一株乳酸菌胞外多糖产生的影响因素及其提取*

应用苯酚—硫酸法对乳酸菌胞外多糖产生的影响因素进行了研究,表明该菌株在培养温度为30℃,培养时间为40~48h,pH值降到4时,胞外多糖的产量最大。葡萄糖是乳酸菌产生多糖的良好碳源。在对乳酸菌的培养物进行离心、透析、脱蛋白、脱色,最后用乙醇沉淀,得到粗品多糖,粗品多糖至少含有两种分子量和含量相差很大的多糖。经过SephadexG-200凝胶柱得到多糖精品EPS-Ⅱ,薄层层析结果显示其为一纯化的样品。     

乳酸菌胞外多糖的研究进展

乳酸菌胞外多糖是乳酸菌生长代谢过程中产生并分泌到细胞外的一种天然高分子聚合物。作为一种新型的天然食品添加剂,乳酸菌胞外多糖因其独特的生理功能和产业潜力而备受研究者青睐。但由于乳酸菌胞外多糖结构组分、功能效用的不同,很难建立一个通用的生产方法和检测标准。另外,如何提高胞外多糖产量也是未来要面临的一大挑战。从乳酸菌胞外多糖的遗传研究、结构修饰、构效关系、生物学活性几个方面进行综述,并对未来研究方向进行展望。     

抑制黑色素合成的乳酸菌胞外多糖的筛选和性质研究

【目的】筛选可抑制黑色素合成的乳酸菌胞外多糖。【方法】通过观察凝乳拉丝外观筛选产胞外多糖的乳酸菌菌株,测量胞外多糖对B16黑色素瘤细胞黑色素合成和细胞活力的影响。对胞外多糖进行纯化,并通过PMP衍生-HPLC、红外光谱、抑制酪氨酸酶活性、抗氧化能力对其单糖组成和结构、作用机制进行研究。【结果】筛选到一株乳酸菌Lactobacillus rhamnosus HLAB122,发酵产生的胞外多糖在5 g/L浓度下可使B16细胞黑色素产量下降至空白对照的32.7%,且在96 h内对细胞活力无影响。纯化后的多糖由鼠李糖、葡萄糖、半乳糖构成,各单糖摩尔比为1?5.44?5.37。该胞外多糖不抑制酪氨酸酶活力且抗氧化性微弱。【结论】L.rhamnosus HLAB122产生的胞外多糖在个人护理产品中有潜在应用价值。     

一株结皮真菌胞外多糖的初步研究

探究一株真菌胞外多糖最佳生产时间及其组成成分。通过对其发酵液胞外多糖含量及上清液黏度的测定,确定其最佳产糖时间,并用此条件提取胞外多糖粗品,用蒽酮-比色法测得提取的胞外多糖粗品的糖含量,薄层色谱法对所得的胞外多糖进行组分分析。当发酵至第5天时该株真菌的生物量、胞外多糖产量及发酵液的黏度均达到最高峰,分别为0.606 4 g/60 mL、20.22 μg/mL和4.74 mPa/s,并且胞外多糖含量与发酵上清液黏度在一定程度上呈正相关。用蒽酮-比色法测得提取的胞外多糖粗品的糖含量为19.58 μg/mL,并用4 mol/L的硫酸完全水解,硅胶G薄层层析,甲醇-氯仿(1:1,体积比）展层,苯胺-二苯胺-磷酸显色,表明其组成成分可能为D-甘露糖、D-半乳糖和D-葡萄糖。该菌株所产的胞外多糖具有提高结皮能力和防沙保水作用,为利用微生物治沙提供参考和种质资源。     

1株结皮真菌胞外多糖的初步研究

探究一株真菌胞外多糖最佳生产时间及其组成成分。通过对其发酵液胞外多糖含量及上清液黏度的测定,确定其最佳产糖时间,并用此条件提取胞外多糖粗品,用蒽酮-比色法测得提取的胞外多糖粗品的糖含量,薄层色谱法对所得的胞外多糖进行组分分析。当发酵至第5天时该株真菌的生物量、胞外多糖产量及发酵液的黏度均达到最高峰,分别为0.606 4 g/60 mL、20.22μg/mL和4.74 mPa/s,并且胞外多糖含量与发酵上清液黏度在一定程度上呈正相关。用蒽酮-比色法测得提取的胞外多糖粗品的糖含量为19.58μg/mL,并用4 mol/L的硫酸完全水解,硅胶G薄层层析,甲醇-氯仿(1:1,体积比)展层,苯胺-二苯胺-磷酸显色,表明其组成成分可能为D-甘露糖、D-半乳糖和D-葡萄糖。该菌株所产的胞外多糖具有提高结皮能力和防沙保水作用,为利用微生物治沙提供参考和种质资源。     

一株胞外多糖产生菌的筛选鉴定及其多糖成分研究

以菌落周围有粘稠分泌物为初筛标准从土壤中筛选胞外多糖产生菌,苯酚-硫酸法测定初筛菌胞外多糖的产量;将胞外多糖产生菌LE-3进行形态学观察、BIOLOG分析与16S rDNA鉴定;提取菌株LE-3胞外粗多糖,该粗多糖经Sevage法除蛋白、透析和CM-琼脂糖凝胶FF、DEAE-琼脂糖凝胶FF、丙烯葡聚糖凝胶S-200HR柱层析进行纯化,傅里叶红外光谱法、薄层层析法和高效液相色谱法分析胞外多糖的单糖组成。结果表明:从土壤中筛出26株符合初筛标准的菌株,3株产糖量在5 g/L以上,其中菌株LE-3产量为5.29 g/L;根据形态学特征、BIOLOG和分子生物学分析,初步鉴定菌株LE-3为一株解淀粉芽孢杆菌亚种(Bacillus amyloliquefaciens subsp.amyloliquefaciens);该菌株胞外粗多糖经Sevage法除蛋白、透析和三次柱层析纯化后,得到单一组分的LE-3胞外多糖;傅里叶红外光谱法、薄层层析法和高效液相色谱法分析确定该多糖为果聚糖。     

发酵乳杆菌CSC-19胞外粗多糖提取物抑制单核细胞增生李斯特菌生物被膜形成能力的研究

【目的】筛选能有效抑制单核细胞增生李斯特菌(Listeria monocytogenes,LM)形成生物被膜的乳酸菌,分析其活性成分并进行功能表征。【方法】采用结晶紫染色法筛选抑制LM形成生物被膜的不同乳酸菌提取物;通过酸中和、蛋白酶处理及热处理,推测抑制生物被膜活性物质以胞外多糖(extracellular crude polysaccharide,ECP)为主;乙醇沉淀法提取目标乳酸菌分离株胞外粗多糖,分析其抑制生物被膜形成活性和对LM生长的影响;运用激光共聚焦扫描显微镜(laser confocal scanning microscopy,LCSM)和扫描电子显微镜(scanning electron microscopy,SEM)观察胞外粗多糖对生物被膜细胞形态和结构的影响。【结果】发酵乳杆菌CSC-19发酵上清液对1516-2LM生物被膜的抑制率为81.7%;经热和蛋白酶处理后,发酵上清抑制生物被膜形成的活性未发生显著变化(P>0.05),表明发酵上清液中抑制生物被膜形成的物质可能为胞外多糖;在不抑制LM生长的条件下所提取的胞外粗多糖抑制生物被膜形成能力具有浓度依赖性。激光共聚焦扫描显微镜和扫描电子显微镜结果显示,胞外粗多糖显著抑制了生物被膜的形成能力,生物被膜三维、有组织的蜂窝状结构被破坏,仅有少量的粘附细胞分散于细胞爬片表面。【结论】发酵乳杆菌CSC-19胞外粗多糖能有效抑制LM生物被膜的形成,有望应用于高效防控该菌污染食品。     

乳酸菌胞外多糖产生菌的 筛选与初步研究

目的从牧区传统乳制品中分离获得胞外多糖产量较高的菌株,并对胞外多糖的结构和功效进行初步研究,以期能为将来生产乳酸菌胞外多糖的可行性提供数据和依据。方法通过涂布平板法从内蒙古传统发酵乳制品中分离乳酸菌,并测定胞外多糖产出量,从中筛选胞外多糖高产菌株,通过生理生化试验和16S rRNA测序鉴定菌株。采用紫外光谱法和高效液相色谱法对胞外多糖的结构进行初步分析。通过测定胞外多糖的吸湿能力和保湿能力初步评价其吸湿保湿性能。结果共分离出90株菌株,筛选出1株胞外多糖高产菌株,并鉴定出该菌株为嗜热链球菌。通过分析得出该菌株产生的胞外多糖主要由4种单糖组成,分别为甘露糖、葡萄糖、半乳糖和阿拉伯糖,其摩尔比为0.25∶3.10∶3.70∶0.10,分子量范围为1.897×10~6～7.257×10~6 Da。通过保湿性能的测定,初步确定该嗜热链球菌产生的胞外多糖有良好的保湿性。结论本实验筛选出的胞外多糖高产菌株嗜热链球菌属于益生菌,有广泛的应用价值。     

乳酸菌胞外多糖对人类肠道菌群的影响

摘要：胞外多糖（EPS）是微生物在生长代谢过程中分泌到细胞壁外及周围生长介质中的一类生物大分子物质。乳酸菌胞外多糖除了具有重要的加工优势外,如提高酸奶等乳制品的粘度、质地和口感,还具有重要的生理活性。本文重点介绍了乳酸菌胞外多糖的分类和主要生物活性,并从胞外多糖的益生元特性、作为肠道能源物质、对肠道细胞的粘附、调节肠道菌群多样性、调节肠道免疫五个方面综述了乳酸菌胞外多糖对人类肠道菌群的影响,同时对胞外多糖的后续研究提出了自己的建议。     

乳酸菌胞外多糖对人类肠道菌群的影响

胞外多糖(EPS)是微生物在生长代谢过程中分泌到细胞壁外及周围生长介质中的一类生物大分子物质。乳酸菌胞外多糖除了具有重要的加工优势外,如提高酸奶等乳制品的粘度、质地和口感,还具有重要的生理活性。本文重点介绍了乳酸菌胞外多糖的分类和主要生物活性,并从胞外多糖的益生元特性、作为肠道能源物质、对肠道细胞的粘附、调节肠道菌群多样性、调节肠道免疫五个方面综述了乳酸菌胞外多糖对人类肠道菌群的影响,同时对胞外多糖的后续研究提出了自己的建议。     

一种简单准确的L-苏氨酸测定方法

通过研究建立了发酵液中L-苏氨酸定性和定量测定的"纸层析-Rf值法"和"纸层析-色斑洗脱比色法",并对该方法的应用条件进行了研究。研究结果表明,该法对测定L-苏氨酸含量具有较高的准确度和精密度。而且该法操作简单、易于掌握,非常适合在L-苏氨酸产生菌筛选中应用。     

The production-influencing factors of extracellular polysacchadde(EPS) from a Strain of lactic acid bacteria and EPS extraction

The influencing factors of extracellular polysaccharide(EPS)produced from a strain of lactic acid bacteria(LAB L15)were studied by using the phenol-H2SO4 method.It was demonstrated that the strain produced EPS at the most amount when it was incubated for 40-48 h and when the pH value was 4 under 30℃.Glucose was the most suitable carbon source for LAB-producing EPS.The rough EPS was obtained from L15 culture after centrifugation,dialysis,deprotein,decoloration,and ethanol-precipitation.The sample was at least composed of two polysaccharides mat were completely different in molecular weight and the amount.The purified EPS was passed through the SephadexG-200 colunm and it showed that it was a sample purified by thin layer chromatography.     

The production-influencing factors of extracellular polysaccharide (EPS) from a strain of lactic acid bacteria and EPS extraction

The influencing factors of extracellular polysaccharide (EPS) produced from a strain of lactic acid bacteria (LAB L15) were studied by using the phenol-H₂SO₄ method. It was demonstrated that the strain produced EPS at the most amount when it was incubated for 40–48 h and when the pH value was 4 under 30°C. Glucose was the most suitable carbon source for LAB-producing EPS. The rough EPS was obtained from L15 culture after centrifugation, dialysis, deprotein, decoloration, and ethanol-precipitation. The sample was at least composed of two polysaccharides that were completely different in molecular weight and the amount. The purified EPS was passed through the SephadexG-200 column and it showed that it was a sample purified by thin layer chromatography. __________ Translated from Microbiology, 2005, 32(4): 85–90 [译自: 微生物学通报, 2005, 32(4): 85–90]     

Relations between extraction protocols for activated sludge extracellular polymeric substances (EPS) and EPS complexation properties: Part I. Comparison of the efficiency of eight EPS extraction methods

The efficiency of eight extracellular polymeric substances (EPS) extraction methods was compared on two different activated sludges. Three chemical methods (EDTA, formaldehyde + NaOH, glutaraldehyde), four physical methods (sonication, cation exchange resin, sonication + cation exchange resin, heating) and a control method (centrifugation alone) were tested.EPS quantities extracted were more greater for chemical methods than those for physical methods. For the chemical methods used EPS contamination due to extracting reagents was pointed out by infra-red analysis. The EPS extracted by physical methods can show a different qualitative composition with protein and carbohydrate as predominant compounds. This study therefore underlines that the choice of EPS extraction method should not only be limited to extraction yield and nucleic acid content but should also consider that the EPS solution may be contaminated by extracting reagents and/or be greatly modified by the extraction protocol.     

慢性前列腺炎患者前列腺液白细胞浓度与前列腺液尿酸 及锌含量的相关性研究

目的:探讨慢性前列腺炎患者前列腺液中白细胞(WBC)数量与前列腺液尿酸(UA)、锌(Zn)含量的关系。方法:选取慢性前列腺炎患者128例,健康对照组52例。分别进行EPS中白细胞(WBC)数量、尿酸(UA)和锌(Zn)含量测定。结果:慢性前列腺炎患者前列腺液UA含量显著高于健康对照组,Zn含量显著低于健康对照组,前列腺液中WBC数量与UA含量呈显著正相关,与Zn含量呈显著负相关(P<0.01)。2慢性前列腺炎患者治疗前后EPS中的UA和Zn对比有显著性差异。结论:EPS中的尿酸(U A)、锌(Zn)含量对慢性前列腺炎的诊断与评估疗效有一定价值。     

Detection ofAspergillus andPenicillium extracellular polysaccharides (EPS) by ELISA: using antibodies raised against acid hydrolysed EPS

Species of the fungal generaAspergillus andPenicillium produce immunologically active extracellular polysaccharides (EPS) in which galactofuranose residues are immunodominant. The antigenic determinant of the EPSA. fumigatus, A. niger andP. digitatum could be removed by acid hydrolysis. Due to the hydrolysis of the EPS the immunological reaction between IgG anti-native EPS and hydrolysed EPS disappeared. Antibodies raised in rabbits against the acid hydrolysed EPS revealed new antigenic determinants that were exposed as a result of the acid hydrolysis. Immunological inhibitory experiments showed that the antibodies were no longer directed to galactofuranose residues.Enzyme Linked Immunosorbent Assay, carried out with antibodies raised against the acid hydrolysed EPS showed that the antibodies against the acid hydrolysed EPS were more species specific in comparison with the antibodies against the native EPS.     

EPS II-Dependent Autoaggregation of Sinorhizobium meliloti Planktonic Cells

Planktonic cells of Sinorhizobium meliloti, a Gram-negative symbiotic bacterium, display autoaggregation under static conditions. ExpR is a LuxR-type regulator that controls many functions in S. meliloti, including synthesis of two exopolysaccharides, EPS I (succinoglycan) and EPS II (galactoglucan). Since exopolysaccharides are important for bacterial attachment, we studied the involvement of EPS I and II in autoaggregation of S. meliloti. Presence of an intact copy of the expR locus was shown to be necessary for autoaggregation. A mutant incapable of producing EPS I displayed autoaggregation percentage similar to that of parental strain, whereas autoaggregation was significantly lower for a mutant defective in biosynthesis of EPS II. Our findings clearly indicate that EPS II is the essential component involved in autoaggregation of planktonic S. meliloti cells, and that EPS I plays no role in such aggregation.     

Quantitative analysis of biofilm EPS uronic acid content

The uronic acids assay was evaluated for its ability to measure the amount of uronic acids contained within a biofilm exopolysaccharide matrix. Cytophaga lytica, a marine bacterium isolated from a naturally occurring biofilm, was used to form single-species biofilms for the method assessment. The assay was found to be simple, reproducible, and sensitive to 1 microg levels, suggesting its potential for application as a screening technique for compounds that inhibit the production of microbial biofilm exopolysaccharide containing uronic acids.     

氧化亚铁硫杆菌胞外多聚物在生物浸出中的作用

氧化亚铁硫杆菌(Thiobacillus ferrooxidans,T.f)是一种重要的浸矿微生物。它与矿物的界面作用机理是复杂的,涉及物理化学的和生物化学的参数。本文运用电镜细胞化学方法对氧化亚铁硫杆菌(Thiobacillus ferrooxidans)的胞外多聚物(EPS)的脂类、多糖、蛋白质等生物大分子以及铁离子进行了研究,并探讨了EPS与吸附、生物膜形成的关系以及生物膜在浸矿过程中的作用。     

Mutational analysis of the Lactococcus lactis NIZO B40 exopolysaccharide (EPS) gene cluster: EPS biosynthesis correlates with unphosphorylated EpsB

AIMS: To determine the role of the EpsA, EpsB, and EpsC proteins encoded at the 5'-end of the exopolysaccharide (EPS) gene cluster in regulation of EPS production in Lactococcus lactis. METHODS AND RESULTS: Deletion and paralog-replacement mutants of epsABCD were used to determine the function of EpsA, EpsB and EpsC in EPS production and polymer chain length determination in L. lactis. EpsA and EpsB appeared to be essential for EPS biosynthesis in L. lactis, while deletion of the phosphatase (EpsC) only had a minor effect on the EPS production level. Determination of the phosphorylation state of EpsB and analysis of a C-terminally truncated EpsB variant indicate that EPS biosynthesis in L. lactis is driven by a nonphosphorylated form of EpsB. CONCLUSIONS: The data presented here show that in L. lactis, EPS production is under control of a phosphoregulatory system and that EPS biosynthesis correlates with an unphosphorylated EpsB. SIGNIFICANCE AND IMPACT OF THE STUDY: This study provides molecular understanding of polysaccharide production in L. lactis that could eventually enable novel approaches to control EPS production by lactic acid bacteria during industrial fermentation processes.