多种微生物搭载返回式卫星的试验研究

利用我国发射的科学返回式卫星,对4种具有实际应用价值的真菌、1种细菌和3种动物病毒的生长及某些特性如产酶、毒力及免疫学等进行了初步研究。结果表明,从4株真菌所选育的变异株产酶活性都得到不同程度的提高,但生长速度有的加快,有的则变慢; 1种动物病毒和1种细菌的毒力降低,并能产生较好的免疫原性。 Abstract:　Four filamentous fungi, one bacterium and three animal viruses were on board retrievable satellite. Some characteristics of them such as production of enzyme, toxicity and immunology were investigated. It showed that the level of producing enzyme of four mutant fungi were enhanced in some degree. The toxicity of one bacterium and one of three viruses become weak, and a good immunogenecity was also obtained.     

快速尿菌计数培养盒的研究

该快速尿菌计数培养盒进行了４种选择性培养基功能试验,共试验２３种９７株细菌,Ｇ－菌１７种７２株,Ｇ＋菌４种１９株,真菌６株。结果表明４种培养基功能特异,即Ⅰ＃为菌落计数,Ⅱ＃只限Ｇ－菌生长,Ⅲ＃只限Ｇ＋菌生长,Ⅳ＃只限真菌生长。该法与微量加样器法进行对比检测１８４份尿菌标本,符合率９６．７％,与日本培养盒平行对比试验１２份,结果一致     

感染瓜实蝇的曲霉菌及其生物学特性

从海南自然发病死亡的瓜实蝇上分离获得2株高毒力的真菌BC-D1和BC-212,经形态学和ITS序列鉴定结果表明, BC-D1为黄曲霉Aspergillus flavus,BC-212为溜曲霉Aspergillus tamarii。室内毒力测定结果发现：菌株BC-D1和BC-212对瓜实蝇成虫均有很高毒力,而对卵、幼虫及蛹的毒力较低。接种8d后成虫的平均死亡率分别为73.5%和85.1%,卵、幼虫及蛹的死亡率均低于50%。两株菌对黄粉虫、斜纹夜蛾及蚜虫的致病率均很低。生物学特性测定,两菌株具有生长速度快、产孢量大的特性,最适合生长的温度范围为30-35℃;在不同营养成分的培养基上,菌株生长速率、产孢量及菌落颜色存在较大差异。     

真菌还原Cr（VI）的研究

从不同来源的样品中分离筛选出几株抗Ｃｒ（ＶＩ）的真菌,他们能在含３００￣５００ｍｇ／ＬＫ２Ｃｒ２Ｏ７的蔗糖合成培养基中生长,其中ＢＳ－１菌株抗Ｋ２Ｃｒ２Ｏ７达９００ｍｇ／Ｌ．ＢＳ－１等４株真菌在含２００ｍｇ／Ｌ Ｋ２Ｃｒ２Ｏ７的培养基中生长４￣６ｄ后,培养液中的Ｃｒ（ＶＩ）已全部消失。这些真菌经鉴定为青霉菌ＢＳ－１和ＢＳ－３,黑曲霉ＢＲ－４和黄曲霉ＢＸ－１。经紫外可见光扫描及化学分析证实,高毒的Ｃ     

中国脊髓灰质炎病毒疫苗株基因特征及其神经毒力的初步观察

中国脊髓灰质炎病毒疫苗株普遍存在基因变异的现象,如重组,点突变等。我们选出１０株有代表性的变异株,在具有人脊灰病毒受体基因的转基因小鼠ＰＶＲ－Ｔｇ２１中做毒力分析,发现Ｓａｂｉｎ １基因型与野毒基因型的重组株显示很强的神经毒力,其ＰＤ５０ｉｎＴＣＩＤ５０值为４．５,而Ｓｂｉｎ１标准株的ＰＤ５０值大于８０。另外两株Ｉ型疫苗株只有关键性核苷酸位点发生突变,只在位点５２５－发生突变的一株,其ＰＤ５０值为     

肠道内产丁酸细菌及其产物丁酸生理功能的研究进展

产丁酸细菌是利用糖类发酵产生丁酸的一类细菌,代表种是丁酸梭菌。在动物及人类肠道内存在的产丁酸细菌主要是梭菌属、柔嫩梭菌属、罗斯式菌属、真菌属及丁酸弧菌属。本文一方面介绍部分肠道内产丁酸细菌的种类、特点及膳食纤维的摄入和肠道益生菌对产丁酸细菌的影响,另一方面对其主要代谢产物丁酸在体内的生理功能进行探讨,以期为产丁酸细菌的应用及产品开发提供理论依据。     

肾综合征出血热病毒核衣壳蛋白在抗感染免疫中的应用

采用区带离心纯化的肾综合征出血热（ＨＲＲＳ）汉滩病毒ＬＲ１株核衣壳蛋白（ＮＰ）分别免疫新西兰白家兔和昆明种小鼠。以ＮＰ免疫家兔后用ＬＲ１株病毒攻击,实验显示,免疫后的家兔可保护１００ＩＤ５０同株病毒的攻击;ＮＰ免疫母鼠所产的乳鼠能抵抗１０＾４－１０＾５ＬＤ５０同株病毒的攻击。以上结果表明：ＨＲＲＳ的病毒ＮＰ组分在抗感染免疫中起重要作用。     

解淀粉芽胞杆菌SSY1菌株的稳定性研究

目的测定产纤维素酶解淀粉芽胞杆菌SSY1株的稳定性。方法在适宜生长条件下连续传代30代。分别取第2、10、15、20、25和30代细菌,对其进行染色镜检、生化试验、药敏试验、产纤维素酶特性及动物安全性试验观察。结果传至第30代,细菌的形态、生化特性、产纤维素酶特性及药敏特性均未发生明显变化。结论产纤维素酶解淀粉芽胞杆菌SSY1株稳定性良好,有望成为中药发酵菌种。     

两株白色不产孢烟曲霉形态学及毒力研究

目的将先后发现的两株白色不产孢的烟曲霉A1j与A2j进行对比,观察其在形态学和毒力方面是否有差异。方法通过真菌基因组DNA的保守序列ITS和β-tub的测序对A2j进行菌种鉴定;采用小培养方法在显微镜下比较A1j、A2j及标准株Af293的菌丝形态;观察A1j和A2j在不同培养时间和不同培养基上生长的菌落形态;在小鼠模型上测试其毒力变化。结果通过ITS和β-tub的测序A2j被鉴定为烟曲霉;小培养发现A1j和A2j与标准菌株Af293不同,两者均为不产孢的烟曲霉,且两者生长速度明显不同;培养不同的时间和不同的培养基均不能诱导A1j和A2j产色和产孢,但是50℃下,A1j被限制生长,而A2j却能生长;在免疫抑制的小鼠模型中,与标准菌株Af293相比,A1j的毒力下降,但A2j小鼠的死亡数量、死亡速度与Af293相当,表明A2j的毒力并没有降低。结论新发现的白色不产孢烟曲霉A2j与A1j在生长速度、耐热性和毒力方面均不同。     

慢性化脓性中耳炎的微生物学及药敏分析

目的：为近两年治疗提出一个合理的抗菌素选择。方法：取慢性化脓性中耳炎的脓液进行细菌和真菌培养,做药敏试验,得出细菌分离率的排序,细菌的耐药特征及耐药率。结果：138耳中培养有微生物生长133耳,其中：细菌培养138耳(培养出142例菌株,混合感染8耳,均为两种致病菌,无细菌生长4耳);真菌培养8耳(培养出5株念株菌,无真菌生长3耳),细菌检出率依次为：金黄色葡萄球51株(占33．12％),铜绿假单胞杆菌33株(占21．43),其次,变形杆菌、肺炎克雷伯秆菌、大肠埃希菌和表皮葡萄球菌等。敏感药物(主要依据细菌检出率的前4种菌株的药敏试验)依次为：头孢菌素类、喹诺酮类、大环内酯类等。结论：定期、系统监测当地慢性化脓性中耳炎的细菌耐药动态和流行动态(细菌分离率的排序,细菌的耐药特征及耐药率,MIC50,MIC90等)。对医生经验用药将会有重要的指导意义。     

Isolation and partial properties of cellulose-decomposing strain of Cytophaga sp. LX-7 from soil

A new facultatively anaerobic, Gram-negative bacterium, Cytophaga sp. LX-7, degrading crystalline cellulose completely, was isolated from soil by dilution plating on cellodextrin agarose plates. This strain could excrete extracellularly all three types of cellulase and cellulosic substrates were the strongest inducer of endocellulase with CMC-liquefying activity production. No reducing sugar was found in cultures of cellulose during incubation. An enzyme which degrades crystalline cellulose was detected in cultures of cellulose by measuring the formation of soluble carbohydrate but was not detected by determining the reducing sugar released. This strain also synthesized cell-bound cellobiose oxidizing enzyme which was previously noted only in fungi. Both cellulose and soluble sugars could promote the production of cellobiose oxidizing enzyme.     

Decolorization and detoxication of reactive industrial dyes by immobilized fungi <Emphasis Type="Italic">Trametes pubescens</Emphasis> and <Emphasis Type="Italic">Pleurotus ostreatus</Emphasis>

Trametes pubescens and Pleurotus ostreatus, immobilized on polyurethane foam cubes in bioreactors, were used to decolorize three industrial and model dyes at concentrations of 200, 1000 and 2000 ppm. Five sequential cycles were run for each dye and fungus. The activity of laccase, Mn-dependent and independent peroxidases, lignin peroxidase, and aryl-alcohol oxidase were daily monitored during the cycles and the toxicity of media containing 1000 and 2000 ppm of each dye was assessed by the Lemna minor (duckweed) ecotoxicity test. Both fungi were able to efficiently decolorize all dyes even at the highest concentration, and the duckweed test showed a significant reduction (p 相似文献   

Kynureninase-Type enzymes of Penicillum roqueforti, Aspergillus niger, Rhizopus stolonifer, and Pseudomonas fluorescens: further evidence for distinct kynureninase and hydroxykynureninase activities.

The kynureninase-type enzymes of three fungi and one bacterium were isolated and examined kinetically for their ability to catalyze the hydrolysis of L-kynurenine and L-3-hydroxykynurenine. The phycomycete Rhizopus stolonifer was found to contain a single, constitutive enzyme with Km for L-3-hydroxykynurenine and L-kynurenine of 6.67 times 10-minus 6 and 2.5 times 10-minus 4 M, respectively. The ascomycetes Aspergillus niger and Penicillium roqueforti each contain an enzyme, induced by L-tryptophan, with similar Km for L-3-hydroxykynurenine and L-kynurenine ranging from 5.9 times 10-minus 5 to 14.3 times 10-minus 5 M, as well as a constitutive enzyme with Km for the two substrates of similar to 4 times 10-minus 6 M and 10-minus 4 M. The bacterium Pseudomonas fluorescens has a single, inducible enzyme with Km for L-3-hydroxykynurenine and L-kynurenine of 5 times 10-minus 4 and 7 times 10-minus 5 M. In addition, significant differences in maximal velocities (Vmax) were observed in two cases. The Vmax of the inducible activity from P. fluorescens was 4.5 times greater for L-kynurenine than L-3-hydroxykynurenine, whereas the Vmax of the constitutive activity from R. stolonifer was 2.5 times greater for L-3-hydroxykynurenine. It is concluded (i) that the constitutive activities are hydroxykynureninases involved in the biosynthesis of nicotinamide adenine dinucleotide from L-tryptophan, (ii) that the inducible activities are kynureninases involved in the catabolism of L-tryptophan to anthranilate, and (iii) that R. stolonifer and P. fluorescens, respectively, carry the most specific examples of each type of enzyme.     

Enterobacter cloacae is an endophytic symbiont of corn

The bacteriumEnterobacter cloacae is presently used for biocontrol of postharvest diseases of fruits and vegetables and as a preplant seed treatment for suppression of damping-off. This bacterium has apparent affinities for several grass species, but it is not considered to be an endophyte. While screening corn for fungi and bacteria with potential for biocontrol of various corn diseases, the surface-sterilized kernels of one unknown Italian corn cultivar produced fungus-free corn seedlings with roots endophytically infected byE. cloacae. This paper describes the microscopic nature ofE. cloacae RRC 101 with corn, and the in vitro control ofFusarium moniliforme and other fungi with this bacterium. Light and electron microscopy determined that this isolate ofE. cloacae was biologically associated with corn seedling roots, where it was distributed intercellularly within the cortex and stele. This is a first report of a strain of this bacterium as an endophytic symbiont of roots. Following a topical application ofE. cloacae to kernels, and upon germination this bacterium readily infected roots of two other corn cultivars. The bacterium was observed within the endosperm of germinating corn seedling, but germination was not affected. Further, the bacterium was isolated from leaves and stems of 3- to 6-week-old seedlings indicating that the above ground portions of corn were also colonized. There was no evidence of damage to cells of the root during a three to four week observation period. This bacterium was antagonistic to several isolates of the corn pathogenFusarium moniliforme, and to two other species of fungi, all of which produce mycotoxins on corn.     

Expression systems of human β-defensins: vectors,purification and biological activities

Human beta-defensins are 2–5 kDa, cationic, microbicidal peptides, which represent the first-line host defense against several Gram-negative and Gram-positive bacteria, fungi and viruses. They contain a conserved disulfide-bridge pattern of three pairs of intramolecular cystine bonds. The well-known public health problem related with the growing number of multiresistant bacteria has driven research to look for novel antibiotics, such beta-defensins and a feasible way to produce them. Heterologous expression of beta-defensins could be one way to generate large quantities of beta-defensins for clinical research; however, heterologous expression of beta-defensins has some biochemical problems, such toxicity toward the host cell, peptide degradation by proteolytic cell enzymes, size, folding constrains and low recombinant peptide yields. In this communication, several heterologous systems for producing human beta-defensins are reviewed.     

阿特拉津降解菌Acinetobacter sp. DNS32对无机氮源的响应

【目的】研究Acinetobacter sp.DNS32的生长、阿特拉津降解能力和降解基因转录水平的表达对无机氮素的响应关系,为菌株的工程应用提供指导与理论基础。【方法】以Acinetobactersp.DNS32为对象,采用摇瓶法研究菌株在阿特拉津培养基中菌株生长情况及降解能力对外加硝态氮与铵态氮的响应关系,利用荧光定量PCR技术检测DNS32降解基因表达量对外加无机氮源的响应关系。【结果】外加无机氮源可以促进DNS32菌株的生长,提高阿特拉津降解能力,无机氮源对DNS32菌株的trzN、atzB和atzC 3种降解基因表达均有促进作用,加入无机氮源的试验处理中DNS32菌株trzN基因的表达量最高可达对照的11.252±2.408倍,推断DNS32菌株的这3种降解基因所编码的酶是稳定表达的组成酶。【结论】DNS32降解阿特拉津不受"氮饥饿"诱导机制调控,且无机氮源的存在对菌株的生长与降解有促进作用,因此菌株在土壤修复实践中具有广阔的应用前景。     

Effect of the carbohydrate growth substrate on polysaccharolytic enzyme formation by anaerobic fungi isolated from the foregut and hindgut of nonruminant herbivores and the forestomach of ruminants

The effect of the carbohydrate growth substrate on polysaccharide-degrading enzyme formation by anaerobic fungi was examined using four strains of Piromyces isolated from hindgut fermenters, three Piromyces isolates from the pre-peptic forestomach of macropodid marsupials, and two ruminal isolates of Neocallimastix spp. The range of enzymes formed by the nine isolates was similar although, under the growth conditions examined, one hindgut isolate did not form amylolytic enzymes. The cellulolytic and xylanolytic enzyme profiles were the same: inter-strain differences in the levels of enzymic activity were apparent, but they were not related to either the genus or intestinal origin of the isolates. Pectin degrading enzymes were not detected in any of the isolates. The cellulolytic and xylanolytic enzymes were formed constitutively during growth on mono-, di- and polysaccharidic carbohydrates but the specific activities were both strain-and substrate-dependent. The activities were considerably lower in glucose-grown preparations of three of the fungi (one each from the hindgut, foregut and rumen) indicating that enzyme synthesis was repressed by glucose; enzyme formation by the other isolates studied was not controlled by catabolite regulatory mechanisms.     

Identification of genes encoding microbial glucuronoyl esterases

One type of covalent linkages connecting lignin and hemicellulose in plant cell walls is the ester linkage between 4-O-methyl-D-glucuronic acid of glucuronoxylan and lignin alcohols. An enzyme that could hydrolyze such linkages, named glucuronoyl esterase, occurs in the cellulolytic system of the wood-rotting fungus Schizophyllum commune. Here we report partial amino acid sequences of the enzyme and the results of subsequent search for homologous genes in sequenced genomes. The homologous genes of unknown functions were found in genomes of several filamentous fungi and one bacterium. The gene corresponding to the cip2 gene of Hypocrea jecorina (Trichoderma reesei), known to be up-regulated under conditions of induction of cellulolytic and hemicellulolytic enzymes, was over-expressed in H. jecorina. The product of the cip2 gene was purified to homogeneity and shown to exhibit glucuronoyl esterase activity.     

Acid Protease Production by Fungi Used in Soybean Food Fermentation

Growth conditions for maximum protease production by Rhizopus oligosporus, Mucor dispersus, and Actinomucor elegans, used in Oriental food fermentations, were investigated. Enzyme yields by all three fungi were higher in solid substrate fermentations than in submerged culture. The level of moisture in solid substrate must be at about 50 to 60%. Very little growth of these fungi was noted when the moisture of substrate was below 35%, whereas many fungi including most storage fungi generally grow well on solid substrate with that level of moisture. Among the three substrates tested—wheat bran, wheat, and soybeans—wheat bran was the most satisfactory one for enzyme production. The optimal conditions for maximum enzyme production of the three fungi grown on wheat bran were: R. oligosporus, 50% moisture at 25 C for 3 to 4 days; M. dispersus, 50 to 63% moisture at 25 C for 3 to 4 days; A. elegans, 50 to 63% moisture at 20 C for 3 days. Because these fungi are fast growing and require high moisture for growth and for enzyme synthesis, the danger of contamination by toxin-producing fungi would be minimal.     

Inactivation of Viruses in Bubbling Processes Utilized for Personal Bioaerosol Monitoring

A new personal bioaerosol sampler has recently been developed and evaluated for sampling of viable airborne bacteria and fungi under controlled laboratory conditions and in the field. The operational principle of the device is based on the passage of air through porous medium immersed in liquid. This process leads to the formation of bubbles within the filter as the carrier gas passes through and thus provides effective mechanisms for aerosol removal. As demonstrated in previous studies, the culturability of sampled bacterium and fungi remained high for the entire 8-h sampling period. The present study is the first step of the evaluation of the new sampler for monitoring of viable airborne viruses. It focuses on the investigation of the inactivation rate of viruses in the bubbling process during 4 h of continuous operation. Four microbes were used in this study, influenza, measles, mumps, and vaccinia viruses. It was found that the use of distilled water as the collection fluid was associated with a relatively high decay rate. A significant improvement was achieved by utilizing virus maintenance fluid prepared by using Hank's solution with appropriate additives. The survival rates of the influenza, measles, and mumps viruses were increased by 1.4 log, 0.83 log, and 0.82 log, respectively, after the first hour of operation compared to bubbling through the sterile water. The same trend was observed throughout the entire 4-h experiment. There was no significant difference observed only for the robust vaccinia virus.