两株芽胞菌对烟草废料烟碱与绿原酸降解的研究

为综合利用烟草废料,筛选得到能有效降解烟碱与绿原酸的两株芽胞菌,考察了所选菌株对烟碱与绿原酸的降解特性。实验结果表明,菌株Bacillus sp．X6表现出较高降解烟碱能力,培养36h可将含烟碱6．04mg／g烟草物料中的烟碱降解60．3％,72h降解率可达87．6％;对绿原酸降解效果最好的是菌株Bacillus sp．Xy,培养48h将含绿原酸10．57mg／g烟草物料中的绿原酸降解了50．5％,72h可将绿原酸降解62．2％,     

一株降烟碱细菌的筛选、鉴定及其降解特性研究

以烟碱为唯一碳源,从湖南张家界烟草种植地的土壤中分离得到一株降解烟碱能力较好的菌株。经常规形态观察和生理生化实验结果表明,该菌为放射形土壤杆菌或根癌土壤杆菌(Agrobacterium radiobacter／tumefaciens)。研究表明,该菌的降解烟碱最适pH和温度分别为7.0和30℃。该菌能够利用烟碱为唯一碳源,在含烟碱的培养基中发酵液呈淡黄色-绿色-墨绿色-深综色变化,培养48h后,烟碱的降解率可达71%,具有较好的烟草工业应用前景。     

1株兼有烟碱降解活性解磷菌的分离鉴定

从烟草(Nicotiana tabacum L.)根际土壤中分离到1株兼有烟碱降解活性的解磷菌株,编号为YF24;菌株YF24经过48 h发酵后,培养基上清液中游离态磷含量达到141.6μg/m L,烟碱降解率达到77%,确定YF24具有解磷和烟碱降解的双重活性;对菌株YF24生长特性的研究表明,其最适生长温度是30~35℃,最适p H值范围是5.5~7.0,耐盐性差。通过形态特征观察、生理生化特性测定和16S r DNA序列分析,确定菌株YF24隶属于不动杆菌属Acinetobacter,暂命名为Acinetobacter sp.YF24。菌株YF24可作为烟草专用菌肥开发、诱变育种的良好出发菌株。     

一株高浓度烟碱降解菌的筛选、分离和初步鉴定

采用以烟碱为唯一碳源氮源的选择培养基,从烟草和植烟土壤中分离筛选出15株高浓度烟碱降解的菌株,其中菌株D9烟碱降解能力最强,其烟碱降解率为82%,耐受烟碱的最高浓度为8 g/L。经常规形态特征、16S rDNA同源序列以及系统进化树分析,初步鉴定该菌株为类似氧化微杆菌,命名为Microbacterium sp. GYC29。本研究为微生物降解烟碱的研究及应用提供了菌种资源。     

烟碱降解细菌的分离、鉴定及其降解性能的初步研究

从福建三明地区的土壤中分离得到一株能够高效降解烟碱的菌株 ,编号为DN2。该菌经常规的形态、生理生化分析以及 16SrDNA序列同源性分析 ,鉴定为Ochrobactrumintermedium ,属于α_变形杆细菌纲。该菌在 30℃～4 0℃和pH 6 . 0～ 9. 0范围内具有较高的降解活性 ,其最适值分别为 30℃和 6 5 ,烟碱的耐受浓度在无机盐培养基中可达到 4 0 0 0mg L。该菌能够以烟碱为唯一碳源生长 ,对于 5 0 0mg L烟碱的降解速率为 15mg L·h ,36h烟碱降解率为97. 6 5 %。该菌在烟草工业和环境保护上可能具有应用前景。     

菌株DN2对烟草薄片制备液中烟碱的降解

使用O.intermedium DN2降解烟草薄片制备液中的烟碱。研究了各种工艺参数对烟碱降解的影响,单因素考察结果表明烟草薄片制备液中烟碱降解的最适条件是:添加0.1%的酵母膏,使用氨水将pH调节到7.0,接种15%种子液,培养温度30oC。在上述条件下,采用30L发酵罐对烟草薄片制备液进行3个批次的半连续发酵,烟碱的平均降解速率为140.55mg/L/h,高于其他烟碱降解菌株。该结果表明菌株DN2可以用来降低烟草薄片中的烟碱含量。     

DN2菌降解烟碱的动力学及其应用研究

研究了菌株DN2降解烟碱的特性和对烟草废弃物中烟碱的降解情况。结果表明,该菌降解烟碱的最适条件为接种量为5 %,温度30 ℃,初始pH值为6.5。在该条件下,对初始烟碱浓度为500 mg/L的降解过程进行考察。结果表明,未经烟碱诱导的降解曲线呈倒S曲线,半衰期为17.43 h;经烟碱诱导的降解曲线符合Eckenfelder动力学模型,半衰期为4.10 h。添加0.1 %(质量分数)葡萄糖,可提高菌株DN2的烟碱耐受浓度,达5000 mg/L。菌株DN2能够降解烟草废弃物水提液中的烟碱（烟碱含量约为2220 mg/L）,60 h时烟碱的降解率为95.22 %,表明该菌在治理烟碱污染环境方面具有应用价值。     

褐黄孢链霉菌原生质体制备与再生

以纳他霉素产生菌株褐黄孢链霉菌SG-2002为出发菌株,考察了菌丝体培养基、甘氨酸浓度、培养时间、溶菌酶浓度、酶解温度、酶解时间及再生培养基对原生质体形成与再生的影响.原生质体形成和再生的最佳条件为S培养基中添加1%的甘氨酸,菌丝体培养 30 h,溶菌酶浓度 40 mg/(g菌体干重),酶解温度 30 ℃,酶解时间 60 min.褐黄孢链霉菌的原生质体形成量达到4.0×106 个/mL,再生培养基选择R5′培养基,再生率为9.0%.     

一株能高效降解梗丝果胶和纤维素的曲霉的筛选和鉴定

用传统培养法从广西梧州六堡茶中初筛获得5株真菌菌株,再用烟草梗丝培养基复筛,得到一株可以高效降解梗丝果胶和纤维素的产香菌菌株,经ITS及部分r DNA序列分析及形态特征观察,将其鉴定为塔宾曲霉(Aspergillus tubingensis),命名为GYC 501。该菌株在发酵培养过程中,能够产生令人愉悦的特殊香气,并且具有很好的果胶酶和纤维素酶活性,在2%蔗糖察氏液体培养基中培养36 h,纤维素酶活力达到418.2 U,培养48 h,果胶酶活力达到471.4 U。该菌株有望用于烟草梗丝发酵,降解梗丝中的果胶和纤维素,提高梗丝的质量和工业可用性。     

甲胺磷降解菌的筛选及降解特性研究

从长期受有机磷农药污染的土壤中分离到1株能降解甲胺磷的菌株B15,经生理生化鉴定为巨大芽孢杆菌(Bacillus megaterium)。在甲胺磷无机盐培养基(甲胺磷浓度为0.5%)生长时,最适生长温度为28℃,最适pH为7.0,摇床培养(28℃190 r/min)48 h降解率达到83%。菌株在甲胺磷浓度为1%的无机盐培养基上能生长,但是在甲胺磷浓度为0.5%的无机盐培养基上生长最好,降解率最高。外加碳氮源对菌株的降解率有所提高,但是超过某一浓度降解率随着浓度的增加反而下降。     

南极抗细菌活性菌株的筛选及系统发育分析

分别以大肠杆菌、枯草芽孢杆菌、金黄色葡萄球菌、青枯假单胞菌、绿脓假单胞菌和苏云金芽孢杆菌为指示菌,采用琼脂扩散法对实验室保存的580株极地细菌进行了抗菌活性菌株的筛选与活性验证,从中筛选出4株对上述指示菌株具有明显抗菌效果的活性菌株,其编号分别为97、Z11、Z18及Z19,并对其生长曲线、抗菌活性曲线和系统发育地位进行研究。结果表明,4株菌均在培养24 h后进入指数生长期,菌株97在培养48 h后达到稳定期,而菌株Z11、Z18及Z19在培养60 h后达到稳定期。抗菌活性分别在培养84、96、72和72 h时达到最高。系统发育分析表明,该4株菌分别属于伦黑墨氏菌属(Rheinheimera)、嗜冷杆菌属(Psychrobacter)、假单胞菌属(Pseudomonas)和嗜冷杆菌属(Psychrobacter)。     

The effect of culture conditions on hydrophobic properties of Pseudomonas aeruginosa

The cell surface hydrophobicity (CSH) plays an important role in a adhesion of bacteria on solid surfaces. CSH of 62 Pseudomonas aeruginosa strains isolated from humans and different animals was assessed using the ammonium sulfate salt aggregation test. Bacteria were grown for 24 h and 48 h at a room temperature (22 degrees C) and 37 degrees C on enrichment broth and agar (Biomed) and tryptic soy agar (Difco). The hydrophobic properties of the Pseudomonas aeruginosa strains were depended on the temperature, time of the culture of bacteria and the kind of media. CSH properties were most frequently expressed when the analyzed strains were cultured in enrichment broth. In a such conditions Pseudomonas aeruginosa strains were more hydrophobic when grown at 22 degrees C (94% after 24 h and 87% after 48%) than those at 37 degrees C (72% after 24 h and 71% after 48 h). Among strains cultured in tryptic soy agar at 37 degrees C, 48% after 24 h and 75% after 48 h were autoaggregating, representing very strong hydrophobic properties.     

Maturation, fertilization, and development of dog oocytes in vitro.

Preovulatory oocytes were collected from ovaries of beagle bitches that had received superovulatory treatment. They were cultured in a modified Krebs-Ringer bicarbonate solution containing 10% fetal calf serum and 30 mg/L gentamicin sulfate for up to 72 h. About 32% of oocytes reached metaphase II by 72 h of culture. When these in vitro-matured oocytes were inseminated with ejaculated beagle spermatozoa that had been preincubated for 4 h, sperm penetration of the zona pellucida started about 1 h after insemination, and both male and female pronuclei were seen in the ooplasm at 8 h after insemination. At 18-20 h after insemination, oocytes were transferred to Whitten's medium and cultured for 76-78 h. The first cleavage was observed at 48 h after insemination, and 15 of 45 oocytes developed to the 2-8-cell stage. These results demonstrate that in vitro-matured canine oocytes can be fertilized and develop to the 8-cell stage in vitro.     

The secretory response of hypothalamic β-endorphin neurons to acute and chronic nicotine treatments and following nicotine withdrawal

In the present study, we determined the effect of acute and chronic nicotine treatments on the secretion of immunoreactive β-endorphin (IR-β-EP) and cell viability of cultured hypothalamic neurons. Also, we determined the secretory response of IR-β-EP following withdrawal from a long-term nicotine treatment. Fetal hypothalamic cells were dissociated and maintained in cultures for 9 days and were treated with various doses of nicotine (1, 6,12 and 18 μM) for 6 h (acute treatment) or treated with nicotine at 12 h intervals for 96 h (chronic treatment). Determination of IR-β-EP concentrations in the media revealed that 6–18 μM doses of nicotine increased IR-β-EP secretion from these cultures for a period of 24 h; after this period, the cultured cells did not respond to these doses of nicotine. The desensitization of β-EP neurons 24 h after treatment with nicotine did not appear to be related to the loss of viable cells. Determination of withdrawal response after 72 h of constant nicotine (6 μM) treatments revealed that the hypothalamic neurons secrete elevated amounts of IR-β-EP for a period of 72 h after nicotine withdrawal. These results suggest that: 1) acute treatment with nicotine stimulates hypothalamic IR-β-EP release; 2) chronic nicotine treatment desensitizes β-EP-secreting neurons and, 3) β-EP neurons in primary culture show withdrawal response to nicotine.     

Quantitative differences in the expression of a 72,000 molecular weight cell surface glycoprotein (GP72) in Trypanosoma cruzi zymodemes

A high affinity monoclonal antibody, 8G2 B9, was used to assess the expression of a 72,000 m.w. glycoprotein ( GP72 ) in isoenzyme-typed T. cruzi strains ( zymodemes ). Western blotting analysis of T. cruzi clones showed that 8G2 B9 bound strongly to GP72 and also suggested that this antigen was absent or weakly detectable in T. cruzi zymodeme 1 (Z1) strains. Purified 8G2 B9 was radiolabeled with 125I and used in an inhibition radioimmune binding assay to compare the quantities of GP72 in different zymodemes . Ninety-six T. cruzi strains were assayed, of which 36 were Z1, 36 were Z2, five were Z3 , and 19 were Z2 (heterozygous). Most (64%) Z1 strains lacked detectable GP72 , whereas this antigen was always detected Z2 and Z2 (heterozygous) strains. There was an 18-fold difference between geometric mean values for the quantities of GP72 (expressed as nanograms per milligram total cell protein) in Z1 and Z2 strains (Z1, 36 ng/mg; Z2, 639 ng/mg; p less than 0.001). There were also significant differences between the geometric mean values for Z2 and Z2 (heterozygous) strains, i.e., 639 ng/mg and 1648 ng/mg, respectively (p less than 0.001). GP72 was detected in four of the Z3 strains in quantities ranging from 740 to 3640 ng/mg. The absolute amounts of antigen in GP72 -positive strains were low, comprising less than 1% of the total cell protein. The specificities of two other anti- GP72 monoclonal antibodies, 7C6 D7 and WIC 29.26, were compared with 8G2 B9. Both antibodies completely inhibited the binding of 8G2 B9 to GP72 in solid phase immunoassays, suggesting that they reacted with the same antigenic determinants. The results show that monoclonal antibody-based assessments of the expression of GP72 correlate with zymodeme classification, and they also suggest that the monoclonal antibodies recognize major antigenic determinants on GP72 . It should be possible to use 8G2 B9 as an immunologic marker to additionally investigate the clinical significance of T. cruzi zymodemes and the biologic significance of GP72 .     

微生物对烟叶蛋白质含量的影响

经菌株不同浓度、不同菌株、及同浓度不同菌株的等量组合处理过的烟叶放置一段时间未经发酵与发酵后对蛋白质检测,结果表明降解K326中部碎烟叶蛋白质的处理中Y菌株106浓度降解率最高,为18.81%;处理烟叶发酵后,降解率最高的处理是S5菌株107浓度,高达24.46%。K326上部碎烟叶处理后检测结果表明,对蛋白质降解率最高的处理是Y与S8混合,降解率为8.98%;K326上部碎烟叶处理发酵后检测结果表明,S8菌株108浓度处理降解率最高,达24.09%,其次为S5菌株108浓度处理降解率达23.48%。整叶处理结果表明S8降解蛋白质效果最好,降解率达5.17%;整叶处理烟叶发酵后检测S5对烟叶降解率最高,为5.17%。     

Nicotine degradation enhancement by <Emphasis Type="Italic">Pseudomonas stutzeri</Emphasis> ZCJ during aging process of tobacco leaves

Nicotine is a key harmful component of tobacco and cigarettes, and the development of low-nicotine cigarettes is of increasing importance in the market. The objectives of this study are to isolate native nicotine-degrading strains and evaluate their feasibility for nicotine reduction during the aging (or fermentation) of tobacco leaves. A novel nicotine-degrading strain was isolated and identified as Pseudomonas stutzeri ZCJ based on its 16S rDNA sequence and morphological-biochemical characteristics. In submerged cultures, P. stutzeri ZCJ could tolerate 4.5 g/L nicotine and completely degrade 1.5 g/L nicotine within 24 h at 37°C and pH 7.4. The addition of glucose (1 g/L) could improve nicotine degradation by P. stutzeri ZCJ in submerged cultures. After submerged culturing, the cell suspension of P. stutzeri ZCJ could be utilized to improve nicotine reduction in tobacco leaves during solid-state fermentation. The nicotine content of tobacco leaves decreased by as much as 32.24% after 7 days of solid-state fermentation by P. stutzeri ZCJ, suggesting the industrial application potential of the native strain to enhance nicotine degradation during the aging of tobacco leaves.