一种简便快速的制备水稻基因组DNA PCR模板的方法

目的：发展一种简便快速的制备水稻基因组DNA PCR模板的方法。方法：用枪头捣碎水稻叶片代替液氮研磨法提取水稻基因组DNA作PCR模板,在去污剂SDS和表面活性剂TrionX-100的存在下在沸水中煮沸10min,然后取上清扩增微管蛋白（TubA1）基因内含子。结果：发现在利用煮沸法提取水稻基因组DNA的过程中,用枪头捣碎叶片可代替液氮碾磨,加入0.1%表面活性剂TrionX-100煮沸叶片对制备模板有促进效果,得到了预期的PCR片断。结论：该方法快速、简便、经济,具有良好的重复性与特异性,便于自动化。     

大肠杆菌和酵母PCR模板制备的优化

对快速制备大肠杆菌和酵母基因组DNA PCR模板的方法进行了优化。实验证明加入0.1%Triton X-100和0.1%SDS的煮沸法能够明显提高大肠杆菌基因组模板的扩增效率,加入0.1%SDS的煮沸法在提高酿酒酵母基因组模板的扩增效率方面也有类似效果,但加入0．1％Triton X—100的煮沸法对酿酒酵母基因组模板的扩增仅有较小的作用。     

快速制备酵母质粒和基因组DNA PCR模板

发展了一个利用煮沸法快速制备酵母质粒和基因组DNA PCR模板的程序,成功地从低拷贝的ARSCEN酵母质粒和酵母基因组扩增到了相应基因。     

快速制备酵母质粒和基因组DNA PCR模板*

发展了一个利用煮沸法快速制备酵母质粒和基因组DNAPCR模板的程序 ,成功地从低拷贝的ARSCEN酵母质粒和酵母基因组扩增到了相应基因。     

快速制备水稻基因组DNA PCR模板的煮沸法

文章发展了一个采用煮沸法快速制备水稻基因组DNA PCR模板的程序,成功地从水稻基因组扩增到了相应基因。     

烟草碱法提取基因组DNA的改进

为能够快速高效的对大量转基因烟草样品进行DNA提取,对碱法提取烟草组织DNA的方法进行了改进。采用0.01mol/L的Na OH溶液为提取液,破碎转基因烟草叶片组织后无需经过加热煮沸中和等步骤,上清液可直接用作PCR反应的模板。结果表明,0.01-0.1 mol/L之间的Na OH溶液制备的DNA模板均能成功扩增,该方法制备的DNA模板不依赖特殊的反应条件,多种品牌的PCR Mix均能成功进行扩增反应。与传统SDS提取法和试剂盒提取法获得的DNA相比,PCR结果没有明显差异。此提取方法在小麦、高粱、水稻、玉米等作物上也取得了很好的实验效果。通过本方法制备的DNA模板,其PCR扩增的产物可直接用来测序分析。该方法使用仪器少,样品消耗少,快速、简便、成本低,没有交叉污染,能够在短时间内处理大量样品,因此能够对大量的转基因烟草样品进行DNA的快速提取和鉴定。     

一种快速高效获取丝状真菌PCR反应模板的方法

建立一种快速高效获取丝状真菌PCR反应模板的方法,提高丝状真菌PCR鉴定效率。通过单因素法对机械破壁联合微波法进行条件优化,利用优化后的方法获取13株不同种属丝状真菌的PCR反应模板,同时与Chelex-100法、机械破壁法作对比,以试剂盒抽提法作为阳性对照,进行ITS序列扩增,琼脂糖凝胶电泳检测扩增结果。机械破壁联合微波法获取丝状真菌PCR反应模板的最佳条件为40 Hz机械破壁1 min、微波700 W高温裂解3 min,采取该法与试剂盒抽提法获得的模板均成功扩增13株不同种属丝状真菌ITS序列,且PCR鉴定结果一致;Chelex-100法获得的模板成功扩增6株丝状真菌ITS序列;机械破壁法获得的模板虽成功扩增9株丝状真菌ITS序列,但扩增效果欠佳。机械破壁联合微波法能够有效获取丝状真菌PCR反应模板,与试剂盒抽提法相比具有操作简便、快速高效的优点,提高丝状真菌PCR鉴定效率。     

一种简单高效的酵母单菌落 PCR 方法

目的:为快速简便地挑选出酿酒酵母重组克隆,探索建立一种经济、直接、高效的酵母单菌落 PCR 方法.方法:以 Leu2MX6基同重组或重组质粒转化得到的酵母突变菌为材料,分别采用传统的提取基组或质粒的方法、煮沸法及化学试剂处理法等制备 PCR 模板进行重组克隆鉴定,并对6种 PCR 模板制备方法的效果进行比较与分析;对加热提取法进行优化并进行重组子的提取和验证.结果与结论:直接以1 mm2单克隆菌株95℃处理5 min 后的酵母菌落水悬浮液为模板进行单菌落 PCR,是一种简单高效的酵母重组克隆鉴定方法.该方法能弥补传统方法的不足,且简便快速、结果稳定,可作为筛选和鉴定阳性克隆的有效手段.同时,这种单菌落 PCR 法也可应用重组毕赤酵母的阳性克隆筛选.     

GISH中杂交鲷亲本封阻DNA不同制备方法的效果

目的:基因组荧光原位杂交(GISH)作为一种细胞遗传学的研究方法,以其特定的优点被越来越广泛的应用于杂种染色体分析、染色体行为考察等方面。采用适当的封阻DNA制备方法得到合适的封阻DNA从而使得在基因组原位杂交中大大提高杂交效率,更能突显GISH方法的优势。方法:采用煮沸法和超声波破碎法对杂交鲷亲本真鲷(♀)、黑鲷(♂)DNA进行剪切研究了两种鲷类封阻DNA的制备。结果:煮沸15 min时DNA已被切断。煮沸70 min以后,DNA片段更加集中,主要分布在500bp左右。煮沸90 min或者煮沸120 min以后发现,DNA电泳条带主要分布于250 bp附近,已达到GISH所需封阻DNA片段大小的要求。结论:煮沸法对基因组DNA的剪切,与超声波清洗仪剪切DNA相比,具有更高的效率。研究结果为基因组荧光原位杂交的顺利进行提供了条件。     

应用RD-PCR技术制备HIV基因芯片探针

利用限制性显示 (RD PCR)技术快速分离HIV 1基因片段制备DNA芯片探针 .以Sau3AⅠ酶切HIV基因 ,得到许多大小适合芯片的限制性酶切片段 .然后在片段两端接上接头 ,根据酶切位点、接头的序列设计通用引物 .在该通用引物的 3′端分别延伸一个碱基后 ,通过引物间的两两组合 ,将PCR反应分成 10个亚组 .纯化各组PCR产物 ,克隆到T载体上 .阳性克隆经鉴定、扩大培养后提取质粒 .以质粒为模板扩增靶片段并进行序列分析 .每个亚型得到了十几个 10 0～ 10 0 0bp的HIV基因片段 .研究表明 ,RD PCR技术是一种有效的快速制备基因芯片探针的方法     

Plasmid analysis and antimicrobial susceptibilities of Peptostreptococcus species

Abstract There are no published methods on plasmid isolation from Peptostreptococcus spp., therefore two methods of plasmid isolation from this genera were analysed: the boiling and alkaline-SDS methods. Plasmid DNA was not recovered by the boiling method, however, with the alkaline-SDS method, cryptic plasmid DNA was detected in two P. asaccharolyticus and one P. magnus strains. To achieve optimum lysis, Peptostreptococcus cells were treated with lysozyme (2 mg/ml) for 15 min. at 37°C followed by proteinase K (0.2 mg/ml) for 1 h at 37°C. In addition we report, the occurence of clindamycin or metronidazole-resistant peptostreptococci, but these phenotypes were not correlated with plasmid carriage.     

Rapid Immunocytochemistry with Simple Heat-Induced Antigen Retrieval Technique for Improvement in the Quality of Cytological Diagnosis

Rapid immunocytochemistry (ICC) can improve the accuracy of intraoperative cytological diagnoses; however, it is usually applied without heat-induced antigen retrieval (HIAR). We established a HIAR method for rapid ICC and evaluated its efficacy and reliability. Rapidly fixed smear samples were immunostained using 35 antibodies. We compared the results of HIAR by boiling in a pot or heating in an electric kettle. The smears were incubated for 3 min with each primary antibody and immuno-enzyme polymer reagent, and for 1 min with diaminobenzidine solution. HIAR for 1 min using the kettle method yielded the best cellular integrity. For 32 out of the 35 antibodies, results achieved using rapid ICC within 11 min were comparable to that achieved using standard ICC. HIAR was essential for 13 antibodies. For two of the antibodies, HIAR was not required when standard ICC was applied, but consistent staining with rapid ICC was obtained only with HIAR. In conclusion, we established a rapid ICC procedure using a simple HIAR method, which allowed efficient immunostaining of a panel of antigens, including nuclear antigens, within only 11 min. The combined use of this rapid ICC technique with other staining techniques could be useful for improving intraoperative cytological diagnoses.     

Identification of 3- and 4-repeat tau isoforms within the PHF in Alzheimer's disease.

The microtubule associated protein tau is incorporated into the pronase resistant core of the paired helical filament (PHF) in such a way that the repeat region is protected from proteases, but can be released as a major 12 kDa species from the PHF core by formic acid treatment and by boiling in SDS. This fragment retains the ability to aggregate in the presence of SDS. Detailed sequence analysis of the 12 kDa species shows that it consists of a mixture of peptides derived from the repeat region of 3- and 4-repeat tau isoforms comigrating as a single electrophoretic band. However, the 4-repeat isoforms released from the core lack either the first or the last repeat. The pronase-protected region of tau within the PHF core is therefore restricted to three repeats, regardless of isoform. The alignment of cleavage sites at homologous positions within tandem repeats after protease treatment indicates that the tau-core association is precisely constrained by the tandem repeat structure of the tau molecule.     

锰——超氧化物歧化酶活力测定的五种方法比较研究

 本文分别以CN~-抑制和SDS处理区分Mn-SOD与CuZn-SOD,对五种SOD活力测定方法进行了比较研究。结果表明:(1)化学发光法和光化学扩增法不适用于Mn-SOD活力测定,CN~-和SDS对这两种方法有明显的干扰作用。(2)NBT还原、Cyt c还原和亚硝酸盐形成法都能用于Mn-SOD活力测定,用这三种方法测得Mn-SOD每活力单位相当于酶的含量分别为2.93μg、0.11μg和0.028μg。说明NBT还原法灵敏度最低,其次是Cyt c还原法。亚硝酸盐形成法灵敏度高,专一性强,为五种测定方法之首。     

Affinity purification of plasmid DNA by temperature-triggered precipitation

This protocol presents a new method to purify plasmid DNA using temperature-triggered precipitation. The principle is based on the specific DNA-binding affinity of a bacterial metalloregulatory (MerR) protein to its cognate DNA sequence and the temperature responsiveness of elastin-like protein (ELP). A bifunctional ELP-MerR fusion protein is created to enable the precipitation of plasmid DNA, designed to contain the MerR recognition sequence, by a simple temperature trigger. The protocol covers all stages of the process from the design of ELP-MerR fusion proteins and MerR-binding plasmids, to the isolation of plasmid DNA from Escherichia coli cultures after boiling lysis, the subsequent temperature-triggered precipitation of plasmid DNA-fusion protein complexes and final elution of plasmid DNA by mild heating. This protocol is well suited to laboratory research-scale applications, producing plasmid DNA of better purity and similar yield as one of the most commonly used laboratory methods, standard alkaline lysis (known as the midiprep procedure). The protocol takes approximately 30 min to obtain pure plasmid DNA from cell cultures using the temperature-triggered precipitation method.     

侧孢芽孢杆菌质粒提取方法的探究

以能够降解有机磷农药的两株侧孢芽孢杆菌BL-21和BL-22为研究对象,分别采用碱裂解法、试剂盒提取法和SDS法对侧孢芽孢杆菌BL-21和BL-22的质粒进行提取,并通过凝胶电泳和紫外分光光度法对提取结果进行分析,试验结果证明,适合侧孢芽孢杆菌BL-21和BL-22的质粒提取方法是SDS裂解法,该方法提取的质粒大小为10kb,且该方法提取的结果稳定,质粒的产量和质量均符合分子生物学实验的要求。     

煮沸裂解法和试剂盒法提取浸矿菌基因组DNA的比较

目的:在生物浸出中,微生物群落结构分析有着重要意义,而群落分析的基础是提取纯度高、损失少的基因组DNA。为了解决这一问题,本实验通过比较两种较常用的DNA提取方法,煮沸裂解法和试剂盒法,寻找一种灵敏、快速、经济实用的制备浸矿细菌基因组DNA的方法。方法:分别用煮沸裂解法和试剂盒法提取6种浸矿菌的基因组DNA,从所提取的基因组DNA浓度、纯度、回收率和对PCR扩增反应的影响方面比较了两种方法的提取效果;用两种方法来处理不同浓度梯度的一种菌,通过实时定量PCR来比较两种方法的灵敏性。结果:相同处理量(108个)的革兰氏阳性菌(1株)、革兰氏阴性菌(4株)、古菌(1株)经两种方法提取的基因组DNA差异较大,煮沸裂解法所得的6组基因组DNA更纯,其OD260/OD280的值更接近1.8-2.0(纯DNA的OD260/OD280在1.8-2.0之间),前者所提DNA回收率最大可达后者的16.7倍;煮沸裂解法只需较少菌(102个)便能让实时定量PCR检测到所提DNA模板浓度,比试剂盒法灵敏。结论:两种方法提取的基因组DNA均可用于后续的PCR扩增,此外,前者提取的DNA浓度随细菌浓度增加而呈线性增大,而后者随菌浓度增大,所提DNA量增加有限,因此,在生物浸出中微生物基因组DNA的提取可直接采用简单快速的煮沸提取法,为实验节约成本和时间。     

煮沸裂解法和试剂盒法提取浸矿菌基因组DNA的比较

目的：在生物浸出中,微生物群落结构分析有着重要意义,而群落分析的基础是提取纯度高、损失少的基因组DNA。为了解决这一问题,本实验通过比较两种较常用的DNA提取方法,煮沸裂解法和试剂盒法,寻找一种灵敏、快速、经济实用的制备浸矿细菌基因组DNA的方法。方法：分别用煮沸裂解法和试剂盒法提取6种浸矿菌的基因组DNA,从所提取的基因组DNA浓度、纯度、回收率和对PCR扩增反应的影响方面比较了两种方法的提取效果;用两种方法来处理不同浓度梯度的一种菌,通过实时定量PCR来比较两种方法的灵敏性。结果：相同处理量（108个）的革兰氏阳性菌（1株）、革兰氏阴性菌（4株）、古菌（1株）经两种方法提取的基因组DNA差异较大,煮沸裂解法所得的6组基因组DNA更纯,其OD260／OD280的值更接近1．8-2．0（纯DNA的OD260／OD280在1．8—2．0之间）,前者所提DNA回收率最大可达后者的16．7倍;煮沸裂解法只需较少菌（102个）便能让实时定量PCR检测到所提DNA模板浓度,比试剂盒法灵敏。结论：两种方法提取的基因组DNA均可用于后续的PCR扩增,此外,前者提取的DNA浓度随细菌浓度增加而呈线性增大,而后者随茵浓度增大,所提DNA量增加有限,因此,在生物浸出中微生物基因组DNA的提取可直接采用简单快速的煮沸提取法,为实验节约成本和时间。