土壤样品中DNA提取方法的比较

对土壤样品中提取DNA方法的有效性进行了比较研究。如果以细胞有效裂解和DNA产率为标准,用冻融进行预处理再结合SDS和溶菌酶的化学裂解方法,是效果最佳的DNA抽提方法,细胞裂解率为82%,DNA产率达20.8μg/g。为了去除PCR抑制物,将DNA样品进一步用柱纯化,回收率为80%。纯化后的DNA样品可用于16SrDNA扩增及其他分子操作。     

A Simple Method of Genomic DNA Extraction from Human Samples for PCR-RFLP Analysis

Isolation of DNA from blood and buccal swabs in adequate quantities is an integral part of forensic research and analysis. The present study was performed to determine the quality and the quantity of DNA extracted from four commonly available samples and to estimate the time duration of the ensuing PCR amplification. Here, we demonstrate that hair and urine samples can also become an alternate source for reliably obtaining a small quantity of PCR-ready DNA. We developed a rapid, cost-effective, and noninvasive method of sample collection and simple DNA extraction from buccal swabs, urine, and hair using the phenol-chloroform method. Buccal samples were subjected to DNA extraction, immediately or after refrigeration (4–6°C) for 3 days. The purity and the concentration of the extracted DNA were determined spectrophotometerically, and the adequacy of DNA extracts for the PCR-based assay was assessed by amplifying a 1030-bp region of the mitochondrial D-loop. Although DNA from all the samples was suitable for PCR, the blood and hair samples provided a good quality DNA for restriction analysis of the PCR product compared with the buccal swab and urine samples. In the present study, hair samples proved to be a good source of genomic DNA for PCR-based methods. Hence, DNA of hair samples can also be used for the genomic disorder analysis in addition to the forensic analysis as a result of the ease of sample collection in a noninvasive manner, lower sample volume requirements, and good storage capability.     

工业化废水处理反应器污泥总DNA提取方法

根据工业化废水处理反应器污泥特性,对常规的溶菌酶-SDS-酚/氯仿环境样品总DNA提取方法进行改进,增强样品预处理,强化细胞裂解,提高杂质去除效率,获得了一种工业化污泥总DNA提取的通用方法,并采用该方法对石家庄若干实际运行的工业化厌氧、好氧反应器的污泥样品进行了总DNA提取研究.结果表明,该方法对所选污泥样品均有效,具有普适性.提取的污泥总DNA杂质含量少,纯度高,A260/A280在1.8左右;提取效率较高.总DNA产率都在0.7 mg/g以上,最大产率可达0.85 mg/g.所提取的污泥总DNA可以直接作为模板进行PCR反应,PCR产物直接进行变性梯度凝胶电泳(DGGE),能够得到较好的DGGE谱图,表明该方法提取的污泥总DNA样品可满足后续分析研究的要求.     

A Simple Silica-based Method for Metagenomic DNA Extraction from Soil and Sediments

A new method is described for extraction of metagenomic DNA from soil and sediments which is based on DNA adsorption to silica without the use of phenol, ethanol precipitation or a cesium chloride gradient. High-quality DNA was obtained, and PCR inhibition was overcome by adding bovine serum albumin and adjusting magnesium concentration. By using PCR-DGGE with Firmicutes and lactic acid bacteria-specific primers the extracted metagenomic DNA was shown to contain a mixture of bacterial genomes. This method can be used for screening bacterial diversity in soil and sediment samples.     

狮子头热泉菌席样品环境总DNA提取方法的比较研究

通过对狮子头热泉7个环境菌席样品所提取的总DNA进行纯度检测、提取得率计算和DGGE分析,比较了3种直接和1种间接DNA提取方法。结果表明：综合利用多种裂解方式比单一裂解方式更能充分释放环境DNA;其中3种方法获得的DNA片段能够进行后续16S rDNA扩增;针对同一样品,不同方法提取的环境DNA,可获得不同DGGE群落指纹图谱;间接提取法提取的总DNA,能更好地反映狮子头热泉菌席的微生物多样性。     

A Simple, Efficient Method for the Separation of Humic Substances and DNA from Environmental Samples

Three different gels (Sepharose 4B, Sephadex G-200, and Sephadex G-50) were evaluated as a means of removing humic contaminants from DNA extracts of environmental samples. Sepharose 4B gave superior separation of DNA from humics, and DNA purified in this way showed consistently greater amplification than DNA purified by the other materials.     

Evaluation and Optimization of DNA Extraction and Purification Procedures for Soil and Sediment Samples

We compared and statistically evaluated the effectiveness of nine DNA extraction procedures by using frozen and dried samples of two silt loam soils and a silt loam wetland sediment with different organic matter contents. The effects of different chemical extractants (sodium dodecyl sulfate [SDS], chloroform, phenol, Chelex 100, and guanadinium isothiocyanate), different physical disruption methods (bead mill homogenization and freeze-thaw lysis), and lysozyme digestion were evaluated based on the yield and molecular size of the recovered DNA. Pairwise comparisons of the nine extraction procedures revealed that bead mill homogenization with SDS combined with either chloroform or phenol optimized both the amount of DNA extracted and the molecular size of the DNA (maximum size, 16 to 20 kb). Neither lysozyme digestion before SDS treatment nor guanidine isothiocyanate treatment nor addition of Chelex 100 resin improved the DNA yields. Bead mill homogenization in a lysis mixture containing chloroform, SDS, NaCl, and phosphate-Tris buffer (pH 8) was found to be the best physical lysis technique when DNA yield and cell lysis efficiency were used as criteria. The bead mill homogenization conditions were also optimized for speed and duration with two different homogenizers. Recovery of high-molecular-weight DNA was greatest when we used lower speeds and shorter times (30 to 120 s). We evaluated four different DNA purification methods (silica-based DNA binding, agarose gel electrophoresis, ammonium acetate precipitation, and Sephadex G-200 gel filtration) for DNA recovery and removal of PCR inhibitors from crude extracts. Sephadex G-200 spin column purification was found to be the best method for removing PCR-inhibiting substances while minimizing DNA loss during purification. Our results indicate that for these types of samples, optimum DNA recovery requires brief, low-speed bead mill homogenization in the presence of a phosphate-buffered SDS-chloroform mixture, followed by Sephadex G-200 column purification.     

一种简单有效且适于土壤微生物多样性分析的DNA提取方法

参照Zhou[11]的方法进行了改进,获得了一种简单、有效的DNA提取方法.此方法操作简单、从大量样品改为小量样品的提取,利用高浓度的PEG沉淀,不作回收纯化,所提DNA片段较大,在23 kb以上,每克土的DNA提取量从3.74～15.28 μg,OD260/OD230比值在0.89～1.21范围内,用真菌和细菌核糖体特异性引物进行PCR扩增,均获得较好的结果,DGGE图谱显示丰富性较高,可用于细菌多样性和真菌多样性的分析.此方法能够从4种不同性质土壤中提取出DNA,但提取盐渍土壤和碱性土壤的效果更好一些,为土壤微生物群落结构的多样性分析奠定良好的基础.     

碱裂解法提取细菌质粒DNA的改良

碱裂解法是目前最为广泛应用的细菌质粒DNA的提取方法。但该法提取DNA所需时间较长,通常需要2h以上。为了快速提取质粒DNA,对常规碱裂法中溶液Ⅰ、Ⅱ、Ⅲ、RNA酶A及无水乙醇的反应时间由原来的5min,5min,10min,30min,10min分别缩短至5s,1min,5s,10min,5min。这种改良方法极大地缩短了DNA的提取时间,可在30min内完成整个DNA的制备,且制备的DNA可直接应用于进一步的酶切,连接及PCR等各种分子生物学分析。     

从土壤中提取DNA方法比较

设计并比较了3种直接从土壤中提取DNA的方法。试验结果表明:3种方法都可以从土壤中提取到分子量大于23.13 kb的DNA的片段,每克干土DNA的提取量为2.5~31μg,不同方法间在DNA产量、纯度等方面存在较大差异。     

A Hybrid DNA Extraction Method for the Qualitative and Quantitative Assessment of Bacterial Communities from Poultry Production Samples

The efficacy of DNA extraction protocols can be highly dependent upon both the type of sample being investigated and the types of downstream analyses performed. Considering that the use of new bacterial community analysis techniques (e.g., microbiomics, metagenomics) is becoming more prevalent in the agricultural and environmental sciences and many environmental samples within these disciplines can be physiochemically and microbiologically unique (e.g., fecal and litter/bedding samples from the poultry production spectrum), appropriate and effective DNA extraction methods need to be carefully chosen. Therefore, a novel semi-automated hybrid DNA extraction method was developed specifically for use with environmental poultry production samples. This method is a combination of the two major types of DNA extraction: mechanical and enzymatic. A two-step intense mechanical homogenization step (using bead-beating specifically formulated for environmental samples) was added to the beginning of the “gold standard” enzymatic DNA extraction method for fecal samples to enhance the removal of bacteria and DNA from the sample matrix and improve the recovery of Gram-positive bacterial community members. Once the enzymatic extraction portion of the hybrid method was initiated, the remaining purification process was automated using a robotic workstation to increase sample throughput and decrease sample processing error. In comparison to the strict mechanical and enzymatic DNA extraction methods, this novel hybrid method provided the best overall combined performance when considering quantitative (using 16S rRNA qPCR) and qualitative (using microbiomics) estimates of the total bacterial communities when processing poultry feces and litter samples.     

An Efficient Extraction Method of Persistent Organic Pesticides in Soil Samples for Their Chromatographic Determination

In order to determine persistent organic pesticides (OPs) and their metabolites in soil samples, an analytical procedure was developed, optimized and validated. It possesses advantages like suitable limits of detection, low solvent volume and time consume, and requires a chromatography detector commonly used in routine laboratories. The method allows the determination of Methoxychlor, p,p’-DDT, Endosulfan sulfate, Endrin aldehyde, p,p’-DDD, Endosulfan II, Endrin, Dieldrin, p,p’-DDE, Endosulfan I, Heptachlor epoxide, Aldrin, Heptachlor, δ-HCH, γ-HCH, β-HCH, α-HCH, Etridiazole, Trifluralin, Hexachlorobencene, Chlorothalonil, Chlorpyrifos, DCPA, γ-Chlordane, α-Chlordane, Clorbenzilate, trans-Permethrin, cis-Permethrin. Linearity is evaluated and the analytical parameters are presented. The average recoveries obtained for each pesticide (28 OPs) by using 3, 15 and 22.5 µg kg^?1 spiked samples ranged between 50 and 97.3%, 57 and 103% and from 60 to 100% for each case. The limits of detection and quantification vary from 0.18 to 1.28 μg kg^?1 and from 0.60 to 4.22 μg kg^?1. The reproducibility obtained as relative standard deviation percentages is less than 7.5, 5.3 and 4.2% for low, middle and high level of concentrations, respectively. The procedure is statistically validated for its application to soil samples and compared with other published methods.     

CTAB法提取野野村菌基因组DNA

针对用常规方法难以提取野野村菌基因组DNA的问题,通过选用添加甘氨酸的不同培养基和不同培养时间获得的菌丝体,采用液氮研磨结合CTAB法提取野野村菌DNA,电泳检测及计算OD260/OD280值。结果表明,在添加0.3%甘氨酸的麦芽汁-酵母膏(YE)培养基中振荡培养培养3d的菌丝体适合于DNA提取,用CTAB法获得的基因组DNA,长度约为20kb,且OD260/OD280在1.8左右,达到基因组DNA-DNA杂交的要求。     

A Simple Method for Selective Isolation of Stenotrophomonas maltophilia from Environmental Samples

Stenotrophomonas maltophilia is a commonly found environmental bacterium that is associated with the plant rhizosphere. It shows increasing prevalence in immunocompromised patients. We report a simple method for selective isolation of S. maltophilia from soils which makes use of both its resistance to imipenem and its requirement for methionine.     

一种棉花线粒体DNA的提取方法

线粒体是重要的细胞器,它有自身的基因组。其基因组DNA与细胞核基因组DNA相比,含量较低。棉花当中富含棉酚、丹宁等物质,这对提取DNA有很大的影响。因此我们根据棉花自身的特点,找到了一种提取棉花线粒体DNA经济有效的方法,其质量可以满足限制性酶切、PCR、分子杂交等实验的要求。     

两种从土壤中提取DNA方法的比较

为土壤微生物多样性研究选取理想的DNA提取方法,该文比较了直接法和间接法从土壤中提取微生物总DNA的效果。结果表明：直接法提取量大,每克土壤提取到DNA约10．26μg,而间接法仅提取到0．55μg,直接法DNA提取量约为间接法的19倍。直接法得到的DNA包含细菌种群较间接法丰富,DGGE分析结果显示,二者的条带数分别为35条和28条,占检测条带总数的92．1%和78．9%。间接法提取到DNA纯度较直接法高,不需纯化即可用于PCR扩增和BamHⅠ酶切反应。     

On the Methodology of Nematode Extraction from Field Samples: Comparison of Methods for Soil Extraction

The commonly used nematode extraction methods were compared using three soil types and four nematode species. The comparison was repeated in three trials by the same operator to estimate operator reproducibility. Extraction efficiency was dependent upon method, soil type, and nematode species, and reproducibility was not particularly satisfactory for routine analyses. Extraction by any method tested was less than 50% efficient. Quantitative nematode extraction methodology needs serious attention.     

一种从鸟类剥制标本提取DNA的改进方法

应用非损伤性取样的方法,收集鸟类剥制标本的皮肤组织和羽毛,用无水乙醇、浸泡液预处理的方法抽提DNA,结果两者都可提取DNA供PCR扩增。将PCR产物经序列测定和比对分析,证明提取的DNA为目的DNA,表明本试验方法可行。鸟类剥制标本的皮肤组织和羽毛可以作为研究种群遗传学的资源。