Titlebook: Genetic Recombination; Reviews and Protocol Alan S. Waldman Book 2004 Humana Press 2004

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書(shū)目名稱Genetic Recombination影響因子(影響力)

書(shū)目名稱Genetic Recombination影響因子(影響力)學(xué)科排名

書(shū)目名稱Genetic Recombination網(wǎng)絡(luò)公開(kāi)度

書(shū)目名稱Genetic Recombination網(wǎng)絡(luò)公開(kāi)度學(xué)科排名

書(shū)目名稱Genetic Recombination被引頻次

書(shū)目名稱Genetic Recombination被引頻次學(xué)科排名

書(shū)目名稱Genetic Recombination年度引用

書(shū)目名稱Genetic Recombination年度引用學(xué)科排名

書(shū)目名稱Genetic Recombination讀者反饋

書(shū)目名稱Genetic Recombination讀者反饋學(xué)科排名

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Detecting Carcinogens With the Yeast DEL Assayaddition to the arsenal of predictive tests for genotoxicity and carcinogenicity. This chapter provides an in-depth description of materials and methods for the yeast DEL assay from a user’s prospective and should allow the assay to be successfully deployed in any laboratory with basic microbiological capability and minimal user training.

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Chromatin Immunoprecipitation to Investigate Protein-DNA Interactions During Genetic Recombination the protein. Polymerase chain reaction (PCR) is then used to determine the relative amounts of DNA associated with the protein of interest throughout the recombination event. This in vivo chemical crosslinking technique can be used to localize proteins to both double-strand breaks and recombination intermediates.

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Barriers to Change and Hope for the Future,cribe a protocol for increasing the frequency of TNE in the true yeast, ., through the use of nonspecific, carrier oligonucleotides. These molecules, when added to the reaction, increase the TNE frequency up to 25-fold in some cases, perhaps by providing a molecular trap to bind factors, which may inactivate the specific targeting oligos.

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https://doi.org/10.1007/978-94-6351-029-5ealing of partially complementary oligonucleotides; and (2) a true recombination intermediate structure formed by RecA protein-mediated strand exchange. The use of these substrates in assays designed to detect Holliday junction branch migration and resolution activities is described.

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DNA Fragment Transplacement in ,tions of transformation efficiency, length of homology, and alternative target site configuration were assessed. This analysis indicates that several genetic parameters are important for optimizing the efficiency of gene transplacement.

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