Molecular Verification of Two Potent Bacteria Isolated from Darfiyeh Cheese: <i>Lactococcus lactis</i>Subsp. <i>Lactis</i>and <i>Lactobacillus plantarum</i>

Raw goat milk cheeses are known for their natural microflora linked to many biodiversity factors such as the use of raw milk. That microflora serves probiotic attribution conferring a beneficial health impact on the consumer. Darfiyeh is an artisanal raw goat milk cheese manufactured traditionally in Northern Lebanese Mountains. To emphasize its clinical significance in both digestive and immune system, and to provide health remunerations to the consumer, the cheese microbiota will be investigated. To serve that purpose, the presence of the two potent probiotic Lactic Acid Bacteria (LAB): Lactococcus lactis subsp. lactis and Lactobacillus plantarum will be investigated. For bacterial identification, selection and isolation: culture-dependent techniques that imply the use of laboratory media will be implemented, and culture independent techniques: Polymerase Chain Reaction (PCR) will be applied for further validation. Both bacteria were further verified as Lactococcus lactis subsp. lactis and Lactobacillus plantarum by implementing specie-specific primers for the qualitative PCR.

Inhibition mechanisms of secretome proteins from Paenibacillus polymyxa Kp10 and Lactococcus lactis Gh1 against methicillin-resistant Staphylococcus aureus and vancomycin-resistant Enterococcus

Objective:To determine the inhibition mechanisms of secretome protein extracted from Paenibacillus polymyxa Kp10(Kp10)and Lactococcus lactis Gh1(Gh1)against methicillin-resistant Staphylococcus aureus(MRSA)and vancomycin-resistant Enterococcus(VRE).Methods:The sensitivity and viability of MRSA and VRE treated with secretome proteins of Kp10 and Gh1 were determined using minimal inhibitory concentration,minimum bactericidal concentration,and time-to-kill assays.The morphological changes were observed using scanning electron microscopy and transmission electron microscopy.To elucidate the antimicrobial mechanism of secretome protein of Kp10 and Gh1 against MRSA and VRE,2D gel proteomic analysis using liquid chromatography-mass spectrometry was run by comparing upregulated and downregulated proteins,and the proton motive force study including the efflux of ATP,pH gradient,and the membrane potential study were conducted.Results:MRSA and VRE were sensitive to Kp10 and Gh1 secretome protein extracts and displayed apparent morphological and internal composition changes.Several proteins associated with cellular component functions were either downregulated or upregulated in treated MRSA and VRE by changing the membrane potential gradient.Conclusions:Kp10 and Gh1 secretome proteins reduce the growth of VRE and MRSA by damaging the cell membrane.Cell division,cell wall biosynthesis,and protein synthesis are involved in the inhibition mechanism.

Prevalence of Clostridium spp.,in Kashar cheese and efficiency of Lactiplantibacillus plantarum and Lactococcus lactis subsp.lactis mix as a biocontrol agents for Clostridium spp.

Clostridium sporogenes and Clostridium tepidium strains were detected in traditional Kashar cheese samples with late blowing characteristics.To control Clostridium spp.,in Kashar cheese,dairy originated Lactic Acid Bacteria(LAB)strains were tested under in vitro conditions and during Kashar production.Two strains,Lactiplantibacillus plantarum and Lactococcus lactis subsp.lactis demonstrated anticlostridial activity in vitro and the co-inoculum of these two strains(107 cfu g^(-1))were tested during the challenge test on Kashar cheese production in which a contamination ratio of 10^(4) cfu g^(-1) with spores of Cl.sporogenes were applied.Kashar samples were stored at 4℃ and 25℃ during 40 days of storage period and microbiological and physicochemical properties of Kashar samples were determined during this period.A decrement of nearly 1 log cfu g^(-1) in Cl.sporogenes numbers was observed in Kashar samples produced with co-inoculum of Lb.plantarum and L.lactis subsp.lactis stored at 4℃ but this was not the case for the Kashar samples stored at 25℃.This study revealed the potential of distinct LAB strains to control Cl.sporogenes spores in semi-hard cheese samples as biocontrol agents at 4℃ storage.

乳酸乳酸球菌AL2产生的乳链菌肽的提纯和性质

用NaCl饱和的乳酸乳酸球菌(Lactococcus lactis subsp. lactis)AL2发酵液经正丙醇提取和CM-Sephadex C-25柱层析,得到聚丙烯酰胺凝胶电泳纯的乳链菌肽组分,比活力从24427IU/mg提高到39865IU/mg,活力回收为41.7％。α—胰凝乳蛋白酶可使乳链菌肽丧失活性;在低pH条件下,乳链菌肽对热较稳定;对许多革兰氏阳性菌有强烈抑制作用,而对革兰氏阴性菌、酵母菌和霉菌没有作用。

乳酸乳球菌发酵液中乳链菌肽的分离纯化

对乳酸乳球菌乳酸亚种SQ80随pH的改变吸附乳链菌肽的规律进行了研究,pH6.5时吸附率达91.5%,pH3以下吸附率为0。通过调整pH,使乳酸乳球菌选择性地吸附、释放乳链菌肽,达到了较好的分离纯化效果,HPLC检测显示单一尖峰,乳链菌肽回收率58.2%,纯化倍数75。

固定化乳酸乳球菌连续生产Nisin的研究

以海藻酸钙为材料 ,固定乳酸乳球菌 (Lactococcuslactissubsp .lactis)SM5 2 6 ,研究不同条件对Nisin合成的影响。结果表明 ,利用 2 %海藻酸钠在 1 0mmol LCaCl2 条件下 ,得到的固定化细胞颗粒稳定性较好 ,可维持 90h无破裂 ;在发酵过程中SYS3培养基中的无机盐成分尤其磷酸盐对固定化颗粒有破坏作用 ;用mSYS3培养基代替SYS3 ,通过 72h三批次循环的半连续培养 ,Nisin活性为 85 0IU mL ,无明显的细胞渗漏现象。连续化生产 70h ,Nisin活性达 1 1 5 0IU mL ,相当于游离细胞的发酵水平。

乳酸菌在大豆黄浆水中发酵条件的优化

以乳酸乳球菌乳亚种为发酵菌株,大豆黄浆水为培养基质,产酸量、pH值为考察指标,探讨不同发酵温度、发酵时间、种子液接种量、葡萄糖添加量对乳酸乳球菌乳亚种在黄浆水中发酵产酸的影响。在单因素试验的基础上,采用均匀设计法对其发酵条件进行优化,并对产酸量进行二次多项式逐步回归分析。结果表明,乳酸乳球菌乳亚种在黄浆水中最适发酵条件为发酵温度35℃、种子液接种量9%(V/V)、发酵时间68h、葡萄糖添加量5%(m/V)、初始pH 6.2,该条件下产酸量达0.791 3g/100mL,pH为3.40。

冷鲜调理肉三种乳酸菌发酵剂的筛选

为筛选出符合冷鲜调理肉制品发酵的优质乳酸菌发酵剂,对3株乳酸菌的发酵特性进行研究,通过耐盐、耐亚硝酸盐、产粘、产酸能力、蛋白质和脂肪分解能力、菌种间的拮抗作用等试验对其进行优势菌种筛选。结果表明,菌株LLSL、LP、LGG对食盐和亚硝酸盐具有较好的耐受性,能在6%的食盐溶液和150 mg/L亚硝酸盐溶液中存活,能有效产酸,无降解蛋白质和脂肪能力,不产气、不产氨、不产H_2S;其中,菌株LLSL、LP不产粘,两者间无拮抗作用,可作为于冷鲜调理肉制品的发酵剂;菌株LGG产粘,影响冷鲜调理肉制品的感官品质和内部组织状态,不适合作为冷鲜调理肉制品的发酵剂。

固定化乳酸乳球菌DL-203发酵生产Nisin的研究

对用固定化乳酸乳球菌DL-203发酵生产Nisin进行了研究。确定采用k-卡拉胶作为固定化载体,并添加磷酸三钙,包埋固定化乳酸乳球菌DL-203发酵生产Nisin。固定化最适条件为3.5%(W/V)k-卡拉胶+0.1%(W/V)磷酸三钙,细胞浓度5%～10%(V/V)。发酵培养基添加0.2%(V/V)吐温-20,30℃摇床培养进行分批重复发酵,可连续使用五批以上,而发酵液Nisin效价未有下降,达游离细胞发酵液的50%～60%。采用柱式填充床反应器进行固定化乳酸乳球菌DL-203连续发酵生产Nisin,停留时间以4～6h比较适宜,可连续稳定生产150h以上,而且固定化小球未有明显的细胞外漏,发酵液Nisin效价可达游离细胞发酵液的30%～40%。

乳酸菌胞外多糖的纯化及对小鼠血清和肝组织抗氧化性的影响

本实验对乳酸乳球菌乳亚种胞外多糖的纯化工艺及其抗氧化活性进行研究。纯化结果表明,选择DA201-C树脂,调节胞外多糖的pH值为3.5,在45℃条件下,树脂用量为2%(V/V),静态吸附20h后糖保留率为81.56%,蛋白脱除率为72.09%,脱色率为81.69%。通过动物实验,检测小鼠血清和肝组织中的过氧化氢酶(CAT)活力、丙二醛(MDA)含量、超氧化物歧化酶(SOD)活力可知,灌胃胞外多糖组的小鼠与对照组小鼠相比,抗氧化能力显著性提高。

1株乳酸链球菌素产生菌的筛选鉴定及其抑菌特性的研究

从白菜叶上分离得到21株对乳酸链球菌素(Nisin)有抗性的乳酸菌株,采用杯碟法从中筛选得到抑菌活性较强的菌株T0625,经鉴定该菌株为乳酸乳球菌乳酸亚种(Lactococcus lactis subsp.Lactis)。经测定,发酵液经加热处理,在低pH条件下能够保持较好的抑菌活性,对革兰氏阳性细菌具有明显的抑制作用,但对革兰氏阴性细菌、酵母菌和霉菌不表现抑制作用。研究还证实,T0625的发酵产物的抑菌活性不受胃蛋白酶和胰蛋白酶的影响。经提取纯化,确定抑菌物质为乳酸链球菌素。

以乳清为原料采用混菌发酵技术促进Nisin生产的研究

采用了一种不用外加碱或移除乳酸来达到控制发酵液中乳酸的新技术,即采用乳酸菌和酵母菌的混和发酵来控制pH值以促进乳酸链球菌素(nisin)的生产。其原理是乳酸菌在发酵生产nisin的过程中所产生的乳酸可以被酵母菌利用,从而达到控制发酵液pH值的目的;同时,混菌培养选用的酵母菌不能利用乳清培养基中的乳糖,从而避免了2株菌之间对碳源的竞争,创造了一个互利共生的微生态环境,从而达到促进nisin生产的目的。实验表明,乳酸根的积累对nisin发酵生产具有抑制作用;混合发酵的酵母菌利用了发酵液中的乳酸,促进了乳酸菌生长和nisin生产;酵母菌较乳酸菌提前3h接入到发酵培养基中时,能更好地控制pH值;最佳的接种比例为乳酸菌3%,酵母菌5%。

营养因素对乳酸乳球菌DL-203生长及其Nisin生物合成的影响

对Nisin高产菌株乳酸乳球菌DL—203的营养要求及其 对Nisin生物合成的影响进行了研究。结果表明,乳链菌 肽的生物合成与DL-203的生长呈极显著正相关,乳酸 乳球菌DL—203生长和合成Nisin的最佳碳源和氮源分 别为蔗糖和大豆蛋白胨,其适宜浓度均为15～20g/L。磷 酸盐对乳酸乳球菌DL—203生长及其Nisin生物合成具 有极大的促进作用,其中以Na_2HPO_4效果最好,其浓度 在224mmol/L以下时对菌体生长和Nisin生物合成具有 较大的促进作用。

乳酸乳球菌SM526产生乳链菌肽的营养调控(英文)

自酸泡菜中分离并鉴定了一株产生乳链菌肽的菌株 -乳酸乳球菌 (Lactococcuslactissubsp .lactis)SM5 2 6 .研究了不同种类与浓度的碳源、氮源和磷源对该菌产生乳链菌肽的影响 ,结果表明乳链菌肽的生物合成受碳源、氮、磷源的调控 ,蔗糖和磷酸二氢钾分别为其最佳碳源和磷源 ,大豆蛋白胨和酵母粉为其理想氮源 .利用分批培养研究乳链菌肽合成的代谢动力学则表明 ,乳链菌肽在SM5 2 6菌株的指数生长期产生 ,到指数生长期末期达到高峰 ,进入稳定期逐渐停止产生 ,表现出一种初级代谢动力学特征 .以植物乳杆菌 (Lactobacillusplantarum)作指示菌株则表明乳链菌肽对细菌的作用方式是杀菌 .图 3表 5参

亚硝基胍诱变选育丁二酮高产菌株

以乳酸乳球菌乳酸亚种丁二酮变种为出发菌株,采用亚硝基胍进行诱变选育,得到高产丁二酮菌株,用邻苯二胺比色法检测突变株丁二酮,其产量达到0.72mg/L,比出发菌株产量0.056mg/L提高12.9倍,且遗传性质稳定。

乳酸乳球菌乳酸亚种T0625菌株产Nisin最佳培养条件的研究

对从大白菜叶片上分离得到的一株乳酸乳球菌乳酸亚种T0625产乳酸链球菌素(Nisin)的适宜培养条件进行了研究。采用单因素分析法首先确定了T0625菌株在改良的M17G培养基中产Nisin的最适碳源、氮源、金属离子的种类,即:碳源为葡萄糖;氮源为蛋白胨、酵母膏和牛肉膏组成的混合氮源;金属离子为Mg2+。并确定了各成分的最适浓度。之后确定了装液量、接种量、起始pH和培养温度的最适指标。最终通过正交试验的方法,确定T0625产Nisin的最佳营养条件:葡萄糖2%、蛋白胨4%、酵母膏2%、牛肉膏1%、MgSO4.7H2O0.003 mol/L、VC0.05%。T0625产Nisin的最佳发酵条件:装液量250 mL(250 mL三角瓶)、接种量7%、起始pH 6.5、35℃下发酵培养12 h。

乳酸乳球菌细胞壁蛋白酶的分离纯化

本研究确定了分离纯化乳酸乳球菌细胞壁蛋白酶(CEP)的最佳技术路线。用裂解液(50mmol/LTris-HCl,2mmol/LEDTA-Na2,100mmol/LNaCl,0.5%Tritonx-100,1mg/ml溶菌酶,pH8.5)悬浮菌体(20ml/g),37℃下保温3h,离心后取上清液即为粗酶液。粗酶液通过45%硫酸铵沉淀,DEAE-SephadexA-25和Sephacryl-S-300HR两步层析,可以得到纯化的细胞壁蛋白酶。蛋白酶提纯倍数达到74.048%,最后回收率为14.865%,PAGE电泳检测为一条带,SDS-PAGE检测蛋白酶为单体结构,分子量大约为53kD。用纯化后CEP酶解乳清蛋白,酶解液ACE抑制率为45%。

乳链菌肽高产菌株的选育及其生理特性

以乳酸乳酸球菌７９ＵＶＳ２２为出发菌株，用紫外线、ＤＥＳ、ＬｉＣｌ等多种理化因子进行诱变处理，获得一株乳链菌肽高产突变株ＤＬ２０３，其效价稳定在２０００ＩＵ／ｍｌ以上。对其生理特性的研究表明，ＤＬ２０３菌的生长及发酵最适温度为３０℃，最适ｐＨ值为７．９，通风可以促进菌体的生长，但对乳链菌肽的产生无影响。

乳酸乳球菌乳脂亚种高产丁二酮的条件优化

分别研究了10种不同因素对乳酸乳球菌乳脂亚种产生丁二酮质量分数的影响。结果表明,各因素产生丁二酮最高量的条件:培养温度为37℃;凝乳后3 h;后熟12 h;培养基pH值调至为5.6;培养基中添加柠檬酸氢二铵的质量浓度为0.15%;培养基中添加Vc的质量浓度为0.3%。培养基中添加金属离子的质量浓度分别为:Mg2+为0.05%,Cu2+为0.04%,Mn2+为0.001%;培养基中添加甘氨酸的质量浓度为1.7%(均为质量分数);培养基中添加碳水化合物的质量浓度分别为:葡萄糖为1%,蔗糖为1.5%(均为质量分数);随着基质浓度增加丁二酮产量也随之增加。

乳酸乳球菌乳脂亚种IMAU60064增殖培养基的优化

以分离自西藏那曲县罗玛镇传统发酵酸牦牛奶中的乳酸乳球菌乳脂亚种（Lactococcus lactis subsp．Cremoris）IMAU60064为试验菌株，研究其最佳的培养条件。对碳源、氮源、缓冲盐等培养基成分及培养条件进行优化，并采用响应面法对优选的碳源、氮源和缓冲盐类的组成含量进行优化，得到IMAU60064的增殖培养基为：葡萄糖23g／L、大豆蛋白胨11g／L、牛肉膏11g／L、胰蛋白胨5g／L、NaAC1．8g／L、K2HP041．2g／L、柠檬酸钠1．2g／L、MgSO4·7H200．4g／L、MnSO4·5H2O54mg／L、L-半胱氨酸盐酸盐0．5g/L、吐温80为1g／L。Lactococcus lactis subsp．cremorisIMAU60064在此增殖培养基中经30℃，14h培养活菌数可达到3．26×10^8cFu／mL，比在MRS中（6．54×10^7CFU／mL）提高近5倍。