Soil microbial community analysis using terminal restriction fragment length polymorphisms

Terminal restriction fragment length polymorphism (T-RFLP) analysis is a polymerase chain reaction (PCR)-fingerprinting method that is commonly used for comparative microbial community analysis. The method can be used to analyze communities of bacteria, archaea, fungi, other phylogenetic groups or subgroups, as well as functional genes. The method is rapid, highly reproducible, and often yields a higher number of operational taxonomic units than other, commonly used PCR-fingerprinting methods. Sizing of terminal restriction fragments (T-RFs) can now be done using capillary sequencing technology allowing samples contained in 96- or 384-well plates to be sized in an overnight run. Many multivariate statistical approaches have been used to interpret and compare T-RFLP fingerprints derived from different communities. Detrended correspondence analysis and the additive main effects with multiplicative interaction model are particularly useful for revealing trends in T-RFLP data. Due to biases inherent in the method, linking the size of T-RFs derived from complex communities to existing sequence databases to infer their taxonomic position is not very robust. This approach has been used successfully, however, to identify and follow the dynamics of members within very simple or model communities. The T-RFLP approach has been used successfully to analyze the composition of microbial communities in soil, water, marine, and lacustrine sediments, biofilms, feces, in and on plant tissues, and in the digestive tracts of insects and mammals. The T-RFLP method is a user-friendly molecular approach to microbial community analysis that is adding significant information to studies of microbial populations in many environments.

PCR-RFLP analysis of mitochondrial DNA ND5/6 region among 3 subspecies of common carp (Cyprinus carpio L.) and its application to genetic discrimination of subspecies

Mitochondrial DNA ND5/6 region was studied by PCR-RFLP analysis among ten representative strains belonging to three subspecies (Cyprinus carpio carpio, Cyprinus carpio haematopterus and Cyprinus carpio rubrofuscus) of common carp (Cyprinus carpio L.). A total of 2.4 kb fragment was amplified and subjected to restriction endonuclease analysis with nine restriction endonucleases subsequently. The results indicated that each subspecies owned one hyplotype and four restriction enzymes (Dde I, HaeIII, Taq I and Mbo I) produced diagnostic restriction sites which could be used for discriminating the three subspecies and as molecular genetic markers for assistant selective breeding of common carp.

光周敏感核不育水稻phyA基因的RFLP分析

本文用RFLP方法分析农垦58和光敏核不育水稻农垦58S以及其他一些水稻品种如IR36等，得到如下结果： 1．以第5染色体上8个RFLP标记(RG】3、RG】19、RG470、RG573、RG360、RG403、RG229、RG556)作探针对58和58S进行RFLP分析．没有发现多态性。 2． 58和58S光敏色素(phyA)基因内部（或附近）一些CpG岛的甲基化程度不同。 以IR36 phyA 基因的c DNA克隆作探针，用限制性内切酶EcoRV、Dra I、HindⅢ、Xba工、BglⅡ、Sca工、Msp工对58和58S进行RFLP分析，没有发现多态性，但用HpaII现了多态性。 3．根据IR36 ph yA序列，在5’一非编码区设计一对PCR引物，在IR36、58、58S等水稻品种中均扩出了一段DNA，此DNA片段大小在这几个不同品种中都相同。以此DNA片段（称为PCRI）作探针进行RFLP分析．发现在58S和IR36之间具有多态性，根据测出的58S的PCRI序列以及RFLP分析结果，推测58S和IR36之间的差异是由于插入或缺失引起的。

分子标记技术在甘兰型杂交油菜育种上的研究与应用

本文应用RAPD分标记技术对我国重要的油料作物“杂油59”杂种种子的Fl代杂种的纯度进了技术鉴定，并完善了这一技术，摸索出这一适合于目前生产应用的实用方法，填补了这一技术在油菜作物应用上的空白。用RFLP技术对我国重要的雄性不育材料“陕2A”细胞质进行了分子水平的鉴定，为证明“陕2A”是一类新型的雄性不育材料提供了重要的实验证据。 对甘蓝型油菜采用DNA快速提取法、酚仿法和CTAB法应用于不同的分子标记分析，实验结果显示： CTAB法适用于样品量大，纯度要术高的RFLP技术，酚仿法适用于引物筛选、DNA模板用量大的PCR反应，而快速提取法特别适合于生产上对种子纯度检测，是生产上推广前景很好的实用技术。 对甘蓝型油菜RAPD技术应用当中PCR体系的建立进行了探讨。实验结果显示：热启动对PCR结果的影响至关重要。而Mg++浓度、dNTP浓度、模板浓度、Tag酶用量对反应结果有不同程度的影响。经过反复实验：当PCR各组分按Mg++，2mM;dNTP，200uM;模板浓度，50ng - lOOng时，PCR的结果最好。PCR反应条件经反复实验后确定为：第一个循环：（热启动）94℃，Imin20sec．OoC 2min循环一次;第二个循环：（解链）94℃ 50sec，（退火）40℃ Imin30sec;（延伸）72℃lmin;循环40次。第三个循环：72℃lOmin，循环1次。反应总体积为20ul时最为适用。 用40个lOmer的RAPD随机引物对“杂油59”的2个亲本“垦C8”和“陕3A” 进行RAPD分析，共出现290条带，分布于3530-220bp之间。引物opA-06、opK-03、opK-13、opj-12出现阳性扩增。经重复实验后确定： opK-03的PCR结果重复性最好，该引物序列为：CCAGCTTAGG。用它对两个亲本进行RAPD分析，PCR结果共出现9条带，其中510bp、260bp为二条特征带。在Fl代中这两条特征带重现性很好。用50个商品用种萌发的F1单株进行验证，检测结果为3个个体没有出现510bp的特征带，4个个体没有出现260bp的特征带，有5个个体出现了其它带，纯度为78%，与生产用种的纯度相符。 通过对“杂优59”不同生育时期及不同取样部位作酯酶同工酶电泳方法与RAPD方法相比较，结果显示：RAPD方法可以弥补同工酶方法的缺限。由于它是基于基因水平的分析技术，可以不受环境条件、发育时期、取材部位等客观条件的限制，并具有取样量小、易操作、费用低、灵敏度高、可以检测出亲缘关系相当近的种闾或种内的材料，具有独到的优点。是值得今后在生产上推广的新技术。 用6个雄性不育材料线粒体的特异探针：ALXR 18（线粒体ATPaseα亚基）;COB 640(脱辅基细胞色素-b);COX -I（细胞色素氧化酶亚基-I）;COX -Ⅱ（细胞色素氧化酶亚基-II;PDC - 12（胡萝卜线粒体随机片断）;C2（玉米线粒随机片断），对“陕2A”，Hybrides Polima，Ogura NSL 94/96, Ogura MLCH036, Ogura NSL, Polima, Fu27,Fu38, Anand等9个材料进行RFLP分析，结果显示：用限制性内切酶EcoR I消化后的DNA与探针COB 640杂交，“陕2A”材料在4.5 kb处缺失，与ALXR 18探针杂交，在4.4 kb、4.2 kb处也明显缺失，证明“陕2A”显然不同与其它不育材料。用ALXR l8为探针，与用内切酶Nc01的酶切片断作Sourthern杂交，在RFLP谱带上6.1 kb、2.4 kb、2.5 kb处明显缺带，进一步为“陕2A”是一种新型的甘蓝型油莱雄性不育系提供了证据。

乌珠穆沁羊mtDNA的RFLP研究

用Apa I等7种识别6碱基的限制性内切酶研究了14只乌珠穆沁羊mtDNA的RFLP。结果表明,在所研究的个体中检测到37个酶切位点,17种限制性态型,其中BamH I和Bgl I表现出多态,Xho I无切点。17种限制性态型可归结为3种基因单倍型,mtDNA多态度π值为0.027%,表明乌珠穆沁羊mtDNA多态性比较贫乏。

绵羊、山羊和岩羊mtDNA的RFLP及其遗传分化研究

用15种识别6碱基的限制性内切酶ApaⅠ、BamHⅠ、BglⅠ、BglⅡ、ClaⅠ、DraⅠ、EcoRⅠ、EcoRⅤ、HaeⅡ、HindⅢ、KpnⅠ、PvuⅡ、PstⅠ、SacⅠ和SalⅠ对绵羊、山羊和岩羊mtDNA的限制性片断长度多态性进行了比较研究,以探讨其遗传分化关系。

Characterization of Sarcocystis species in domestic animals using a PCR-RFLP analysis of variation in the 18S rRNA gene: a cost-effective and simple technique for routine species identification

Thirteen restriction endonucleases were used to investigate nucleotide sequence variation in the 18S rRNA DNA of 88 individuals from ten Sarcocystis taxa collected as cysts from their intermediate hosts, swine, cattle and water buffalo. A DNA sequence of

A PCR-based RFLP analysis of Sarcocystis cruzi (Protozoa : Sarcocystidae) in Yunnan province, PR china, reveals the water buffalo (Bubalus bubalis) as a natural intermediate host

A polymerase chain reaction-based restriction fragment length polymorphism (RFLP) approach is used to examine Sarcocystis cruzi-like taxa from the atypical intermediate host, water buffalo, in Yunnan, People's Republic of China. The loci examined lie with