多型FMDV VP1表位嵌入型载体pMG-SLPMultiVP1的构建及其表达产物鉴定

构建出表达载体pMG-SLPMultiVP1,并对其进行双酶切鉴定及PCR鉴定。将阳性重组质粒转入到发酵乳杆菌中进行表达,并对表达产物进行SDS-PAGE、Western blot和IFAT鉴定。多型FMDV VP1表位嵌入的SLPMultiVP1融合基因成功克隆入穿梭质粒pMG36e中,其表达产物大小约为35ku,部分表达产物位于发酵乳杆菌表面。成功构建了一个乳杆菌嵌入型表达载体pMG-SLPMultiVP1,为以发酵乳杆菌为活菌载体的表位疫苗研究奠定了基础。     

Lactobacillus rhamnosus GG SpaC pilin subunit binds to the carbohydrate moieties of intestinal glycoconjugates

Lactobacillus rhamnosus GG (LGG) is a well‐established probiotic strain. The beneficial properties of this strain are partially dependent on its prolonged residence in the gastrointestinal tract, and are likely influenced by its adhesion to the intestinal mucosa. The pilin SpaC subunit, located within the Spa pili structure, is the most well studied LGG adhesion factor. However, the binding epitopes of SpaC remain largely unknown. The aim of this study was to evaluate the binding properties of SpaC to the carbohydrate moieties of intestinal glycoconjugates using a recombinant SpaC protein. In a competitive enzyme‐linked immunosorbent assay, SpaC binding was markedly reduced by addition of purified mucin and the mucin oligosaccharide fraction. Histochemical staining revealed that the binding of SpaC was drastically reduced by periodic acid treatment. Moreover, in the surface plasmon resonance‐based Biacore assay, SpaC bound strongly to the carbohydrate moieties containing β‐galactoside at the non‐reducing terminus of glycolipids. We here provide the first demonstration that SpaC binds to the oligosaccharide chains of mucins, and that the carbohydrate moieties containing β‐galactoside at the non‐reducing termini of glycoconjugates play a crucial role in this binding. Our results demonstrate the importance of carbohydrates of SpaC for mucus interactions.     

乳酸杆菌LH对水产常用药物的敏感性

采用试管法,以金黄色葡萄球菌ATCC25922为质控菌,研究乳酸杆菌LH菌株对氟苯尼考、土霉素、二氧化氯、二溴海因、强力碘的敏感性。结果显示,在5.0×105cfu/mL时,最小抑菌浓度分别为2μg/mL、4μg/mL、16μg/mL、32μg/mL、32μg/mL,最小杀菌浓度分别为16μg/mL、64μg/mL、128μg/mL、128μg/mL、128μg/mL;最小抑菌浓度随着菌悬液浓度(104~107cfu/mL)的增大而升高;在杀菌曲线中,药物对菌的抑制作用随着作用时间的延长而逐渐减弱。     

油茶籽提取废液中乳酸菌的分离鉴定与发酵性能

从自然发酵的油茶籽提取废液中发现1种产乳酸的细菌.以一定时间内产乳酸量的多少和耐酸性强弱为指标,经分离纯化、鉴定后初步确定为乳酸杆菌属微小乳杆菌种变种.采用接种量3%,发酵时间48h,发酵温度38℃的发酵条件测试此菌种的发酵产酸量及活菌数,其48h产酸量可达2.02%,生长稳定期活菌密度达1011cfu/mL,为具有工业利用价值的优良乳酸菌种.     

表达猪细小病毒VP2蛋白的重组干酪乳杆菌的构建

利用Oligo设计合成一对引物P1、P2,分别含有BamHI和XhoI酶切位点,以猪细小病毒株LJL12的DNA为模板,采用PCR技术扩增VP2基因,克隆到pMD18-TSimple载体,并进行酶切、PCR鉴定和序列测定。将VP2基因分别亚克隆到干酪乳杆菌细胞表面表达型载体pPG1和分泌型表达载体pPG2的BamHI和XhoI酶切位点,电转化干酪乳杆菌Lactobacillus casei393,获得阳性重组菌株。成功构建了猪细小病毒VP2蛋白的干酪乳杆菌表达系统,命名为pPG1-VP2/L.casei393和pPG2-VP2/L.casei393。     

猪源发酵乳杆菌的筛选及其潜在益生性能

【目的】对从健康仔猪粪便中筛选分离出一株发酵乳杆菌的益生性能进行测试,为其在畜禽动物养殖中的应用提供参考。【方法】采用Rogosa SL完全选择性培养基分离出106株乳酸菌,通过革兰氏染色、酸和胆盐耐受初步筛选出1株潜在的饲用乳酸菌,经16S rDNA序列鉴定为发酵乳杆菌LF1,并对其益生性能潜力进行评估,包括抑菌活性(针对大肠杆菌K88、金黄色葡萄球菌、猪链球菌、沙门氏菌以及弧菌等12种病原菌)、对模拟胃液中酸性环境的耐受性、对胆盐的耐受性以及对小肠上皮细胞的粘附性。【结果】发酵乳杆菌LF1耐酸和耐胆盐的能力较强,显示出较强的益生菌潜力,但LF1菌株对猪肠道上皮细胞的粘附能力不强。在生物拮抗作用方面,发酵乳杆菌LF1的培养上清可以显著抑制多种常见动物病原菌生长。【结论】发酵乳杆菌LF1具有较好的益生性能,通过进一步的动物实验评估后,可以作为应用于畜禽养殖业的益生菌候选菌株。     

柑橘溃疡病拮抗菌的分离筛选及其田间防效

从湖南衡阳、常德、长沙、永州等地的柑橘园采集标本,分离、筛选柑橘叶表微生物,共分离到225株细菌,9株真菌.平板拮抗试验结果表明,其中6个菌株有较好的防效,占分离菌株的13.7%.通过对菌株过滤液和定殖力的测定,菌株Kx15和Kx48效果明显,在温室对柑橘溃疡病的防治效果分别达到45.6%和55.6%,在重病果园中的防治效果分别为40.3%,47.7%,且Kx48要优于Kx15.菌株Kx15初步鉴定属于葡萄糖杆菌属,Kx48属于乳酸杆菌属.     

Evaluation and characterization of a novel probiotic Lactobacillus pentosus PL11 isolated from Japanese eel (Anguilla japonica) for its use in aquaculture

In the present study, a potential Lactobacilli probiotics were isolated from Japanese eels (Anguilla japonica) and characterized and evaluated for their possible use in eel farming. Sixteen Lactobacilli were isolated from intestines of Japanese eels, using selective media. The lactobacilli strains (represented as PL1 to PL16) were screened by their ability to produce digestive enzyme. Among these, three strains (PL11, PL13 and PL16) producing four digestive enzymes (amylase, cellulase, protease and phytase) simultaneously were characterized further using API ZYM kit. From these, PL11 (Lactobacillu (L.) pentosus) was identified as potential probiotics candidate producing 15 enzymes among 20 tested. Further examination of biological activities of PL11 revealed tolerance against pH, artificial bile juice and antibacterial activity against several fish pathogenic bacteria. The in vitro competitive exclusion assay also revealed 88.4% reduction in adhesion of fish pathogen (Edwardsiella tarda) by PL11 to host intestinal mucus. In vitro incubation of Japanese eel foregut with Baclight‐labelled PL11 showed colonization of the enterocyte surface by confocal and scanning electron microscopy. In summary, PL11 isolated from eels could serve as a potential probiotics with acid and bile tolerance, production of digestive enzymes, antibacterial activity and inhibition of fish pathogen adhesion to intestinal mucus.     

团头鲂肠黏膜益生乳酸菌的分离及体外抗逆性研究

从团头鲂肠黏膜上分离筛选出2株对嗜水气单胞菌有较强的抑制作用的乳酸菌菌株JK-1和JK-2,通过耐受胆盐、耐受pH值、耐受蛋白酶和耐高温等试验对这2株乳酸菌进行体外抗逆性试验研究.其中在胆盐耐受性试验中,JK-1和JK-2在胆盐浓度0.4%、培养4 h时仍有35%以上的存活率;在pH值耐受性试验时,2株乳酸菌均可在一定的酸性和碱性条件下存活;胰蛋白酶对2株菌的存活率没有影响;在70 ℃的高温中,2株乳酸菌均有一定的耐受性.     

一株干酪乳杆菌对养殖水体亚硝酸盐去除机理的研究

为了解乳酸菌去除养殖水体亚硝酸盐的作用机理,实验研究了一株干酪乳杆菌L821a(Lactobacillus casei)对淡水鱼养殖水体亚硝酸盐的去除状况,通过对菌体、酶及代谢产物的实验,证明其去除亚硝酸盐的机理包括胞内酶作用、代谢产物乳酸的直接化学反应2H++3NO2-=NO3-+2NO↑+H2O作用和间接促进微生物反硝化作用3种作用机理。在养殖水体中主要以间接作用方式发挥作用。分析认为乳酸促进反硝化作用的原因在于为反硝化微生物提供了易于利用的有机碳源(能量物质)。