高效解磷细菌的筛选及其对玉米苗期生长的促进作用

采用改良后的PVK平板,从石灰性土壤上长势良好的野生植物根表分离到44株解磷细菌,通过NBRIP液体摇瓶实验,培养7 d后发现：K₃菌株培养液中全磷浓度高达643.2 μg·ml^-1,可溶性磷为584.8 μg·ml^-1,约有12.9%的磷酸三钙被溶解出来,为对照(CK)的10.5倍;K₉菌株培养液的全磷浓度为608.5 μg·ml^-1,可溶性磷浓度为606.4 μg·ml^-1.盆栽试验的结果表明：接种解磷细菌的处理玉米株高、茎粗和干质量显著高于CK;将有机肥作为载体和解磷细菌一同混合施入土壤的处理,玉米苗干质量较单施解磷菌显著增加.经初步鉴定, K₃、K₉为假单胞菌属.     

不同品系萼花臂尾轮虫休眠卵的形态特征

对采自青岛和芜湖两地的萼花臂尾轮虫在3种温度(20 ℃、25 ℃和30 ℃)和2种藻类食物浓度(1.0×10⁶和5.0×10⁶ cells·ml^-1)下所产休眠卵的长径、短径和体积等形态特征进行了显微测量、计算和分析.结果表明,2种食物浓度下,培养温度以及培养温度和品系间的交互作用均对轮虫休眠卵的长径、短径和体积具有显著影响.当食物浓度分别为1.0×10⁶和5.0×10⁶ cells·ml^-1时,轮虫在20 ℃下所产休眠卵的长径、短径和体积均最大;在25 ℃和30 ℃下所产休眠卵的短径和体积均最小.品系对轮虫休眠卵长径、短径和体积的影响也取决于食物浓度.当食物浓度为1.0×10⁶ cells·ml^-1时,芜湖品系轮虫的休眠卵长径、短径和体积(156.00 μm、99.95 μm和12 269.11 μm³)均显著大于青岛品系轮虫的休眠卵(145.13 μm、91.97 μm和10 498.19 μm³);而当食物浓度为5.0×10⁶ cells·ml^-1时,芜湖品系轮虫的休眠卵长径、短径和体积(155.68 μm、100.85 μm和12 348.59 μm³)均与青岛品系轮虫的休眠卵(156.63 μm、98.04 μm和12 054.20 μm³)之间无显著差异.两品系中,仅芜湖品系轮虫休眠卵的长径、短径和体积分别与温度呈曲线相关.同一温度下,两品系轮虫的休眠卵体积均随着食物浓度升高而增大;但30 ℃下芜湖品系轮虫所产休眠卵体积却随着食物浓度的升高而减小.     

银离子抗性细菌质粒的分离与鉴定

通过对不同化工厂废水处理池的活性污泥进行富集、不同浓度银离子驯化后,分离得到30株银离子抗性细菌,最大硝酸银耐受量可达80 mg·ml^-1.对这些细菌进行质粒抽提与鉴定,质粒检出率为76.67％.40 mmol·L^-1的苯甲酸钠对HAg4细菌质粒的消除率可达98.75％;而350 μg· ml^-1的吖啶橙对HAg4细菌质粒的消除率只有77.78％.细菌质粒与银离子抗性密切相关.     

青海盐湖嗜盐微生物类群及F16菌株生长特性和抗菌、抗肿瘤活性

从青海盐湖底泥中分离出45株嗜盐微生物.其中,丝状真菌F16的抗菌和抗肿瘤活性最强,其发酵液的乙酸乙酯粗提物能抑制4种细菌的生长,尤其对大肠杆菌的抑制作用最强,具有较强的细胞毒活性,当粗提物浓度为50 μg·ml^-1时对肝癌细胞BEL7402的抑制率可达76.91％.F16菌株的最适生长温度为15 ℃;培养基盐度升高,对F16的抑制性增强,当盐度超过15％时,F16不生长;在pH值为5～9范围内,F16生长良好.     

苦瓜叶提取物对美洲斑潜蝇取食和产卵行为的抑制作用

美洲斑潜蝇是危害蔬菜、观赏植物的重大害虫之一.苦瓜叶乙醇提取物(浓度为2000～4000 μg·ml^-1)对美洲斑潜蝇成虫的取食和产卵都具有较强的抑制作用.用环己烷、乙酸乙酯、正丁醇和水依次对乙醇提取物进行萃取,并测试了4种萃取物对美洲斑潜蝇成虫取食和产卵的抑制作用.结果表明: 环己烷、乙酸乙酯、正丁醇和水萃取物在浓度为1000 μg·ml^-1时,处理后2 d对美洲斑潜蝇成虫的拒食率分别是11.08%、34.89%、22.99%和 0,产卵抑制率分别是0、30.91%、6.45%和 0.其中,乙酸乙酯萃取物的活性最强,当其浓度为4000 μg·ml^-1时,处理后2 d对美洲斑潜蝇成虫的拒食率和产卵忌避率分别为70.95％ 和69.49％.乙酸乙酯萃取物经硅胶柱层析分离得到(19S,23E)-5β,19-环氧-19-甲氧葫芦素-6,23-二烯-3β,25-二醇 (化合物1)、(19R,23E)-5β,19-环氧-19-甲氧葫芦素-6,23-二烯-3β,25-二醇(化合物2) 和3β,7β,25-三羟基葫芦素-5,23-二烯-19-醛缩-3-O-β-D-吡喃葡糖苷（化合物3）,3种化合物在供试的浓度（100～400 μg·ml^-1）条件下对美洲斑潜蝇的取食和产卵行为都有明显的抑制作用.在400μg·ml^-1浓度时,化合物1、化合物2和化合物3对美洲斑潜蝇成虫的拒食率分别是66.89%、53.53%和78.02%,产卵抑制率分别是76.32%、58.36%和78.36%.     

龙须菜对重金属铜胁迫的生理响应

研究了大型海藻龙须菜(Gracilaria lemaneiformis)对不同浓度重金属铜(0、25、50、100、250和500 μg·L^-1)胁迫的生理响应.结果表明:当Cu²⁺浓度≥50 μg·L^-1时,龙须菜藻体的相对生长速率显著下降,最大光化学量子产量、最大相对电子传递速率和相对电子传递效率呈相同的变化趋势.随着Cu²⁺浓度的升高,龙须菜藻体最大净光合速率和光饱和点显著降低,而光补偿点显著升高,叶绿素a、类胡萝卜素和藻胆蛋白含量则呈先升高后下降的趋势;当Cu²⁺浓度达到500 μg·L^-1时,叶绿素a、类胡萝卜素和藻胆蛋白含量显著下降.说明龙须菜在低浓度Cu²⁺胁迫下具有一定的抵抗能力,而当Cu²⁺浓度≥50 μg·L^-1时,会对藻体生理活动造成显著的抑制作用.     

DDT对多刺裸腹溞的急性毒性和生命表参数的影响

采用48 h急性毒性试验研究了DDT对多刺裸腹溞的48小时LC₅₀值,采用生命表试验方法研究了暴露于不同浓度（1、8、16、24、32和40 μg·L^-1）DDT溶液中的多刺裸腹溞的生命表统计学参数.结果表明：DDT对多刺裸腹溞48小时LC₅₀值为324 μg·L^-1;浓度在1～40 μg·L^-1的 DDT对多刺裸腹溞的生命期望、净生殖率、世代时间和总繁殖率均没有显著影响(P>0.05),但对种群内禀增长率(r_m)影响显著 (P<0.05).与空白对照组相比,浓度为8、16和40 μg·L^-1的DDT显著地提高了多刺裸腹溞种群r_m.在使用多刺裸腹溞的生命表统计学参数监测亚致死浓度的DDT的生态影响时,r_m是较敏感的指标.     

青岛近海及其临近海域冬季微微型浮游植物的分布

微微型浮游植物（0.2～2.0 μm） 是海水中最小的自养浮游生物, 在世界各海域广泛分布, 并在海洋有机物质循环中起着非常重要的作用.利用荧光显微技术对青岛近海及其邻近海域冬季微微型浮游植物丰度进行了调查,研究了微微型浮游植物的空间变化和昼夜变化的特征, 并分析了微微型浮游植物丰度与环境因子的相关性. 结果显示, 冬季该海域以富含藻红素（Phycoerythrin-rich, PE）的聚球藻(Synechococcus, Syn)细胞占优势,微微型真核藻类（Picoeukaryote, Euk）次之,而富含藻蓝素（Phycocyanin-rich, PC）的聚球藻细胞数量很低, 未发现原绿球藻（Prochlorococcus, Pro）的存在.Syn 的变化范围为8.97×10³～1.95×10⁵ cells·ml^-1, 平均4.67×10⁴ cells·ml^-1; Euk的变化范围为1.95×10²～1.01×10⁴ cells·ml^-1, 平均2.39×10³ cells·ml^-1. Syn丰度在胶南以南海域出现高值区域, 在即墨海域和崂山东南海域出现低值区域. Euk丰度在日照海域出现高值区域; 崂山海域为低值区域; 各水层Syn和Euk丰度均无明显差异(P﹥0.05). 对胶州湾中部连续站4层水体的24 h昼夜连续变化进行观测发现, Syn、Euk丰度都有明显昼夜波动.相关性分析表明： Syn与温度、 电导率呈正相关, 与溶氧浓度呈显著负相关; Euk与盐度和溶氧浓度呈显著负相关. 微微型浮游植物对总浮游植物生物量的贡献约为20％.     

一摸香叶精油对致倦库蚊的生物活性及其成分分析

参照“农药登记卫生用杀虫剂的室内药效评价/驱避剂GB/T 17322.10—1998”,研究了一摸香鲜叶的水蒸汽蒸馏精油对致倦库蚊的驱避作用;参照“电热片蚊香的室内药效测定方法GB 13917.5—1992”,测试了该精油对致倦库蚊成蚊的熏杀效果;采用浸液法测试了其对致倦库蚊幼虫及蛹的毒杀活性;并用GC-MS测试分析了其化学成分.结果表明：一摸香叶精油在1.5 mg·cm^-2剂量下对实验室饲养的未吸血致倦库蚊雌成蚊的驱避100%保护时间为(6.54±0.17) h,对成蚊的熏杀24 h LC₅₀值为6.895 μg·cm^-3,对成蚊的熏蒸KT₅₀值为6.46 min (熏蒸剂量为11.850 μg·cm^-3),对Ⅳ龄期幼虫的24 h毒杀LC₅₀值为119.020 μg·ml^-1.精油中共鉴定出17种化合物,占该精油挥发性成分总量的97.4%.说明一摸香叶精油对致倦库蚊具有显著的驱避作用和极强的毒杀活性.     

二氧化氮对樟树幼苗生长及光合作用的影响

采用开顶式人工熏气装置,对1年生樟树幼苗进行了为期2个月不同体积分数NO₂(0.1、0.5和4.0 μl·L^-1)熏气试验,研究其对幼苗生长及光合作用的影响.结果表明:0.5和0.1 μl·L^-1 NO₂处理促进了樟树幼苗生长,而4.0 μl·L^-1 NO₂处理则抑制其生长.各处理樟树幼苗叶片净光合速率(P_n)日变化呈不对称的双峰型曲线,存在光合“午休”现象;在光合日进程中,0.5 μl·L^-1 NO₂处理使叶片P_n提高,最大值达8.542 μmol CO₂·m^-2s^-1,4.0 μl·L^-1NO₂处理的大多数时段使P_n降低,而0.1 μl·L^-1 NO₂处理对P_n的影响则依时段而不同;0.5和4.0 μl·L^-1 NO₂处理提高了叶片气孔导度(G_s)和胞间CO₂浓度(C_i)的最大值和最小值,0.1 μl·L^-1 NO₂处理提高了C_i的最大值和最小值,降低了G_s的最大值和最小值.熏气处理中、后期,0.5μl·L^-1 NO₂处理叶片的日均净光合速率显著高于其他处理.在熏气处理前期,0.5和4.0 μl·L^-1 NO₂处理使叶片最大PSⅡ的光能转换效率(F_v/F_m)显著下降;在熏气处理后期,4.0 μl·L^-1 NO₂处理的叶片F_v/F_m仍显著低于对照.     

Multi-sited mutations of beta-tubulin are involved in benzimidazole resistance and thermotolerance of fungal biocontrol agent Beauveria bassiana

Fungicide resistance and thermotolerance of biocontrol agents in mitosporic fungi are of merits for enhancing fungal formulations against insect pests in the field. Among 20 wild strains of Beauveria bassiana (a well-known fungal biocontrol agent) tested in this study, 19 were sensitive or highly sensitive to carbendazim (methyl 2-benzimidazole carbamate), a typical benzimidazole fungicide, despite low resistance found in one strain. Sequential mutagenesis of a carbendazim-sensitive wild strain [minimal inhibitory concentration (MIC) = 1.32 microg ml(-1)] under artificial selection pressure generated 11 mutants sharing a common MIC of > 1000 microg ml(-1) without visible variation in colony growth and conidiation capacity. This represents at least 758-fold enhancement of the resistance among the mutants. However, accompanied with the enhanced resistance, all the mutants became less thermotolerable. Stressed at 48 degrees C, conidial LT(50)s of the mutants varied from 1.8 to 9.6 min and were lower than the parental LT(50) (36 min). Moreover, the contents of hydrophobin-like proteins in conidial walls declined significantly among the mutants compared with that of the wild parent. Mutations commonly relating to benzimidazole resistance in fungi were located at Q134, F167 and/or E198 around the taxol-binding site of beta-tubulin by sequencing the beta-tubulin of the mutants. Also, mutations of other 37 amino acid residues in the sequences (each having one to five residues mutated) were found for the first time and they were diverse in spatial structure. All mutations restricted to the half of beta-tubulin close to alpha-tubulin were likely involved in variation in each of the traits concerned but their interactions were complicated.     

Baseline sensitivities to azoxystrobin and tebuconazole in Sclerotinia sclerotiorum isolates from sunflower in Iran related to sensitivities to carbendazim and iprodione

In this study, sensitivities of 156 Sclerotinia sclerotiorum isolates collected from sunflower fields of West Azarbaijan province, Iran, were assessed to carbendazim and iprodione, and the baseline sensitivities were established for azoxystrobin and tebuconazole. Resistance to carbendazim and iprodione was observed in 53.85% and 4.49% of the isolates, respectively. The 50% effective concentration (EC₅₀) values of azoxystrobin for the isolates ranged from 0.017 to 3.515 μg/ml with a mean of 0.330 μg/ml, and 8.97% of the strains showed low levels of resistance to the fungicide. However, in the presence of salicylhydroxamic acid, all isolates were sensitive to azoxystrobin and EC₅₀ values ranged from 0.015 to 0.263 μg/ml with a mean of 0.086 μg/ml. All isolates were found to be sensitive to tebuconazole, and EC₅₀ values ranged from 0.003 to 0.177 μg/ml with a mean of 0.036 μg/ml. Among the multiple-resistant isolates, the strains exhibiting resistance to both carbendazim and iprodione were detected in the highest frequency (4.49%). No correlation was observed between mycelial growth and aggressiveness with fungicide sensitivity of the isolates suggesting the absence of fitness cost associated with resistance to the studied fungicides. The results indicated that iprodione, azoxystrobin and tebuconazole could be effectively used in rotation or mixture in spray programmes to manage S. sclerotiorum in the region. The baselines established for azoxystrobin and tebuconazole would be useful in monitoring the fungal populations in the province to assess possible shifts in fungicide sensitivity of S. sclerotiorum isolates in the future.     

Antifungal pharmacodynamic characteristics of amphotericin B against Trichosporon asahii, using time-kill methodology

We determined the MIC of amphotericin B against 45 Trichosporon asahii isolates from various clinical and environmental sources, and used in vitro time-kill methods to characterize the relationship between amphotericin B concentrations and MIC for four representative T. asahii isolates. Amphotericin B had concentration-dependent antifungal activity. MICs ranged from 0.5 to 16 microg/ml, and most T. asahii isolates (76%, 34/45) were inhibited at safely achievable amphotericin B serum concentrations (< or = 2 microg/ml). However, 40% (18/45) of isolates were not killed at these concentrations (MFCs from 1.0 to 32 microg/ml). At concentrations > or = 2 x MIC, amphotericin B exhibited fungicidal activity (< 99.9% reduction in CFU) over a 12-hr time-period; the maximal effect was achieved at > or =4 x MIC. Susceptibility testing confirmed the resistance of T. asahii to amphotericin B, and in vitro pharmacodynamic results also suggest that amphotericin B is not suitable therapy for T. asahii infection.     

Immobilization in alginate as a technique for the preservation of Bacillus thuringiensis var. israelensis for long-term preservation

Technique for immobilization using sodium alginate as the matrix to preserve Bacillus thuringiensis var. israelensis isolates for long time storage was developed. Two strains of B. thuringiensis var. israelensis viz., VCRC B-17 and WHO standard strain IPS-82 were immobilized in alginate matrix and preserved at 4 degrees C and when tested both were found to have maintained excellent viability and mosquito larvicidal activity for 10 years. Mosquito larvicidal activity of B-17 and IPS-82 alginate beads, in term of LC(50) values before storage was 72.07 ng/ml and 47.07 ng/ml, respectively and after storage at 4 degrees C for a period of 1 to 10 years the values ranged from 69.88 to 73.86 ng/ml with a mean of 72.38 ng/ml and 45.32 to 48.60 ng/ml with a mean of 47.49 ng/ml, respectively. Similarly spore count of the beads of the respective strains was 4.37 x 10(8) and 3.33 x 10(10) CFU/mg before storage. After storage at 4 degrees C for a period of 1 to 10 years the counts of the beads of the respective strains ranged from 4.23 x 10(8) to 4.83 x 10(8) CFU/mg (mean of 4.49 x 10(8) CFU/mg) and 3.2 x 10(10) to 3.87 x 10(10) CFU/mg (mean of 3.54 x 10(10) CFU/mg). The alginate matrix immobilization technique has many advantages over free cells are that they enhance the stability of both spores and toxin against several physicochemical conditions and confer reduced susceptibility to contamination.     

Use of ethidium bromide monoazide for quantification of viable and dead mixed bacterial flora from fish fillets by polymerase chain reaction

Ethidium bromide monoazide (EMA) was utilized to selectively allow conventional PCR amplification of target DNA from viable but not dead cells from a broth culture of bacterial mixed flora derived from cod fillets. The universal primers designated DG74 and RW01 that amplify a 370-bp sequence of a highly conserved region of all eubacterial 16S rDNA were used for the PCR. The use of 10 microg/ml or less of EMA did not inhibit the PCR amplification of DNA derived from viable bacteria. The minimum amount of EMA to completely inhibit the PCR amplification of DNA derived from dead bacterial cells was 0.8 microg/ml. Amplification of target DNA from only viable cells in a suspension with dead cells was selectively accomplished by first treating the cells with 1 microg/ml of EMA. A standard curve was generated relating the intensity of fluorescence of DNA bands to the log of CFU of mixed bacterial cultures for rapidly assessing the number of genomic targets per PCR derived from the number of CFU. A linear range of DNA amplification was exhibited from 1 x 10(2) to 1 x 10(5) genomic targets per PCR. The viable/dead cell discrimination with the EMA-PCR method was evaluated by comparison with plate counts following freezing and thawing. Thawing frozen cell suspensions initially containing 1 x 10(5) CFU/ml at 4, 20, and 37 degrees C yielded a 0.8 log reduction in the number of viable cells determined by both plate counts and EMA-PCR. In contrast, thawing for 5 min at 70 degrees C resulted in a 5 log reduction in CFU derived from plate counts (no CFU detected) whereas the EMA-PCR procedure resulted in only a 2.8 log reduction in genomic targets, possibly reflecting greater damage to enzymes or ribosomes at 70 degrees C to a minority of the mixed population compared to membrane damage.     

Multiple characterizations of Listeria monocytogenes sensitive and insensitive variants to divergicin M35, a new pediocin-like bacteriocin

AIMS: Divergicin M35 is a new class IIa bacteriocin produced by Carnobacterium divergicin M35. The bactericidal activity of this antimicrobial peptide was tested against a set of 11 strains of Listeria monocytogenes isolated from food. METHODS AND RESULTS: The minimal inhibitory concentration (MIC) was determined by the microdilution method. The strains tested displayed a different level of sensitivity to divergicin M35. L. monocytogenes LSD530, referred to as DivS strain, was the most sensitive and appeared to be inhibited by concentration of divergicin M35 below 0.13 microg ml(-1). The mutant resistant to divergicin M35, called DivM, was obtained from L. monocytogenes LSD530 (DivS) by gradually increasing the amounts of divergicin M35 until 1.3 microg ml(-1). Notably, DivM was stable after 50 generations. DivS parental strain was inhibited by a concentration of 4 microg ml(-1). L. monocytogenes LSD530 was shown to be resistant to divergicin M35 at 1.3 microg ml(-1). Remarkably, in the presence of divalent cations such as Ca(2+), Mg(2+) and Mn(2+), the lethality caused by divergicin M35 was reduced by 0.48, 0.54 and 0.63 log CFU per ml (after 18 h at 30 degrees C), respectively. The total DNA profiles of DivS and DivM were similar. DivS and DivM showed variable sensitivity to antibiotics. The two-dimensional (2-D) electrophoresis of cell wall proteins did not show any significant difference between DivS and DivM strains but their fatty acid composition showed a significant difference in C(16:0) content. CONCLUSIONS: Resistance to divergicin M35 is likely ascribed to modification in cell wall fatty acid composition rather than protein modification. SIGNIFICANCE AND IMPACT OF THE STUDY: This study provides original results contributing to understanding of the resistance of L. monocytogenes to divergicin M35, a new class IIa bacteriocin.     

拮抗木霉耐多菌灵菌株的筛选

该文进行了耐多菌灵生防木霉菌株的筛选和生防效果的测定研究。为获得对灰葡萄孢霉等病原菌有显著拮抗能力的耐多菌灵木霉菌株,通过含药平板诱导和紫外线诱变,获得5株耐药性菌株,在多菌灵2.0g/L浓度下生长较好,Ec50值提高了40多倍;抗性菌株在含药培养基上连续继代转移培养10次,抗性程度未见下降;经过平板对峙和活体拮抗性测定,确定T42-2为最佳拮抗性耐多菌灵菌株,其对黄瓜灰霉病的防效达92.13%,并且对多菌灵、速克灵和三唑铜存在交互抗性。     

Vancomycin-resistant Staphylococcus aureus

The evolution and molecular mechanisms of vancomycin resistance in Staphylococcus aureus were reviewed. Case reports and research studies on biochemestry, electron microscopy and molecular biology of Staphylococcus aureus were selected from Medline database and summarized in the following review. After almost 40 years of successful treatment of S. aureus with vancomycin, several cases of clinical failures have been reported (since 1997). S. aureus strains have appeared with intermediate susceptibility (MIC 8-16 microg/ml), as well as strains with heterogeneous resistance (global MIC < or =4 microg/ml), but with subpopulations of intermediate susceptibility. In these cases, resistance is mediated by cell wall thickening with reduced cross linking. This traps the antibiotic before it reaches its major target, the murein monomers in the cell membrane. In 2002, a total vancomycin resistant strain (MIC > or =32 microg/ml) was reported with vanA genes from Enterococcus spp. These genes induce the change of D-Ala-D-Ala terminus for D-Ala-D-lactate in the cell wall precursors, leading to loss of affinity for glycopeptides. Vancomycin resistance in S. aureus has appeared; it is mediated by cell wall modifications that trap the antibiotic before it reaches its action site. In strains with total resistance, Enterococcus spp. genes have been acquired that lead to modification of the glycopeptide target.     

Amino acid substitutions in the VanS sensor of the VanA-type vancomycin-resistant Enterococcus strains result in high-level vancomycin resistance and low-level teicoplanin resistance

The vancomycin-resistant enterococci GV1, GV2 and GV3, which were isolated from droppings from broiler farms in Japan have been characterized as VanA-type VRE, which express high-level vancomycin resistance (256 or 512 microg ml(-1), MIC) and low-level teicoplanin resistance (1 or 2 microg ml(-1), MIC). The vancomycin resistances were encoded on plasmids. The vancomycin resistance conjugative plasmid pMG2 was isolated from the GV2 strain. The VanA determinant of pMG2 showed the same genetic organization as that of the VanA genes encoded on the representative transposon Tn1546, which comprises vanRSHAXYZ. The nucleotide sequences of all the genes, except the gene related to the vanS gene on Tn1546, were completely identical to the genes encoded on Tn1546. Three amino acid substitutions in the N-terminal region of the deduced VanS were detected in the nucleotide sequence of vanS encoded on pMG2. There were also three amino acid substitutions in the vanS gene of the GV1 and GV3 strains in the same positions as in the vanS gene of pMG2. Vancomycin induced the increased teicoplanin resistance in these strains.