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1.
This article describes the direct sequencing of PCR-amplified DNA, a technique that bypasses the problem of replication errors sometimes associated with other PCR procedures. The direct sequencing procedure produces an “average sequence” of all the copies of the target. Any miscopied molecule usually represents only a small proportion of the total. The technique described here is based on the “traditional” ddNTP sequencing method of Sanger et al. 相似文献
2.
Thermal cycle dideoxy DNA sequencing 总被引:1,自引:0,他引:1
Barton E. Slatko 《Molecular biotechnology》1996,6(3):311-322
Thermal cycle dideoxy DNA sequencing eliminates the requirements for independent primer annealing and double-stranded DNA
denaturation steps. The method enables sequencing from nanogram amounts of DNA from double-stranded and single-stranded PCR
products, and plasmid or phage DNA templates. Thermal cycle sequencing also enables direct sequencing from bacterial colonies
or phage plaques. Protocols using the Vent exo− DNA polymerase, helpful suggestions, and a troubleshooting guide are also presented. 相似文献
3.
4.
Taq DNA聚合酶具有反应速度快、温度作用范围广及良好的续进性等特点,可视为一种理想的DNA顺序分析酶。本文首先对非对称性PCR扩增过程中单、双链DNA产物的积累情况进行了分析,然后采用标记延伸二步法,对Taq DNA聚合酶的性质及影响因素进行分析。为进一步改进Taq DNA聚合酶测序的方法,本反应建立了“Klenow-型”的直接掺入标记同位素测序法,即在反应液中加入与标记核苷酸相应的一定浓度的冷dNTP。此法不但解决了二步法中引物后部分DNA顺序无法读出的缺点,而且简化了反应步骤,亦能得到令人满意的顺序分析结果,每次可读出至少400碱基的序列。 相似文献
5.
We describe here methods and strategies for amplifying and sequencing the genes encoding the small subunits (16/18S) of nuclear
and chloroplast ribosomal DNA (rDNA) from total plant DNA. These methods were developed in response to technical difficulties
we encountered in our molecular systematic work with members of various plant families. These protocols have proved useful
when the amount of tissue available for study is limited and when the tissues have high concentrations of undesirable secondary
metabolites which are often co-isolated with nucleic acids. 相似文献
6.
We have developed a polymerase chain reaction (PCR) method for sequencing of tobacco chloroplast genome. In a mixture containing chloroplast DNA, 5-end-labeled oligonucleotide primer, Taq DNA polymerase and reaction buffer, we were able to sequence a segment of chloroplast 16S rRNA gene. The results showed that the 750 bp of DNA sequenced were identical to the sequence reported, indicating that direct sequencing method that we have developed is useful for the sequencing of chloroplast genome. To analyze the chloroplast genome more rapidly in those in vitro grown plantlets, we also developed a simple method which is applicable for the amplifications and sequencing of chloroplast 16S rRNA fragment from either 0.15 g of tobacco leaf or stem tissue. The readable sequences obtained from the presented methods were consistent with the published sequence. 相似文献
7.
David Needleman Debbie Adam Michelle Detwiler Helaman Escobar Jan Kieleczawa Rashmi Pershard Peter Schweitzer Glenis Wiebe 《Journal of biomolecular techniques》2007,18(2):113-119
Over the past few years, technological advances in automated DNA sequencing have had a profound effect on the nature of DNA sequencing laboratories. To characterize the changes occurring within DNA sequencing facilities, the DNA Sequencing Research Group conducted three previous studies, in 1998, 2000, and 2003. A new general survey has been designed and conducted by the DSRG to capture the current status of DNA sequencing facilities in all sectors. Included were questions regarding facility administration, pricing, instrumentation, technology, protocols, and operation. The results of the survey are presented here, accompanied by comparisons to the previous surveys. These comparisons formed a basis for the discussion of trends within the facilities in response to the dynamics of a changing technology. 相似文献
8.
DNA coding for the 16S rRNA of an intracellular bacterium was directly amplified from lysed cells of a host amoebae using the polymerase chain reaction and primers specific for eubacteria. The amoebae had been used to recover an uncultured bacterium observed in the sputum of a patient with pneumonia. The amplified DNA was sequenced directly and compared with published 16S rRNA sequences. The analysis revealed that the intracellular bacterium is a member of the genus Legionella and that it is different from species, including L. pneumophila, for which 16S ribosomal RNA sequence data are available. 相似文献
9.
Identification and authentication of animal cell culture by polymerase chain reaction amplification and DNA sequencing 总被引:1,自引:0,他引:1
Liu MY Lin SC Liu H Candal F Vafai A 《In vitro cellular & developmental biology. Animal》2003,39(10):424-427
Polymerase chain reaction (PCR) amplification and deoxyribonucleic acid (DNA) sequence analysis were used to identify the species origin of cell lines used in a cell culture facility where various cell lines of different species are routinely propagated. The aldolase gene family was selected for PCR amplification because the DNA sequences of this gene are highly conserved over a wide range of animals and humans. A total of 36 cell lines representing 13 different species were selected for this study. The DNA from each cell line was amplified, and PCR products were analyzed by agarose gel electrophoresis. The results showed unique profiles of amplified bands on agarose gels that allowed differentiation among non-closely related species. However, DNA amplification of closely related species, including rat and mouse or human and primate, resulted in similar and indistinguishable banding patterns that could be further differentiated by DNA sequence analysis. These results suggested that aldolase gene amplification coupled with DNA sequence analysis is a useful tool for identification of cell lines and has potential application for use in identification of interspecies cross-contamination. 相似文献
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11.
The treatment of DNA with bisulfite, which converts C to U but leaves 5-methyl-C unchanged, forms the basis of many analytical techniques for DNA methylation analysis. Many techniques exist for measuring the methylation state of a single CpG but, for analysis of an entire region, cloning and sequencing remains the gold standard. However, biases in polymerase chain reaction (PCR) amplification and in cloning can skew the results. We hypothesized that single-molecule PCR (smPCR) amplification would eliminate the PCR amplification bias because competition between templates that amplify at different efficiencies no longer exists. The amplified products can be sequenced directly, thus eliminating cloning bias. We demonstrated this accurate and unbiased approach by analyzing a sample that was expected to contain a 50:50 ratio of methylated to unmethylated molecules: a region of the X-linked FMR1 gene from a human female cell line. We compared traditional cloning and sequencing to smPCR and sequencing. Sequencing smPCR products gave an expected methylated to unmethylated ratio of 48:52, whereas conventional cloning and sequencing gave a biased ratio of 72:28. Our results show that smPCR sequencing can eliminate both PCR and cloning bias and represents an attractive approach to bisulfite sequencing. 相似文献
12.
Wen L 《Molecular biotechnology》2001,17(2):135-142
The use of automated fluorescent DNA sequencer systems and PCR-based DNA sequencing methods plays an important role in the
actual effort to improve the efficiency of large-scale DNA analysis. While dideoxy-terminators labeled with energy-transfer
dyes (BigDyes) provide the most versatile method of automated DNA sequencing, premature terminations result in a substantially
reduced reading length of the DNA sequence. Premature terminations are usually evidenced by base ambiguities and are often
accompanied by diminished signal intensity from that point on in the sequence. I studied a two-step protocol for Taq cycle
sequencing using the ABI BigDye terminator for reducing premature terminations in DNA sequences. I demonstrate that combining
the annealing step with the extension step at one temperature (60°C) reduces premature terminations in DNA sequences that
regularly contain premature terminations when the three temperature steps are used. This modification significantly increases
the number of accurately read bases in DNA sequences. 相似文献
13.
We surveyed exemplars from all 12 infrageneric taxa ofRibes (Grossulariaceae) for restriction site variation in two cpDNA regions, fromrbcL toaccD and fromrpoC1 torpoC2, in order to develop an explicit phylogenetic hypothesis and to assess the validity of infrageneric classifications. Maximum parsimony analysis resolves sect.Ribes (red currants), sect.Berisia (European alpine currants), sect.Symphocalyx (golden currants), sect.Grossularia plus sect.Grossularioides (true gooseberries and spiny currants), andHesperia, Lobbia, and probably sect.Robsonia (west North American gooseberries) as well-supported monophyletic groups. The clade of sectionsGrossularioides andGrossularia is unexpected, and suggests that subgenusGrossularia is not monophyletic. Alternatively, sect.Grossularioides may have acquired its cpDNA via hybridization and introgression. SectionsCoreosma (black currants) andHeritiera (dwarf currants) are apparently non monophyletic. Relationships among the well-supported lineages and the other sampled taxa remain unresolved. Maximum likelihood analysis is consistent with the parsimony results. 相似文献
14.
The purpose of this study was to sequence the central part of the coding region of the Clostridium tyrobutyricum fiagellin gene to improve the immunoenzymatic counting of cells after milk filtration. The coding region was amplified by PCR, and the amplified products were cloned. A DNA sequence analysis of positive clones gave us 1,131 nucleotides with a partial calculated flagellin molecular mass of 40,143 Da. The flagellar filament protein sequence exhibited high levels of homology to sequences of flagellin protein from other bacteria in both N- and C-terminal parts, but little homology in the central domain. A PCR-restriction fragment length polymorphism analysis of amplified C. tyrobutyricum flagellin gene products confirmed the variability of the central domain. The flagellin mRNA was determined to be 1.1 kb in size, which suggests a monocistronic mRNA. Furthermore, the deduced protein flagellin contains eleven potential N-glycosylation sites and one sequence rich in serine, which could be modified by O-glycosylation. 相似文献
15.
DNA microarray and next-generation DNA sequencing technologies are important tools for high-throughput genome research, in
revealing both the structural and functional characteristics of genomes. In the past decade the DNA microarray technologies
have been widely applied in the studies of functional genomics, systems biology and pharmacogenomics. The next-generation
DNA sequencing method was first introduced by the 454 Company in 2003, immediately followed by the establishment of the Solexa
and Solid techniques by other biotech companies. Though it has not been long since the first emergence of this technology,
with the fast and impressive improvement, the application of this technology has extended to almost all fields of genomics
research, as a rival challenging the existing DNA microarray technology. This paper briefly reviews the working principles
of these two technologies as well as their application and perspectives in genome research.
Supported by the National High-Tech Research Program of China (Grant No.2006AA020704) and Shanghai Science and Technology
Commission (Grant No. 05DZ22201) 相似文献
16.
A label-free method for DNA sequencing based on the principle of the Millikan oil drop experiment was developed. This sequencing-by-synthesis approach sensed increases in bead charge as nucleotides were added by a polymerase to DNA templates attached to beads. The balance between an electrical force, which was dependent on the number of nucleotide charges on a bead, and opposing hydrodynamic drag and restoring tether forces resulted in a bead velocity that was a function of the number of nucleotides attached to the bead. The velocity of beads tethered via a polymer to a microfluidic channel and subjected to an oscillating electric field was measured using dark-field microscopy and used to determine how many nucleotides were incorporated during each sequencing-by-synthesis cycle. Increases in bead velocity of approximately 1% were reliably detected during DNA polymerization, allowing for sequencing of short DNA templates. The method could lead to a low-cost, high-throughput sequencing platform that could enable routine sequencing in medical applications. 相似文献
17.
P. Barbier H. Morishima A. Ishihama 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1991,81(5):693-702
Summary The phylogenetic relationships between Asian wild rice strains were analyzed by direct sequencing of PCR-amplified DNA fragments. The sequence of three introns located in the phytochrome gene was determined for eight strains of the Asian wild rice, Oryza rufipogon, and one strain of the related African species, Oryza longistaminata. The number of nucleotide substitutions per site between various strains within a single species, O. rufipogon, ranged between 0.0017 and 0.0050, while those between two related species, O. rufipogon and O. longistaminate, were 0.043–0.049 (23–26 within 532 bp). Taken together with the sequence differences of the 10-kDa prolamin gene, a model is proposed for the phylogenetic relationships and evolutionary history of annuals and perennials within O. rufipogon. 相似文献
18.
Napier stunt phytoplasma (16SrXI and 16SrIII) in eastern Africa is a serious threat to the expansion of Napier grass (Pennisetum purpureum) farming in the region, where it is widely cultivated as fodder in zero grazing livestock systems. The grass has high potential for bio-fuel production, and has been adopted by farmers as a countermeasure to cereal stem borer Lepidoptera, since it attracts and traps the insect. Diagnosis of stunt phytoplasma have been largely by nested polymerase chain reaction (nPCR) targeting the 16S rRNA gene. However, the method is laborious, costly and technically demanding. This investigation has developed a simpler but effective phytoplasma diagnostic tool, called; loop-mediated isothermal amplification of DNA (LAMP). The assay was tested on 8 symptomatic and 8 asymptomatic plants, while its detection limit was compared to nested PCR using samples serially diluted from 3 ng/μl to 0.38 pg/μl. Molecular typing of LAMP products was determined by BsrI restriction digestion and Southern blot analysis. The assay sensitivity, positive and negative predictive values were estimated, while the specificity was tested on 11 phytoplasma groups. LAMP was specific to 5 phytoplasma groups: 16SrVI, X, XI and XVI. BsrI restriction digestion produced two predicted fragments, and there was specific binding of probe DNA to the LAMP amplicons in Southern blot analysis. The assay sensitivity was 100%, while the positive and negative predictive values were 63 and 100% respectively. LAMP was 20-fold more sensitive than nested PCR. This study validates LAMP for routine diagnosis of Napier stunt and other closely related phytoplasmas. 相似文献
19.
锌指基因是一种造血调节基因,编码锌指结构蛋白,主要在髓细胞中表达,促进髓细胞分化,在急性早幼粒白血病维甲酸治疗中,促使病情缓解。本文报道了我们从基因分子上研究锌指基因作用中,探索并建立了单向聚合酶链反应(PCR)扩增特定单链DNA,直接测序的新方法。它能产生质和量均佳的单链DNA,无需纯化即可直接用于测序,使复杂的测序研究简便易行,可在2,3天内完成。这种单向PCR扩增特定单链DNA直接测序的方法,经对锌指基因的cDNA测序,得到验证。此法不仅适用于疾病研究中的DNA测序,还可制各单链DNA探针,更利于基因结构组成的研究。 相似文献
20.
Fabian Ripp Christopher Felix Krombholz Yongchao Liu Mathias Weber Anne Sch?fer Bertil Schmidt Rene K?ppel Thomas Hankeln 《BMC genomics》2014,15(1)