一种快速握取植物总DNA的良好材料与方法

本文介绍以种子植物幼嫩胚乳为材料,用改良的氯仿－异戊醇快速提取方法提取植物总ＤＮＡ。这种材料和方法,细胞磨碎容易,ＤＮＡ收取量大,操作简便,适用于遗传操作及教学实验等方面的ＤＮＡ快速制备。     

木根麦冬（Ophiopogon xylorrhizus）干叶提取DNA用于RAPD分析

木根麦冬（Ｏｐｈｉｏｐｏｇｏｎｘｙｌｏｒｒｈｉｚｕｓ）是我国珍稀濒危植物,分布仅限于云南西双版纳雨林,在植物系统学和保护生物学研究中具有独特的意义。随机扩增多态ＤＮＡ（ＲＡＰＤ）方法是揭示群体遗传多样性的高效、简便方法,但一般均以新鲜材料提取总ＤＮＡ,对一些分布边远地区物种难以采用此法。本文研究从木根麦冬干叶片中提取总ＤＮＡ,进行ＲＡＰＤ分析。样品取自４个居群、４９个个体。选取生长旺盛的叶片,在野外用硅胶快速干燥保存样品。采用高盐低ｐＨ值法提取总ＤＮＡ,每克鲜重所得的干叶可得８０～１６０μｇ。通过对模板ＤＮＡ的各种处理和ＰＣＲ扩增程序的调整,解决了扩增片段边缘弥散、界线模糊、产率低等问题,获得了理想的扩增带型。这一成果对其它从野外直接采样的干叶提取ＤＮＡ进行ＲＡＰＤ研究具有指导意义     

植物总DNA样品的快速制备

利用Ｑｉａｇｅｎ微量植物ＤＮＡ提取试剂盒,在１小时内即可从植物组织获得总ＤＮＡ,提取过程中勿需酚／氯仿和ＳＤＳ抽提,操作简便、快捷。所得ＤＮＡ样品的ＯＤ２６０／ＯＤ２８０值在１．７－１．９之间。样品纯度高;该样品不含ＰＣＲ反应抑制剂及其他酶反应抑制剂,可被各种限制性内酶完全降解,适合于ＰＣＲ、印迹、ＲＡＰＤ、ＡＦＬＰ和ＲＦＬＰ分析等各种下游应用。     

香蕉不同组织中总RNA的有效分离

从植物组织中提取总ＲＮＡ是进行植物分子生物学某些方面研究的必要前提。如进行Ｎｏｒｔｈｅｍ杂交分析,纯化ｍＲＮＡ以用于体外翻译或建立ｃＤＮＡ文库,ＲＴ－ＰＣＲ及差示分析等分子生物学实验,都需要高质量的总ＲＮＡ。因此,从植物组织中提取高质量的总ＲＮＡ是顺利进行上述研究的关键所在。目前常用于植物材料ＲＮＡ提取的方法有脱法［１～４］苯酚法［５,６］和ＣＴＡＢ［７,８］法等。这些方法对于提取某些植物的总ＲＮＡ是有效的,但对另外一些植物来说,却并不一定是好的方法。因为不同植物组织的细胞内外成分复杂多变,在使…     

一种提取果树叶片DNA的简便方法

植物ＤＮＡ的提取是分子遗传学及遗传工程的根本前提。通常ＤＮＡ提取方法应满足以下几个主要条件：（１）所得ＤＮＡ具备理想的纯度,如ＲＦＬＰ技术对ＤＮＡ纯度要求高,因为纯度高的ＤＮＡ便于酶切及膜转移等操作,而对于涉及ＰＣＲ扩增的技术,ＤＮＡ提取则尤为注意样...     

甘薯叶片超氧化物歧化酶基因克隆及测序

以甘薯（Ｉｐｏｍｏｅａｂａｔａｔａｓ（Ｌ．）Ｐｏｉｒ）叶为材料提取植物总ＲＮＡ,经反转录后,利用多聚酶链式反应技术,扩增并克隆超氧化物歧化酶基因的ｃＤＮＡ,并进行测序分析。该序列全长４８２ｂｐ,其读码框编码１５２个氨基酸,与国外文献报道的甘薯块根ＳＯＤ基因的ｃＤＮＡ序列相比,具有９９％的同源性。     

猪瘟病毒石门株特异cDNA片段的扩增与序列分析

以猪瘟病毒感染细胞中提取的细胞总ＲＮＡ为模板,应用反转录─聚合酶链反应,在化学合成的两对特异引物引导下,成功地扩增出了两个石门株的ｃＤＮＡ片段。电泳证明它们的大小与预计的３４６ｂｐ和１２０ｂｐ完全一致。酶切分析证实了它们应有的酶切位点。随后对这两个片段进行了克隆和序列测定,并与国外株的序列进行了比较。结果证明本实验扩增的两个ｃＤＮＡ序列与Ａｌｆｏｒｔ株和Ｂｒｅｓｉａ株的同源性分别是９５．２％和９８．５％。     

大豆分子育种研究获重大突破“转基因大豆”新品系性状优良

大豆分子育种研究获重大突破“转基因大豆”新品系性状优良黑龙江省农科院雷勃均研究员和卢翠华副研究员在其所主持的“导入外源总ＤＮＡ获得优质高蛋白和双高大豆新品系”课题研究中,带领课题组成员刻苦攻关,先后完成了对大豆供体总ＤＮＡ的提取和直接导入受体的组合配...     

一种简便的海藻DNA提取方法

把包裹缠绕在大量粘性多糖中的海藻ＤＮＡ提取出来是一个十分困难的。研究表明,ＤＮＡ样品中的酸性多糖会抑制限制性酶切反应和ＰＣＲ扩增,而海藻组织中主要的碳水化合物是硫多糖和羧酸多糖,而且比陆生植物的中性多糖更易水溶,使溶液高度粘稠,在ＤＮＡ提取中很难去除...     

鸢尾属药用植物总DNA提取方法的比较研究

以鸢尾属（Iris L．）药用植物鸢尾Iris tectorum Maxim．叶片为材料,分别采用CTAB法、高盐低pH法、SDS法和试剂盒法四种方法提取植物总DNA,并通过琼脂糖凝胶电泳、紫外分光光度计、ISSR和RAPD四种方法对所提取的DNA样品进行检测。结果表明,用SDS—I法提取的植物总DNA纯度、浓度和完整性都很高,从经济角度考虑优于用试剂盒提取,从提取效果考虑不亚于用CTAB法和高盐低pH法提取,是比较适合鸢尾属植物总DNA提取的方法。     

Leaf age affects the quality of DNA extracted from Dimorphandra mollis (Fabaceae), a tropical tree species from the Cerrado region of Brazil

Isolation of high-quality DNA from plants, especially plants from the Cerrado, is notoriously difficult because of polysaccharides and secondary compounds produced by plants from this biome. DNA isolation and its quality may be compromised by chemical defenses such as tannins and phenols. Quantitative plant defenses tend to have a cumulative effect, increasing in concentration during leaf development, reducing DNA quality extracted in mature compared to young leaves. We report the effect of leaf age on DNA extraction of Dimorphandra mollis. Our working hypothesis was that the young leaves have more DNA than old leaves of the same individual because chemical defenses accumulate in older leaves. Young and old leaves were sampled from eight mature trees as well as leaves from eight seedlings in the north region of Minas Gerais State. Genomic DNA extraction followed the standard CTAB procedure. DNA isolation was very successful from young leaves of 16 individuals of D. mollis. The extracted DNA exhibited high quality and the DNA quantity was also high, with an A(260)/A(280) ratio above 1.8, which is within the optimal sample range. In contrast, DNA isolation from old leaves was not successful. When the DNA was extracted from old leaves, the DNA was brownish, indicating contamination by phenolic compounds. These metabolites oxidize the DNA irreversibly, which hinders amplification of DNA by PCR by inhibiting the action of enzymes such as Taq polymerase. PCR performed with DNA from young leaves of D. mollis was successful and produced strong bands for RAPD markers.     

栗属植物基因组DNA的提取及RAPD、SSR分析

以中国板栗、茅栗和锥栗的叶片为材料,提取栗属的DNA。针对栗属植物富含多酚类等次生物质的特点对栗属DNA的提取方法进行了改良,采用CTAB-蛋白酶K法加重复抽提,去除栗属植物中的相关次生物质,获得了高质量的DNA。所提取的DNA完全满足PCR、RAPD、SSR等一些分子生物学实验要求。     

Rapid isolation of DNA from Dioscorea species suitable for PCR,restriction digestion and pathogen screening

The methods employed for DNA extraction from many plants is difficult because of the metabolites that interfere with DNA isolation procedures. We have developed a reliable and efficient method for isolating genomic DNA free from polysaccharide, polyphenols and protein contaminants from Dioscorea spp. The method involves inactivation of contaminant proteins by using CTAB/Proteinase K and precipitation of polysaccharides in the presence of high concentration of salt. The purity of genomic DNA was confirmed by A260/280 and A260/230 ratios calculated from the spectrophotometric readings and further by restriction analysis of the isolated DNA using restriction enzymes Eco RI. The total genomic DNA extracted by the new protocol was used for polymerase chain reaction amplification, RAPD analysis, restriction digestion and pathogen screening. The new protocol can be successfully used for both small- and large-scale preparation of genomic DNA from different tissues of Dioscorea spp. The quarantine of seed tubers and use of pathogen-free tubers for planting is a prerequisite for integrated disease management strategy. The protocol can be used for the isolation of genomic DNA from other crop plants too.     

植原体DNA提取方法的改良

在总结多种植原体DNA提取方法的基础上 ,发展了一种提取植原体DNA新方法。用此方法提取的DNA经琼脂糖凝胶电泳检测到大于 15kb的DNA主带 ,基本无DNA碎带 ,不用RNase处理 ,也无RNA干扰 ,OD2 60 / 2 80 值显示产物纯度较高 ,无需任何处理 ,即可以作为模板扩增     

A rapid and efficient DNA minipreparation suitable for screening transgenic plants

We present a modified method for DNA minipreparation suitable for large-scale screening of transgenic plants. The method is rapid and efficient—one person can prepare DNA from approximately 50 samples per day. The average yield was about 40 μg DNA per 100 mg of fresh tissue, and the A₂₆₀/A₂₈₀ was 1.89–2.03. The total DNA extracted by this method could be used for PCR, restriction enzyme digestion, and Southern blotting.     

A strategy for optimizing quality and quantity of DNA extracted from soil

The efficiency of a bead beating method was studied in detail with regard to a variety of factors including beating time and speed, volume and temperature of the buffer, as well as amount and type of beads employed. The results presented here reveal that all of these parameters have a significant effect on yield and quality of DNA extracted from soils. Precise adjustment of extraction conditions allows for significantly higher yields of high quality DNA from soils than previously reported. We further evaluated the effect of the extraction conditions on the apparent soil microbial community structures, as observed by polymerase chain reaction (PCR) and RFLP. Differences in the fingerprints of DNA extracted under different conditions suggest that results could be biased when using gentle extraction procedures. Based on multiple subsequent extractions using very harsh extraction conditions, we propose a protocol for the quantification of the total DNA content in soils. Extractions from six soils of different texture and chemical characteristics with selected bead beating protocols revealed that the quality (fragment size and purity) of the extracted DNA was generally very good, but also depended on the soil characteristics. While a single, general protocol for optimal DNA recovery from all soils cannot be given, this study provides detailed guidelines on how to optimize the general method to obtain optimal DNA from individual soils.     

DNA isolation protocol for red seaweed (rhodophyta)

We report a DNA isolation protocol for red seaweed. The method is a modification of the Dellaporta et al. (1983) protocol for land plants. Our simplified version can be used to process large sample numbers and to minimise polysaccharide co-isolation. The protocol was applied to 12 red seaweed species as well as one green alga and one land plant. The protocol yields about 5 μg of high molecular weight DNA from 10 mg of dried material, with no RNA. No sign of degradation was observed after agarose gel electrophoresis for both freshly extracted DNA and DNA stored for 18 months at 4°C. DNA isolated by our protocol was suitable for genomic library construction (tested for one species), endonuclease restriction, and PCR amplification for all species.     

Universal and rapid salt-extraction of high quality genomic DNA for PCR-based techniques.

A very simple, fast, universally applicable and reproducible method to extract high quality megabase genomic DNA from different organisms is described. We applied the same method to extract high quality complex genomic DNA from different tissues (wheat, barley, potato, beans, pear and almond leaves as well as fungi, insects and shrimps' fresh tissue) without any modification. The method does not require expensive and environmentally hazardous reagents and equipment. It can be performed even in low technology laboratories. The amount of tissue required by this method is approximately 50-100 mg. The quantity and the quality of the DNA extracted by this method is high enough to perform hundreds of PCR-based reactions and also to be used in other DNA manipulation techniques such as restriction digestion, Southern blot and cloning.     

琼脂固体培养基培养蜜环菌菌索总DNA的提取

野外采集的蜜环菌[Armillaria mellea(Vahl.ex Fr.)Quel]在提取DNA前需要分离获得纯化的菌丝体。常规液体培养获得菌丝团的方法感杂率较高,采集固体培养基表面cellophane膜上形成的菌丝则难以获得足量的DNA提取材料。蜜环菌细胞内含有大量多醣类物质,也使得蜜环菌高质量DNA的提取存在一定的困难。本研究通过改进试验,提供一个直接从琼脂固体培养基培养的蜜环菌菌索中提取高质量DNA的方法。其中样品的预先冻融处理方法可以促使蜜环菌菌索与琼脂分离;而在裂解提取缓冲液裂解材料细胞后加入1.25 mol/L KAc溶液,则有利于除去蜜环菌细胞内的多醣类物质以及残留的少量琼脂。通过琼脂糖电泳、紫外分光光度计对DNA浓度及OD值的测定、ISSR引物的PCR扩增以及酶切产物的PCR扩增等方法的检测,结果均表明该方法提取的DNA质量较好,符合进一步进行分子生物学研究的要求。     

一种动物基因组DNA提取方法的改进

介绍一种动物基因组ＤＮＡ提取方法。该方法具有简便、快速、实用的特点,所获得的ＤＮＡ数量和质量都很高,可用于各种分子生物学实验。