1株产纤维素酶细菌的筛选、鉴定及生长特性

分离筛选高效降解纤维素的菌株,并研究其生物学特性。利用刚果红染色法从腐烂的玉米秸秆中分离纤维素降解菌,再通过测定滤纸的降解率及多种酶活复筛。综合考虑水解圈和菌落直径(HC值),滤纸的降解率和酶活,对所筛选的菌株进行纤维素降解能力综合评价,最终获得1株具有纤维素降解能力的菌株DX4,其滤纸酶活(FPA酶活)、内切葡聚糖酶活力(CMC酶活)和外切葡聚糖酶活力(Cex酶活)分别为256.051、358.276和5.536 U/m L。结合形态学、生理生化特性和分子生物学鉴定,将该菌株鉴定为枯草芽胞杆菌(Bacillus subtilis),命名为Bacillus subtilis DX4,简称BS-DX4。研究表明,BS-DX4的最适生长温度为40℃,最适生长pH为7.0,低盐浓度下生长旺盛,是具有开发潜力的纤维素酶高产菌株。     

一株产纤维素酶菌株的分离、鉴定及产酶特性

【目的】筛选并鉴定一株产纤维素酶的菌株,初步探究该菌的产酶特性,为综合利用纤维素筛选菌源。【方法】在常温条件下,采用滤纸培养基对菌种富集,采用CMC-Na初筛纤维素降解菌,采用LB培养基分离纯化菌株,经形态学、生理生化特征试验、16S r RNA基因序列测定等分析筛选菌株的系统分类地位。单因素试验确定培养时间、培养温度、初始p H及Na Cl浓度对筛选菌株产酶活力的影响。【结果】从腐烂的玉米秸秆中分离出一株在常温下产纤维素酶细菌KZ-2,根据菌落形态特征、生理生化特征鉴定以及16S r RNA基因序列分析,初步鉴定KZ-2为肠杆菌(Enterobacter sp.),为潜在新种。产酶条件实验显示:该菌使用产酶发酵培养基120 h产酶量达到最大值,在25–35°C、初始p H 4.5–5.5、Na Cl浓度1.0%–2.0%范围内为最佳产酶条件,在最适条件下酶活可达80.93 U/m L。该菌株所产纤维素酶最适反应p H为7.0,最适反应温度为50°C。【结论】KZ-2是一株具有降解纤维素能力的细菌,在常温下即可分泌纤维素酶,并且该菌株为潜在新种,具有潜在的开发价值。     

三株高效秸秆纤维素降解真菌的筛选及其降解效果

【目的】利用多种筛选方法,获得高效秸秆纤维素降解真菌,并研究其秸秆纤维素的降解能力。【方法】采用滤纸片孔洞法、滤纸条降解法、羧甲基纤维素钠(CMC-Na)水解圈测定法、秸秆失重法、纤维素分解率测定法、胞外酶活测定法等常规秸秆纤维素降解菌的筛选方法。【结果】筛选到3株具有较强纤维素降解能力的真菌菌株,经初步鉴定菌株98MJ为草酸青霉(Penicillium oxalicum)、菌株W3为木霉(Trichoderma sp.)、菌株W4为扩张青霉(Penicillium expansum)。菌株W4具有非常强的秸秆纤维素降解能力,10d内对秸秆的降解率可达56.3%,对纤维素、半纤维素和木质素的分解率分别为59.06%、78.75%和33.79%。菌株W4的胞外纤维素酶活力在14.25-49.75U/mL之间。【结论】筛选获得3株高效秸秆纤维素降解真菌菌株,其中菌株W4的纤维素酶活高于已报道的菌株,是一株十分具有研究开发潜力的纤维素酶生产菌株。     

产纤维素菌株的分离鉴定及产量相关性

【背景】细菌纤维素是一种性能优异的新型天然生物纳米材料,但其发酵产量低、生产成本高,尚未得到大规模生产与应用。【目的】自然选育细菌纤维素高产菌株,并探索菌株产量与菌落形态、水果来源、菌株种属之间的关联。【方法】从15个不同种类的576份腐烂水果中自然选育产纤维素菌株,并按菌落形态进行分类。静置培养筛选高产纤维素菌株,并对所得菌株进行16SrRNA基因测序,鉴定其种属。【结果】获得134株产纤维素菌株,其中一株分离自芒果的汉氏驹形杆菌(Komagataeibacter hansenii)产量最高,为11.24 g/L。所得菌株按菌落形态可分为10个类别,高产纤维素菌株形态共同特征为黄色、圆形、边缘整齐或不规则、表面粗糙或褶皱、凸起(形态4、5、9)。苹果和梨来源中分离得到的菌株菌落形态多样性丰富,高产纤维素菌株的水果来源中芒果所占比值最高,其次为梨和苹果。所有菌株鉴定为5个属13个种,包含了醋酸杆菌属(Acetobacter)、驹形杆菌属(Komagataeibacter)、葡糖醋杆菌属(Gluconacetobacter)、沙雷氏菌属(Serratia)和乳酸杆菌属(Lactobacillus),其中高产纤维素菌株集中分布于汉氏驹形杆菌(K.hansenii)和中间驹形杆菌(K.intermedius)。【结论】筛到的菌株多样性丰富,并且得到多株高产纤维素菌株,其传代稳定性好,丰富了细菌纤维素生产菌株的来源。分析所得菌株产量与菌落形态、水果来源之间的关系可以为今后菌株筛选工作提供参考。     

一株降解纤维素放线菌的产纤维素酶基因克隆与表达

【背景】纤维素在自然界中储量丰富,但天然纤维素的难降解性成为广泛应用纤维素资源的壁垒,近年来利用微生物来降解纤维素成为热点研究。【目的】筛选分离得到一株具有降解纤维素功能的放线菌菌株Lb1,通过全基因组测序确定其产纤维素酶关键基因5676,对基因5676进行克隆转化,使其在大肠杆菌中进行表达。【方法】通过基因工程技术将产纤维素基因连接到表达质粒上并导入表达菌株,对其降解纤维素生成葡萄糖的能力进行探究。【结果】将Lb1菌株的16S rRNA基因进行比对,确定菌株Lb1属于链霉菌属,命名为Streptomyces sp. Lb1。成功构建出纤维素酶表达载体,并且导入表达菌株大肠杆菌BL21(DE3),重组菌株的产纤维素酶能力大于空载菌株。【结论】通过基因工程技术成功克隆出产纤维素酶基因,从而表达纤维素酶,为今后利用微生物降解纤维素的大规模应用提供参考。     

纤维素分解菌的选育及酶活测定

纤维素是地球上最丰富的有机物质,这些丰富的宝贵资源大部分被浪费了,而且由于部分地区焚烧秸杆造成了严重的环境污染。为了充分利用纤维素,纤维素分解菌的筛选研究逐步展开。通过新华滤纸为唯一碳源的杜氏培养基和刚果红纤维素培养基,从堆肥、污泥、马粪和土壤中分离得到7株纤维素分解菌。以5号菌株为出发菌株,经过紫外线诱变,用刚果红纤维素平板透明圈选育法得到8号菌株。为了评价筛选工作,对8株纤维素分解菌进行酶活测定。结果表明,8号菌株具有最高的CMC酶活和FPA酶活。     

解糖热解纤维素菌F32降解未预处理秸秆及产纤维素酶特性分析

【目的】明确极端嗜热厌氧木质纤维素降解菌解糖热解纤维素菌F32代谢特征,并分析其产酶特性。【方法】使用细胞计数法绘制菌株的生长曲线,使用离子色谱及气相色谱进行产物和残糖量分析,以DNS法及对硝基苯酚法检测菌株胞外蛋白的酶活性。【结果】解糖热解纤维素菌F32在以葡萄糖、微晶纤维素和未经预处理小麦秸秆为碳源时生长状况优于解糖热解纤维素菌DSM 8903。在以葡萄糖为碳源进行培养时,与菌株DSM 8903相比,菌株F32具有产乳酸较多,而产氢气较少的特点。在以微晶纤维素和未经预处理小麦秸秆为碳源进行培养时,与菌株DSM 8903相比,菌株F32胞外蛋白具有较高的内切纤维素酶活性和木聚糖酶活性。【结论】解糖热解纤维素菌F32表现出较强的木质纤维素降解能力,其与DSM 8903的产物组成及胞外蛋白的酶活性具有明显差异。     

嗜热厌氧纤维素降解细菌的分离、鉴定及其系统发育分析

利用纤维素降解细菌和纤维素粘附的方法分别从新鲜牛粪、高温堆肥和本实验室保存的纤维素降解富集物中分离得到4株嗜热厌氧纤维素降解细菌。分离菌株为革兰氏染色阴性,直的或稍弯曲杆菌,菌体大小为0.4μm～0.6μm×3μm～15μm,严格厌氧,不还原硫酸盐,形成芽孢。多数芽孢着生于菌体顶端。分离菌株能利用纤维素滤纸、纤维素粉Whatman CFII、微晶纤维素、纤维素粉MN300和未经处理的玉米秆芯、甘蔗渣、水稻秸杆。分离菌株在pH6.2～8.9、温度45℃～65℃范围内利用纤维素,最适pH为7.0～7.5,最适温度为55℃～60℃,发酵纤维素产生乙醇、乙酸、H2和CO2。分离菌株还可利用纤维二糖、葡萄糖、果糖、麦芽糖、山梨醇作为碳源。部分长度的16S rDNA序列分析表明,分离菌株EVAI与Clostridium thermocellum具有99.8%相似性。     

一组降解纤维素细菌的分离筛选及产酶特性研究

用稀释法从腐殖泥中分离菌株,根据它们在羧甲基纤维素钠(CMC-Na)-刚果红培养基上的透明圈直径及对滤纸的崩解能力,获得7株纤维素分解细菌(编号:B-37、B-35、B-31、B-25、B-17、Z-a和Z-b),其中菌株Z-b的纤维素崩解能力最强,分子鉴定结果表明它与Stenotrophomonas maltophilia的16S rDNA序列有99.8%的同源性,初步确定为嗜麦芽窄食单胞菌。适合7个菌株生长的C源为马铃薯浸出液,无机盐组分为:CaCl_2 0.20、MgSO_4 1.25、NaCl 5.00、(NH_4)_2SO_4 1.30、KH_2PO_4 1.35、FeSO_4·7H_2O 0.015、Na-EDTA 0.02g/L。在滤纸为唯一碳源的培养基中,菌株Z-b的滤纸酶(FPase)和CMC酶(CMCase)活性最大,为0.099 U/mL和0.075 U/mL,而在固体PSA上,菌株B-31和B-37的FPase和CMCase活性最高,为0.131 U/mL和0.175 U/mL。7个细菌单独发酵,Z-b对滤纸的崩解能力最强,滤纸块完全崩解成粉未状;与真菌34混合发酵,菌株组合Z-a+34、Z-b+34、B-31+34、B-25+34将滤纸完全水解为水溶性物质。可见,各菌株的纤维素酶活与培养条件密切相关,某些真菌、细菌间存在协同作用,它们混合发酵可大大提高纤维素的水解效率。     

纤维素降解菌的筛选与复合菌系的初步构建

目的针对大庆地区土地盐碱化较严重,盐碱面积较大等现状,从大庆特征性盐碱地区土壤样品中分离出能够降解纤维素的菌株,为降解植物废料以及缓解土壤盐碱化改善土壤环境提供功能菌株。方法通过刚果红染色法初步筛得到具有纤维素降解能力菌株,进一步用比色法测定其纤维素降解率,同时测定菌株耐盐、耐碱、产酸性能,选择性能优良的3株菌作为纤维素降解菌复合菌系构建菌株,通过耐盐性、耐碱性和纤维素降解率实验测定复合菌系菌株最佳组合,进一步通过上述实验确定复合菌系菌株最佳混合比例。结果得到由DX-5和DX-9按照2∶3进行组合复合菌系纤维素降解率最高,达到87.96%,且具有较高的耐盐以及耐碱能力。结论通过实验得到纤维素降解菌的复合菌系,具有较高纤维素降解率以及改善土壤盐碱性能力。     

phbC基因敲除对土壤杆菌产可得然胶的影响

本文构建了phbC基因无痕敲除菌株ΔphbC,分析了ΔphbC菌株生长代谢情况和产生的可得然胶在产量、凝胶性质和红外结构的变化。结果显示,ΔphbC菌株在发酵过程中氨基氮消耗情况与野生型菌株一致,在蔗糖消耗方面,ΔphbC菌株与野生型菌株在18 h之后出现显著差异,蔗糖消耗比野生型菌株明显降低。ΔphbC菌株可得然胶产量约24 g/L,相对于野生型菌株降低了45%;胶凝胶强度为812.521 g/cm^2,相对于野生型菌株降低了21%;红外结构与野生型菌株一致,无明显差异。phbC基因不影响菌体生长,不影响可得然胶结构,但是影响可得然胶的合成。     

Transductional construction of a threonine-producing strain of Serratia marcescens.

A threonine-producing strain of Serratia marcescens Sr41 was constructed according to the following process. Thr- strain E-60 was derived from strain HNr59 having constitutive levels of threonine-sensitive aspartokinase and homoserine dehydrogenase. Thr+ transductant T-570 was constructed from strain E-60 and phage grown on strain HNr21 having feedback-resistant threonine-sensitive aspartokinase and homoserine dehydrogenase. This transductant lacked both feedback inhibition and repression for the two enzymes. Thr- strain N-11 was derived from strain AECr174 lacking feedback inhibition and repression of lysine-sensitive aspartokinase. Subsequently, the threonine region of strain T-570 was transduced into strain N-11. One of the THR+ transductants, strain T-693, produced markedly high levels of the two aspartokinases and homoserine dehydrogenase, which were insensitive to feedback inhibition. This strain produced about 25 mg of threonine per ml in the medium containing sucrose and urea.     

Transductional construction of a threonine-producing strain of Serratia marcescens.

A threonine-producing strain of Serratia marcescens Sr41 was constructed according to the following process. Thr- strain E-60 was derived from strain HNr59 having constitutive levels of threonine-sensitive aspartokinase and homoserine dehydrogenase. Thr+ transductant T-570 was constructed from strain E-60 and phage grown on strain HNr21 having feedback-resistant threonine-sensitive aspartokinase and homoserine dehydrogenase. This transductant lacked both feedback inhibition and repression for the two enzymes. Thr- strain N-11 was derived from strain AECr174 lacking feedback inhibition and repression of lysine-sensitive aspartokinase. Subsequently, the threonine region of strain T-570 was transduced into strain N-11. One of the THR+ transductants, strain T-693, produced markedly high levels of the two aspartokinases and homoserine dehydrogenase, which were insensitive to feedback inhibition. This strain produced about 25 mg of threonine per ml in the medium containing sucrose and urea.     

高产γ-氨基丁酸低产桔霉素红曲霉(Monascus ruber)突变子1047筛选与发酵特性研究

以红曲米中筛选到的红色红曲霉菌株G为原始菌株,通过农杆菌介导T-DNA插入突变技术,成功构建了含有1 483株红曲霉突变子的T-DNA插入突变库。用HPLC等方法从突变库中筛选出10株γ-氨基丁酸(GABA)产量稳定高于原始菌株G的突变子,薄层层析结合HPLC技术分析了10株突变子发酵液中桔霉素的含量;其中突变子1047的GABA产量较高,为1.169g/L,是原始菌株G(GABA产量0.472g/L)的247.67%,桔霉素含量稳定低于原始菌株G。以红曲霉菌株G和突变子1047为实验材料,通过5 L发酵罐发酵并定时取样,HPLC等方法精确分析发酵液各种活性物质的含量;结果显示,突变子1047生长速度稍快于原始菌株G;GABA、莫纳可林K(Monacolin K)、红曲色素色价分别为2.201 g/L、83.892 mg/L、21.984 U/mL,是原始菌株G的279.67%、108.01%和182.35%;而桔霉素产量为1.976 mg/L,是原始菌株G的41.71%。因此,利用TDNA插入的方法对红曲霉进行育种,能产生稳定的遗传变化,在红曲霉资源的保护和利用上有一定潜力。     

灰黄霉素菌的诱变效应

以灰黄霉素产生菌D－756为出发菌株,经过三代紫外线＋氯化锂诱变处理,获得耐氯变株F－1012,该变株在形态特征及产量、耐氯性等方面均发生变化,当发酵培养基中的氯化物浓度由1.5%提高到2.0%,F－1012的大米孢子效价提高了34.5%;当固体平板培养基中氯化物浓度提高到11％时,F－1012的孢子存活率比出发菌株提高了25.5％。     

以耐赖氨酸为标记的金霉素产生菌抗噬菌体变株的选育

本文以金霉素产生菌Ｆ－３０３作为出发菌株,通过ＵＶ＋ＥＭＳ复合处理,双层法不同梯度耐赖氨酸作标记,进行抗噬菌体的金霉素菌株选育,获得Ｆｓ－４８－１４菌株。该菌株不但表达了抗噬菌体的特性,而且产素效价超过Ｆ－３０３。通过无机盐正交条件试验,取得抗性变株最佳的发酵培养基配方。     

Comparative studies of strains Ictero No. I and RGA as the type strain of Leptospira interrogans: agglutinin absorption test, protein and antigen profiles, and enzyme activities

Strain Ictero No. I, the first isolate of Leptospira, isolated by Inada and Ido in 1914, was found to be sufficiently qualified to be the type strain of Leptospira interrogans rather than strain RGA. In an agglutinin absorption test, anti-Ictero No. I serum was not absorbed completely with strain RGA, and 25% of the homologous titer remained unabsorbed, while anti-RGA serum was completely absorbed with strain Ictero No. I. Thus, strain Ictero No. I was not serologically identical with strain RGA, and the two strains were considered to be different serovars. A protein band with a molecular weight of approximately 33,000 daltons was detected in strain Ictero No. I but not in strain RGA by SDS-PAGE. By Western blotting, this protein band was detectable with anti-Ictero No. I serum but not with anti-RGA serum. The presence of the 33K protein in strain Ictero No. I, but not in strain RGA, was confirmed by radioimmunoprecipitation using [125I]-labeled antigens, indicating that the protein antigen was surface-exposed. Only 8 of the 89 enzymes activities were different between strains Ictero No. I and RGA (line Sapporo). From the above results, we propose that strain Ictero No. I should be designated as the type strain of L. interrogans instead of strain RGA.     

Compressive axial strain distributions in cancellous bone specimens

The compressive axial strain distribution in cylindrical trabecular bone specimens was studied using digitized images of the specimen surface. Specimens were tested with strain rate 0.00015 s-1. Images were taken at 0, 1, 2, 3, 4, 6, 8 and 10% strain. Using an optical illusion of movement by rapidly changing succeeding images, failures were classified as transverse (33%) or oblique collapses (67%). The location of failure was not determined by the specimen density gradient. Local axial strain in the distal, intermediate and proximal third was measured throughout the compression in the transversely failing specimens, whereas local strain in the obliquely failing specimens was measured in the pre-failure phase only. Axial strain inhomogeneity was observed in the pre-failure as well as in the post-failure phase. In the pre-failure phase the intermediate third was strained significantly less than the thirds near the ends. In the post-failure phase specimen strain occurred solely in the collapsed part. Ultimate strain of the transversely failing specimens was 2.5% and ultimate strain of the failing third was 3.7%. At failure less than 1% strain was observed in the intermediate third and at 10% specimen strain 1.5% local strain was found in the intermediate third. The results indicate unreliability of conventional stiffness and strain measurements in trabecular bone specimens probably due to lack of trabecular constraint at the end surfaces. Conventional measurements tend to underestimate stiffness and, by giving an average value of strain in spite of considerable strain inhomogeneity, to underestimate failure strain.     

Arctic charr strain crosses: effects on growth and sexual maturity

Three Arctic charr strains and their crosses were evaluated with respect to growth and sexual maturation frequency. No significant heterosis was observed for growth. One out of five crosses was heavier, but not significantly so, than the best performing parental strain at ages 1 + and 2. The five other crosses did not perform better than the best performing parental strain at any age. Cross-breeding was not recommended as an effective method to improve growth performance in Arctic charr. Growth performance of reciprocal crosses differed significantly in all strain combinations: crosses resembled more the male parent strain than the female parent strain. ANOVA for male maturation frequency showed a highly significant effect of the male parent strain and a weakly significant effect of female parent strain. In the Ottsjö strain mature males were significantly larger than immature fish and females. Such size difference was also observed in the offspring when sires of the Ottsjö strain were crossed with dams of the faster growing Honavan strain or with dams of the Rensjö strain. When Ottsjö dams were crossed to sires of the other strains no significant size difference between mature males and other fish was found.