基于ERIC-PCR指纹图谱技术的小鼠肠道菌群失调分析方法的建立

目的采用常规菌群分析方法和ERIC-PCR技术对正常小鼠和抗生素相关性腹泻小鼠模型分别进行肠道菌群检测,结合细菌培养和DNA指纹图谱检测结果分析小鼠肠道内主导菌群数量和种类的改变情况,建立利用ERIC-PCR技术分析小鼠肠道菌群失调的检测方法。方法先利用常规菌群分析方法鉴定正常小鼠和抗生素相关性腹泻小鼠的菌群状况,再提取其基因组DNA,最后以肠杆菌科基因间重复序列(ERIC)为模板,利用ERIC-PCR方法获得正常小鼠和模型小鼠的肠道菌群指纹图谱,与常规菌群分析结果作比较,验证ERIC-PCR技术的准确性。结果常规菌群分析结果表明四种优势菌群在数量上出现明显的变化,证实造模成功。经ERIC-PCR技术成功获得两组小鼠粪便基因组DNA图谱,两组间呈现具有一定对比性的特异性指纹图谱。结论从小鼠粪便基因组经ERIC-PCR后的图谱中特异性条带的分布、数目和亮度来看,能说明肠道菌群的分布状况存在明显差异,结合常规菌群分析方法作对比,说明ERIC-PCR技术是一种分析小鼠肠道菌群失调高效快捷的检测方法。     

不同寡营养培养条件下南海水体细菌群落结构及其对碳源的利用特征

【背景】绝大多数海洋微生物不可培养,为挖掘海洋生态系统中可培养的微生物资源,研究者尝试寡营养培养等方法。【目的】比较不同寡营养培养条件下南海水体细菌数量、群落结构及其对碳源的利用特征差异。【方法】采用原2216E培养液(Y)、稀释10倍(Y-10)和稀释50倍(Y-50)的2216E培养液培养南海海水样品,用荧光定量PCR法和16S rRNA基因检测细菌数量和菌群结构;利用平板计数法计数异养细菌的数量,纯化鉴定可培养细菌;采用Biolog EcoPlateTM微板法分析不同培养基中细菌群落对碳源的利用特征。【结果】Y组细菌总数高于Y-10组和Y-50组,差异不显著(P>0.05),但异养细菌数量显著高于Y-10组和Y-50组(P<0.05)。16S rRNA基因测序结果表明,不同稀释倍数下的细菌群落结构差异明显,Y组检测出10门193属,优势类群为Proteobacteria(56.44%)和Bacteroides (37.27%);Y-10组检测出15门220属,优势类群为Proteobacteria (40.30%)、Bacteroides(36.91%)和Firmic...     

不同培养基组合提高土壤细菌可培养性的研究

为选择性采用多培养基组合以提高土壤细菌可培养性,利用变性梯度凝胶电泳(DGGE)技术研究了贫营养、富营养和自然营养培养基在3种培养方式下获得细菌种群的差异。结果表明:平板培养条件下,细菌在贫营养培养基上生长较慢,菌落连续稳定形成。培养5d后,富营养的LB培养基和贫营养的R2A培养基获得菌落数最多,分别是贫营养的0.1×LB培养基获得菌落数的5.1倍和5.3倍。7种培养基中,LB培养基获得细菌种群数目最多,营养成分适当稀释后,培养物中有新的种群出现。贫营养培养基和富营养培养基培养物DGGE图谱相似性低,条带互补性强。三角瓶静置培养时,R2A和LB培养基获得细菌种群数目较多,其它几种培养基获得的细菌类群都能在这2种培养基中找到。试管静置培养条件下,LB培养基获得细菌种群数目最多,某些种群也只出现在R2A培养基和TSB培养基上,R2A及LB培养基与TSB培养基获得的细菌种群差异较为明显。研究结果为特殊培养基设计及选用合适培养基分离土壤细菌提供参考。     

Biolog和PCR-DGGE技术解析施肥对德惠黑土细菌群落结构和功能的影响

试验采用Biolog和PCR-DGGE技术研究了不同施肥处理对吉林省德惠市黑土细菌群落结构和功能的影响.Biolog试验结果表明,单施有机肥处理的土壤细菌群落对底物碳源利用种类最多,代谢功能多样性最高;而施用化肥处理降低了土壤细菌群落代谢功能.DGGE图谱表明,不同施肥处理的土壤细菌16S rDNA多数条带分布相同,说明这些细菌类群在黑土中较稳定,在本试验中未受到施肥的影响,但也有一些特殊条带出现或缺失,施用化肥处理降低了土壤细菌群落结构组成多样性.对Biolog和DGGE试验结果的主成分分析显示,未施肥和单施有机肥处理的土壤细菌群落结构和功能相似,表明单施有机肥处理主要是增加了土壤微生物的总量,而对黑土细菌群落结构组成影响是次要的;单施化肥和半量有机肥 化肥处理的土壤细菌群落代谢功能多样性相似,但其结构组成产生了分离.研究表明化肥处理主要是影响到土壤中快速生长和富营养的细菌类群,施用化肥降低了这些细菌类群的代谢活性.     

风干土壤中氨氧化微生物的恢复

【目的】比较历史风干土壤与加水恢复培养土壤中氨氧化古菌AOA和细菌AOB的组成与数量差异,探究风干土壤用于后续微生物生理生态学研究的可能性;明确我国典型酸性森林土壤中,海洋类Group 1.1a是否为数量上占据优势的古菌AOA生态型。【方法】针对中国生态系统研究网络10个台站的典型森林土壤样品,围绕风干保存和加水培养两种处理,通过高通量测序土壤氨氧化古菌及细菌amoA标靶基因,分析氨氧化微生物群落组成的变化规律;利用实时荧光定量PCR和DGGE指纹图谱技术,研究森林土壤微生物群落16S rRNA基因的数量变化规律,以及氨氧化细菌和古菌群落结构的差异。【结果】10个历史风干土壤加水培养28天后,土壤细菌和古菌数量均急剧增加,最高可达3230倍和568倍;其中8个土壤中氨氧化古菌AOA明显增加,5个土壤中氨氧化细菌AOB表现出明显的增加趋势。然而,高通量测序和系统发育分析表明,历史风干土壤与加水恢复培养土壤中AOA和AOB的群落组成无明显变化。Group 1.1b是氨氧化古菌的优势类群,而氨氧化细菌的主要类群是Nitrosospira螺菌属。氨氧化古菌和细菌的比例与总氮浓度呈显著正相关(r2=0.54,P0.05),表明酸性条件下土壤矿化并提供铵态氮底物可能是古菌氨氧化的驱动机制。【结论】风干土壤加水恢复培养后,AOA和AOB的种群数量大多出现增加的趋势,但其物种组成未发生显著变化,表明风干保存的土壤样品可用于后续室内培养,开展微生物生理生态学研究。与已有的海洋AOA生态型主导酸性土壤氨氧化类群的报道不同,土壤Group 1.1b是本研究森林土壤中的优势类群。     

茶树根际微生物研究

利用选择性培养基,对土壤肥力肥沃、中等、贫瘠茶园的茶树根际细菌、真菌和放线菌进行了分离。根据菌体形态及培养特征、生理生化指标、DNA的G Cmol％值等,对根际细菌进行了鉴定和分类。研究了不同肥力、不同茶龄的茶园根际细菌的数量和类群的变化;根际真菌的数量变化;根际放线菌的数量变化。主要结果为：土壤肥沃的茶园根际细菌的数量最多,土壤贫瘠的茶园数量最少;相同土壤肥力的茶园,10年生茶园根际细菌的数量最多,4年生的次之,20年生的最少。根际真菌的数量,土壤肥沃茶园的较少,中等和贫瘠茶园的较多。根际放线菌的数量,20年生茶园的明显高于4年生和10年生茶园的,而且,土壤贫瘠茶园的数量较多。从9种不同类型茶园中分离获得的纯化细菌经鉴定分别属于20个属,中等肥力的茶园最适于多数细菌的生长与繁殖,类群最为丰富,但类群的优势度低于另外两种土壤;不同茶龄的茶园随着茶龄的增加,肥沃茶园和中等茶园的根际中有较多的细菌类群定殖,但20a茶龄的类群较少;贫瘠茶园类群的优势度最大。     

健康儿童与发育不佳儿童肠道菌群结构的比较研究

目的对健康儿童与发育不佳(FTT)儿童肠道中微生物区系的ERIC-PCR指纹图谱异同进行研究。方法根据美国疾病预防控制中心(CDC)对儿童生长发育的评价指标对某幼儿园200例4～6岁儿童进行评价,筛选出16例健康儿童和13例FTT儿童,每周1次连续3周跟踪取样,提取粪便样品中细菌总DNA,获得其ERIC-PCR指纹图谱,再将其中一个样品的ERIC-PCR产物作为混合探针通过杂交对指纹图谱上DNA条带序列的异同进一步比较。结果同一个体的肠道菌群结构在取样期间稳定性较好;虽然健康儿童间的肠道菌群结构也有一定差异,但它们却有着共同的结构特征;而健康儿童与FTT儿童的肠道菌群结构差异较大。结论儿童发育状况与肠道菌群结构有一定的关系。     

一株嗜麦芽寡养单胞菌的分离及其生物学特性

近年来,基于高通量测序技术对植物根际土壤微生物菌群结构的测定结果表明,土壤中绝大多数微生物难以通过传统的富营养培养基实现培养和分离。为进一步探索分离土壤中寡营养微生物的方法,结合多种培养因素,以土壤浸出液为基础培养基设计寡营养培养基分离土壤细菌菌株。并通过菌株的细胞形态、生理生化特征、16S rRNA和gyrB基因序列等对其中一株菌进行鉴定,同时对其蛋白酶与铁载体的产生能力进行检测以评价其在植物根际促生方面的应用潜力。利用土壤浸出液做培养基是有效分离土壤寡营养细菌的方法 ;编号为S35的菌株鉴定为嗜麦芽寡养单胞菌(Stenotrophomonas maltophilia),具有蛋白酶和铁载体产生能力。采用的寡营养培养基可以分离获得在富营养培养基上不易分离的细菌,得到S. maltophilia S35菌株在植物促生方面具有一定的应用潜力。     

多点接种方法计数土壤细胞生理类群的研究

多点接点计数方法是根据细菌分解固体培养基上不同的有机化合物的能力确定为不同的生理类群,由有机化合物的降解点数和根据MPN方法进行计数,对不同的耕作方法进行了测定表明,秸秆覆盖免肾够明显提高土壤中分解淀粉,木聚糖,纤维素,果胶,几丁质,卵磷质,脂类和蛋白质类群的细菌数量。     

多点接种方法计数土壤细菌生理类群的研究

多点接种计数方法是根据细菌分解固体培养基上不同的有机化合物的能力确定为不同的生理类群 ,由有机化合物的降解点数和根据MPN方法进行计数。对不同的耕作方法进行的测定表明 ,秸秆覆盖免耕能够明显提高土壤中分解淀粉、木聚糖、纤维素、果胶、几丁质、卵磷质、脂类和蛋白质类群的细菌数量。     

利用DGGE评价不同培养基回收番茄根际细菌类群的能力

用营养肉汤、YG、根系分泌物、土壤浸渍液4种培养基从番茄根际分离培养细菌,并结合变性梯度凝胶电泳(DGGE)技术,对4种培养基回收番茄根际细菌种群的能力进行了比较研究。结果表明,不同培养基和培养温度,回收到的细菌种群有一定差异;低营养浓度的YG培养基在较低的培养温度20℃下进行较长时间的培养,比高营养浓度营养肉汤培养基产生更多、更具代表性的细菌;以根系分泌物为基础的培养基从番茄根际回收到的优势菌群最多。该研究初步建立了用DGGE技术对不同培养基回收分离细菌种群能力进行评价的方法。     

Isolation and characterization of bacteria associated with two sand dune plant species, Calystegia soldanella and Elymus mollis

Little is known about the bacterial communities associated with the plants inhabiting sand dune ecosystems. In this study, the bacterial populations associated with two major sand dune plant species, Calystegia soldanella (beach morning glory) and Elymus mollis (wild rye), growing along the costal areas in Tae-An, Chungnam Province, were analyzed using a culture-dependent approach. A total of 212 bacteria were isolated from the root and rhizosphere samples of the two plants, and subjected to further analysis. Based on the analysis of the 16S rDNA sequences, all the bacterial isolates were classified into six major phyla of the domain Bacteria. Significant differences were observed between the two plant species, and also between the rhizospheric and root endophytic communities. The isolates from the rhizosphere of the two plant species were assigned to 27 different established genera, and the root endophytic bacteria were assigned to 21. Members of the phylum Gammaproteobacteria, notably the Pseudomonas species, comprised the majority of both the rhizospheric and endophytic bacteria, followed by members of Bacteroidetes and Firmicutes in the rhizosphere and Alphaproteobacteria and Bacteroidetes in the root. A number of isolates were recognized as potentially novel bacterial taxa. Fifteen out of 27 bacterial genera were commonly found in the rhizosphere of both plants, which was comparable to 3 out of 21 common genera in the root, implying the host specificity for endophytic populations. This study of the diversity of culturable rhizospheric and endophytic bacteria has provided the basis for further investigation aimed at the selection of microbes for the facilitation of plant growth.     

Effects of the symbiosis between fungal endophytes and Atractylodes lancea on rhizosphere and phyllosphere microbial communities

Tissue-cultured plantlets of Atractylodes lancea were inoculated with the endophytes AL4 (Cunninghamella sp.) and AL12 (Gilmaniella sp.), and subsequently transplanted into soil after hardening of the tissue-cultured plantlets. We investigated rhizospheric and phyllospheric microbial communities using culture-based and culture-independent methods. Energy spectrum analysis, high performance liquid chromatography, and other assay methods were employed to quantify the elements in the leaves, and the soluble sugars, free amino acids and organic acids in the rhizosphere. The results showed that the endophytes enhanced the diversity and size of the rhizospheric microbial populations. In the phyllosphere, AL4 (Cunninghamella sp.) enhanced the diversity and size of bacterial populations, while AL12 (Gilmaniella sp.) enhanced the diversity and size of fungal populations. The dominant bacterial genera were Microbacterium, Kocuria and Sphingomon in the endophytes-inoculated groups, and Acinetobacter and Bacillus in the endophytes-free group. While Acremonium and Curvularia were the dominant fungal genera in the phyllosphere of endophytes-inoculated groups, Fusarium and Penicillum were most common in the endophytes-free group. AL4 (Cunninghamella sp.) enhanced the rhizospheric microbial population size and diversity by increasing rhizospheric free amino acids, while AL12 (Gilmaniella sp.) altered the rhizospheric microbes by changing concentration of soluble sugars in the rhizosphere. Elemental levels in the phyllosphere and the nutrients in the rhizosphere varied among the treatments and may also have influenced the microbial communities.     

Diversity of Culturable Bacteria Isolated from Root Domains of Moso Bamboo (Phyllostachys edulis)

The distribution of culturable bacteria in the rhizosphere, rhizoplane, and interior root tissues of moso bamboo plants was investigated in this study. Of the 182 isolates showing different colony characteristics on Luria–Bertani and King B plates, 56 operational taxonomic units of 22 genera were identified by 16S ribosomal RNA gene sequence analysis. The majority of root endophytic bacteria were Proteobacteria (67.5%), while the majority of rhizospheric and rhizoplane bacteria were Firmicutes (66.3% and 70.4%, respectively). The most common genus in both the rhizosphere and on the rhizoplane was Bacillus (42.4% and 44.4%, respectively), while Burkholderia was the most common genus inside the roots, comprising 35.0% of the isolates from this root domain. The endophytic bacterial community was less diverse than the rhizoplane and rhizospheric bacterial communities. Members of Lysinibacillus, Bacillus, and Burkholderia were found in all three root domains, whereas many isolates were found in only a single domain. Our results show that the population diversity of culturable bacteria is abundant in the root domains of moso bamboo plants and that obvious differences exist among the rhizospheric, rhizoplane, and endophytic bacterial communities.     

转基因生防菌308R(pCPP430)对番茄根围菌群的影响

研究目的在于了解转基因生防菌308R(pCPP430)对番茄根围菌群代谢能力和群落结构的影响。实验中使用了两种互为补充的方法,即单一碳源利用测试(SCSU)和ERIC-PCR,对分别以308R(pCPP430)悬液、308R悬液和无菌水蘸根处理的番茄植株根围菌群进行比较。SCSU菌落计数的聚类分析表明,308R(pCPP430)和308R处理的根围菌重复之间相似性好,水处理的相似性差。主成分分析也得到了相同的结果。ERIC-PCR聚类结果表明,10种碳源,其中8种水处理和308R处理聚为一类。实验为生防菌与植物的互作提供一些依据,为根围菌群结构研究提供一些新的思路。     

转Bt基因抗虫棉根际微生物区系和细菌生理群多样性的变化

在大田栽培条件下 ,以转 Bt基因抗虫棉 GK-12和常规棉花泗棉 3号作为材料 ,在棉花不同发育时期 ,于 2 0 0 1和 2 0 0 2连续两年测定棉花根际土壤细菌、放线菌和真菌数量的变化 ,并在 2 0 0 2年棉花的花铃期和吐絮期对根际细菌生理群的数量和多样性进行了分析 ,结果表明 :虽然不同年份和生育期棉花根际微生物数量存在差异 ,但是 ,年度间和相同的发育时期棉花根际微生物的数量变化趋势一致。在棉花的苗期和吐絮期 ,转 Bt基因抗虫棉根际微生物的数量与对照差异不显著 ;在棉花的花铃期 ,转 Bt基因抗虫棉根际细菌的数量比对照增加 ,放线菌的数量差异不显著 ,而真菌的数量变化没有规律。在棉花发育的花铃期和吐絮期 ,Bt棉根际细菌生理群的总数量比常规棉增加 ,但是根际细菌生理群的 Simpson指数、Shannon-Wiener指数和细菌生理群分布的均匀度下降     

Comparison of culturable Gram-negative bacterial community structures in the rhizosphere of three fruit plants

This research work was oriented to outlining the diversity of Gram-negative culturable portion of the bacterial community in three fruit plants rhizosphere. Rhizosphere samples were taken from European chestnut (Castanea sativa Mill), true service tree (Sorbus domestica L.) and cornelian cherry (Cornus mas L.) plants. Experiments were conducted for three years during the vegetation period, and the bacterial community structure was assessed with cultivation-dependent approach. Many Gram-negative isolates (n = 251) from the rhizosphere survived sub culturing and were identified by biochemical tests. A total of 57 species belonging to 29 genera were identified and assigned to four broad taxonomic groups (Bacteroidetes, Alpha-, Beta- and Gamma-proteobacteria). Several specific bacterial cluster communities were identified inside all the three rhizospheres. Most of the species belonged to the genera Moraxella, Pseudomonas, Pantoea, Enterobacter and Acinetobacter. In addition, while, using the plate count analysis, large discrepancies in numbers among physiological groups of bacteria cultured from three rhizosphere samples have not been revealed, more expressive distinctions among bacterial populations were obtained concerning the relative abundance of different genera, different taxonomic groups as well as different diversity indices. Furthermore, the number of cultured bacteria and their taxonomic distribution in the rhizosphere of all three plants changed not only explicitly during vegetation period but continually during the three years of investigation. It seems that rhizosphere bacterial populations of each plant are under the influence of the specific root-released materials.     

Comparison of Parental and Transgenic Alfalfa Rhizosphere Bacterial Communities Using Biolog GN Metabolic Fingerprinting and Enterobacterial Repetitive Intergenic Consensus Sequence-PCR (ERIC-PCR)

Abstract Rhizosphere bacterial communities of parental and two transgenic alfalfa (Medicago sativa L.) of isogenic background were compared based on metabolic fingerprinting using Biolog GN microplates and DNA fingerprinting of bacterial communities present in Biolog GN substrate wells by enterobacterial repetitive intergenic consensus sequence-PCR (ERIC-PCR). The two transgenic alfalfa expressed either bacterial (Bacillus licheniformis) genes for alpha-amylase or fungal (Phanerochaete chrysosporium) genes for Mn-dependent lignin peroxidase (Austin S, Bingham ET, Matthews DE, Shahan MN, Will J, Burgess RR, Euphytica 85:381–393). Cluster analysis and principal components analysis (PCA) of the Biolog GN metabolic fingerprints indicated consistent differences in substrate utilization between the parental and lignin peroxidase transgenic alfalfa rhizosphere bacterial communities. Cluster analysis of ERIC-PCR fingerprints of the bacterial communities in Biolog GN substrate wells revealed consistent differences in the types of bacteria (substrate-specific populations) enriched from the rhizospheres of each alfalfa genotype. Comparison of ERIC-PCR fingerprints of bacterial strains obtained from substrate wells to substrate community ERIC-PCR fingerprints suggested that a limited number of populations were responsible for substrate oxidation in these wells. Results of this study suggest that transgenic plant genotype may affect rhizosphere microorganisms and that the methodology used in this study may prove a useful approach for the comparison of bacterial communities. Received: 1 June 1998; Accepted: 20 October 1998     

Bacterial community structure in the rhizosphere of three cactus species from semi-arid highlands in central Mexico

The nature reserve of Tehuacan-Cuicatlan in central Mexico is known for its diversity and endemism mainly in cactus plants. Although the xerophytic flora is reasonably documented, the bacterial communities associated with these species have been largely neglected. We assessed the diversity and composition of bacterial communities in bulk (non-rhizospheric) soil and the rhizosphere of three cactus plant species: Mammillaria carnea, Opuntia pilifera and Stenocereus stellatus, approached using cultivation and molecular techniques, considering the possible effect of dry and rainy seasons. Cultivation-dependent methods were focused on putative N₂-fixers and heterotrophic aerobic bacteria, in the two media tested the values obtained for dry season samples grouped together regardless of the sample type (rhizospheric or non-rhizospheric), these groups also included the non-rhizospheric sample for rainy season, on each medium. These CFU values were smaller and significantly different from those obtained on rhizospheric samples from rainy season. Genera composition among isolates of the rhizospheric samples was very similar for each season, the most abundant taxa being α-Proteobacteria, Actinobacteria and Firmicutes. Interestingly, the genus Ochrobactrum was highly represented among rhizospheric samples, when cultured in N-free medium. The structure of the bacterial communities was approached with molecular techniques targeting partial 16S rRNA sequences such as denaturing gradient gel electrophoresis and serial analysis of ribosomal sequence tags. Under these approaches, the most represented bacterial phyla were Actinobacteria, Proteobacteria and Acidobacteria. The first two were also highly represented when using isolation techniques.