北京引进树种火炬树和水曲柳的光合特征

应用LI-6400便携式红外气体分析仪,研究了北京市两种引进乔木生长旺季的光合作用的日变化规律和光响应曲线.结果表明:①水曲柳和火炬树的光合速率(Pn)、蒸腾速率(Tr)的日变化均为"双峰"曲线,而水分利用效率(WUE)的日变化为"单峰"曲线,但三者峰值出现的时刻和大小有所不同.②火炬树的光合速率(Pn)和水分利用效率(WUE)均高于水曲柳,但蒸腾速率(Tr)要低于水曲柳.③从光响应曲线来看,两种引进乔木均为阳生植物,其中火炬树对光的适应性范围较广,而水曲柳的耐阴性较强.④逐步回归分析表明:影响光合速率的主要因子是光合有效辐射、气孔导度、胞间CO₂浓度.⑤与原产地进行对比可知:火炬树光合能力有所增加,水曲柳变化不大.研究认为,在北京,火炬树与水曲柳相比具有较强的竞争优势.研究结果可为首都园林绿化树种选择提供科学依据.     

Interactions between rumen anaerobic fungi and ciliate protozoa in the degradation of rice straw cell walls

Suspensions of mixed rumen protozoa were added to incubations of the anaerobic fungus Neocallimastix patriciarum with rice straw cell walls. The protozoa did not influence the dry matter lost from the straw, or the solubilization of monosaccharides, but they had a marked effect on the fermentation products formed. Studies with ¹⁴C-labelled protozoa suggested that the presence of protozoa reduced the fungal carboxymethylcellulase activity to around half of that found in pure cultures of the fungus.     

Field Evaluation of Fungal Competitors of Fusarium culmorum and F. graminearum, Causal Agents of Ear Blight of Winter Wheat, for the Control of Mycotoxin Production in Grain

Thirty-seven antagonists, from a collection of 113 pre-screened microorganisms, were tested in field experiments on winter wheat for their ability to control ear blight and production of mycotoxins, particularly deoxynivalenol (DON), in grain by Fusarium culmorum and F. graminearum. Ears were spray-inoculated during anthesis with spore suspensions, first of test fungi and then of the pathogen. Isolates of F. equiseti were the most effective treatments. A strain of F. equiseti (G9) decreased DON consistently on wheat inoculated with F. culmorum, compared with the control, often by more than 70%. It performed well under severe disease pressure (F. culmorum at 10⁵ conidia mL^-1) and similarly to a standard fungicide, tebuconazole. Percentages of diseased grains and amounts of DON corresponded well. Small quantities of nivalenol (NIV) occurred in grain samples after treatment with some F. equiseti strains. On wheat inoculated with F. graminearum, F. equisti G2 decreased the percentage diseased grains by 92% and DON by 94%. One strain of F. equiseti (G2) was found to produce small amounts of NIV in pure culture.     

Rapid molecular technique for identification of a biological control agent Rhodosporidium diobovatum

The purpose of this study was to develop a rapid molecular technique for identification of the biological control agent, Rhodosporidium diobovatum. DNA from all yeast cultures described below was extracted, amplified by PCR using primers specific to septate fungi, and fixed to nylon membranes. Using sequence information obtained from the GenBank database, Rhodosporidium diobovatum-specific oligonucleotides were designed and, after labeling with digoxigenin-d-UTP, were used as probes in a dot-blot hybridization assay. After preliminary testing, two probes were selected for further study. For probe RD3, a positive reaction was obtained at 38, 42 and 48°C with R. diobovatum in pure culture. Other yeast isolates such as Rhodosporidium toruloides, R. fluviale, R. babjevae, R. sphaerocarpum, R. kratochvilovae, R. azoricum, Pichia anomala, and some common greenhouse pathogens tested gave a negative result. The other probe (RD1) reacted with two species, R. diobovatum and R. babjevae at 42°C. The present dot-blot assay can be used reliably to identify the biocontrol agent, Rhodosporidium diobovatum, from pure culture and plant tissue.     

Growth inhibition of the cereal root pathogens Rhizoctonia solani AG8, R. oryzae and Gaeumannomyces graminis var. tritici by a recombinant 42-kDa endochitinase from Trichoderma harzianum

The objective of this study was to determine the effectiveness of a 42-kDa endochitinase coded by the ThEn42 gene from Trichoderma harzianum as a potential source of transgenic resistance to Rhizoctonia root rot of barley caused by Rhizoctonia solani AG8 and/or R. oryzae. The gene cThEn42 was codon optimized (GC content increased from 53.3 to 65.1%) and then synthesized to produce the modified cThEn42GC in Pichia pastoris for in vitro tests. Two expression vectors were constructed: one with the fungal signal peptide and the fungal activation peptide [FSP-FAP-cThEn(GC)] and the other with barley chitinase 26 signal peptide followed by the fungal signal and activation peptides [SP(HVChi26)-FSP-FAP-cThEn(GC)]. N-terminal sequencing showed that, of two proteins secreted into liquid medium, FSP was cleaved off faithfully in one protein and both FSP and FAP were cleaved from the other protein. Purified endochitinase provided strong in vitro inhibition of both R. solani AG8 and R. oryzae. The enzyme had an intermediate inhibitory activity against Gaeumannomyces graminis var. tritici, and no inhibitory activity against Fusarium graminearum, F. pseudograminearum, and F. culmorum.     

Interactions between rumen bacterial strains during the degradation and utilization of the monosaccharides of barley straw cell-walls

Pure cultures and pair-combinations of strains representative of the rumen cellulolytic species Ruminococcus flavefaciens, Fibrobacter succinogenes and Butyrivibrio fibrisovens were grown on cell-wall materials from barley straw. Of the pure cultures, R. flavefaciens solubilized straw most rapidly. The presence of B. fibrisolvens , which was unable to degrade straw extensively in pure culture, increased the solubilization of dry matter by R. flavefaciens and the solubilization of cell-wall carbohydrates by both R. flavefaciens and F. succinogenes. During fermentation, both R. flavefaciens and F. succinogenes released bound glucose and free and bound arabinose and xylose into solution. The accumulation of these sugars, especially arabinose and xylose, was greatly reduced in co-cultures containing B. fibrisolvens , suggesting that significant interspecies cross feeding of the products of hemicellulose hydrolysis (particularly soluble bound xylose released by F. succinogenes ) occurs during straw degradation by mixed cultures containing this species.     

镉胁迫对绢毛委陵菜-丛枝菌根真菌共生体根系结构和生理的影响

为从生理水平上揭示绢毛委陵菜（Potentilla sericea L.）-丛枝菌根真菌共生体对镉胁迫的应答机制,以绢毛委陵菜多年生植株为试验材料,分别接种根内根生囊霉（Rhizophagus intraradices）和摩西球囊霉（Funneliformis mosseae）,80 d后以不同浓度的镉胁迫处理并测定菌根侵染率,研究侵染率较高菌种的共生体植株的生理指标变化和结构变化。结果表明：摩西球囊霉较根内根生囊霉对绢毛委陵菜菌根侵染率高,达100%,而根内根生囊霉侵染率为89.33%;接种摩西球囊霉真菌的植物,当镉质量浓度达10 mg?L^-1时,细胞壁小范围破裂、液泡出现变小的趋势,高浓度镉（20 mg?L^-1）处理时,根系细胞壁破裂,细胞无法维持原有形态;镉胁迫下,Cd（5 mg?L^-1）~ Cd（10 mg?L^-1）MDA含量显著上升（P<0.05）,Cd（0 mg?L^-1）~Cd（5 mg?L^-1）SOD活性和脯氨酸含量变化显著（P<0.05）,可溶性蛋白含量和叶绿素含量显著减少（P<0.05）,Cd（10 mg?L^-1）~Cd（15 mg?L^-1）可溶性蛋白含量和叶绿素含量变化不显著（P>0.05）,植物可以抵抗一定浓度范围的镉胁迫。综合来看,接种摩西球囊菌可以增强绢毛委陵菜耐镉胁迫能力,为利用绢毛委陵菜修复镉污染土壤提供了理论依据。     

Interaction of the rumen fungus Orpinomyces joyonii with Megasphaera elsdenii and Eubacterium limosum

The degradation and fermentation of microcrystalline cellulose were studied in monoculture of the polycentric anaerobic fungus Orpinomyces joyonii and in co-cultures with the rumen bacteria Megasphaera elsdenii and Eubacterium limosum. More than 25% of cellulose hydrolysis products (glucose and cellodextrins) were released by the fungus into the medium after 8 d of cultivation. These products were metabolized by bacteria in mixed cultures. In co-culture with the fungus M. elsdenii and E. limosum . increased the extent of microcrystalline cellulose degradation by 10·12% and 7·96%, respectively. Biomass yield in co-cultures was increased by 89·9% and 59·4% for M. elsdenii and E. limosum . Y_cellulose for fungus alone was 52·29 g dry matter mol^-1 glucose. These values were 64·93 and 55·92 g mol^-1 glucose unit in co-culture with M. elsdenii and E. limosum , respectively.     

Poly-beta-hydroxybutyrate accumulation in Nostoc muscorum and Spirulina platensis under phosphate limitation

Nostoc muscorum and Spirulina platensis were grown under phosphate deficiency in order to investigate the role of internal phosphate pool and activity of alkaline phosphatase on poly-β-hydroxybutyrate (PHB) accumulation. PHB accumulation in N. muscorum increased to 22.7% of dry weight (dw) after 4 day of phosphate deficiency, while the internal phosphate pool reduced to the level of 0.02 μM mg dw⁻¹ at a maximum APase activity of 2.57 nM PNP mg dw⁻¹ h⁻¹. In contrary, S. platensis depicted maxima of 1.39 nM PNP mg dw⁻¹ h⁻¹ on day 30 of incubation, which was about 2 fold lower than the observed value of N. muscorum. PHB content in S. platensis remained low even after prolonged phosphate starvation, and a rise only up to 3.5% of dw was recorded on day 60 of phosphate deficiency. Supplementation of NADPH exogenously to S. platensis cultures grown under phosphate deficiency favoured PHB accumulation in 10, 20 and 30 days old cultures, but not in the cultures grown under phosphate deficiency for 60 days. The possible role of phosphate limitation on PHB accumulation is discussed.     

Transformation of callus cultures of nine plant species mediated by agrobacterium

A simple method for the Agrobacterium-mediated transformation of callus cultures of nine plant species, Lycopersicum esculentum Mill, Petunia hybrida Vilm, Pimpinella anisum L., Solanum melongena L., S. tuberosum L., Nicotiana glauca Graham, N. glutinosa L., N. plumbaginifolia Viviani and N. tabacum L., is described. Plant calli were resuspended in liquid media, co-cultivated with A. tumefaciens, and plated on restrictive media. The combination of a gene for kanamycin resistance and a gene for firefly luciferase was convenient in the selection and confirmation of hundreds of transformants. Four strains of A. tumefaciens, A208, A348, A281, and PC2760, were employed. All of the callus cultures were successfully transformed with at least one strain of A. tumefaciens, and A281 was the most effective of the four strains. N. glutinosa, N. plumbaginifolia, N. tabacum, P. hybrida and L. esculentum were transformed more efficiently than the other species tested.     

金针菇基因组测序及萜类合成关键基因分析

金针菇是我国一种重要的食药用真菌,具有较高的营养和药用价值,尤其是从金针菇中分离得到了多种麦角甾醇、倍半萜等萜类,具有抗菌、抗肿瘤和降血脂等功效。以往关于金针菇的研究多集中在营养成分、栽培和市场开发等方面,而很少报道有关生物活性成分的合成和代谢研究。从福建省金针菇主要栽培品种中获得原生质体单核化L11菌株,我们进行了金针菇基因组测序与初步分析,并利用生物信息学手段,研究了其主要的生物活性成分——萜类合成途径中的关键基因。结果显示,金针菇单孢全基因组序列长度为34.75Mb。通过分析萜类合成途径中的相关基因,确定了4个萜类合成关键基因的基因结构,并且表明其蛋白结构具有稳定性,该类基因还含有多个信号肽和跨膜结构。金针菇基因组测序的完成,为下一步功能基因的筛选、分析等研究工作奠定了基础。     

准噶尔盆地东南缘多枝柽柳、白刺和红砂水分来源的异同

荒漠生态系统中, 水是植物生长最主要的限制因子。为了比较同一生境下不同荒漠植物的水分来源特征, 选取了同一生境下的多枝柽柳(Tamarix ramosissima)、白刺(Nitraria sibirica)和红砂(Reaumuria soongorica), 测定了这3种植物茎水和各潜在水源(降水、土壤水和地下水)的氢、氧稳定同位素比率(δD和δ¹⁸O)值, 并利用IsoSource软件计算了3种植物对潜在水源的利用比例。结果表明: 红砂和白刺的茎水δD和δ¹⁸O值及其水分来源有明显的季节波动特征。其中, 红砂为浅根系植物, 春季(3-5月)以表层土壤水为主要水源, 夏秋季节(6-10月)表层土壤含水量显著降低, 其主要的水分来源逐渐偏向于较深层的土壤水; 白刺的根系分布范围介于红砂和多枝柽柳之间, 在春季能够较多地利用表层土壤水, 而到了夏秋季节, 所利用的水分更多地来源于深层土壤水或地下水; 多枝柽柳为深根系植物, 其90%以上的水分来源于深层土壤水和地下水, 而且茎水δD和δ¹⁸O值及其水分来源没有季节波动特征。3种植物水分来源特征的差异与其水分利用策略密切相关, 同时, 也说明荒漠灌木可以通过自身调节向着最优(最有利)表现型发展, 从而最大限度地获取水分。     

黄顶菊入侵对土壤中主要功能细菌的影响

以我国北方大面积发生的入侵植物黄顶菊为研究对象,对黄顶菊根际土壤中可培养的主要功能细菌进行了分离筛选,通过rep-PCR聚类和多样性分析研究了其群落结构的变化,并利用16S rRNA序列比对,对主要优势菌群进行鉴定.结果表明: 相对于本地植物万寿菊和空白对照,黄顶菊显著增加了根际土壤中固氮菌、有机磷细菌、无机磷细菌和钾细菌的数量.rep-PCR分析显示,黄顶菊根际4种功能细菌的种群结构与本地植物和对照相比有显著差异,3种土壤中相同的聚类群极少.多样性分析表明,黄顶菊根际微生物物种多样性更加丰富,群落结构更加复杂,优势种群比较明显,生态多样性较高.对从3种土壤中分离得到的主要优势菌群的鉴定结果也进一步证明了这一结论.研究结果为阐明黄顶菊入侵的微生态机制提供了理论基础.     

兰州市南北两山5种典型人工林凋落物的水文功能

结合野外实地观测和室内浸水试验,对兰州市南北两山5种典型人工林(侧柏林、刺槐林、新疆杨林、侧柏+刺槐混交林、新疆杨+刺槐混交林)凋落物的持水特性进行研究。结果表明: 不同林分类型凋落物的蓄积量在13.50～47.01 t·hm^-2,依次为新疆杨+刺槐混交林＞侧柏+刺槐混交林＞侧柏林＞刺槐林＞新疆杨林。除侧柏林外,其他林分类型的半分解层蓄积量所占比例均高于未分解层。凋落物最大持水率在190.8%～262.7%,新疆杨+刺槐混交林最大,侧柏林最小。凋落物最大持水量在35.29～123.59 t·hm^-2,依次为新疆杨+刺槐混交林＞侧柏+刺槐混交林＞刺槐林＞侧柏林＞新疆杨林。凋落物的吸水速率在浸水0～1 h直线下降,1 h后降幅减缓,未分解层凋落物吸水速率小于半分解层。最大拦截量和有效拦截量(深)均为新疆杨+刺槐混交林＞侧柏+刺槐混交林＞侧柏林＞刺槐林＞新疆杨林,且新疆杨+刺槐混交林有较高的有效拦截率,表明新疆杨+刺槐混交林在兰州市南北两山有较好的保持水土和涵养水源能力。     

绿色荧光蛋白标记下镰刀菌侵染地黄的组织学观察

为分析对地黄有较强致病性的尖孢镰刀菌的侵染机制,本研究采用携带有潮霉素抗性标记的强组成型表达载体pCT74,经PEG-CaCl₂介导的原生质体转化法导入镰刀菌,获得荧光信号强烈的sGFP标记菌株,并采用喷施接种和根部灌根接种。研究发现镰刀菌首先在地黄外部聚集繁殖,并通过伤口或气孔等通道侵入地黄维管组织,后逐渐导致周围海绵组织破裂,进而致使地下根茎逐渐变黑腐烂;由于地黄叶部气孔发达,使得镰刀菌由叶部侵入速度要快于根部灌根接种;不同孢子浓度接种实验表明镰刀菌对寄主的致害程度与其在叶部与根部的接种浓度并不呈相关性。进一步在接种处理后采集地黄叶部、茎部和根部组织提取真菌DNA后进行PCR扩增发现：在根部接种60h后即能检测到镰刀菌的侵入,经84h后侵入到地黄茎部组织,经96h后侵入到地黄叶部组织。该标记菌株可为今后探索地黄连作栽培中真菌病害大规模爆发的根际生物学过程提供研究材料。     

AM真菌摩西管柄囊霉对干旱胁迫下枳抗氧化酶基因表达的影响

测定分析了接种丛枝菌根（AM）真菌摩西管柄囊霉Funneliformis mosseae对正常供水与干旱处理的盆栽枳Poncirus trifoliata实生苗生长、活性氧代谢及抗氧化酶基因表达量的影响。结果表明,7周干旱处理显著降低了根系菌根侵染率。接种摩西管柄囊霉显著促进了干旱处理的枳植株生长,增加了根系体积和叶片相对含水量,显著降低了叶片脯氨酸含量,同时也上调了干旱处理的枳叶片精氨酸脱羧酶基因（PtADC1和PtADC2）和超氧化物歧化酶基因（PtFe-SOD和PtMn-SOD）、过氧化物酶基因（PtPOD）和过氧化氢酶基因（PtCAT1）的表达,因而维持了一个相对更低的活性氧水平（如过氧化氢）,有利于增强植株的抗旱性。     

Isolation of Cuticle and Vascular Bundles of Leaves by Maceration in Rumen Fluid

We report a new macerating technique for plant leaves which permits the isolation of cuticle and vascular bundles. The maceration medium is rumen fluid, a complex mixture of interacting microorganisms, used full strength or diluted with a nutrient buffer solution in the ratio of 2:5. An incubation period of up to 72 hours at 39 C permits cuticle and vascular-bundle networks to be isolated. The technique is illustrated with fresh leaf samples from pearl millet, Pennisetum typhoides; orchardgrass, Dactylis glomerata; and alfalfa, Medicago sativa.     

Metabolism of CO2 by leaves of different photosynthetic types of Neurachne species

Following a series of continuous exposures to ¹⁴CO₂ for different lengths of time, leaves from Neurachne munroi (C₄), N. minor (C₃-C₄) and N. tenuifolia (C₃| were estimated to assimilate 100%, 9% and 2–4%, respectively, of atmospheric CO₂ by the C₄ pathway. The percentage of ¹⁴C-label appearing in malate and aspartate in leaves of N. minor progressively increased with longer exposure times indicating that a significant proportion of its C₄ acids are formed as secondary products. In ¹⁴CO₂/¹²CO₂ pulse/chase experiments, the ¹⁴C-label in leaves of N. munroi was rapidly transferred from C₄ acids to sugar monophosphates plus sugar diphosphates, and finally to sucrose. In leaves of N. minor, the ¹⁴C-label was slowly metabolized from the C-4 carboxyl of malate and asparate (apparent half-time = 250 s), and the formation of C₄ acids as secondary products was again evident. ¹⁴C-label in serine/glycine accumulated to comparable magnitudes in both N. minor and in N. tenuifolia, but there was an initial lag phase in the accumulation of label in N. minor. C₄ photosynthesis is apparently of minimal importance in reducing photorespiration in N. minor, but leaf anatomical specializations and a possible compartmentation of photorespiratory metabolism may be of considerable importance.     

The degradation and utilization of wheat-straw cell-wall monosaccharide components by defined ruminal cellulolytic bacteria

Cell walls (CW) of untreated wheat straw and sulphur-dioxide (SO₂)-treated wheat straw were used as model substrates for the hydrolysis and utilization of CW carbohydrates by pure cultures or pair-combinations of defined rumen bacterial strains. Fibrobacter succinogenes S85 and BL2 strains and their co-cultures with D1 were the best degraders of CW among ruminal cultures, solubilizing 37.2–39.6% of CW carbohydrates of untreated straw and 62.2–74.5% of SO₂-treated straw. Complementary action between Butyrivibrio fibrisolvens D1 and the F. succinogenes strains was identified with respect to co-culture growth and carbohydrate utilization. However, the extent of CW solubilization was determined mainly by the F. succinogenes strains. In both substrates, utilization of solubilized cellulose by F. succinogenes S85 and BL2 monocultures was higher than that of xylan and hemicellulose: 96.5–98.3%, 34.4–40.5% and 33.5–36.2%, respectively. Under scanning electron microscopy visualization, S85 and BL2 cells of the co-cultures comprised the most dense layer of bacterial cell mass attached to and colonized on straw stems and leaves, whereas D1 cells were always nearby. Stems and leaves of the untreated straw were less crowded by attached bacteria than that of the SO₂-treated straw. In both materials, the cell surface topography of S85 and BL2 bacteria attached to CW particles was specified by a coat of characteristic protuberant structures, polycellulosome complexes.     

Potential of fungal antagonists for biocontrol of Fusarium spp. in wheat and maize through competition in crop debris

Pathogenic Fusarium spp. cause head blight in wheat or ear rot in maize leading to yield losses and also a reduction in quality due to mycotoxin contamination of the grain. Infected crop residues are the main inoculum source for epidemics. Saprophytic fungi, obtained from cereal tissues or necrotic tissues of other crops, were screened for their ability to colonise wheat straw and maize stalks and to suppress sporulation of pathogenic Fusarium spp. Results of bio-assays conducted under controlled conditions were variable among Fusarium spp. and host substrates for most antagonists tested, such as yeasts, Trichoderma spp. and non-pathogenic Fusarium spp. Isolates of Clonostachys rosea consistently suppressed sporulation of F. culmorum and F. graminearum on wheat straw, and of F. culmorum, F. graminearum, F. proliferatum and F. verticillioides on maize stalks. Isolates of C. rosea, C. cladosporioides and F. equiseti were applied to pieces of maize stalks or flowering ears in preliminary experiments conducted under field conditions. The colonisation of stalk pieces by pathogenic Fusarium spp. was assessed after 9 months. Colonisation of stalk pieces by pathogenic Fusarium spp. was significantly reduced at several sampling dates. However, results obtained with the antagonists were not consistent for all sampling dates and between experiments.