Probiotic Leuconostoc mesenteroides ssp. cremoris and Streptococcus thermophilus induce IL-12 and IFN-γ production

AIM： To investigate the capacity of potentially probiotic strains from six bacterial genera to induce cytokine production alone or in combinations in order to identify potential enhancing or synergistic effects in order to select probiotic bacteria for in vivo purposes.METHODS： Cytokine production in human peripheral blood mononuclear cells （PBMC） in response to stimulation with eleven different potentially probiotic bacterial strains from Streptococcus, Lactobacillus, Bifidobacterium, Lactococcus, L euconostoc a n d Propionibacterium genera was analysed. Production and mRNA expression of TNF-α, IL-12, IFN-y and IL-10 were determined by ELISA and Northern blotting, respectively.RESULTS： All tested bacteria induced TNF-α production. The best inducers of Thl type cytokines IL-12 and IFN-y were Streptococcus and Leuconostoc strains. All BiHdobacterium and Propionibacterium strains induced higher IL-IO production than other studied bacteria. Stimulation of PBMC with any bacterial combinations did not result in enhanced cytokine production suggesting that different bacteria whether gram-positive or gram- negative compete with each other during host cell interactions.CONCLUSION： The probiotic S. thermophilus and Leuconostoc strains are more potent inducers of Thl type cytokines IL-12 and IFN-γ than the probiotic Lactobacillus strains. Bacterial combinations did not result in enhanced cytokine production.

Isolation, Purification, and Characterization of Exopolysaccharide Produced by Leuconostoc Citreum N21 from Dried Milk Cake

A strain with high production of exopolysaccharide(EPS) was isolated from dried milk cake(a traditional fermented food from Inner Mongolia). The strain was called N21 and later identified as Leuconostoc citreum( Leu. citreum). The strain was cultured in Man-Rogosa-Sharpe medium containing 50 g/L of sucrose for 48 h at 30 °C and the EPS purified, with a yield of 24.5 g/L. An average molecular weight of 6.07 × 10~6 g/mol was determined by high-performance size-exclusion chromatography. The structure of the purified EPS was investigated through gas chromatography, ~1H and ^(13)C nuclear magnetic resonance spectroscopy, and Fourier transform infrared spectroscopy. The results demonstrated a polysaccharide composed of D-glucopyranose units in a linear chain with consecutive α(1 → 6) linkages. No branching was found in the structure of the exopolysaccharide. The purified EPS showed high water solubility and emulsibility. Based on the thermogravimetric curve, the degradation temperature of the EPS was 308.47 °C, which suggested that the dextran in the study exhibited high thermal stability. The results indicated that Leu. citreum N21 could be widely used to produce linear EPS and that the EPS has potential applications in food science and processing as a food additive.

Production and characterization of insoluble α-1,3-linked glucan and soluble α-1,6-linked dextran from Leuconostoc pseudomesenteroides G29

Exopolysaccharides can be produced by various bacteria and have important biological roles in bacterial survival depend on molecular weight,linkage,and conformation.In this study,Leuconostoc pseudomesenteroides G29 was identified and found to produce two types of exopolysaccharides from sucrose including soluble and insoluble a-glucans.By regulation of pH above 5.5,soluble a-glucan production was increased to 38.4 g∙L^(-1) from 101.4 g∙L^(-1) sucrose with fewer accumulation of lactic acid and acetic acid.Simultaneously,the quantity of thick white precipitate,that is insoluble a-glucan,was also increased.Then,a-glucans were prepared by enzymatic reaction with crude glucansucrases from the supernatant of G29 fermentation broth and purified for structure analysis.Based on the integration analysis of FT-IR and NMR,it was observed that soluble a-glucan is a highly linear dextran with α-1,6 glycosidic bonds while the insoluble a-glucan has 93%of α-1,3 and 7%of α-1,6 glycosidic bond.The results extend our understanding of exopolysaccharides production by L.pseudomesenteroides,and this water insoluble α-1,3-glucan might have potential application as biomaterials and/or biochemicals.

乳酸明串珠菌(Leuconostoc lactis)L2体内耐受性及产胞外多糖条件研究

通过对乳酸明串珠菌(Leuconostoc lactis,Leu.lactis)L2进行耐pH、耐胆盐、耐NaCl能力的测定,评价其体内益生特性。结果表明,该菌株具有较强耐酸、耐胆盐及耐NaCl能力,是具有益生潜力的优良菌株。为提高Leu.lactis L2胞外多糖(Exopolysaccharide, EPS)的产量,结合单因素试验,对该菌株产EPS的培养基组分和发酵条件进行优化。优化后的条件为:蔗糖80 g·L^-1、蛋白胨10 g·L^-1、酵母提取物15 g·L^-1、乙酸钠3 g·L^-1、柠檬酸铵3 g·L^-1、磷酸氢二钾6 g·L^-1、吐温80 3 mL·L^-1、初始pH值6.5、摇床转速120 r·min^-1、培养温度30°C时,Leu.lactis L2 EPS产量达到18.31 g·L^-1,比优化前提高了2.36倍,为乳酸菌EPS的规模化生产提供理论依据。

Carotenoid productivity in human intestinal bacteria Eubacterium limosum and Leuconostoc mesenteroides with functional analysis of their carotenoid biosynthesis genes

The human intestinal microbiota that comprise over 1,000 species thrive in dark and anaerobic environments.They are recognized for the production of diverse low-molecular-weight metabolites crucial to human health and diseases.Carotenoids,low-molecular-weight pigments known for their antioxidative activity,are delivered to humans through oral intake.However,it remains unclear whether human intestinal bacteria biosynthesize carotenoids as part of the in-situ microbiota.In this study,we investigated carotenoid synthesis genes in vari-ous human gut and probiotic bacteria.As a result,novel candidates,the crtM and crtN genes,were identified in the carbon monoxide-utilizing gut anaerobe Eubacterium limosum and the lactic acid bacterium Leuconostoc mesenteroides subsp.mesenteroides.These gene candidates were isolated,introduced into Escherichia coli,which synthesized a carotenoid substrate,and cultured aerobically.Structural analysis of the resulting carotenoids re-vealed that the crtM and crtN gene candidates of E.limosum and L.mesenteroides mediate the production of 4,4′-diaponeurosporene through 15-cis-4,4′-diapophytoene.Evaluation of the crtE-homologous genes in these bacteria indicated their non-functionality for C40-carotenoid production.E.limosum and L.mesenteroides,along with the known carotenogenic lactic acid bacterium Lactiplantibacillus plantarum,were observed to produce no carotenoids under strictly anaerobic conditions.The two lactic acid bacteria synthesized detectable levels of 4,4′-diaponeurosporene under semi-aerobic conditions.The findings highlight that the obligate anaerobe E.limo-sum retains aerobically functional C30-carotenoid biosynthesis genes,potentially with no immediate self-utility,suggesting an evolutionary direction in carotenoid biosynthesis.(229 words)

Effects of mixed inoculation of Leuconostoc citreum and Lactobacillus plantarum on suansun(Sour bamboo shoot)fermentation

To study the effects of mixed starter consisted of different fermentative type of lactic acid bacteria(LAB)on the fermentation of suansun,two lactic acid bacteria(Leuconostoc citreum NM-12 and Lactobacillus plantarum L01)isolated from Chinese traditional fermented vegetable were used in the preparation of suansun.The fermentation was carried out at ambient temperature(around 25℃)for 96 h by inoculating different mixing ratios of LAB(inoculated fermentation)or using natural microbes(natural fermentation).The changes of pH,titratable acid(TA),microbe communities,free sugars,organic acids,nitrite and volatile compounds during fermentation were evaluated.Suansun treated with high Leuconostoc citreum ratio inoculation exhibited a quickly change in pH and TA,resulting from the rapid increase in the number of viable cells,at the early stage of fermentation and produced more mannitol(0.12–0.46 mg/mL)and acetic acid(0.93–3.56 mg/mL).However,Suansun treated with high Lactobacillus plantarum ratio inoculation had lower pH and higher TA at the later stage of fermentation and produced more lactic acid(5.32–7.68 mg/mL).No mannitol was detected in suansun when only Lactobacillus plantarum was inoculated in fermentation.No p-cresol was produced in the inoculated fermentation with mixed starter culture,in addition to the production of ethyl acetate and 2.3-butanedione,which had a positive effect on the flavor of suansun.In summary,this study demonstrated the application value of mixed starter consisted of different fermentative type of LAB.LAB types and mixing ratios greatly affected the types and concentration of metabolites in suansun fermentation.

Fermentative production of dextran using Leuconostoc spp. isolated from fermented food products

Leuconostoc spp. （LSland LI1） isolated from sauerkraut and idli batter was selected for dextran production. To enhance the yield of dextran, effects of various parameters such as sucrose concentration, pH, temperature, incubation and inoculum percentage were analyzed. The optimum sucrose concentration for the Leuconostoc spp. （LS1 and LI1） was found to be 15% and 25% respectively. Isolates produced maximum dextran after 20 h of incubation at 29℃ and the optimum pH was found between 8 and 8.5. The inoculum concentration of 7.5% was more favorable for the production of dextran by Leuconostoc spp. （LS1 and LI1）. The growth kinetic parameters were studied and compared for the strains LS1 and LI1. Mass production of dextran was carried out using a stirred tank batch reactor. FTIR analysis was done to determine the functional groups of dextran, sephadex is prepared by cross linking dextran using epichlorohydrin and the functional groups are determined by FTIR analysis.

Spatiotemporal variations of sand hydraulic conductivity by microbial application methods

The spatiotemporal distributions of microbes in soil by different methods could affect the efficacy of the microbes to reduce the soil hydraulic conductivity.In this study,the specimens of bio-mediated sands were prepared using three different methods,i.e.injecting,mixing,and pouring a given microbial so-lution onto compacted sand specimens.The hydraulic conductivity was measured by constant-head tests,while any soil microstructural changes due to addition of the microbes were observed by scan-ning electron microscope(SEM)and mercury intrusion porosimetry(MIP)tests.The amount of dextran concentration produced by microbes in each type of specimen was quantified by a refractometer.Results show that dextran production increased exponentially after 5-7 d of microbial settling with the supply of culture medium.The injection and mixing methods resulted in a similar amount and uniform dis-tribution of dextran in the specimens.The pouring method,however,produced a nonuniform distri-bution,with a higher concentration near the specimen surface.As the supply of culture medium discontinued,the dextran content near the surface produced by the pouring method decreased dramatically due to high competition for nutrients with foreign colonies.Average dextran concentration was negatively and correlated with hydraulic conductivity of bio-mediated soils exponentially,due to the clogging of large soil pores by dextran.The hydraulic conductivity of the injection and mixing cases did not change significantly when the supply of culture medium was absent.

在明串珠菌构建高产甘露醇的细胞工厂

甘露醇是一种具有多种功效的六糖醇,被广泛应用于医药、食品、化工和电子等行业。为构建高产甘露醇的明串珠菌,建立了将底盘细胞转化为高产目标产物菌株的理论:细胞工厂的“源-库”学说。通过2次同源重组,打破染色体中基因的操纵子和重叠基因模式,并将甘露醇外排泵蛋白(mannitol efflux pump,MEP)基因序列和再生NADH的酶(甲酸脱氢酶)基因序列定点插入到染色体上。蔗糖为90 g/L时,打破mep基因的操纵子和重叠基因模式的菌株甘露醇产量比原始菌株(CGMCC1.10327)提高了9.5%。原始菌株染色体上敲入一个拷贝mep基因序列的菌株,底物蔗糖能添加到120 g/L,甘露醇产量也达到55.18 g/L。CCTCC M2020762菌株染色体上敲入一个拷贝甲酸脱氢酶基因序列的菌株,底物蔗糖能添加到145 g/L,甘露醇产量也达到101.6 g/L。使细胞工厂具备更强的“源”能(NADH再生等)和更大的“库”容(提高MEP活性),实现目标产物的超高产。

乳酸菌与酵母菌联合发酵对芥菜理化性质及保藏期品质的影响

为了探究肠膜明串珠菌(Leuconostoc mesenteroides)L5与少孢哈萨克斯坦酵母(Kazachstania exigua)M1联合发酵对低盐低酸发酵芥菜发酵过程及保藏期理化性质的影响,本研究将其与自然发酵组和乳酸菌L5单独发酵组进行了对比,测定了发酵过程及保藏期的pH、总酸、总酯和亚硝酸盐含量等指标,分析了发酵成熟泡菜和加速保藏泡菜的质构和色差,并进行了感官评定。结果表明,L5+M1共发酵组在发酵成熟时亚硝酸盐含量最低为1.45 mg/kg,总酸含量(2.46 g/kg)显著低于其他两组(P<0.05),总酯含量(3.79 g/kg)和感官评分均显著高于其他两组(P<0.05);成品在37℃加速保藏75 d后,总酸含量仅增加至3.10 g/kg、总酯含量增加至4.16 g/kg、亚硝酸盐含量进一步降至0.91 mg/kg,仍能维持低酸状态和较好的感官、质构和色泽品质。本研究证明了添加合适的酵母菌与乳酸菌联合发酵不仅能提升泡菜的风味和品质,对维持其保藏性也有一定作用。

柠檬明串珠菌KM20中D-乳酸脱氢酶的特性

目的:分析柠檬明串珠菌中D-乳酸脱氢酶(D-LDH)的酶学特性。方法:对柠檬明串珠菌KM20中D-乳酸脱氢酶基因进行克隆表达并构建表达质粒,转化至Escherichia coli BL21(DE3)中实现过表达。结果:经Ni-NTA柱亲和层析纯化后,D-LDH-1与D-LDH-2编码的蛋白分子质量分别为40.0,38.5 kDa;比活力分别为2.18,153.10 U/mg;在丙酮酸还原中两种酶的最适pH值与最适温度均为8.0与40℃;而乳酸氧化时D-LDH-2的最适pH值与最适温度分别为12.0与30℃。D-LDH-1与D-LDH-2对草酰乙酸、苯丙酮酸和2-酮戊二酸具有较强的催化能力,且Ca^(2+)、Cu^(2+)和Na+对其酶活性均具有促进作用,Zn^(2+)与SDS对酶活性有极高的抑制作用。此外,两种酶对丙酮酸的Km值分别为2.98,6.11 mmol/L,对丙酮酸的K_(cat)/K_(m)分别为6.04×10^(2),2.28×10^(4)L/(mol·s),LDH-2对D-乳酸的K_(cat)/K_(m)为65.0 L/(mol·s)。结论:D-LDH-1与D-LDH-2为柠檬酸明串珠菌中催化D-乳酸合成的关键酶。

肠膜明串珠菌葡聚糖蔗糖酶的生物信息学分析

葡聚糖蔗糖酶是一种糖苷转移酶(Glucosyltransferase,GTF),可以催化蔗糖合成胞外多糖(Exopolysaccharides,EPS)。由于葡聚糖蔗糖酶来源和催化中心的氨基酸序列不同,所以其合成的EPS的结构和性质存在差异。解析GTF的结构和催化机制是探究EPS生物合成和构效关系的关键。本研究利用生物信息学方法对肠膜明串珠菌(Leuconostoc mesenteroides,Ln.mesenteroides)GtfA蛋白序列进行结构和性质分析。结果表明,GtfA属于GH70家族,是一种位于细胞外的亲水蛋白,存在跨膜区,含有19个开放阅读框和7个保守区域,与Ln.mesenteroides CBA3607 Gtf相似性为100%。该蛋白具有一般葡聚糖蔗糖酶的“桶”状结构,其活性口袋能够与蔗糖紧密结合,催化蔗糖合成EPS。本研究结果可为后期探究葡聚糖蔗糖酶的结构和功能提供参考和依据。

1株甜菜糖蜜源高产胞外多糖明串珠菌的分离鉴定、发酵工艺优化及抗氧化活性研究

为挖掘甜菜糖蜜中高产胞外多糖乳酸菌菌种资源,对分离自甜菜糖蜜中的1株产胞外多糖菌株M1进行分类鉴定,分析其生长特性;采用单因素试验结合Box-Behnken响应面法优化该菌株利用甜菜糖蜜作为底物发酵胞外多糖的发酵工艺参数,并对提取的粗胞外多糖的抗氧化活性进行分析。结果表明:菌株M1为明串珠菌属的苏奥古姆明串珠菌(Leuconostoc suionicum),其延滞期短(仅2 h),最适生长温度为35℃,最适pH值为8.0,最高可耐受质量分数为60%的蔗糖;优化后的胞外多糖发酵培养基为甜菜糖蜜300.0 g/L,酵母粉20.0 g/L,K 2HPO_(4)·3H_(2)O 15.0 g/L,MgSO_(4)·7H_(2)O 0.2 g/L,NaCl 0.01 g/L,CaCl_(2)·2H_(2)O 0.01 g/L,MnSO_(4)·4H_(2)O 0.01 g/L,FeSO_(4)·7H_(2)O 0.01 g/L;最优发酵工艺参数为装液量200 mL/250 mL、接种量5%、初始pH值8.1、发酵温度38.5℃、发酵时间41.1 h,此条件下的胞外多糖产量最高,为39.1 g/L;菌株M1所产胞外多糖具有良好的抗氧化活性,质量浓度为6.0 mg/mL的胞外多糖对DPPH自由基、·OH自由基和ABTS+自由基的清除率分别为70.25%、47.16%和35.92%,对Fe^(3+)的总还原力为0.42。菌株M1能够利用甜菜糖蜜发酵生产具有较好抗氧化活性的胞外多糖,在生物转化甜菜糖蜜生产功能性胞外多糖产品方面具有良好的应用前景。

发酵蔬菜来源具抑菌活性明串珠菌的筛选及其细菌素基因簇挖掘

为提高发酵蔬菜的安全性和保藏性,从来自云南传统发酵蔬菜的8株明串珠菌中筛选出1株对食源性致病菌和引起泡菜过酸化的细菌抑制效果好的肠膜明串珠菌AP7。通过排除酸和H2O2影响及蛋白酶敏感性确定AP7的主要抑菌物质,分析其酸稳定性和热稳定性,根据AP7的全基因组序列挖掘潜在的细菌素基因簇。结果表明:排除酸及H2O2的影响后,菌株的发酵上清液仍具有明显抑菌活性,经蛋白酶处理后,抑菌效果明显下降,推测AP7发酵上清液浓缩液中的抑菌物质为细菌素;该细菌素对pH变化敏感,热稳定性高,分子质量在6.51~14.4 kDa;全基因组测序表明,菌株AP7全基因组包含1条染色体(1948310 bp)和2个质粒(37366和20698 bp),GC含量37.7%;存在1个以Enterocin_X_chain_beta细菌素为核心的基因簇,其编码产物预测为带正电的亲水性稳定蛋白,二级结构以α-螺旋为主,三级结构主要由两端松散肽链和中间α-螺旋构成。综上,产细菌素的肠膜明串珠菌AP7具有优良抑菌性能,有潜力应用于酸性食品的发酵和防腐。

肠膜明串珠菌二鸟苷酸环化酶生物信息学分析

环二鸟苷酸(Cyclic diguanosine monophosphate,c-di-GMP)可以调控细菌的生存优势,从而使细菌适应环境的改变。二鸟苷酸环化酶(Diguanylate cyclase,DGC)可以通过催化2个GTP分子合成c-di-GMP,虽然不同来源的DGC的催化功能类似,但是催化方式及调控通路存在较大差异,因此表征新来源的DGC具有重要的意义。以肠膜明串珠菌(Leuconostoc mesenteroides,Ln.mesenteroides)DRP105中的DGC序列为基础,进行了生物信息学分析。结果表明,DGC含有5个开放阅读框和1个保守结构域,并且与Ln.mesenteroides CBA3607中含有GGDEF结构域的蛋白高度相似。理化性质分析结果表明,DGC是一种定位于细胞膜上的亲水蛋白,存在6段跨膜螺旋结构。结构预测结果显示,DGC含有3段保守序列,主要由α-螺旋和β-折叠组成,含有GGEEF结构域和Mg 2+结合位点。分子对接结果表明,2个GTP分子与c-di-GMP的活性口袋稳定结合。本研究结果可为后续深入探索Ln.mesenteroides DGC的催化功能提供理论基础。

生物信息学分析葡聚糖蔗糖酶的结构和功能特性

葡聚糖蔗糖酶是一种重要的糖基转移酶(Glucosyltransferase,GTF),对于乳酸菌合成胞外多糖具有关键作用,能够以蔗糖为底物合成葡聚糖或低聚糖,是乳酸菌(Lactic acid bacteria,LAB)合成胞外多糖(Exopolysaccharide,EPS)的关键酶蛋白。然而乳酸菌代谢系统复杂,EPS生物合成机制未得到全面解析,限制了EPS的应用。为了进一步解析乳酸菌EPS的生物合成机制,表征不同来源葡聚糖蔗糖酶的结构,探明酶的催化调控机制是必要手段。本研究以肠膜明串珠菌(Leuconostoc mesenteroides)DRP105的葡聚糖蔗糖酶gtfB基因为目标序列,利用生物信息学技术对葡聚糖蔗糖酶GtfB结构和功能进行了预测分析。研究结果显示:GtfB属于GH70家族,是一种胞外酶,不存在跨膜区,含有7个保守区域和39条重复序列。其理论分子量为308986.21,理论等电点为4.59,属于酸性蛋白质。磷酸化位点含110个Thr、89个Ser、53个Tyr,GtfB含有5个结构域,呈U型折叠,活性中心在A结构域,含有(β/α)8桶状结构。分子对接预测分析表明,蔗糖与GtfB的活性口袋结合紧密。这些结果初步探明了GtfB具有葡聚糖蔗糖酶的特征结构和功能,证明其在乳酸菌EPS合成途径中的关键调控作用,为其在EPS生产过程中的应用提供了理论基础。

产D-乳酸假肠膜明串珠菌生长特性分析

研究假肠膜明串珠菌(Pseudomesenteroides leuconostoc)在不同条件下的生长特性,结果表明,假肠膜明串珠菌最适生长温度为35℃,最适p H为6.5;代谢生成D-乳酸的适宜发酵条件为4%初始葡萄糖,6%的接种量,35℃有助于发酵产酸,35℃条件下耗糖速度最快。

酿酒酵母产D-乳酸重组菌的构建与发酵

采用基因工程方法对酿酒酵母进行代谢改造,使酵母产生乳酸代谢途径。将来源于L.mesenteroides和E.coli的D-乳酸脱氢酶基因,分别插入带有G418抗性的酵母穿梭质粒p YX212-kan MX上,电转化酵母,得到2株生产D-乳酸的酿酒酵母重组菌S.cerevisiae WE1510和S.cerevisiae WB1186。进一步摇瓶发酵试验表明:重组菌S.cerevisiae WB1186在YEPD培养基、20 g/L糖、p H 5的条件下生长条件最好,并具有更好的产乳酸能力。经3 L发酵罐条件下验证,S.cerevisiae WB1186分批发酵96 h,最终乳酸积累量达到18.0 g/L;发酵条件为培养基YEPD,接种量10%,溶解氧(DO)30%,转速150 r/min,初始葡萄糖质量浓度10 g/L,控制pH 5.0,通气量3 L/min,OD600最大值转为厌氧发酵。

发酵法生产右旋糖酐的工艺研究

文章对由肠膜状明串珠菌L.M-0326(Leuconostocmesenteriodes)发酵生产右旋糖酐的工艺过程及条件进行了探讨,通过对其发酵过程中的粘度、pH值、果糖、右旋糖酐生成和分子量变化的研究及对发酵诱导物的考察,得到了右旋糖酐发酵工艺的相关工程曲线。结果表明:通过定向发酵技术可得到符合要求的不同分子量的右旋糖酐,避免了老工艺中酸水解工艺;控制发酵培养基pH值为8.0,可使产率最大;无机盐离子Mn2+和Ca2+能促进L.M菌的生长,其促进菌生长的程度大小依次为:Mn2++Ca2+>Mn2+>Ca2+。

泡菜纯种发酵优良乳酸菌的筛选及菌株特性研究

从不同时期的新鲜泡菜汁中分离得到18株乳酸菌,筛选出2株发酵萝卜产酸能力强、风味好、亚硝酸盐含量低的菌株,经鉴定分别为肠膜明串珠菌肠膜亚种和戊糖乳杆菌。对这2株菌生长特性的测试结果表明:2株菌的生长温度范围较宽,最适生长温度均为37℃,最适生长pH值均为6~8,肠膜明串珠菌对酸度和盐度的耐受性比戊糖乳杆菌差,肠膜明串珠菌在pH值【4和盐浓度】8%时生长停滞,戊糖乳杆菌能够耐受pH值【3和盐浓度】8%的生长条件。肠膜明串珠菌和戊糖乳杆菌在MRS培养基中对初始亚硝酸盐的降解率分别为84.96%和93.17%。