产氢产乙酸菌互营共培养体7-m-2a的基础上,探讨了丙酸质量浓度、氮源、Ca2+、Fe2+、Mg2+和泛酸等对其生长代谢的影响.结果表明,培养基中适宜的丙酸钠和Fe2+、Mg2+、泛酸质量浓度分别为10 g/L和88、38、30 mg/L,最佳氮源是由质量浓度为0.33 g/L的酵母膏、胰蛋白胨和NH4Cl组成的复合氮源.在优化条件下38℃培养30 d,7-m-2a对丙酸的降解速率和乙酸产量分别可达998 mg/(L.d)和3 947 mg/L.

丁酸甲烷发酵优势菌群的选育及其丁酸降解特性

选育以产氢产乙酸菌为优势的复合菌群,对于开发基于强化产氢产乙酸菌群功能作用的高效厌氧生物处理技术具有重要意义。研究表明,以厌氧折流板反应器中的厌氧活性污泥为出发菌群,通过丁酸盐培养基的定向培育,可选育到以降解丁酸的产氢产乙酸菌和产甲烷菌为优势的复合菌群。该菌群在初始pH 7.0、初始丁酸浓度9 319 mg/L和35℃等条件下,经过27 d的培养,其丁酸降解率达到95%,平均降解速率为39.2 mg/d,累积产气量为290 mL,丁酸的比产气速率达到3.95 mL/g,发酵气中的CH_4含量为61%,CO_2含量为22%。

一种产氢产乙酸菌互营共培养体的筛选及其群落结构解析

厌氧消化系统中的产氢产乙酸菌在营养生态位上位于产酸发酵菌群和产甲烷菌群之间,在功能上起着承上启下的重要作用。该菌群具有与耗氢菌互营共生的特性,其分离纯化非常困难。为了深入了解其生理生态特性,为开发高效的厌氧生物处理技术提供理论基础,采用丙酸和丁酸混合培养基,以具有甲烷发酵功能的厌氧活性污泥为出发菌群,进行了产氢产乙酸菌互营共培养体的选育,并借助于PCR-DGGE技术对其菌群结构进行了解析。经过选择培养基的不断传代培养,最终筛选到2个产氢产乙酸互营共培养体7-m-2a和11-O-1。这2个共培养体不仅对丙酸和丁酸具有很强的降解和产乙酸能力,而且不产甲烷和硫化氢。在这种非产甲烷菌和非硫酸盐还原菌与产氢产乙酸菌组成的互营共培养体中,含有专性的互营产乙酸菌Desulfotomaculum sp.Iso-W2及其伴生菌,其中的伴生菌是能利用甲酸盐和H2/CO2的Uncultured bacterium 054E12_B_DI_P58和Sedimenti bactersp.JN18_A14_H。对这一新的产氢产乙酸菌互营共培养体的发现和选育成功,为更全面地研究产氢产乙酸菌的生理生态特性提供了样本。

pH对UASB运行效能及产甲烷互营菌群的影响

研究产甲烷互营菌群对pH变化的响应,对于寻求提高有机废水厌氧生物处理效能的策略具有重要意义.以处理制糖废水的升流式厌氧污泥床(UASB)反应器的运行为基础,考察不同pH对反应器运行效能及产甲烷互营菌群的影响.结果表明,在进水COD 20 000 mg.L-1、HRT 8 h的条件下,当进水pH分阶段由6.9降至5.4时,UASB系统的pH随之从6.8～7.4下降至5.7～6.7,导致COD去除率降低了23.3%,出水中残留丙酸提高了3.9倍.聚合酶链式反应-变性梯度凝胶电泳(PCR-DGGE)分析结果表明,产氢产乙酸菌群在UASB中的多样性显著低于产甲烷菌群,其分布和优势度受pH降低的影响显著.以Eub 19(Pelotomaculum)为代表的食丙酸产氢产乙酸菌在偏酸环境中的优势度明显减弱,而食乙酸产甲烷菌及部分食氢产甲烷菌对pH下降响应并不显著,且随着pH下降,耐酸的食氢产甲烷菌Methanobacterium ferruginis和Uncultured Methanobrevibacter的优势度逐渐增强.由此可见,与产甲烷菌群相比,UASB系统中的产氢产乙酸菌群对pH的变化更加敏感.

ABR启动期运行效能及互营产甲烷菌群的分布特征

为探讨厌氧折流板反应器(ABR)启动期运行效能和互营产甲烷菌群的空间分布特征,考察了ABR反应器处理制糖废水启动期的运行特征,并采用聚合酶链式反应-变性梯度凝胶电泳(PCR-DGGE)技术分析了互营产甲烷菌群在ABR各格室的分布规律.结果表明,在污泥驯化阶段,ABR的COD去除率为61.5%,出水挥发酸总量高达1808mg/L.经过2个阶段的调控运行后,ABR出水挥发酸明显降低,甲烷含量增加至55%以上,COD去除率达到了94.8%.而且ABR第2～4格室形成了沉降性能良好的颗粒污泥.PCR-DGGE检测结果表明,该ABR系统中的主要产氢产乙酸菌为Syntrophobacter和Pelotomaculum,主要分布在ABR系统第3,4格室.ABR第1,2格室的产甲烷菌主要为耐酸的氢营养型产甲烷菌(Methanoregula和Methanosphaerula),而乙酸营养型产甲烷菌(Methanosaeta和Methanothrix)主要分布在第3,4格室.ABR系统中产甲烷菌的多样性要明显高于产氢产乙酸菌,说明当系统受到冲击时,产氢产乙酸作用比产甲烷作用更易成为限速步骤.

产乙酸复合菌系Th3培养及其在沼气厌氧发酵中的应用

为有效提高厌氧发酵过程中乙酸转化率和甲烷产量,将CD-2(Clostridium sordellii)、ZY-3(Clostridium bifermentans)和ZQ-1(Clostridium butyricum)3株利用不同底物的产乙酸菌混合培养,人工构建一个高效产乙酸复合菌系Th3,通过试验确定其最佳发酵条件为:初始pH值为7.0-8.0,按ZQ-1、ZY-3、CD-2顺序接种,CD-2:ZY-3:ZQ-1接种比例(体积比)为1:2:1,总接种量6%,30°C静置培养,乙酸产率达0.65g/(L·d)。经过代谢稳定性测定,Th3连续培养10代,乙酸产量维持稳定。复合菌系Th3应用于室内沼气发酵,(26±1)°C,在发酵初期和中期加入复合菌系Th3均能显著提高沼气日均产气量和产气率,初期添加可缩短发酵启动时间2～3d。在发酵末期加入复合菌剂对整个发酵产气过程没有显著影响。该研究不仅为构建高效微生物菌剂、提高厌氧发酵效率和发酵过程优化提供基础参数,而且表明该复合菌在沼气生产中有一定的应用价值。

工业化UASB厌氧颗粒污泥产氢产乙酸菌群分析

合成特异性探针,应用荧光原位杂交(FISH)技术分析阿维菌素废水处理工业化升流式厌氧污泥床(UASB)反应器颗粒污泥产氢产乙酸菌群分布和相对丰度,并测定菌群活性.结果表明:不同形成阶段颗粒污泥表面和内部剖面,产氢产乙酸菌、食丙酸盐产氢产乙酸菌和食丁酸盐产氢产乙酸菌的分布形态相同;产氢产乙酸菌平均相对丰度范围为(10.08±0.81)%～(28.06±2.12)%.成熟期颗粒污泥中产氢产乙酸菌相对丰度最大;颗粒污泥表面产氢产乙酸菌相对丰度大于内部剖面;食丙酸盐产氢产乙酸菌相对丰度大于食丁酸盐产氢产乙酸菌.阿维菌素残留对产氢产乙酸菌群具有抑制作用.不同形成阶段颗粒污泥最大比产乙酸速率范围为0.912～1.145g/(g.d),且与产氢产乙酸菌群相对丰度变化趋势一致.

一株产氢产乙酸菌的生长条件及产乙酸特性

在参与有机废水厌氧生物处理的各类微生物菌群中,产氢产乙酸菌群在功能生态位上起着承上启下的作用,对产氢产乙酸过程的强化,将有助于提高厌氧生物处理系统的效能。在前期研究中,通过丙酸和丁酸混合培养基,从厌氧活性污泥中筛选到一株双歧杆菌属(Bifidobacterim)的产氢产乙酸菌AX3。间歇培养试验结果表明,菌株AX3可在pH7.0、30℃条件下获得最佳增殖,不仅对丁酸和丙酸具有很高的乙酸转化率,同时也可发酵多种双糖和淀粉,并产生一定数量的乙酸。作为氮源,氯化铵比尿素更能有效地促进菌株AX3的增殖。

合成气生物利用的研究进展

对近年来利用合成气生产有机酸或醇、甲烷和氢气以及生物脱硫方面的相关研究进行了全面的介绍与评述,认为较低的发酵生产能力和产物浓度是目前该技术存在的最大问题,同时提供了一些可供选择的解决途径。

含硫酸盐废水厌氧处理过程中底物的竞争

在含硫酸盐有机工业废水的厌氧处理过程中,硫酸盐还原菌和产甲烷菌以及产乙酸菌之间的竞争是不可避免的,值得注意的是有些硫酸盐还原菌可以和产甲烷菌或产乙酸菌构成一个有效的降解丙酸和丁酸的共生生物群。从增长动力学上看,硫酸盐还原菌在底物的竞争中占有明显的优势,但是有些因素诸如:温度,pH,以及游离态硫化氢的浓度也影响到它们之间的竞争关系。有几种硫酸盐还原菌还可以像发酵菌和产乙酸菌那样进行代谢活动。

产氢产乙酸菌株AX2的生长条件及产乙酸特性

产氢产乙酸菌群在参与厌氧消化过程的各类微生物菌群中起着承上启下的作用,然而,目前产氢产乙酸菌的纯培养物很少,对其生理生态习性的了解也十分有限.为增加产氢产乙酸菌资源,了解其生理生化特性,通过丙酸和丁酸混合培养基,从厌氧活性污泥中筛选到一株具有产氢产乙酸特性的葡萄球菌(Staphylococcus)AX2,对其生长条件及转化丙酸和丁酸为乙酸的能力进行研究.结果表明,菌株AX2在丁酸培养基(2.4 g/L)和丙酸培养基(2.31 g/L)中的乙酸产量可分别达到278 mg/L和222 mg/L,并在以氯化铵为无机氮源、pH为7.0、35℃等条件下具有最佳的增殖能力.菌株AX2对丙酸、丁酸有较强的乙酸转化能力.

硬脂酸降解菌与嗜氢产甲烷杆菌共培养物的研究

本文介绍基本纯化的产氢乙酸的硬脂酸降解菌与嗜氢产甲烷杆菌的共培养物(LDB2-M2)在等当量的CaCl_2存在下,能降解C_1～C_18饱和脂肪酸;游离的硬脂酸能抑制M2的产甲烷活性;LDB 2短时间接触H_2,导致其活性暂时性抑制;当氢营养细菌数明显高于产氢产乙酸细菌数时,在分离过程中不必加其他氢营养菌作为伴生菌。