桔梗RAPD反应体系的优化

以通化桔梗为材料,用改进的CTAB法提取桔梗叶片的总DNA,通过对不同镁离子浓度、dNTP浓度、模板DNA含量、引物浓度、DNA聚合酶量条件下的RAPD扩增反应的效果,建立了一个适合桔梗的比较稳定的RAPD反应体系,用于桔梗遗传多样性分析。结果表明,桔梗RAPD扩增反应的最佳体系为:模板DNA20ng,dNTP150μmol/L,引物0.3μmol/L,Mg2+浓度2.0mmol/L,TaqDNA聚合酶1Unit,10×Buff-er2.0μL,PCR反应总体积为20μL。按此优化RAPD条件进行实验,重现性良好。     

苏铁属植物RAPD反应体系的优化及部分种类亲缘关系的探索

通过优化苏铁属植物的RAPD反应体系,进而探讨苏铁属部分种类的亲缘关系。结果表明,Mg~(2+)、dNTP、Taq酶及随机引物浓度在RAPD反应中有重要影响,而模板DNA浓度有一个很大的适应范围。适合苏铁属植物RAPD分析的反应体系:20μL反应体系中,含有10 mmol/L Tris-HCl(pH8.3)、50 mmol/L KCl、2.0mmol/L MgCl_2、200μmol/L dNTP、0.3μmol/L随机引物、模板DNA 50ng、Taq酶1.0 U。聚类分析结果基本反应了苏铁属各个种间的亲缘关系,证明了RAPD适用于苏铁属种间亲缘关系分析。RAPD聚类分析结合形态学研究表明:海南苏铁、台湾苏铁、广东苏铁、滇南苏铁和仙湖苏铁之间的亲缘关系较远,支持各自成为独立的种。     

Use of a subset of doubled-haploid lines for RAPD interval mapping in barley.

Molecular markers have been used in barley to locate genes and quantitative trait loci. Only a few RAPD markers have been located on barley marker maps. The objectives of this study were (i) to place RAPD markers in specific intervals on the barley linkage map developed from the cross Steptoe (S) x Morex (M), (ii) to examine the distribution of RAPD markers, and (iii) to compare markers amplified by Taq DNA polymerase with those amplified by the Stoffel fragment of Taq DNA polymerase. Screening of DNA from S and M with 362 decamer primers identified 85 that amplified 127 reliable RAPDs. A subset of 15 doubled-haploid (DH) lines from the 150 DH line mapping population was used to place these RAPD markers in intervals on the SM map. This subset can be used for rapid placement of any new markers on the SM linkage map. Most of the RAPD markers were dominant but four codominant RAPDs were identified. The RAPDs were not evenly distributed, with many clustered around the centromeric region of each chromosome. Two of these clusters were located in intervals larger than 15 cM. Testing of 38 to 42 additional DH lines provided more precise placement of eight of the markers in these clusters. Reliable RAPDs were detected with 44% of the primers tested with the Stoffel fragment, but with only 17% of the primers tested with Taq DNA polymerase. These RAPDs provide additional markers for use in barley improvement.     

濒危植物七子花RAPD条件的优化

以改进SDS法抽提濒危植物七子花嫩叶总DNA,进行随机扩增多态DNA（RAPD）分析,分别测试了镁离子, dNTP,模板DNA含量,引物和DNA聚合酶量对反应结果的影响,通过各因子的组合研究,可知七子花RAPD分析较适宜的扩增条件是：15 μL PCR反应体积,1×Taq酶配套缓冲液（10 mmol/L Tris·HCl pH 9.0, 50 mmol/L KCl, 0.1% Triton X_100）,2.5 mmol/L MgCl2,2U Taq酶（上海华美公司）,10 ng模板DNA,20 pmol引物（上海Sangon公司）;dATP、dCTP 、dGTP 、dTTP 各0.1 mmol/L。     

柱花草RAPD反应体系的建立及其8个品种遗传多样性分析

采用两种不同的方法分别从柱花草嫩叶及种子萌发芽中提取了高质量的DNA ,并对柱花草RAPD反应中的各组分浓度及热循环因素进行优化 ,建立了柱花草RAPD反应的最佳条件。在此基础上 ,用 2 0条随机引物对 8个柱花草品种进行了RAPD扩增 ,结果表明 ,其多样性达 5 1 .9% ,品种间的遗传相似系数在 0 .5 3～0 .88之间 ;根据非加权成对平均数法 (UPGMA)进行分类 ,获得了品种聚类树形图 ,8个柱花草品种均被明显分开。     

一种新的分子标记方法－随机微卫星扩增多态DNA (RMAPD)

随机微卫星扩增多态DNA（RMAPD）是利用随机引物和微卫星的上游或下游引物一起作为该扩增的引物,在Taq DNA聚合酶、MgCl2、dNTPs和模板DNA等共同作用下进行PCR扩增的一种新型分子标记方法。其核心是RMAPD引物的有效性问题。通过对西农萨能奶山羊群体RMAPD电泳检测、数据统计分析及验证实验等证明RMAPD的引物是有效的。通过与微卫星和RAPD标记比较,发现RMAPD标记在扩增引物、扩增程序和重复性等方面区别于微卫星和RAPD标记;它是RAPD标记的一种广义的延伸,但又不完全等同于RAPD标记。因此,确定RMAPD是一种新的分子标记方法。该方法也具有DNA标记的特点,在群体遗传结构和亲缘关系分析以及标记辅助选择等遗传育种领域具有广阔的应用前景。     

皮下盘菌属及其近似类群RAPD-PCR反应条件的优化

以悬钩子皮下盘菌等总基因组DNA为皮下盘菌属(Hypodermade Not.)及其近似类群RAPD体系优化的模板,对模板DNA浓度、dNTPs浓度、Mg2+浓度、引物浓度、TaqDNA聚合酶浓度等反应体系以及退火温度和时间、延伸时间、循环次数等扩增程序条件进行优化,寻找出适合此类菌物RAPD-PCR反应的最佳反应体系和最佳扩增程序。     

扩增条件对茶类植物RAPD带的影响

采用梯度分析的方法试验了模板ＤＮＡ、引物、镁离子、ｄＮＴＰ和Ｔａｑ酶的浓度对茶类植物进行ＲＡＰＤ分析中ＤＮＡ扩增结果的影响。实验表明这些条件的变化对扩增出来的ＲＡＰＤ带的数目和强弱会产生影响。经过比较分析,筛选出对于茶类植物进行ＲＡＰＤ分析较理想的扩增条件：２．０ｍｍｏｌ／ＬＭｇＣｌ２,２００ｕｍｏｌ／ＬｄＮＴＰ,１５ｎｇ引物／２０ｕｌ反应体积,４ｎｇ模板ＤＮＡ／ｕｌ反应体积,１ＵＴａｑ酶／２０ｕｌ反应体积。     

Amplification of bacterial DNA bound on clay minerals by the random amplified polymorphic DNA (RAPD) technique

Abstract: Chromosomal DNA from Bacillus subtilis , bound on the clay minerals, montmorillonite (Wyoming (W) and Apache County (Ap)) and kaolinite (K), was subjected to the random amplified polymorphic DNA (RAPD) technique. DNA bound on the clays was not amplified with 0.625, 1.875, 6.25, and 12.5 U of Taq DNA polymerase, but amplification occurred when the clay-DNA complexes were diluted 10- and 20-fold or when 21 U of Taq DNA polymerase was added. DNA desorbed from the Ap-DNA and K-DNA equilibrium complexes was amplified with 0.625 U of Taq DNA polymerase, whereas amplification of DNA desorbed from the W-DNA complex occurred only after a 10-fold dilution or when 1.875 U of Taq DNA polymerase was used. These observations indicate that clay minerals differentially affect the amplification process, probably by inhibiting the activity of Taq DNA polymerase.     

白色念珠菌RAPD反应体系优化的研究

建立白色念珠菌RAPD的最佳反应体系,并应用于其基因组DNA扩增。通过单因子试验分别研究了Mg^2＋、dNTPs、Taq酶、引物和模板DNA等浓度对RAPD反应的影响;同时,应用L16（4^5）正交试验研究了DNA模板、Mg^2＋、Taq酶、dNTPs和引物浓度对RAPD反应的影响。以条带稳定、丰富、清晰为标准,获得了白色念珠菌基因组DNA的RAPD扩增优化条件;对于白色念珠菌的最适RAPD反应体系为Mg^2＋1．5mmol／L、dNTPs250μmol／L、引物0．6μmol／L、模板100ng／25μL、TaqDNA聚合酶1．5U／25μL。     

飞蝗总DNA的抽提及其RAPD分析条件的摸索

通过试验寻求得到一种快速、简便抽提飞蝗（Ｌocusta sp.)总DNA方法,使每头雄性和雌性成虫分别可以得以５０和１００μg的总ＤＮＡ。所得到的总ＤＮＡ ＯＤ２６０／ＯＤ２８０为１．５－２．２,分子量４５kb。为了获得高分子量的ＤＮＡ产品,使ＲＰＡＤ结果具重复性,酚氯仿抽提后的ＤＮＡ沉淀用灭菌Ｔip头挑出,而不用离心收集。对各种分析条件如摸板、Ｔaq酶、dNTP及引物的浓度、不同的ＰＣＲ仪、反应管进行了比较试验,发现在一定的范围内,它们对ＲＡＰＤ结果影响。用优化的试验条件对我国３个飞蝗亚种５个地理种群进行ＲＡＰＤ分析。结果在３个亚种ＵＰＧＭＡ聚类图中,东亚飞蝗和西藏飞蝗珠２个种群以１００％Ｂootstrap分别聚类在一起,亚洲飞蝗与东亚飞蝗的２个种群以６６％的Ｂootstrap聚类在一起,在３个亚种所有个体的ＵＰＧＭＡ聚类图中,亚种内的所有个体都聚类在一起,各自形成独立分支,说明３个飞蝗亚种有明显的区别。西藏飞蝗的２个种群之间,群居型与散居型东亚飞蝗之间在聚类图中混合聚类,说明它们之间存在基因交流。     

荔枝DNA提取及RAPD扩增条件优化

为应用RAPD技术开展对荔枝种质资源的分析,以S43(GTCGCCGTCA)为引物,通过试验设计,分别研究了退火温度、模板浓度、引物浓度、dNTP浓度、Taq DNA聚合酶用量对荔枝RAPD-PCR反应的影响。建立并优化了适宜荔枝RAPD分析的扩增体系:20μL的反应体系,30ng的模板DNA度,0.25μmol/LRAPD引物、1.0UTaqDNA聚合酶,0.2μmol/LdNTP为荔枝适宜的RAPD-PCR扩增条件。     

穗花杉ISSR引物反应条件的优化与筛选

在研究穗花杉(Amentotaxus aragotaenia)的遗传多样性过程中,为了获得清晰、重复性好ISSR扩增结果,对影响ISSR-PCR的多个因素包括模板浓度、Taq酶的选择和用量、Mg²⁺和dNTPs浓度及退火温度等指标等进行了筛选和优化,确定了穗花杉ISSR-PCR分析的最适扩增条件： 20 μL PCR反应体系中,2 μL 10×Taq酶配套缓冲液,1.8 U Taq聚合酶（上海生工公司）,0.2 μmol·L^-1引物,0.18 mmol·L^-1 dNTP,1.5～2.5 mmol·L^-1 MgCl₂,10 ng·μL^-1模板DNA。用来自不同居群7个个体,以100个ISSR引物进行PCR扩增,筛选出扩增效果较好的10个引物。得到了92个位点,其中45个多态性位点,多态性位点比例为49%。     

Fidelity of Thermococcus litoralis DNA polymerase (Vent) in PCR determined by denaturing gradient gel electrophoresis.

DNA synthesis fidelities of two thermostable DNA polymerases, Thermus aquaticus (Taq) and Thermococcus litoralis (Tli, also known as Vent), and a non-thermostable enzyme, a modified T7 DNA polymerase (Sequenase), were determined by analyzing polymerase chain reaction (PCR) products using denaturing gradient gel electrophoresis (DGGE). The error rates were 4.4, 8.9, and 2.4 x 10(-5) errors/bp for modified T7, Taq, and Tli polymerase, respectively. Reducing the nucleotide triphosphate concentration for Tli polymerase during PCR did not alter the fidelity. The ability of DGGE to detect a mutant present at several percent in a wild type population is related to the polymerase fidelity. To examine the sensitivity of mutant detection, human genomic DNA containing a 1% fraction of a known base pair substitution mutant was PCR-amplified with the three enzymes using primers that flank the mutant sequence. The PCR products were analyzed by DGGE. The signal from the mutant present at 1% was visible in the samples amplified with modified T7 and Tli polymerase, but the higher error rate of Taq polymerase did not permit visualization of the signal in DNA amplified with Taq polymerase.     

香蕉RAPD分析初步研究

比较了不同提取方法对香蕉植株不同部位组织提取 DNA的质量及其 PCR扩增结果 ,对香蕉 RAPD分析中引物种类和浓度 ,复性温度 ,d NTPs,Taq DNA聚合酶浓度 ,热循环数等因素进行了比较影响分析。结果表明 ,虽然改良的 SDS法、CTAB法和 PVP法提取的植株嫩叶和吸芽 DNA提取量和纯度各不相同 ,但其 PCR扩增结果基本相同 ;相同克隆不同植株的 DNA其 PCR扩增结果也基本相同 ;建立了适合香蕉大规模 DNA多态性分析 RAPD反应体系 :2 5 μL反应液中 ,含 1倍缓冲液 ,0 .2 m Md NTPs,0 .3 2 p M随机引物 ,IUTaq酶 ,2 0 ng模板 DNA;反应循环数为 45 ,热循环条件为 94°C,1 min;3 7°C,1 min;72°C,1 .5 min;之前为 94°C,5 min;之后为72°C,1 0 min。在筛选的 2 49个随机引物中 ,有 1 8个在 7个品种上都能扩增出 3～ 1 0条比较清晰条带。     

Improvement of single nucleotide polymorphism genotyping by allele-specific PCR using primers modified with an ENA residue

When we placed an ENA residue into primers at the 3' end, or the n-1, n-2, or n-3 position, which included a single nucleotide polymorphism (SNP) site at the 3' end, only primers containing the ENA residue at the n-2 position were read by Taq DNA polymerase for amplification. The use of the ENA primers avoided the generation of undesired short products, which are thought to be derived from primer-dimers. A greater discrimination of the SNP site by these primers containing the ENA residue was observed compared with that of the corresponding unmodified DNA primers that are often used for allele-specific polymerase chain reaction (AS-PCR). This improvement is probably due to the difficulty of incorporating a nucleotide into the mismatched ENA primer by Taq DNA polymerase in the modified primer-template duplex. These results demonstrate that ENA primer-based AS-PCR would enable a rapid and reliable technique for SNP genotyping.     

几种因素对山茶属植物RAPD分析的DNA扩增的影响

多种因素会影响ＲＡＰＤ扩增,本研究试验了引物、Ｍｇ２＋和ｄＮＴＰ的浓度以及Ｔａｑ酶来源对山茶属植物进行ＲＡＰＤ分析的ＤＮＡ扩增的影响。结果表明这些因素对扩增结果都会产生影响,通过比较分析,得到了一个对于山茶属植物进行ＲＡＰＤ分析较理想的扩增条件。     

牛血清白蛋白在植物RAPD分析中的作用

以水杉、七子花DNA为模板,添加牛血清白蛋白（BSA）,观察其对植物RAPD扩增效果的改善情况。研究显示,在水杉及七子花RAPD扩增体系中,改善RAPD扩增反应的最佳的BSA浓度是不同的,分别为06μg/μl与1μg/μl。另外,BSA还可以封闭乙酰BSA对RAPD扩增反应的抑制作用,降低RAPD反应系统中Taq酶的用量。 Abstract:Using Metasequoia glyptostroboides and Heptacodium miconioides DNA as templates,the effect of bovine serum albumin(BSA) on RAPD in plants was studied.The results showed that suitable concentrations of BSA used in Metasequoia glyptostroboides and Heptacodium miconioides RAPD were different,which were 06μg/μl and 1μg/μl,respectively.The inhibition of acetylated BSA on the amplification of plant RAPD could be relieved by BSA.BSA could reduce the dosage of Taq DNA polymerase.     

Optimizing Taq Polymerase Concentration for Improved Signal-to-Noise in the Broad Range Detection of Low Abundance Bacteria

Background

PCR in principle can detect a single target molecule in a reaction mixture. Contaminating bacterial DNA in reagents creates a practical limit on the use of PCR to detect dilute bacterial DNA in environmental or public health samples. The most pernicious source of contamination is microbial DNA in DNA polymerase preparations. Importantly, all commercial Taq polymerase preparations inevitably contain contaminating microbial DNA. Removal of DNA from an enzyme preparation is problematical.

Methodology/Principal Findings

This report demonstrates that the background of contaminating DNA detected by quantitative PCR with broad host range primers can be decreased greater than 10-fold through the simple expedient of Taq enzyme dilution, without altering detection of target microbes in samples. The general method is: For any thermostable polymerase used for high-sensitivity detection, do a dilution series of the polymerase crossed with a dilution series of DNA or bacteria that work well with the test primers. For further work use the concentration of polymerase that gave the least signal in its negative control (H₂O) while also not changing the threshold cycle for dilutions of spiked DNA or bacteria compared to higher concentrations of Taq polymerase.

Conclusions/Significance

It is clear from the studies shown in this report that a straightforward procedure of optimizing the Taq polymerase concentration achieved “treatment-free” attenuation of interference by contaminating bacterial DNA in Taq polymerase preparations. This procedure should facilitate detection and quantification with broad host range primers of a small number of bona fide bacteria (as few as one) in a sample.     

散斑壳属真菌RAPD-PCR反应条件的优化

以分离自四川省二郎山林场云南松上的松针散斑壳菌(Lophodermium pinastri)为材料,提取其总基因组DNA做为RAPD-PCR体系优化的模板。研究了dNTPs、Mg~(2+)、DNA模板、Taq酶、引物等组分对RAPD反应结果的影响,并建立了最佳反应体系:25μL PCR反应体积,10×Taq酶缓冲液2．5μL,1．5 U Taq酶,20 ng DNA模板,0．4 mmol/L dNTPs,4．0 mmol/L Mg~(2+),0．48μmol/L引物,10．2μL ddH_2O。