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PCR amplification of DNA microdissected from a single polytene chromosome band: a comparison with conventional microcloning.

机译：从单个多染色体染色体条带上显微切割的DNA的PCR扩增：与常规微克隆的比较。

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摘要

A novel alternative to microcloning for the production of region specific chromosomal DNA is described. In this method, 'microamplification', single bands are dissected from polytene chromosomes and digested with Sau3A. Oligonucleotide adaptors are ligated to these fragments to provide convenient priming sites for polymerase chain reaction amplification. In this way, as much as 1 microgram of DNA can be amplified from a single band. Probes made from PCR amplified DNA from two such dissections have been used to probe cloned DNA form a 100 kb chromosome walk. Whereas conventional microcloning has generated cloned EcoRI fragments corresponding to 3-4 kb of the walk, the PCR probes cover greater than 90% of this chromosomal region. Thus microamplification is significantly more effective than microcloning in providing probes for establishing chromosomal walks.

机译：描述了用于产生区域特异性染色体DNA的微克隆的新型替代方法。在这种方法中，“微扩增”是从聚乙烯染色体上切出单条带，并用Sau3A消化。将寡核苷酸衔接子连接至这些片段，以提供用于聚合酶链反应扩增的方便的引发位点。以此方式，可从单个条带扩增多达1微克的DNA。由来自两个此类解剖结构的PCR扩增DNA制成的探针已用于探针从100 kb染色体步移中克隆出的DNA。常规的微克隆已产生了对应于步行3-4 kb的克隆EcoRI片段，而PCR探针覆盖了该染色体区域的90％以上。因此，微扩增在提供用于建立染色体步移的探针方面比微克隆显着更有效。

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作者
Saunders, R D; Glover, D M; Ashburner, M; Siden-Kiamos, I; Louis, C; Monastirioti, M; Savakis, C; Kafatos, F;
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年度 1989
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正文语种 en
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专利

1. PCR amplification of DNA microdissected from a single polytene chromosome band: a comparison with conventional microcloning [J] . Charalambos Savakis, Christos Louis, David M. Glover, Nucleic acids research . 1989,第22期

机译：从单个多染色体染色体条带上显微切割的DNA的PCR扩增：与常规微克隆的比较
2. Comparison of Chironomus usenicus and Chironomus curabilis with species of the group plumosus (Diptera) inferred from the mitochondrial DNA Gene COI and by the polytene chromosomes banding pattern [J] . Polukonova NV, Djomin AG, Mugue NS, Russian journal of genetics . 2009,第8期

机译：用线粒体DNA基因COI和多态性染色体条带图谱推论的Useronus chinicomus usenicus和Chironomus curabilis与plumosus（Diptera）物种的比较
3. Comparison of DNA Extraction Methods Between Conventional, Kit, Alkali and Buffer-Only for PCR Amplification on Raw and Boiled Bovine and Porcine Meat [J] . Arif Yahya, Marindra Firmansyah, Annisa Arlisyah, Journal of Experimental Life Science . 2017,第2期

机译：常规，试剂盒，碱和仅缓冲液之间DNA提取方法的比较，用于生，煮牛和猪肉的PCR扩增
4. Amplification of Y-chromosome Specific DNA Sequence of Sheep and Goat by PCR [C] . International symposium on bioanalytical chemistry . 1995

机译：绵羊和山羊的Y-染色体特异性DNA序列的扩增PCR
5. Optimization and validation of the Bode Buccal DNA Collector with the AmpFLSTR Identifiler Direct PCR Amplification Kit for single-source reference samples. [D] . DeLillo, Sandy. 2010

机译：使用AmpFLSTR标识符直接PCR扩增试剂盒对Bode颊部DNA收集器进行优化和验证，用于单源参考样品。
6. PCR amplification of DNA microdissected from a single polytene chromosome band: a comparison with conventional microcloning. [O] . R D Saunders, D M Glover, M Ashburner, 1989

机译：从单个多染色体染色体条带上显微切割的DNA的PCR扩增：与常规微克隆的比较。
7. PCR amplification of microdissected wheat chromosome arms in a simple 'single tube' reaction [O] . Diego Albani, Marie-Jose Cote, Ken C. Armstrong, 1993

机译：PCR扩增微小物质染色体臂的简单“单管”反应
8. Quantitation of DNA for Forensic DNA Typing by qPCR (quantitative PCR): Singleplex and Multiplex Modes for Nuclear and Mitochondrial Genomes, and the Y Chromosome [R] . Timken, M. D., Swango, K. L., Orrego, C., 2005

机译：通过qpCR（定量pCR）进行法医DNa分型的DNa定量：核和线粒体基因组的单重和多重模式，以及Y染色体

PCR amplification of DNA microdissected from a single polytene chromosome band: a comparison with conventional microcloning.

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