海洋真菌Fusarium sp.LD8岩藻多糖酶的液态发酵条件研究

通过对海洋真菌Fusarium sp.LD8产岩藻多糖酶发酵培养基组成及工艺条件的研究,得到较优培养基配方为:麸皮5%,海带粉2%,(NH4)2SO40.8%。以人工海水代替蒸馏水,接种量为3%,在恒温振荡器中以180r/min的速度振荡培养,岩藻多糖酶活可达2.10IU/mL。     

海洋真菌Dendryphiella Arenaria TM94产岩藻多糖酶发酵及酶学性质

通过对海洋真菌Dendryphiella Arenaria TM94产岩藻多糖酶发酵培养基组成及工艺条件的研究,并经正交实验,得到较优培养基配方为：麸皮3％,海带1％,葡萄糖0．3％,复合氮源为NaNO33％,(NH4)2SO40．5％,蛋白胨3％和酵母浸膏0．6％时,培养基的起始pH为6．5。在恒温振荡器中以120rpm的速度振荡培养,岩藻多糖酶活可达24．3IU／ml。     

黄杆菌菌株RC2-3基因组生物信息学分析及高效降解岩藻多糖功能基因的挖掘

以从海带中筛选获得的一株具有降解岩藻多糖能力的黄杆菌菌株RC2-3为研究对象，该菌株产的岩藻多糖酶可以高效降解不同来源的岩藻多糖。为进一步探究菌株RC2-3降解岩藻多糖的机制，推动岩藻寡糖的酶法生产，采用Illumina测序技术对菌株RC2-3进行基因组测序、基因功能注释和碳水化合物活性酶注释以及岩藻多糖降解相关基因的生物信息学分析。结果表明，黄杆菌菌株RC2-3基因组全长3 414 532 bp,共编码2 967个基因，GC含量为30.92%。经碳水化合物活性酶数据库注释获得213个基因，与岩藻多糖降解有关的包括7个岩藻糖结合结构域的基因；2个β-D-岩藻糖苷酶(EC 3.2.1.38)基因；2个属于GH141家族的α-L-岩藻糖苷酶(EC 3.2.1.51)基因；12个属于GH29家族的α-1, 3/1, 4-L-岩藻糖苷酶(EC 3.2.1.111)基因；9个属于GH95家族的α-1, 2-L-岩藻糖苷酶(EC 3.2.1.63)基因。此外，通过与已报道的蛋白序列比对发现，岩藻多糖酶基因RC2.3＿GM001247编码的蛋白序列与FunA蛋白序列同源性达到70.98%,岩藻多糖酶...     

海洋真菌岩藻多糖酶的固态发酵条件研究*

本文对海洋真菌Dendryphiella arenaria(TM94)岩藻多糖酶的固态发酵条件进行了研究,主要内容包括碳源、氮源、添加物、起始pH、接种量及温度等.固态发酵最佳培养基组成麸皮7.5g,葡萄糖0.5g,海带粉0.6g,NaNO3为4g/L最佳培养条件为培养温度28℃,起始pH6,接种量3ml(孢子浓度为106个/ml).在28℃培养24h,酶活力可达35.5IU/g干培养基,比活力为1.39IU/mg蛋白质.对岩藻多糖酶酶学性质也进行了研究.     

硅藻金色奥杜藻色素的HPLC分析与超临界CO2萃取研究

以硅藻金色奥杜藻(Odontella aurita)为实验材料,利用高效液相色谱法分析了其色素组成与含量,采取超临界CO2萃取技术研究了从干藻粉内提取岩藻黄素的条件。结果表明,该藻主要含有岩藻黄素、硅甲藻黄素、β-胡萝卜素、硅藻黄素等类胡萝卜素以及叶绿素a和叶绿素c1,其中岩藻黄素为该藻含量最高的类胡萝卜素。色素的萃取率与压强、温度、夹带剂含量以及萃取时间呈正相关,夹带剂含量对萃取率影响最大,CO2流速的影响最小;与有机溶剂法相比,超临界CO2萃取岩藻黄素效率略低,而更利于岩藻黄素的选择性萃取及分离提纯;岩藻黄素的SFE-CO2适宜条件为压强400 bar、温度50℃、CO2流速0.2 L/min、夹带剂比例10%、萃取时间2～3 h。     

高产岩藻黄素的海洋硅藻筛选及光照条件优化

为提高岩藻黄素(Fucoxanthin)提取效率, 对16株海洋硅藻岩藻黄素的检测含量和实际含量进行了分析, 并以一株牟氏角刺藻(Chaetoceros muelleri)为对象, 研究了岩藻黄素与另外两种关键光合色素(即叶绿素a和β-胡萝卜素)的含量及其消长受光强和光质影响的特征。研究结果显示, 不同种或同种不同株的海洋硅藻, 在相同的培养条件、收获时期、提取方法下, 其提取率差异大, 可从不足1%到89.78%; 岩藻黄素的检出含量各异, 从0.03到5.02 mg/g。受不同光照强度[低: 50 μmol/(m2·s); 中: 100 μmol/(m2·s); 高: 200 μmol/(m2·s)和光质(红光、蓝光)]的影响, 岩藻黄素产量呈现不同特征。在低光照强度下, 单位细胞岩藻黄素的含量相对较高。在红光条件下, 岩藻黄素的产量高于蓝光。在相同光强条件下, 岩藻黄素含量随增殖周期变化; 在单色光质条件下, 几种光合色素均在生长平台期后期含量增加。岩藻黄素的含量变化与叶绿素a和β-胡萝卜素的含量及其消长关系密切。研究为筛选藻株、优化硅藻培养条件以累积岩藻黄素提供了参考。     

铁皮石斛组织培养与快速繁殖(简报)

以铁皮石斛种子为外植体进行组培快繁技术研究,筛选出适合各个阶段培养的培养基配方。种子萌发的培养基1/2MS+马铃薯汁15%;原球茎分化的培养基1/2MS+马铃薯汁20%+NAA 0.1 mg/L;壮苗培养基MS+香蕉汁10%+NAA 0.2 mg/L;生根培养1/2 MS+香蕉汁15%+NAA 0.5 mg/L。     

植酸酶和非淀粉多糖酶对鲈鱼生长和消化酶活性的影响

以初始体重为(6.26 ± 0.10)g鲈鱼(Lateolabrax japonicus Cuvier)为研究对象,探讨饲料中添加植酸酶（PY）和非淀粉多糖酶（WX和VP）（WX为木聚糖酶和葡聚糖酶的复合酶制剂,VP为纤维素酶、半纤维素酶、葡聚糖酶和果胶酶的复合酶制剂）对鲈鱼生长、体组成以及胃和肠道消化酶活性的影响。以含36.1%鱼粉和18.0%复合蛋白(豆粕：肉骨粉：花生粕：菜籽粕 = 4：3：2：1并添加赖氨酸、蛋氨酸和异亮氨酸以模拟鱼粉必需氨基酸含量)的饲料为基础饲料(Diet 1),分别向每千克基础饲料中添加200 mg PY (Diet 2)和400 mg VP + 800 mg WX (Diet 3),配制出3种等氮(粗蛋白43%)等能(20 kJ/g)的实验饲料。实验在1.5 m× 1.5 m × 2.0 m的浮式海水网箱中进行,每个处理设3个重复,每个重复放养60尾鲈鱼。 每天饱食投喂2次(06：00和18：00)。实验期间水温为27.5－29.5 ℃, 盐度为25‰－28‰,溶解氧大于7 mg / L。实验结果表明饲料中添加外源酶对鲈鱼的成活率无显著影响（92%－95%）,但却显著提高了鲈鱼的增重百分率（从859.3%提高到947.2%和905.2%）和特定生长率（从4.0提高到4.2和4.1） (p<0.01)。与基础饲料组相比,饲料中添加非淀粉多糖酶对鲈鱼鱼体水分、粗蛋白、粗脂肪、灰分以及身体总能均无显著影响;饲料中添加植酸酶对鲈鱼鱼体水分、粗脂肪含量以及身体总能也无显著影响,但却显著提高了鱼体的粗蛋白和灰分含量（p<0.05）。饲料中添加植酸酶和非淀粉多糖酶后,鲈鱼胃和肠道消化酶均有上升趋势。饲料中添加植酸酶对鲈鱼胃和肠道中的脂肪酶和淀粉酶的活性无显著影响,但是显著提高了其胃和肠道中蛋白酶的活性（分别从0.74 U / mg提高到1.02 U / mg和1.09 U / mg提高到1.71 U / mg）(p<0.01)。而饲料中添加非淀粉多糖酶对鲈鱼胃和肠道中的蛋白酶和脂肪酶活性无显著影响,但显著提高了其胃和肠道中淀粉酶的活性（分别从0.05 U / mg提高到0.16 U / mg和0.12 U / mg提高到0.21 U / mg）(p<0.01)。     

岩藻糖基化人乳低聚糖在新生儿无乳链球菌肺炎治疗中的作用

目的探讨岩藻糖基化人乳低聚糖在新生儿无乳链球菌肺炎中的治疗作用。方法收集本院2015年7月至2017年2月痰培养阳性新生儿无乳链球菌、大肠埃希菌和肺炎克雷伯菌感染性肺炎病例,分析不同喂养方式、不同病原类别肺炎在住院时间、炎症、并发症等指标差异,探讨岩藻糖基化人乳低聚糖对无乳链球菌感染的独特治疗作用;使用含有不同浓度岩藻糖基化人乳低聚糖的培养基对无乳链球菌进行培养,研究岩藻糖基化人乳低聚糖抑制无乳链球菌的最佳浓度;分别使用岩藻糖基化人乳低聚糖或酸性人乳低聚糖加入培养基中对无乳链球菌、大肠埃希菌、肺炎克雷伯菌进行培养,进一步探讨岩藻糖基化人乳低聚糖对无乳链球菌的独特抑制作用。结果无乳链球菌肺炎患儿,母乳喂养组的住院时间较人工喂养组住院时间减少[(8.35±0.77)d vs(10.91±0.54)d,t=1.557 676,P<0.05)],PCT值较人工喂养组低[(2.38±0.63)ng/mL vs(8.69±2.23)ng/mL,t=1.419 964,P<0.05],白细胞计数较人工喂养组低[(13.28±1.08)×10^9/L vs(16.16±0.98)×10^9/L,t=1.878 447,P<0.05],脑膜炎发生率较人工喂养组低(5%vs 35%,χ^2=5.601 353,P<0.05),呼吸机使用率较人工喂养组低(10.0%vs 36.4%,χ^2=4.005 042,P<0.05);大肠埃希菌肺炎患儿、肺炎克雷伯菌肺炎患儿,母乳喂养组与人工喂养组比较,住院时间稍减少,PCT值、白细胞计数、脑膜炎发生率和呼吸机使用率均有所降低,差异无统计学意义;细菌培养实验发现岩藻糖基化人乳低聚糖在2.5 mg/L浓度的时候可以明显抑制无乳链球菌的生长,对大肠埃希菌和肺炎克雷伯菌无明显抑制作用,酸性人乳低聚糖对3种细菌均无抑制作用。结论岩藻糖基化人乳低聚糖可以明显抑制无乳链球菌的生长,可能成为未来无乳链球菌感染性肺炎治疗中新的靶点,值得深入研究。     

野生碧玉兰组培快繁技术

以云南野生碧玉兰（Cymbidium lowianum）种子无菌萌发的试管苗为试验材料,进行其丛生芽诱导增殖、生根的组培快繁技术体系研究。结果表明：适宜的增殖培养基配方为1/2MS＋6-BA 2.0 mg/L＋KT 0.5 mg/L＋NAA 0.2 mg/L,增殖率可达300%;生根培养基的配方为1/2MS＋NAA 1.5 mg/L＋6-BA 0.3 mg/L,其根数多,健壮。     

The characteristics and enzyme activities of 4-chlorophenol biodegradation by Fusarium sp

The effects of pH, temperature and sucrose addition on biodegradative capacity of Fusarium sp. HJ01 for 4-chlorophenol (4-CP) were examined, the property of dioxygenases produced by Fusarium sp. HJ01 during 4-CP degradation was investigated. The results show that Fusarium sp. HJ01 has a high capacity on degrading 4-CP in solution. The optimum values of pH, sucrose concentration and temperature are pH 7,1 g/L and 30°C, respectively. The strain can produce chlorocatechol 1,2-dioxygenase (CC12O) and chlorocatechol 2,3-dioxygenase (CC23O), which show the highest activities when 4-CP is used as the sole carbon source and energy, and the optimal values of pH and temperature are pH 7 and 50°C for CC12O as well as pH 8 and 60°C for CC23O. The kinetics of enzyme-catalyzed reactions accord with the Michaelis-Menten equation. To our knowledge, this is the first study on biodegradation of 4-CP by Fusarium sp. HJ01.     

生防菌根系定殖竞争作用对西瓜枯萎病发病机理的影响

【目的】西瓜枯萎病是由西瓜专化型尖孢镰刀菌(Fusarium oxysporum f.sp.niveum)引起的一种常见的毁灭性土传病害,对镰刀菌同属非致病性菌株与致病性菌株存在的竞争作用进行研究,有助于获得新的具有生防效果的菌株,从而拓宽西瓜枯萎病生物防治的手段。【方法】利用选择性培养基和稀释平板计数法对温室盆栽试验中西瓜根际和非根际土壤及植物组织中非致病性轮枝镰刀菌菌株(Fusarium verticillioides XA)与致病性尖孢镰刀菌(Fusarium oxysporum LD)进行计数,确定其在西瓜植株根际和组织中的定殖情况。【结果】将从田间西瓜枯萎病发病植株根部分离获得的菌株XA和LD接入健康土壤中,接种菌株XA既不会引起西瓜枯萎病发病症状,也不会影响西瓜植株生物量,但接种菌株LD导致严重发病症状。与单接种LD处理相比较,双接种(XA+LD)处理地上部鲜重和地上部干重都分别增加了151.2%和110%。XA菌株能成功定殖于西瓜根系,但在茎基部没有检测到。在接种菌株LD的处理中植物组织和土壤中致病性镰刀菌的数量达到(1.58 4.85)×104CFU/g。与单接种LD处理相比,双接种菌株XA和LD处理植物茎基部、根系、根际土壤和土体土壤致病性镰刀菌的数量分别下降63.3%、66.1%、3.3%和24.4%,根系、根际土壤和土体土壤非致病性镰刀菌的数量增加到(0.35 3.84)×104CFU/g;双接种处理对西瓜枯萎病的防效达57.8%。【结论】非致病性轮枝镰刀菌菌株XA可有效降低致病性尖孢镰刀菌LD对西瓜植株的定殖侵染能力,对西瓜枯萎病具有一定的生防效果。     

除虫菊内生镰孢菌Y2发酵条件优化及其抑菌活性

从除虫菊叶中筛选到1株内生真菌Fusarium sp．Y2,对其进行了基础培养基的筛选及培养条件优化研究。结果表明,Y2菌株的较佳发酵培养基为：每L培养基中含有麦芽糖10g、蛋白胨6g、KH2PO42g、KCl 1g、FeSO40．02g、MgSO4·7H2O1g;较佳发酵条件为：初始pH8．5,250mL三角瓶装液100mL,摇床转速180r／min,培养温度28．0℃,接种量21％。在此条件下与原始发酵条件相比,Y2菌株发酵液对番茄灰霉病菌菌丝生长抑制率达98．6％,提高了6．8％;对其孢子萌发抑制率达95．4％,提高了16．1％;其茵丝生长量（干质量）达8．975mg／mL,增加了7．8％。     

Population structure and linkage disequilibrium in a large collection of Fusarium oxysporum strains analysed through iPBS markers

In the current study, 160 pathogenic strains of Fusarium oxysporum collected from tomato, eggplant and pepper were studied. Eighteen inter‐primer binding site (iPBS)‐retrotransposon primers were used, and these primers generated 205 scorable polymorphic bands. The number of polymorphic bands per primer varied between 9 and 19, with a mean of 11 bands per primer. The highest polymorphism information content (PIC) value was determined as 0.27, and the lowest was 0.05. The unweighted pair‐group method with arithmetic averages (UPGMA) dendrogram including a heat map revealed that the 160 pathogenic strains of F. oxysporum were divided into two main clusters. The first cluster mainly included F. oxysporum f. sp. capsici (FOC) and F. oxysporum f. sp. melongenae (FOMG) isolates. The second cluster mainly comprised F. oxysporum f. sp. lycopersici (FOL) and F. oxysporum f. sp. radicis lycopersici (FORL) isolates. The highest percentage of loci in significant linkage disequilibrium (LD) was detected for FOL, whereas the lowest level of LD was found for FOC, and 95.2%, 99.4%, 99.1% and 97.4% of the relative kinship estimates were less than 0.4 for FOL, FOMG, FORL and FOC, respectively. LD differences were detected among formae speciales, and LD was higher in FOL as compare to FOC species. The findings of this study confirm that iPBS‐retrotransposon markers are highly polymorphic at the intraspecific level in Fusarium spp.     

Extracellular xylanase production by Fusarium species in solid state fermentation

Fusarium sp. has been shown to be a promising organism for enhanced production of xylanases. In the present study, xylanase production by 21 Fusarium sp. isolates (8 Fusarium culmorum, 4 Fusarium solani, 6 Fusarium verticillioides and 3 Fusarium equiseti) was evaluated under solid state fermentation (SSF). The fungal isolate Fusarium solani SYRN7 was the best xylanase producer among the tested isolates. The effects of some agriculture wastes (like wheat straw, wheat bran, beet pulp and cotton seed cake) and incubation period on xylanase production by F. solani were optimized. High xylanase production (1465.8 U/g) was observed in wheat bran after 96 h of incubation. Optimum pH and temperature for xylanase activity were found to be 5 and 50 degrees C, respectively.     

Biotransformation of (±)-2-methylcyclohexanone by fungi

The biotransformation of 2-methylcyclohexanone (1) using 16 fungal strains and some mushroom cultures was investigated. Fusarium sp. was one of the effective biocatalysts for oxidoreduction of 2-methylcyclohexanone (1). cis-2-Methylcyclohexanol (2a) was isomerized to trans-2-methylcyclohexanol (2b) by Fusarium sp. In addition, the corresponding lactones 3 was obtained by Baeyer-Villiger oxidation using Fusarium sp. AP-2 (46%, 94% ee).     

蔗渣发酵菌剂培养基的筛选及发酵条件的优化

采用单因素和正交试验研究了蔗渣高效发酵菌剂(芽孢杆菌B-A、曲霉菌F-A、链霉菌A-B)的摇瓶发酵最佳工艺条件.结果表明:芽孢杆菌B-A的最佳培养基配方:牛肉膏0.3%、蛋白胨1%、葡萄糖1%、NaCl 0.5%、可溶性淀粉0.5%、3.08%浓度的MnSO4溶液0.1;最适发酵条件为pH7、装液量100 ml(250 ml三角瓶)、36℃培养27 h.曲霉F-A的最佳培养基配方:葡萄糖3%、豆饼粉3%、蛋白胨1.2%、酵母膏0.3%、K2HPO4 0.05%、KH2PO40.05%、CaCl20.08%、MgSO40.04%、MnSO40.04%、ZnSO40.02%;最适发酵条件为pH6、装液量50 ml、30℃培养3 d.链霉菌A-B的最佳培养基配方:可溶性淀粉4.5%、蔗糖1%、豆饼粉3%、NaNO30.2%、ZnSO40.01%、KH2PO40.001%;最适发酵条件为pH7、装液量50 ml、30℃培养3 d.     

The distribution and partial characterization of the serum apolipoproteins in the guinea pig.

1. Very-low-density (VLD), low-density (LD) and high-density (HD) lipoproteins were isolated by sequential ultracentrifugation from the serum of male guinea pigs fed on a diet containing 3--4% fat. The apoproteins of these lipoproteins (apo-VLD, apo-LD and apo-HD lipoproteins) were studied after delipidation with organic solvents or extraction with tetramethylurea. 2. The major apolipoprotein of LD lipoprotein isolated by gel filtration was found to closely resemble apolipoprotein B of human serum in its chemical and physical properties. Electrophoresis in sodium dodecyl sulphate-polyacrylamide gel showed that this apoprotein consisted of a number of polypeptides. 3. Tetramethylurea precipitated an apoprotein from guinea-pig serum lipoproteins that is probably the apolipoprotein B-like component. This apoprotein accounted for about 80% of the apo-LD lipoprotein, about 55% of the apo-VLD lipoprotein and about 50% of the apo-HD lipoprotein. 4. The distribution of apolipoproteins soluble in tetramethylurea was determined by densitometric scanning of stained polyacrylamide disc gels. 5. A glycine-rich component of high electrophoretic mobility (band I) and a triplet of soluble apolipoproteins (bands II-IV) were present in both VLD and LD lipoprotein classes. These components constituted a higher proportion of the tetramethylurea-soluble apoproteins of VLD lipoprotein (60--80%) than of LD lipoprotein (40--55%). 6. Small amounts (10--15%) of a component of intermediate mobility, which contained traces of half-cystine, were also present in both VLD and LD lipoproteins. 7. A group of soluble components of basic character (bands VI-X), present as minor components of VLD lipoprotein (10--20%), constituted a major proportion (30--45%) of the soluble apoproteins of LD lipoprotein. Two of these apoproteins were rich in lysine, and two of lower electrophoretic mobility were rich in arginine. 8. The pattern of tetramethylurea-soluble apoproteins in HD lipoprotein was distinguished by the presence of two polypeptides of low electrophoretic mobility as its predominant components. One of these components, band VI, resembled the A-I apolipoprotein of man in both its amino acid profile and in its electrophoretic mobility. The second major component, band VI-B, was rich in lysine and resembled the C-I apolipoprotein of man in amino acid composition. 9. The soluble components of bands I and IX were analogous in physicochemical properties to the R-X1 and R-X2 (high-arginine polypeptide) peptides of human serum lipoproteins respectively.     

棉花枯萎病菌异核体的三个不同核型分离子DNA碱基组成及18S rDNA序列

从棉花枯萎病菌（Fusarium oxysporum f.sp.vasinfectum）异核体菌株Ag149的菌落我变处分离得到3个培养特征和致病性差异明显的单孢分离子。分别测定了这3个分离子的总DNA和核DNA的碱基组成,以及它们的18S rDNA的部分序列（1477个碱基对）。它们的总DNA（G＋C）mol%差异在0.1%-0.4%之间;核DNA（G＋C）mol%的差异在0.4%-0.8%范围内;而18S rDNA的部分序列则完全相同。     

绿色木霉菌LTR-2孢子提取物的抑菌活性及化学成分分析

通过研究绿色木霉菌LTR-2分生孢子提取物的抑菌活性及化学成分,为进一步提取纯化新型抗生素提供依据。采用固体麸皮培养基培养绿色木霉菌LTR-2,以二氯甲烷浸提法提取分生孢子中的抗菌物质,采用菌丝生长法测定提取物的抑菌活性,并用气相色谱-质谱联用仪进行分析,峰面积归一法计算有关成分的相对含量。绿色木霉菌LTR-2分生孢子的提取物抑菌谱广,对供试11种植物病原真菌均有不同程度的抑制作用;抑制效果好,对禾谷丝核菌的抑制率为89.3%。从提取物中分离鉴定出60多种化学成分,其中烷烃类成分数量最多,为43种,其他成分有酮类、有机酸类、醇类、烯类等,主要成分是麦角固醇,含量为41.90%。结论:绿色木霉菌LTR-2分生孢子提取物具有抑菌作用。通过化学成分分析,提取物中含有化合物5,6-二氢-6-戊基-2H-吡喃-2-酮,含量为2.35%,结合文献报道,推测5,6-二氢-6-戊基-2H-吡喃-2-酮是提取物中起抑菌作用的物质。