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Titlebook: Clinical Applications of PCR; Y. M. Dennis Lo Book 1998 Humana Press 1998

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Long Range PCRThe . polymerase lacks proofreading properties (.) and thus is unable to correct such misincorporations. The higher extension K. value for a misincorporated nucleotide is thought to cause detachment of the . polymerase from template DNA.
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Sequencing of PCR ProductsIt is often necessary to obtain DNA sequence information following successful amplification. Although polymerase chain reaction (PCR) products may be cloned into a vector and sequenced at a later stage, it is often preferable to sequence PCR products directly, without subcloning, and it is this approach that is addressed in this chapter.
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Amplificationtissue specimens. . hybrrdization (ISH) does permit localization of specific nucleic acid sequences at the individual cell level. In conventional nonisotopic . (IS) detection systems, most protocols do not detect single copy genes, except for those incorporating elaborate sandwich detection techniques as described by Herrington et al. (.).
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PCR Analysis of CD44 Variants in Tumorshain disulfide bonds. It is essentially composed of a 37-kDa protein core highly glycosylated by .- and .-linked sugars to form an 85–90-kDa product and is sometimes additionally linked to chondroitin sulfate side chains to produce a 180–220 kDa form on sodium dodecyl sulfate (SDS) gels (.,.).
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