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Suppression subtractive hybridization.

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TLDR
In the authors' hands, the SSH technique has enriched over 1000-fold for rare sequences in a single round of subtractive hybridization.
Abstract
Suppression subtractive hybridization (SSH) is a widely used method for separating DNA molecules that distinguish two closely related DNA samples. Two of the main SSH applications are cDNA subtraction and genomic DNA subtraction. To our knowledge, SSH is one of the most powerful and popular methods for generating subtracted cDNA or genomic DNA libraries. It is based primarily on a suppression polymerase chain reaction (PCR) technique (described narrowly in Chapter 3) and combines normalization and subtraction in a single procedure. The normalization step equalizes the abundance of DNA fragments within the target population, and the subtraction step excludes sequences that are common to the populations being compared. This dramatically increases the probability of obtaining low-abundance differentially expressed cDNAs or genomic DNA fragments and simplifies analysis of the subtracted library. SSH technique is applicable to many comparative and functional genetic studies for the identification of disease, developmental, tissuespecific, or other differentially expressed genes, as well as for the recovery of genomic DNA fragments distinguishing the samples under comparison. This chapter provides an insight into SSH practical use and contains detailed protocol for generation of subtracted cDNAs (which is the most frequent SSH application) and differential screening of the resulting subtracted cDNA library. As shown in many examples, the SSH technique may result in over 1000-fold enrichment for rare sequences in a single round of subtractive hybridization. Finally, we discuss the characteristics of cDNA-subtracted libraries, the nature and level of background nondifferentially expressed clones in the libraries, as well as procedure for rapid identification of truly differentially expressed cDNA clones.

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References
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TL;DR: A new method of total RNA isolation by a single extraction with an acid guanidinium thiocyanate-phenol-chloroform mixture is described, providing a pure preparation of undegraded RNA in high yield and can be completed within 4 h.
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A simple and very efficient method for generating cDNA libraries

TL;DR: Using the fully sequenced 1300 nucleotide-long bovine preproenkephalin mRNA, it is established by sequencing that the method yields faithful full-length transcripts.
Journal ArticleDOI

Suppression subtractive hybridization: a method for generating differentially regulated or tissue-specific cDNA probes and libraries

TL;DR: The results suggest that the SSH technique is applicable to many molecular genetic and positional cloning studies for the identification of disease, developmental, tissue-specific, or other differentially expressed genes.
Journal ArticleDOI

Isolation of cDNA clones encoding T cell-specific membrane-associated proteins.

TL;DR: Of 10 distinct cloned DNA copies of mRNAs expressed in T lymphocytes but not in B lymphocytes and associated with membrane-bound polysomes, one hybridizes to a region of the genome that has rearranged in a T- cell lymphoma and several T-cell hybridomas, suggesting that it encodes one chain of the elusive antigen receptor on the surface of T lymphocyte.
Journal ArticleDOI

An improved PCR method for walking in uncloned genomic DNA

TL;DR: Improvements are improved upon the adaptor ligation method by combining 'vectorette PCR' with a newly developed method termed 'suppression PCR' (12), which is based upon adaptors ligated to the ends of DNA fragments generated by digestion of human genomicDNA.
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