Patent ID: 7202022

Claim:
A method for sequence-specific identification, separation, and quantitation of an amplified subset of restriction fragments in a population of restriction fragments, the method comprising: (a) reverse transcribing an RNA population to provide a double-stranded cDNA population; (b) digesting said cDNA population with one or more restriction endonucleases having a degenerate recognition or cleavage sequence, wherein said restriction endonuclease is a three- to eight-base cutter and wherein the degenerate recognition or cleavage sequence is represented by the formula N m , where N is the extent of degeneracy, and m is the number of degenerate bases, and wherein for at least one of said restriction endonucleases N is 2–4 and m is 1–5, to produce restriction fragments having N m different single-stranded overhangs for each restriction endonuclease; (c) ligating said restriction fragments to a series of adapters lacking restriction endonuclease sites, each adapter having a sequence complementary to one of said N m different single-stranded overhangs such that restriction fragments having identical overhangs are ligated to the same adapter, wherein each ligating reaction is performed with one adapter of said series of adaptors and said one adapter can be ligated to only a subset of said N m different single-stranded overhangs on said restriction fragments; (d) amplifying said subset of said restriction fragments for no more than 25 cycles with a primer comprising a detectable label, wherein said primer is designed to amplify only those restriction fragments to which said one adapter of said series of adapters has been ligated, and wherein the amplifying for no more than 25 cycles produces an amplified subset of restriction fragments that are linearly representative of the RNA population; and (e) detecting and quantifying said amplified subset of restriction fragments.