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Titlebook: Basic Cloning Procedures; Valdis Berzins Book 1998 Springer-Verlag Berlin Heidelberg 1998 DNA.RNA.gene.nucleic acid.protein.protein synthe

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PCR-Based Site-Specific Mutagenesis,on of DNA for different needs to be made more rapidly and easily than was previously possible. In the course of mutagenesis the relevant sequence changes can be introduced more readily by chemically synthesized oligonucleotide primers than by manipulating DNA fragments with restriction and ligation enzymes.
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Immunological Methods for Analysis of Recombinant Proteins,translational products of cloned genes can be used. Selected clones could be chosen for further studies such as determination of their primary structure by DNA sequencing and for characterization of an appropriate expressed protein.
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Book 1998interaction, cell-free protein synthesis and product electrophoretic and immunological analysis. Each protocol includes short background information, a detailed description of the necessary materials, step-by-step procedures, a troubleshooting guide and useful practical hints.
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Adornos ambivalente Heine-Rezeptionalysis and in situ hybridization. Another important application of RNA templates is the construction of representa­tive cDNA libraries in order to clone genes, to investigate their molecular structure and to express them in prokaryotic and/or eukaryotic cells (Belyaysky 1989).
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Heine’s Flowers in Schumann’s „Myrthen“translational products of cloned genes can be used. Selected clones could be chosen for further studies such as determination of their primary structure by DNA sequencing and for characterization of an appropriate expressed protein.
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Adornos ambivalente Heine-Rezeptionng DNA. Both of these methods depend on analytical polyacrylamide gel electrophoresis to resolve oligonucleotides with one identical end and one end varying in length by a single nucleotide. The enzymatic method has been improved over recent years. The Sanger method was developed as a basic method f
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Zwischen Europa und „Nazionalkatzenjammer“ant DNA technology. Nucleotide changes are necessary not only for the analysis of the structural basis of gene and corresponding protein function, but also for the generation of novel gene products. The availability of the polymerase chain reaction (PCR) in the last decade has enabled the modificati
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Zwischen Europa und „Nazionalkatzenjammer“ication, recombination and DNA condensation in chromatin are steered by binding of regulatory protein ligands to specific sites in DNA. Numerous methods have been developed to study protein-DNA interactions. In this chapter we discuss two widely used and straightforward approaches to address this pr
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