共查询到20条相似文献,搜索用时 93 毫秒
1.
黄檗根围丛枝菌根真菌菌群组成 总被引:5,自引:3,他引:2
从东北林业大学林场采集黄檗Phellodendron amurense根系及根围土壤,采用Nested-PCR技术扩增黄檗菌根及根围土壤AM真菌18S rDNA NS31/Glol区域,利用该产物进行DGGE分析,并结合DNA测序、系统发育分析及DGGE图谱分析技术对黄檗AM真菌菌群组成进行分析.结果表明:Nested-PCR技术具有较高的灵敏性,可有效地从微量DNA中扩增出约230bp的目的片段;黄檗根系及根围土壤具有不同的DGGE指纹图谱特征,DGGE带谱在条带的数量、亮度、优势度等方面均存在较大差异,全部序列可分为3类菌群,即球囊霉属Glomus、盾孢囊霉属Scutellospora及植物病原菌黄杨亚赤壳Hyponectria buxi,其中Glomus sp.(EF177624)和Glomus sp.(DQ085205)分别为黄檗根系和根围土壤样品中最具优势的AM真菌. 相似文献
2.
3.
4.
5.
利用DGGE法研究不同种植体系中根际微生物群落结构 总被引:7,自引:0,他引:7
利用DGGE技术研究不同间作和轮作种植体系对作物根际细菌和真菌群落结构的影响.运用16SrDNA和18SrDNA特异引物对,将土壤中提取的总DNA进行PCR扩增后,通过DGGE技术对PCR产物进行分析,结果表明:玉米-蚕豆轮作对蚕豆根际细菌和真菌群落结构影响明显,二者都与单作蚕豆有较大差异;小麦/蚕豆间作明显改变两种作物根际细菌群落结构和蚕豆根际真菌群落结构;玉米/蚕豆间作明显改变玉米根际细菌、真菌群落结构和蚕豆根际真菌群落结构. 相似文献
6.
PCR-DGGE技术在农田土壤微生物多样性研究中的应用 总被引:49,自引:6,他引:43
变性梯度凝胶电泳技术(DGGE)在微生物生态学领域有着广泛的应用。研究采用化学裂解法直接提取出不同农田土壤微生物基因组DNA,并以此基因组DNA为模板,选择特异性引物F357GC和R515对16S rRNA基因的V3区进行扩增,长约230bp的PCR产物经变性梯度凝胶电泳(DGGE)进行分离后,得到不同数目且分离效果较好的电泳条带。结果说明,DGGE能够对土壤样品中的不同微生物的16S rRNA基因的V3区的DNA扩增片断进行分离,为这些DNA片断的定性和鉴定提供了条件。与传统的平板培养方法相比,变性梯度凝胶电泳(DGGE)技术能够更精确的反映出土壤微生物多样性,它是一种有效的微生物多样性研究技术。 相似文献
7.
AM真菌对青枯菌和根际细菌群落结构的影响 总被引:12,自引:0,他引:12
利用传统的平板培养与DGGE相结合的技术手段,研究了接种AM真菌对番茄根际土壤中的青枯菌和细菌群落结构的影响。结果表明,菌根根际土壤中的细菌总量和总DNA量都高于非菌根根际土壤,其中前者的青枯菌种群数量比后者低60倍;DGGE图谱也证实了AM真菌对青枯菌的抑制效应,还揭示出接种AM真菌对根际土壤中细菌群落结构所产生的复杂的影响。文章对AM真菌抑制青枯菌的机制进行了探讨。 相似文献
8.
在PCR-DGGE研究土壤微生物多样性中应用GC发卡结构的效应 总被引:30,自引:1,他引:29
应用普通细胞裂解法提取 3株实验菌株 (Escherichia coli DH5α,Staphylococcus aureus SA- 1和 A-grobacterium tumerfaciens 1 31 2 9)的基因组 DNA和应用基于高盐和长时高热的细胞裂解法提取 7种不同土壤样品中的微生物的基因组 DNA,两组不同结构的引物 F3 57GC,R51 8(在正向引物的 5′端有 GC发卡结构 )和 F3 57,R51 8,分别对实验菌株和土壤样品中微生物的 1 6Sr RNA基因 V3区进行扩增 ,均得到了目的片段。比较了不同引物扩增的 1 6S r DNA片段在 DGGE中的不同电泳行为 ,结果表明 ,含 GC发卡结构的PCR扩增产物在 DGGE中能够得到很好的分离 ,而无 GC发卡结构的 PCR产物则不能在 DGGE中获得满意分离。引入 GC发卡结构 ,使得对不同微生物的定性和分类更深入细致 相似文献
9.
研究确定土壤微生物基因组DNA提取方法、PCR扩增条件、DGGE电泳条件,为进一步研究分析土壤中微生物结构变化规律提供理论依据。土壤微生物基因组DNA提取采用直接法和间接法进行比较; PCR扩增条件调整扩增体系、DGGE电泳条件调整变性剂范围,并对其结果进行比较分析。通过对DGGE电泳相关条件的研究,结果显示,土壤中粗基因组DNA采用直接法提取,然后进行纯化; PCR扩增体系中加入BSA,DGGE电泳系统组成中变性剂浓度范围为35%~55%。确定了土壤微生物基因组DNA提取方法、PCR扩增条件、DGGE电泳条件,为后续的相关研究提供理论依据。 相似文献
10.
鸡肠道微生物菌群经PCR-DGGE分析,回收PCR-DGGE分析胶上的一条DNA片段,回收的DNA片段再重复进行2次PCR-DGGE分析,以及分别用PCR反复循环扩增和PCR高保真酶扩增后再进行DGGE分析等方法研究PCR-DGGE分析中多条带产生原因。结果显示PCR-DGGE分析中多条带产生原因可能是作PCR扩增模板的DNA混杂有少量其他DNA片段,多条带现象不易被消除。DGGE分析胶上的DNA片段测序时,将该DNA片段回收、PCR扩增后克隆,提取多个阳性克隆菌的质粒DNA片段,分别与其原目的DNA片段进行DGGE分析,在DGGE分析胶上选取与原目的DNA片段处于同一电泳位置的质粒DNA测序,提高测序的准确性。 相似文献
11.
喀斯特地区丛枝菌根真菌遗传多样性 总被引:7,自引:0,他引:7
为探明喀斯特地区丛枝菌根真菌( AMF)的遗传多样性特征,利用巢式PCR和DGGE相结合的分子生物学方法对茂兰喀斯特多个植被类型下的AMF遗传多样性进行了研究.结果表明,喀斯特地区AMF遗传多样性指数和物种丰富度分别平均为3.50和41,远高于非喀斯特对照样地的2.68和17,分析表明,喀斯特地区较高的AMF多样性与此地区丰富的植物多样性以及特殊的生态环境有关,是与喀斯特生态系统长期相互选择的结果.不同植被类型下的AMF多样性差异显著,相似性指数最高为0.34,喀斯特地区AMF的群落结构随着植被类型的改变发生显著变化;基因测序显示,喀斯特地区AMF的优势菌属是生态适应性很强的球囊霉属,在喀斯特石漠化生态恢复中具有较强的利用潜力. 相似文献
12.
Haoqiang Zhang Ming Tang Hui Chen Zhiqiang Tian Yaoqin Xue Ye Feng 《Plant and Soil》2010,326(1-2):415-424
The process of ecological restoration and reconstruction in Zhifanggou watershed forms a special ecosystem on the Loess Plateau. Little is known about the communities of arbuscular mycorrhizal fungi (AMF) and bacteria in this ecosystem. The aim of this study was to analyze the communities of AMF and bacteria, and their relationship in the rhizosphere of Caragana korshinkii and Hippophae rhamnoides in Zhifanggou watershed. Soil samples were collected from Zhifanggou watershed. The communities of AMF and bacteria were analyzed by using nested PCR of rDNA fragments and denaturing gradient gel electrophoresis (DGGE). Diversity analysis revealed that the bacterial Shannon diversity index was higher than that of AMF, and the AMF and bacterial Shannon diversity index in the rhizosphere of H. rhamnoides was higher than that of C. korshinkii. Principal component analysis (PCA) revealed that host plant had a significant influence on the bacterial community structure, but no strict specificity with AMF. Correlation analysis showed that the AMF communities had a significant positive correlation with the bacterial communities, and that indicated a significant effect of AMF on bacteria. 相似文献
13.
Identification of arbuscular mycorrhizal fungi (AMF) on roots is almost impossible with morphological methods and, due to the presence of contaminating fungi, it is also difficult with molecular biological techniques. To allow broad investigation of the population structure of AMF in the field, we have established a new method to selectively amplify the internal transcribed spacer (ITS) region of most AMF with a unique primer set. Based on available sequences of the rDNA, one primer pair specific for AMF and a few other fungal groups was designed and combined in a nested PCR with the already established primer pair ITS5/ITS4. Amplification from contaminating organisms was reduced by an AluI restriction after the first reaction of the nested PCR. The method was assessed at five different field sites representing different types of habitats. Members of all major groups within the Glomeromycota (except Archaeosporaceae) were detected at the different sites. Gigasporaceae also proved detectable with the method based on cultivated strains. 相似文献
14.
Elisabeth W. Vissers Paul L.E. Bodelier Gerard Muyzer & Hendrikus J. Laanbroek 《FEMS microbiology letters》2009,298(2):193-198
In a survey on the presence of archaea in a number of European lakes, it was found that known archaeal primer sets for PCR were not suited for use in freshwater environment, as some lack selectivity, while others were too selective. A nested PCR was developed for denaturing gradient gel electrophoresis (DGGE) with primer sets 21F–958R and Parch519f–Arch915r, respectively. After sequencing of the DGGE bands obtained by this nested method, 93% of the sequences were of archaeal origin. More diverse archaeal DGGE patterns were found as compared with other PCR methods. The nested PCR-DGGE method presented here is therefore a reliable tool to analyze the archaeal diversity in freshwater habitats, revealing even more widespread diversity of the archaea. 相似文献
15.
16.
The community of arbuscular mycorrhizal fungi (AMF) colonizing the roots of Festuca pratensis and Achillea millefolium was characterized in a Swedish pasture at different times, along a gradient of fertilization. The small subunit ribosomal RNA gene was subjected to PCR and denaturing gradient gel electrophoresis (DGGE), sequencing and phylogenetic analysis. The sequences found in this study clustered in 10 discrete sequence groups, seven belonging to Glomus, two to Scutellospora and one to Diversispora. A negative correlation was observed between soil mineral nitrogen and the number of AMF sequence groups in the roots. The frequency of occurrence of AMF in roots decreased dramatically between June and September. No plant-host specificity could be detected. 相似文献
17.
AIMS: To screen for bacterial contamination during gelatine production by means of denaturing gradient gel electrophoresis (DGGE). As members of Bacillus and related genera were found to persist in the final product, this study focussed on these taxa. METHODS AND RESULTS: Template DNA was extracted from gelatine samples at five crucial points of a gelatine production process. A primer specific for Bacillus and related genera was designed and used in a selective PCR, followed by a nested DGGE-PCR targeting the V9 region of the 16S rDNA. DGGE analysis of the resulting amplicons, and sequence analysis of selected bands, showed high sequence similarities of these bands with Bacillus fumarioli, B. licheniformis, B. coagulans and Clostridium perfringens. When the selective PCR was omitted, primarily Lactobacillus bands were retrieved. CONCLUSIONS: PCR-DGGE analysis of gelatine extracts can be used for tracing and screening of bacterial contamination during gelatine production. A selective PCR, nested with DGGE-PCR, gave much more accurate information about endospore-forming contaminants than did the direct DGGE procedure alone. Significance AND IMPACT OF THE STUDY: Use of this nested DGGE-PCR protocol may provide important information about possible hazards to the final microbiological quality and/or safety of gelatine, so allowing production parameters and/or remediation procedures may be adjusted on-line. 相似文献
18.
Yun Hou Zheng Ma Shengzhang Dong Yolanda H. Chen Xiaoping Yu 《Current microbiology》2013,67(3):263-270
Yeast-like symbiotes (YLS) are endosymbionts that are intimately associated with the growth, development, reproduction of their host, the brown planthopper, Nilaparvata lugens (Hemiptera: Delphacidae). However, it is unclear how many species of YLS are found within N. lugens, and how they are related to each other. Traditional methods or simple amplification based on 18S rDNA sequence does not reliably identify new species quickly and efficiently. Therefore, a novel nested PCR-denaturing gradient gel electrophoresis (DGGE) strategy was developed in this article to analyze the YLS of brown planthopper using a nested PCR protocol that involved the 18S rDNA gene and the 5.8S–ITS gene using fungal universal primers. The nested PCR protocol was developed as follows: firstly, the 18S rDNA gene, and 5.8S–ITS gene were amplified using fungal universal primers. Subsequently, these products were used as a template in a second PCR with primers ITS1GC–ITS2, ITS1FGC–ITS2, and NFGC-NR, which was suitable for DGGE. Using this highly specific molecular approach, we found several previously detected fungi: Noda, Pichia guilliermondii, Candida sp., and some previously undetected fungi, such as Saccharomycetales sp., Debaryomyces hansenii, and some uncultured fungi. In conclusion, the nested PCR system developed in this study, coupled with DGGE fingerprinting, offers a new tool for uncovering fungal endosymbiont diversity within planthoppers. 相似文献
19.
应用巢式PCR并进行梅根系与根围土壤丛枝菌根真菌(arbuscular mycorrihizal fungi,AMF)DNA扩增片段长度多态性(amplified fragment length polymorphism,AFLP)的差异比较,研究梅共生AMF的作用机理。结果表明,从18个梅品种的30个根围土壤样品中有28个样品获得纯化的DNA片段,占样品数93.3%,样品平均多态性位点数为6.5个,Nei’s基因多样性为0.3559±0.1382,Shannon信息指数为0.5299±0.1676。与梅根系AMF DNA多态性比较,根围土壤的平均多态性位点数明显较多;且根系AMF的DNA多态性位点绝大多数存在于土壤AMF的DNA多态性位点中,表明根系内AMF是由土壤AMF发育而来;根系与根围土壤AMF DNA的聚类均与梅品种群、品种关联性不强,表明AMF对宿主梅品种或品种群没有特异的共生关系。 相似文献