WO2017048982A1 - Extincteurs non-fluorescents oligophosphates et leurs utilisations - Google Patents

Extincteurs non-fluorescents oligophosphates et leurs utilisations Download PDF

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WO2017048982A1
WO2017048982A1 PCT/US2016/051976 US2016051976W WO2017048982A1 WO 2017048982 A1 WO2017048982 A1 WO 2017048982A1 US 2016051976 W US2016051976 W US 2016051976W WO 2017048982 A1 WO2017048982 A1 WO 2017048982A1
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nucleic acid
quencher
alkyl
moiety
fluorophore
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Robert Dempcy
Albert Wong
Hans Johansson
Ronald M. Cook
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Biosearch Technologies, Inc.
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    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07FACYCLIC, CARBOCYCLIC OR HETEROCYCLIC COMPOUNDS CONTAINING ELEMENTS OTHER THAN CARBON, HYDROGEN, HALOGEN, OXYGEN, NITROGEN, SULFUR, SELENIUM OR TELLURIUM
    • C07F9/00Compounds containing elements of Groups 5 or 15 of the Periodic Table
    • C07F9/02Phosphorus compounds
    • C07F9/547Heterocyclic compounds, e.g. containing phosphorus as a ring hetero atom
    • C07F9/6558Heterocyclic compounds, e.g. containing phosphorus as a ring hetero atom containing at least two different or differently substituted hetero rings neither condensed among themselves nor condensed with a common carbocyclic ring or ring system
    • C07F9/65583Heterocyclic compounds, e.g. containing phosphorus as a ring hetero atom containing at least two different or differently substituted hetero rings neither condensed among themselves nor condensed with a common carbocyclic ring or ring system each of the hetero rings containing nitrogen as ring hetero atom
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07FACYCLIC, CARBOCYCLIC OR HETEROCYCLIC COMPOUNDS CONTAINING ELEMENTS OTHER THAN CARBON, HYDROGEN, HALOGEN, OXYGEN, NITROGEN, SULFUR, SELENIUM OR TELLURIUM
    • C07F9/00Compounds containing elements of Groups 5 or 15 of the Periodic Table
    • C07F9/02Phosphorus compounds
    • C07F9/547Heterocyclic compounds, e.g. containing phosphorus as a ring hetero atom
    • C07F9/6561Heterocyclic compounds, e.g. containing phosphorus as a ring hetero atom containing systems of two or more relevant hetero rings condensed among themselves or condensed with a common carbocyclic ring or ring system, with or without other non-condensed hetero rings
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6813Hybridisation assays
    • C12Q1/6816Hybridisation assays characterised by the detection means
    • C12Q1/6818Hybridisation assays characterised by the detection means involving interaction of two or more labels, e.g. resonant energy transfer

Definitions

  • DNA sequence between individuals include single polymorphisms (SNPs), mutations, and tandem repeats. Sequences with the highest degree of variations are very useful in the fields of forensics, epidemiology, infectious disease, population characterization, human gene mapping, identification of genes involved in disease, relationship testing, crop and animal breeding and identifying genes of interest. Genetic markers which are sufficiently polymorphic with respect to length or sequence have long been sought for use in identity applications, such as paternity testing and identification of tissue samples collected for forensic analysis.
  • DNA markers which are simple base substitutions i.e., simple sequence polymorphisms
  • Southern hybridization assays For examples of references describing the identification of such markers, designed to be used to analyze restriction endonuclease-digested DNA with radioactive probes, see: Southern, E. M. (1975), J. Mol. Biol. 98(3):503-507; Schumm, et al. (1988), American Journal of Human Genetics 42: 143-159; and Wyman, A. and White, R. (1980) Proc. Natl. Acad. Sci, U.S.A. 77:6754- 6758.
  • DNA markers based on size variants i.e., length polymorphisms, such as "variable number of tandem repeat” (VNTR) markers and polymorphic short tandem repeat (STRs) markers, also have been identified (Nakamura Y., et al. (1987), Science 235: 1616-1622; and U.S. Pat. Nos. 4,963,663 and 5,411,859; (Jeffreys et al. (1985a), Nature 314:67-73; Jeffreys et al. (1985b) Nature 316:76-79.; and U.S. Pat. No. 5,175,082).
  • the genomes of different individuals in a population may contain different numbers of these repeats.
  • VNTRs and STRs are more highly polymorphic than base substitution polymorphisms, sometimes displaying up to forty or more alleles at a single genetic locus.
  • the discovery and development of VNTRs and STRs as genetic markers have stimulated progress in the development of linkage maps, the identification and characterization of diseased genes, and the simplification and precision of DNA typing (Mizutani et al. (2001), J Hum Genet 46:448-55; Sprecher et al, (1996) Biotechniques, 20:266-76; Haaf et al, (1996) Nat. Genet. 12: 183-5; Wooster et al, (1994), Nat. Genet. 6: 152-6; Vergnaud (1989) Polynucleotides Res. 17:7623-30).
  • DNA markers which are polymorphic loci also have been identified by applying polymerase chain reaction (PCR) (U.S. Pat. Nos. 4,683,202; 4,800,159; 5,468,613; and 5,604,099 by Mullis, K.) technology to the analysis of polymorphic loci (Pertl et al, (2000) Hum. Genet. 106:45-9; Deng et al, (2000) Biotechniques 29:298-304; Hohoff and
  • the predominant probe type in the qPCR market is linear hydrolysis probes for use in the 5' nuclease assay. They are traditionally labeled with two dyes, generally located at the termini of a nucleic acid oligomer, for example, a 5' fluorescent reporter and 3' quencher, e.g., a dark quencher.
  • the 3' modification can serve the dual purpose of prohibiting polymerase extension from the probe upon hybridization; and quenching signal from the fluorophore before the probe hybridizes to its target sequence.
  • the quencher and fluorophore may interact through either Forster Resonance Energy Transfer (FRET) and/or static quenching, which it is hypothesized that they contact one another to form a ground-state complex that is non-fluorescent (Marras, S.A.E., Kramer, F.R., and Tyagi, S. (2002) Nucleic Acids Res. 30, el22; Johansson M.K., Fidder, H., Dick, D., Cook, R.M. J. Am. Chem. Soc. (2002); Johansson, M.K. (2006) Methods Mol. Biol. 335, 17-29). This interaction suppresses the signal when the probe is free in solution.
  • FRET Forster Resonance Energy Transfer
  • the duplex formed is quite rigid and so increases the effective length compared to single-stranded oligo, which is much more flexible. Binding of the probe to the target sequence is therefore sufficient to disrupt the interaction between dyes positioned at opposite ends of an oligo and release fluorescent signal (Parkhurst, K.M., and Parkhurst, L.J. (1995). Biochemistry 34, 285-292).
  • the signal release upon hybridization can be made permanent by hydrolyzing the oligo between the fluorophore and the quencher. In fact, cleavage is accomplished when Taq polymerase extends from a primer and encounters the probe in its path. The nuclease activity of the polymerase cleaves the probe one or several bases from its 5' end until the probe loses binding stability and is displaced from the strand. This hydrolysis is the basis for the signaling mechanism in TaqMan® probes.
  • Probe performance can be quantified in a general sense by a signal-to-noise ratio: the final fluorescence following amplification divided by the initial fluorescence preceding amplification.
  • the initial fluorescence represents the quenching efficiency, and so to double this background signal reduces the S:N by a factor of two.
  • Quenching efficiency depends, in part, upon the oligo length. This is because FRET quenching diminishes quite rapidly with increasing separation between the dyes according to a relationship of (1/r 6 ), where r is the distance through space (Cardullo et al. (1988). Proc. Natl. Acad. Sci. U. S. A. 85, 8790- 8794.).
  • Single-stranded oligos are thought to behave as a random coil and so the effective distance is the average of many conformations, but the principle remains the same: increasing sequence length diminishes the quenching efficiency, resulting in probes with elevated baseline fluorescence and poor signal-to-noise values. For this reason, probe designs are typically limited to 30 nucleotides or shorter to achieve sufficient quenching efficiency for the final application.
  • Oligonucleic acid lengths are selected with consideration not only to quenching efficiency but also their binding stability.
  • a common design guideline is to select probe sequences with a TM of 70 ° C, elevated above that of the primers. Probes must typically be longer than 20 bases to accomplish that TM depending on the base composition, and in the absence of special modifications to promote hybridization. Sequence design is thus a careful compromise between binding stability and quenching efficiency, but that 20-30 base window is inadequate for many difficult targets. For example, SNP genotyping requires probes shorter than 20 bases in order to achieve the enhanced specificity needed for mismatch discrimination.
  • TM SNP probes would be nonfunctional without the use of chemical moieties to increase their binding stability— a Minor Groove Binder (MGB) (Kutyavin et al. (2000). Nucleic Acids Res. 28, 655-661) or the propynyl residues used in BHQplus probes, among others. These chemical modifications serve to relax the lower limitation, allowing the design of compact sequences beneath 20 bases in length.
  • MGB Minor Groove Binder
  • Quenchers which can be incorporated in to oligonucleotides during PCR (or other amplification modality) provide a unique entry point to quencher-derivatized
  • the present invention provides quenchers of excited state energy, probes and other conjugates comprising these quenchers, and methods of their use. Other objects, advantages and aspects of the present invention will be apparent from the detailed description below. BRIEF DESCRIPTION OF THE DRAWINGS
  • FIG. 1A - FIG. IB Characterization of BHQlO-dUTP is an HPLC chromatogram of BHQlO-dUTP.
  • FIG. IB is an absorbance spectrum of BHQlO-dUTP.
  • FIG. 2A - FIG. 2B Characterization of BHQIO-dCTP is an HPLC chromatogram of BHQIO-dCTP.
  • FIG. 2B is an absorbance spectrum of BHQIO-dCTP.
  • FIG. 3A - FIG. 3B Characterization of BHQIO-ddCTP is an HPLC chromatogram of BHQIO-ddCTP.
  • FIG. 3B is an absorbance spectrum of BHQIO-ddCTP.
  • FIG. 4A- FIG. 4B Characterization of BHQIO-dATP.
  • FIG. 4A is an HPLC chromatogram of BHQIO-dATP.
  • FIG. 4B is an absorbance spectrum of BHQIO-dATP.
  • FIG. 5A is an HPLC chromatogram of BHQIO-ddATP.
  • FIG. 5B is an absorbance spectrum of BHQIO-ddATP.
  • FIG. 6A - FIG. 6B Characterization of BHQIO-dGTP.
  • FIG. 6A is an HPLC chromatogram of BHQIO-dGTP.
  • FIG. 6B is an absorbance spectrum of BHQIO-dGTP.
  • FIG. 7A - FIG. 7B Characterization of BHQlO-dUTP.
  • FIG. 7A is an HPLC chromatogram of BHQ 10-dUTP.
  • FIG. 7B is an absorbance spectrum of BHQ 10-dUTP.
  • FIG. 8 QIAxcel DNA High Resolution Cartridge capillary gel electrophoresis analysis of desalted double stranded DNA PCR products with and without incorporation of BHQlO-dNTPs.
  • Lane 17 is the QX DNA Size Marker 25-500 bp v2.0.
  • Control reactions of unlabeled PCR products are in Lane (Reactions) 1, 5, 9, and 13.
  • Lanes 2 to 4 are decreasing concentrations of BHQlO-dUTP in the PCR reaction, resulting in decreasing incorporation of BHQlO-dUTP.
  • Lanes 6 to 8 are decreasing concentrations of BHQIO-dATP in the PCR reaction, resulting in decreasing incorporation of BHQIO-dATP.
  • Lanes 10 to 12 are decreasing concentrations of BHQIO-dCTP in the PCR reaction, resulting in decreasing incorporation of BHQIO-dCTP.
  • Lanes 14 to 16 are decreasing concentrations of BHQ 10- dGTP in the PCR reaction, resulting in decreasing incorporation of BHQIO-dGTP.
  • the control reactions were used to compare to the BHQIO-dNTP incorporation into the dsDNA PCR product. By increasing the concentration of BHQlO-dNTPs in the PCR reaction, more labeled dNTPs are incorporated into the dsDNA PCR product, and thus slower migration is observed in the capillary gel electrophoresis.
  • FIG. 9 QIAxcel DNA High Resolution Cartridge capillary gel electrophoresis analysis of desalted single stranded DNA products with and without incorporation of BHQIO-ddATP or BHQIO-ddCTP.
  • Lane 4 is reaction 13, where the reaction contained no BHQlO-ddNTPs.
  • Lanes 1 thru 3 contain decreasing concentrations of BHQIO-ddCTP.
  • Lanes 5-7 contain decreasing concentrations of BHQIO-ddATP.
  • BHQIO-ddATP generates different ssDNA pattern than the incorporation of BHQIO-ddCTP.
  • FIG. 10 Absorbance at 260 nm (RNA absorbance) and 517 nm (BHQ 10 absorbance) measured on a Nano-Drop Spectrophotometer ND- 1000.
  • RNA absorbance RNA absorbance
  • BHQ 10 absorbance 517 nm
  • BHQ refers generally to dark quenchers including one or more diazo bond and specifically to "Black Hole Quenchers®.” Exemplary BHQ's are described in U.S. Patent No. 7,019,129.
  • FET refers to "Fluorescence Energy
  • FRET Fluorescence Resonance Energy Transfer
  • SNP Single Nucleotide Polymorphism
  • alkyl by itself or as part of another substituent, means, unless otherwise stated, a straight- or branched-chain, or cyclic hydrocarbon radical, or combination thereof, which may be fully saturated, mono- or polyunsaturated and can include mono-, di-, tri- and tetra-valent radicals, having the number of carbon atoms designated (i.e. Ci-Cio means one to ten carbons).
  • saturated hydrocarbon radicals include, but are not limited to, groups such as methyl, ethyl, n-propyl, isopropyl, n-butyl, t-butyl, isobutyl, sec-butyl, cyclohexyl, (cyclohexyl)methyl, cyclopropylmethyl, homologs and isomers of, for example, n-pentyl, n-hexyl, n-heptyl, n-octyl, and the like.
  • An unsaturated alkyl group is one having one or more double bonds or triple bonds.
  • unsaturated alkyl groups include, but are not limited to, vinyl, 2-propenyl, crotyl, 2-isopentenyl, 2-(butadienyl), 2,4-pentadienyl, 3- (1,4-pentadienyl), ethynyl, 1- and 3-propynyl, 3-butynyl, and the higher homologs and isomers.
  • alkyl unless otherwise noted, also optionally include those derivatives of alkyl defined in more detail below, such as “heteroalkyl.” Alkyl groups that are limited to hydrocarbon groups are termed “homoalkyl”.
  • alkyl refers to alkyl, alkenyl and alkynyl moieties, each of which can be mono-, di- or polyvalent species as appropriate to satisfy valence requirements.
  • Alkyl groups are optionally substituted, e.g., with one or more groups referred to herein as an "alkyl group substituent.”
  • alkylene by itself or as part of another substituent means a divalent radical derived from an alkyl moiety, as exemplified, but not limited, by -CH 2 CH 2 CH 2 CH 2 -, and further includes those groups described below as “heteroalkylene.”
  • an alkyl (or alkylene) group will have from 1 to 24 carbon atoms, with those groups having 10 or fewer carbon atoms being preferred in the present invention.
  • alkylene and heteroalkylene linker groups it is optional that no orientation of the linker group is implied by the direction in which the formula of the linker group is written.
  • the formula -C(0) 2 R'- represents -C(0) 2 R'- and, optionally, -R'C(0) 2 -.
  • a "lower alkyl” or “lower alkylene” is a shorter chain alkyl or alkylene group, generally having eight, seven, six, five or fewer carbon atoms.
  • alkoxy alkylamino and “alkylthio” (or thioalkoxy) are used in their conventional sense, and refer to those alkyl groups attached to the remainder of the molecule via an oxygen atom, an amino group, or a sulfur atom, respectively.
  • heteroalkyl by itself or in combination with another term, means, unless otherwise stated, a stable straight- or branched-chain, or cyclic alkyl radical consisting of the stated number of carbon atoms and at least one heteroatom selected from the group consisting of B, O, N, Si and S, wherein the heteroatom may optionally be oxidized and the nitrogen atom may optionally be quatemized.
  • the heteroatom(s) may be placed at any internal position of the heteroalkyl group or at a terminus of the chain, e.g., the position through which the alkyl group is attached to the remainder of the molecule. Examples of
  • heteroalkylene by itself or as part of another substituent refers to a substituted or unsubstituted divalent heteroalkyl radical, as exemplified, but not limited by, -CH2-CH2-S-CH2-CH2- and -CH2-S-CH2-CH2-NH-CH2-.
  • heteroatoms can also occupy either or both of the chain termini (e.g., alkyleneoxy, alkylenedioxy, alkyleneamino, alkylenediamino, and the like).
  • heteroalkyl a heteroatom can occupy the position at which the heterocycle is attached to the remainder of the molecule.
  • cycloalkyl include, but are not limited to, cyclopentyl, cyclohexyl, 1 -cyclohexenyl, 3- cyclohexenyl, cycloheptyl, and the like.
  • heterocycloalkyl examples include, but are not limited to, l-(l,2,5,6-tetrahydropyridyl), 1 -piperidinyl, 2-piperidinyl, 3-piperidinyl, 4- mo holinyl, 3-morpholinyl, tetrahydrofuran-2-yl, tetrahydrofuran-3-yl, tetrahydrothien-2-yl, tetrahydrothien-3-yl, 1-piperazinyl, 2-piperazinyl, and the like.
  • halo or halogen
  • haloalkyl by themselves or as part of another substituent, mean, unless otherwise stated, a fluorine, chlorine, bromine, or iodine atom.
  • terms such as “haloalkyl,” are meant to include monohaloalkyl and polyhaloalkyl.
  • halo(Ci-C4)alkyl is meant to include, but not be limited to,
  • aryl means, unless otherwise stated, a polyunsaturated, aromatic, substituent that can be a single ring or multiple rings (preferably from 1 to 3 rings, one or more of which is optionally a cycloalkyl or heterocycloalkyl), which are fused together or linked covalently.
  • heteroaryl refers to aryl groups (or rings) that contain from one to four heteroatoms selected from N, O, and S, wherein the nitrogen and sulfur atoms are optionally oxidized, and the nitrogen atom(s) are optionally quatemized. A heteroaryl group can be attached to the remainder of the molecule through a heteroatom.
  • Non-limiting examples of aryl and heteroaryl groups include phenyl, 1 -naphthyl, 2-naphthyl, 4-biphenyl, 1-pyrrolyl, 2-pyrrolyl, 3-pyrrolyl, 3-pyrazolyl, 2-imidazolyl, 4-imidazolyl, pyrazinyl, 2- oxazolyl, 4-oxazolyl, 2-phenyl-4-oxazolyl, 5-oxazolyl, 3-isoxazolyl, 4-isoxazolyl, 5- isoxazolyl, 2-thiazolyl, 4-thiazolyl, 5-thiazolyl, 2-furyl, 3-furyl, 2-thienyl, 3-thienyl, 2- pyridyl, 3-pyridyl, 4-pyridyl, 2-pyrimidyl, 4-pyrimidyl, 5-benzothiazolyl, purinyl, 2- benzimidazolyl, 5-indolyl,
  • aryl when used in combination with other terms (e.g. , aryloxy, arylthioxy, arylalkyl) optionally includes both homoaryl and heteroaryl rings as defined above.
  • arylalkyl optionally includes those radicals in which an aryl group is attached to an alkyl group (e.g. , benzyl, phenethyl, pyridylmethyl and the like) including those alkyl groups in which a carbon atom (e.g., a methylene group) has been replaced by, for example, an oxygen atom (e.g. , phenoxymethyl, 2-pyridyloxymethyl, 3-(l- naphthyloxy)propyl, and the like).
  • R', R", R'" and R" each preferably independently refer to hydrogen, substituted or unsubstituted heteroalkyl, substituted or unsubstituted aryl, e.g., aryl substituted with 1-3 halogens, substituted or unsubstituted alkyl, alkoxy or thioalkoxy groups, or arylalkyl groups.
  • each of the R groups is independently selected as are each R', R", R'" and R"" groups when more than one of these groups is present.
  • R' and R" are attached to the same nitrogen atom, they can be combined with the nitrogen atom to form a 5-, 6-, or 7-membered ring.
  • -NR'R is meant to include, but not be limited to, 1-pyrrolidinyl and 4-morpholinyl.
  • alkyl includes groups with carbon atoms bound to groups other than hydrogen, such as haloalkyl (e.g. , -CF 3 and -CH 2 CF 3 ) and acyl (e.g. , -C(0)CH 3 , -C(0)CF 3 , -C(0)CH 2 OCH 3 , and the like).
  • alkyl group substituents include those groups referred to herein as “reactive functional groups” and "linkage sites.”
  • the alkyl group substituent is a phosphorus- containing moiety, e.g., a phosphodiester or a phosphodiester modification such as those described herein.
  • substituents for the aryl and heteroaryl groups are generically referred to as "aryl group substituents.”
  • Two of the substituents on adjacent atoms of the aryl or heteroaryl ring may optionally be replaced with a substituent of the formula -T-C(0)-(CRR') q -U-, wherein T and U are independently -NR-, -0-, -CRR'- or a single bond, and q is an integer from 0 to 3.
  • two of the substituents on adjacent atoms of the aryl or heteroaryl ring may optionally be replaced with a substituent of the formula -A-(CH 2 ) r -B-, wherein A and B are independently -CRR'-, -0-, -NR-, -S-, -S(O)-, -S(0) 2 -, -S(0) 2 NR'- or a single bond, and r is an integer of from 1 to 4.
  • One of the single bonds of the new ring so formed may optionally be replaced with a double bond.
  • two of the substituents on adjacent atoms of the aryl or heteroaryl ring may optionally be replaced with a substituent of the formula -(CRR') s -X-(CR"R"') d -, where s and d are independently integers of from 0 to 3, and X is - 0-, -NR'-, -S-, -S(O)-, -S(0) 2 -, or -S(0) 2 NR'-.
  • the substituents R, R', R" and R'" are preferably independently selected from hydrogen or substituted or unsubstituted (Ci- Ci 6 )alkyl.
  • Exemplary aryl group substituents include those groups referred to herein as "reactive functional groups" and "linkage sites.”
  • heteroatom includes oxygen (O), nitrogen (N), sulfur (S) and silicon (Si).
  • R is a general abbreviation that represents a substituent group that is selected from H, substituted or unsubstituted alkyl, substituted or unsubstituted heteroalkyl, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl, and substituted or unsubstituted heterocyclyl groups. R can also refer to alkyl group substituents and aryl group substituents.
  • salt(s) includes salts of the compounds which are prepared with relatively nontoxic acids or bases, depending on the particular substituents found on the compounds described herein.
  • base addition salts can be obtained by contacting the neutral form of such compounds with a sufficient amount of the desired base, either neat or in a suitable inert solvent.
  • base addition salts include counterions such as sodium, potassium, calcium, ammonium, organic amino, or magnesium salt, or a similar salt.
  • acid addition salts can be obtained by contacting the neutral form of such compounds with a sufficient amount of the desired acid, either neat or in a suitable inert solvent.
  • acid addition salts include those derived from inorganic acids like hydrochloric, hydrobromic, nitric, carbonic, monohydrogencarbonic, phosphoric, monohydrogenphosphoric, dihydrogenphosphoric, sulfuric, monohydrogensulfuric, hydriodic, or phosphorous acids, and the like, as well as the salts derived from relatively nontoxic organic acids like acetic, propionic, isobutyric, butyric, maleic, malic, malonic, benzoic, succinic, suberic, fumaric, lactic, mandelic, phthalic, benzenesulfonic, p-tolylsulfonic, citric, tartaric, methanesulfonic, and the like.
  • inorganic acids like hydrochloric, hydrobromic, nitric, carbonic, monohydrogencarbonic, phosphoric, monohydrogenphosphoric, dihydrogenphosphoric, sulfuric, monohydrogensulfuric, hydriodic, or phospho
  • salts of amino acids such as arginate, and the like, and salts of organic acids like glucuronic or galactunoric acids and the like (see, for example, Berge et al, Journal of Pharmaceutical Science, 66: 1 -19 (1977)).
  • Certain specific compounds of the present invention contain both basic and acidic functionalities that allow the compounds to be converted into either base or acid addition salts. Hydrates of the salts are also included. Those of skill in the art will immediately recognize the counterions associated with these and other salt forms of the compounds of the invention.
  • nucleic acid means nucleosides, nucleotides and
  • oligonucleotides e.g., DNA, RNA, whether single-stranded, double-stranded, or in more highly aggregated hybridization motifs, and any chemical modifications thereof.
  • Modifications include, but are not limited to, those providing chemical groups that incorporate additional charge, polarizability, hydrogen bonding, electrostatic interaction, and reactivity to the nucleic acid ligand nucleobases or to the nucleic acid ligand as a whole. Such modifications include, but are not limited to, phosphodiester group modifications (e.g.
  • nucleomonomer refers to a species of nucleic acid having a single nucleic acid unit, which can be a nucleoside, nucleotide or a modification thereof.
  • Exemplary nucleic acids of the invention include a nucleotide having a
  • oligophosphate moiety e.g., pyrophosphate or a higher homologue, such as the 3-mer, 4-mer, 5-mer, 6-mer, 7-mer, 8-mer and the like.
  • exemplary nucleic acids include such a
  • polyphosphate moiety bonded to the 3' or the 5 '-oxygen of a nucleoside.
  • oligophosphate moiety can include a modified phosphate bridge, such as those exemplified herein.
  • the modified phosphate bridge is modified with a linker dye (e.g., fluorophore) conjugate.
  • linker dye e.g., fluorophore
  • Nucleobase as used herein includes those moieties which contain not only the known purine and pyrimidine heterocycles and the invention pyrimidines, but also heterocycle analogs and tautomers thereof.
  • Purines include adenine and guanine, and exemplary purine analogs include 8-oxo-N 6 -methyladenine and 7-deazaxanthine.
  • Pyrimidines include thymine, uracil and cytosine, and their analogs such as 5-methylcytosine, 5- methyluracil and 4,4-ethanocytosine. This term also encompasses non-natural nucleobases.
  • Non-natural nucleobases include 5-fluorouracil, 5-bromouracil, 5-chlorouracil, 5-iodouracil, hypoxanthine, xanthine, 4-acetylcytosine, 5-(carboxyhydroxylmethyl) uracil, 5- carboxymethylaminomethyl-2-thiouridine, 5-carboxymethylaminomethyluracil,
  • nucleobase mimetics e.g., those in which a nitrogen is missing from the five-membered ring of a purine. Such mimetics fall within the scope of the term "nucleobase”.
  • the inventive compounds include pyrimidines derivatized at the 5 -position.
  • the derivatives are 1 -alkenyl-, 1 -alkynyl-, heteroaromatic- and 1-alkynyl- heteroaromatic modifications.
  • 1-Alkenyl means an olefinically-unsaturated (double bond containing) acyclic group.
  • 1-Alkynyl means an acetylenically-unsaturated (triple bond containing) acylic group.
  • nucleoside means a subset of nucleic acid in which a nucleobase is covalently attached to a sugar or sugar analog and which optionally includes a phosphite, phosphoramidite or phosphine.
  • nucleoside includes ribonucleosides,
  • deoxyribonucleosides or any other nucleoside which is an N-glycoside or C-glycoside of a nucleobase.
  • the stereochemistry of the sugar carbons can be other than that of D-ribose.
  • Nucleosides also include those species which contain modifications of the sugar moiety, for example, wherein one or more of the hydroxyl groups are replaced with a halogen, a heteroatom, an aliphatic groups, or are functionalized as ethers, amines, thiols, and the like.
  • the pentose moiety can be replaced by a hexose or an alternate structure such as a cyclopentane ring, a 6-member morpholino ring and the like.
  • Nucleosides as defined herein also include a nucleobase linked to an amino acid and/or an amino acid analog having a free carboxyl group and/or a free amino group and/or protected forms thereof. Nucleosides also optionally include one or more nucleobase modification, e.g., modified with a fluorocarbyl, alkenyl or alkynyl moiety. A nucleoside including a phosphodiester or phosphodiester modification, is referred to herein as a nucleotide. Nucleosides as defined herein are also intended to include a nucleobase linked to an amino acid and/or an amino acid analog having a free carboxyl group and/or a free amino group and/or protected forms thereof.
  • sugar modification means any pentose or hexose moiety other than 2'-deoxyribose.
  • Modified sugars include, for example, D-ribose, 2'-0-alkyl, 2'-amino, 2'-halo functionalized pentoses, hexoses and the like.
  • Exemplary sugar modifications include those sugars in which one or more of the hydroxyl groups is replaced with a halogen, a heteroatom, an alkyl moiety, or are functionalized as ethers, esters, and the like.
  • the pentose moiety can be replaced by a hexose or an alternate structure such as a cyclopentane ring, a 6- member morpholino ring and the like. Sugars having a stereochemistry other than that of a D- ribose are also included.
  • Substitute linkages include phosphodiester analogs, e.g. such as phosphorothioate and methylphosphonate, and nonphosphorus containing linkages, e.g. such as acetals and amides.
  • Nucleic acid modification also include 3', 5', and base modifications such as labeling with a quencher (e.g., a BHQ), a fluorophore, intercalator, minor groove binder, a fluorocarbon, a stabilizing group or another moiety.
  • a quencher e.g., a BHQ
  • the modification or label is covalently conjugated to the oligomer through a linker group.
  • Oligomers are defined herein as two or more nucleomonomers covalently coupled to each other by a phosphodiesester or modified phosphodiester moiety.
  • an oligomer can have as few as two nucleomonomers (a dimer), and have essentially no upper limit of nucleomonomers.
  • Oligomers can be binding competent and, thus, can base pair with cognate single-stranded or double-stranded (or higher order aggregation) nucleic acid sequences. Oligomers are also useful as synthons for longer oligomers as described herein. Oligomers can also contain abasic sites and pseudonucleosides. In various embodiments, the oligomers of the invention are functionalized.
  • oligomer is used interchangeably to refer to the nucleic acid sequence of the oligomer, the modified nucleic acid sequence providing a probe of the invention or the modified nucleic acid sequence providing a solid support of the invention.
  • Peptide refers to an oligomer in which the monomers are amino acids and are joined together through amide bonds, alternatively referred to as a polypeptide.
  • amino acids are a-amino acids
  • either the L-optical isomer or the D-optical isomer can be used.
  • unnatural amino acids for example, ⁇ -alanine, phenylglycine and homoarginine are also included.
  • Commonly encountered amino acids that are not gene- encoded may also be used in the present invention. All of the amino acids used in the present invention may be either the D - or L -isomer.
  • the L -isomers are generally preferred.
  • other peptidomimetics are also useful in the present invention.
  • a "solid support” is a solid material having a surface for attachment of molecules, compounds, cells, or other entities, or to which surface such species are attached.
  • the surface of a solid support can be flat or otherwise configured.
  • a solid support can be porous or non-porous.
  • a solid support can be a chip or array that comprises a surface, and that may comprise glass, silicon, nylon, polymers, plastics, ceramics, or metals.
  • a solid support can also be a membrane, such as a nylon, nitrocellulose, or polymeric membrane, or a plate or dish and can be comprised of glass, ceramics, metals, or plastics, such as, for example, a 96- well plate made of, for example, polystyrene, polypropylene, polycarbonate, or polyallomer.
  • a solid support can also be a bead or particle of any shape, and is preferably spherical or nearly spherical, and preferably a bead or particle has a diameter or maximum width of 1 millimeter or less, more preferably of between 0.1 to 100 microns.
  • Such particles or beads can be comprised of any suitable material, e.g., glass or ceramics, and/or one or more polymers, such as, for example, nylon, polytetrafluoroethylene, TEFLONTM, polystyrene, polyacrylamide, sepaharose, agarose, cellulose, cellulose derivatives, or dextran, and/or can comprise metals, particularly paramagnetic metals, such as iron.
  • suitable material e.g., glass or ceramics
  • polymers such as, for example, nylon, polytetrafluoroethylene, TEFLONTM, polystyrene, polyacrylamide, sepaharose, agarose, cellulose, cellulose derivatives, or dextran
  • metals particularly paramagnetic metals, such as iron.
  • Supports for solid phase synthesis include, but are not limited to, high cross-linker polystyrene (McCollum, et al, Tetrahedron Lett. 32: 4069-4072 (1991), polystyrene/PEG copolymer (Gao, et al, Tetrahedron Lett. 32: 5477-5480 (1991), silica gel (Chow, et al., Nucl. Acids Res. 9: 2807-2817 (1981)), polyamide bonded silica gel (Gait, et al, Nucl. Acids Res. 10: 6243-6254 (1982)), cellulose (Crea, et al, Nucl. Acids Res.
  • CPG beads can be derivatized for the attachment of a nucleomonor or oligomer in a variety of ways.
  • CPG beads can be treated with 3-aminopropyltriethoxysilane to add an amino propyl linker handle for the attachment of oligonucleotide analogue monomers or dimers (Koster, et al,
  • an "intercalator” refers to a planar aromatic or heteroaromatic moiety that is capable of partial insertion and stacking between adjacent nucleobases. These moieties may be small molecules or part of a larger entity, such as a protein.
  • Non-limiting examples of intercalators include acridines, anthracenes, anthracyclines, anthracyclinone, methylene blue, indole, anthraquinone, quinoline, isoquinoline, dihydroquinones, tetracyclines, psoralens, coumarins, ethidium halides, ethidium homodimers, homodimeric oxazole yellow (YOYO), thiazole orange (TOTO), dynemicins, 1,10-phenanthroline-copper, calcheamicin, porphyrins, distamycins, netropcins, and viologens.
  • a “minor groove binder” refers to a moiety typically having a molecular weight of approximately 150 to approximately 2000 Daltons. The moiety binds in a non-intercalating manner into the minor groove of double stranded (or higher order aggregation) DNA, RNA or hybrids thereof, preferably, with an association constant greater than approximately 10 3 M "1 .
  • Minor groove binding compounds have widely varying chemical structures, however, exemplary minor groove binders have a crescent shape three dimensional structure.
  • Certain bisquarternary ammonium heterocyclic compounds, diarylamidines such as pentamidine, stilbamidine and berenil, CC- 1065 and related pyrroloindole and indole polypeptides, Hoechst 33258, 4'-6-diamidino-2- phenylindole (DAP I) as well as a number of oligopeptides consisting of naturally occurring or synthetic amino acids are minor groove binder compounds.
  • Exemplary minor groove binders are described in U.S. Patent No. 6,084,102. This type of binding can be detected by well established spectrophotometric methods, such as ultraviolet (u.v.) and nuclear magnetic resonance (NMR) spectroscopy and also by gel electrophoresis. Shifts in u.v. spectra upon binding of a minor groove binder molecule, and NMR spectroscopy utilizing the "Nuclear Overhauser" (NOSEY) effect are particularly well known and useful techniques for this purpose.
  • Gel electrophoresis detects binding of a minor groove binder to double stranded DNA or fragment thereof, because upon such binding the mobility of the double stranded DNA changes.
  • the minor groove binder is typically attached to the oligomer or solid support through a linker comprising a chain about 20, about 15 atoms, about 10 or about 5 atoms.
  • Intercalating moieties or agents are readily distinguished from minor groove binders on the basis that the intercalating agents are flat aromatic (preferably poly cyclic) molecules versus the "crescent shape" or analogous geometry of the minor groove binders.
  • An experimental distinction can also be made by NMR spectroscopy utilizing the Nuclear Overhauser effect.
  • linker refers to a single covalent bond ("zero- order") or a series of stable covalent bonds incorporating 1-30 nonhydrogen atoms selected from the group consisting of C, N, O, S, Si and P that covalently link together the components of the compounds of the invention, e.g., linking a solid support to a stabilizing agent, a quencher, a nucleomonomer or oligomer of the invention; or linking a quencher or stabilizing moiety to a nucleobase in an amidite of the invention.
  • Exemplary linkers include 1 , 2, 3, 4, 5, 6, 7, 8, 9, 10, 1 1, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21 , 22, 23, 24, 25, 26, 27, 28, 29 or 30 non-hydrogen atoms.
  • linking “linked,” “linkage,” “conjugating,” “conjugated” and analogous terms relating to attachment refer to techniques utilizing and species incorporating linkers.
  • Exemplary linkers include a linkage site as defined herein.
  • a linker is of use to attach an oligomer or nascent oligomer (during oligomer synthesis) to the solid support of the invention.
  • the invention also provides an oligomer of the invention covalently attached to a solid support (e.g., a solid support of the invention) through a linker.
  • the solid supports and oligomers of the invention optionally include a cleavable linker between two components of the solid support and oligomer (e.g., between the oligomer and the solid support, between the fiuorophore and oligomer, between the quencher and oligomer, between the fiuorophore and quencher, etc.).
  • the linker joining the solid support to the oligomer is a cleavable linker.
  • An exemplary linker includes an alkenyl or an alkynyl moiety covalently attached though an unsaturated carbon to a purine or a pyrimidine of a nucleobase.
  • a "cleavable linker” is a linker that has one or more cleavable groups that may be broken by the result of a reaction or condition.
  • An exemplary cleavable linker is located within R 8 of Formula I or II, serving to allow for the expedient separation of a synthesized oligomer of the invention from the solid support upon which it was synthesized.
  • cleavable group refers to a moiety that allows for release of a component of the solid support or oligomer of the invention by cleaving a bond linking the released moiety to the remainder of the conjugate.
  • exemplary cleavage mechanisms of use both in preparing and using the oligomers and solid supports of the invention are enzymatically or otherwise chemically mediated.
  • cleaved groups include one or more sites that are cleaved by the action of an agent other than an enzyme.
  • exemplary non-enzymatic cleavage agents include, but are not limited to, acids, bases, light (e.g., nitrobenzyl derivatives, phenacyl groups, ortho-hydroxcinnamate esters, benzoin esters), and heat.
  • Many cleaveable groups are known in the art. See, for example, Jung et al, Biochem. Biophys. Acta, 761 : 152-162 (1983); Joshi et al, J. Biol.
  • Afunctional (both homo- and hetero-bifunctional) spacer arms are commercially available.
  • An exemplary cleavable group is cleavable by a reagent, e.g. sodium hydroxide, ammonia or other amine.
  • a reagent e.g. sodium hydroxide, ammonia or other amine.
  • the cleavable linker is readily cleaved at room temperature or under heat.
  • R 8 of Formula I or II comprises a cleavable linker that is cleaved by treatment with an amine, e.g., ammonia or an essentially anhydrous amine in an organic solvent.
  • a "linkage site,” is a moiety that connects two or more components (e.g., functional component, solid support, oligonucleotide, or linker). This term refers to a covalent bond that is formed by reaction of complementary reaction partners, each of which has a functional group of complementary reactivity to that of its partner. Linkage sites in the solid support and oligomers of the invention are independently selected.
  • Exemplary linkage sites include, but are not limited to S, SC(0)NH, HNC(0)S, SC(0)0, O, NH, NHC(O), (O)CNH and NHC(0)0, and OC(0)NH, CH 2 S, CH 2 0 , CH 2 CH 2 0, CH 2 CH 2 S, (CH 2 ) 0 O, (CH 2 ) 0 S or (CH 2 ) 0 Y X -PEG wherein, Y x is S, NH, NHC(O), C(0)NH, NHC(0)0, OC(0)NH, or O and o is an integer from 1 to 50.
  • NH can be NR l in which R l is substituted or unsubstituted alkyl or substituted or unsubstituted heteroalkyl.
  • a linkage site can also be a phosphodiester group.
  • the linkage site is between a linker and a fluorophore, a linker and a quencher, a linker and a stabilizing moiety or a linker and a solid support.
  • each linkage site is different.
  • fluorophore refers to a moiety that is inherently fluorescent or demonstrates a change in fluorescence upon binding to a biological compound or metal ion, or metabolism by an enzyme, i.e., fluorogenic. Fluorophores may be substituted to alter the solubility, spectral properties or physical properties of the fluorophore.
  • fluorophores are known to those skilled in the art and include, but are not limited to coumarins, acridines, furans, dansyls, cyanines, pyrenes, naphthalenes, benzofurans, quinolines, quinazolinones, indoles, benzazoles, borapolyazaindacenes, oxazines and xanthenes, with the latter including fluoresceins, rhodamines, rosamines and rhodols.
  • fluorophores of use in the invention are described in Haugland, MOLECULAR PROBES HANDBOOK OF FLUORESCENT PROBES AND RESEARCH CHEMICALS. Further useful fluorophores are described in commonly owned U.S. Patent Application Publication No. 2005/0214833 and 2005/0170363 and herein below.
  • quencher refers to any fluorescence-modifying moiety of the invention that can attenuate at least partly the light emitted by a fluorophore. This attenuation is referred to herein as "quenching". Hence, in various embodiments, excitation of the fluorophore in the presence of the quenching group leads to an emission signal that is less intense than expected, or even completely absent. Quenching typically occurs through energy transfer between the excited fluorophore and the quenching group.
  • the fluorophore or quencher may include substituents enhancing a desirable property, e.g., solubility in water, cell permeability or an altered absorption and emission spectrum, relative to the "parent" compound in the absence of such substituent.
  • a desirable property e.g., solubility in water, cell permeability or an altered absorption and emission spectrum
  • the fluorophore or quencher of use in the invention include substituents that enhance a desirable property relative to an identical parent compound in the absence of the improving substituent.
  • a "functional component” is a generic term for a moiety in a compound of the invention having a structure selected from a quencher, a fluorophore or a stabilizing moiety (including, but not limited to, intercalators, minor groove binding moieties, nucleobases modified with a stabilizing moiety (e.g., alkynyl moieties, and fluoroalkyl moieties), and conformational stabilizing moieties, such as those described in commonly owned U.S. Patent Application Publication No. 2007/0059752).
  • a stabilizing moiety including, but not limited to, intercalators, minor groove binding moieties, nucleobases modified with a stabilizing moiety (e.g., alkynyl moieties, and fluoroalkyl moieties), and conformational stabilizing moieties, such as those described in commonly owned U.S. Patent Application Publication No. 2007/0059752).
  • amplification of polynucleotides includes but is not limited to methods such as polymerase chain reaction (PCR), ligation amplification (or ligase chain reaction, LCR) and amplification methods based on the use of Q-beta replicase. These methods are well known and widely practiced in the art. See, e.g., U.S. Pat. Nos. 4,683,195 and 4,683,202 and Innis et al, 1990 (for PCR); and Wu et al, 1989a (for LCR). Reagents and hardware for conducting PCR are commercially available.
  • PCR polymerase chain reaction
  • LCR ligase chain reaction
  • Primers useful to amplify sequences from a particular gene region are preferably complementary to, and hybridize specifically to sequences in the target region or in its flanking regions. Nucleic acid sequences generated by amplification may be sequenced directly. Alternatively the amplified sequence(s) may be cloned prior to sequence analysis. A method for the direct cloning and sequence analysis of enzymatically amplified genomic segments has been described by Scharf (1986).
  • the present invention provides oligomeric primers of use in amplification processes. Moreover, there is provided a solid support of use in synthesizing such primers. In addition to primers, the invention provides probes, and methods of using such probes, to detect, characterize and/or quantify the products of amplification: also provided are solid supports of use to synthesize these oligomeric probes.
  • base-stacking perturbations refers to any event that causes a perturbation in base-stacking such as, for example, a base-pair mismatch, a protein binding to its recognition site, or any other entities that form oligonucleotide adducts.
  • Various probes of the invention are capable of detecting, characterizing and/or quantifying such base-stacking perturbations.
  • the invention provides solid supports of use in synthesizing probes capable of detecting, characterizing and/or quantifying such base-stacking perturbations.
  • hybridized refers to two nucleic acid strands associated with each other which may or may not be fully base-paired: generally, this term refers to an association including an oligomer of the invention whether bound to a solid support or in solution.
  • denaturing refers to the process by which strands of nucleic acid duplexes (or higher order aggregates) are no longer base-paired by hydrogen bonding and are separated into single-stranded molecules. Methods of denaturation are well known to those skilled in the art and include thermal denaturation and alkaline denaturation. This term generally refers to the dissociation of a probe of the invention from its target nucleic acid.
  • mismatches refers to nucleic acid nucleobases within hybridized nucleic acid duplexes (or higher order aggregates) which are not 100% complementary.
  • a mismatch includes any incorrect pairing between the nucleobases of two nucleobases located on complementary strands of nucleic acid that are not the Watson-Crick base-pairs, e.g., A:T or G:C.
  • the lack of total homology may be due to deletions, insertions, inversions, substitutions or frameshift mutations.
  • the oligomer of the invention includes a mismatch relative to its target nucleic acid, preferably allowing detection and/or
  • the mismatch is a single nucleotide mismatch.
  • polymorphism refers to a sequence variation in a gene
  • mutation refers to a sequence variation in a gene that is associated or believed to be associated with a phenotype.
  • gene refers to a segment of the genome coding for a functional product protein control region. Polymorphic markers used in accordance with the present invention for subject identification may be located in coding or non-coding regions of the genome, and various probes of the invention are designed to hybridize to nucleic acid regions including these markers.
  • the term "subject,” as used herein refers to a subject providing a test sample from which target nucleic acids are obtained for the purpose of genetic testing.
  • the oligomers of the invention are of use in detecting and/or characterizing and/or quantifying polymorphisms and mutations.
  • the solid supports of the invention are of use in synthesizing oligomers of use to detect and/or characterize and/or quantitate polymorphisms and mutations.
  • probe refers to nucleic acid oligomers prepared using a solid support or amidite of the invention.
  • the probes produce a detectable response upon interaction with a binding partner.
  • the probes include at least one detectable moiety, or a pair of moieties that form an energy transfer pair detectable upon some change of state of the probe in response to its interaction with a binding partner.
  • the present invention provides probes and amidites and solid supports of use to synthesize probes. Exemplary probes of the invention are of use to detect a polymorphism.
  • the polymorphism is a single nucleotide polymorphism (SNP).
  • detectable response refers to a change in or an occurrence of, a signal that is directly or indirectly detectable either by observation or by instrumentation and the presence of or, preferably, the magnitude of which is a function of the presence of a target binding partner for a probe in the test sample.
  • the detectable response is an optical response from a fluorophore resulting in a change in the wavelength distribution patterns or intensity of absorbance or fluorescence or a change in light scatter, fluorescence quantum yield, fluorescence lifetime, fluorescence polarization, a shift in excitation or emission wavelength or a combination of the above parameters.
  • the detectable change in a given spectral property is generally an increase or a decrease in fluorescence intensity.
  • the change in fluorescence on ion binding is usually due to conformational or electronic changes in the indicator that may occur in either the excited or ground state of the fluorophore, due to changes in electron density at the ion binding site, due to quenching of fluorescence by the bound target metal ion, or due to any combination of these or other effects.
  • the detectable response is an occurrence of a signal wherein the fluorophore is inherently fluorescent and does not produce a change in signal upon binding to a metal ion or biological compound.
  • the present invention provides probes providing a detectable response and solid supports of use to synthesize such probes.
  • carrier molecule refers to any molecule to which a compound of the invention is attached.
  • Representative carrier molecules include a protein (e.g., enzyme, antibody), glycoprotein, peptide, saccharide (e.g., mono-, oligo-, and polysaccharides), hormone, receptor, antigen, substrate, metabolite, transition state analog, cofactor, inhibitor, drug, dye, nutrient, growth factor, etc., without limitation.
  • Carrier molecule also refers to species that might not be considered to fall within the classical definition of "a molecule,” e.g., solid support (e.g., synthesis support, chromatographic support, membrane), virus and microorganism.
  • the present invention provides a conjugate between a nucleic acid and quencher of excited state energy having a structure comprising at least three radicals selected from substituted aryl, substituted heteroaryl and combinations thereof, wherein at least two of the residues are covalently linked via an exocyclic diazo bond.
  • One of of the substituted aryl or heteroaryl rings includes a linker covalently joining the quencher to the nucleobase of the nucleic acid.
  • the 5 '-hydroxyl of the ribose moiety is derivatized with a phosphate or an oligophosphate.
  • Exemplary oligophosphates include di-, tri-, tetra-, penta-, and higher order phosphates.
  • the oligophosphate conjugate of the invention can be enzymatically incorporated in to an oligonucleotide, e.g., during PCR.
  • an oligonucleotide having incorporated therein the conjugate between the quencher and the nucleic acid and methods of incorporating the conjugate in to an oligonucleotide using the oligophosphate as an enzyme substrate.
  • One, two or three of the substituted aryl or heteroaryl rings is derivatized with at least one water-solubilizing moiety, e.g., sulfonate, carboxylate, phosphate, phosphonate, charged amine (e.g., quaternized), hydroxy, oligohydroxy, ether.
  • the substituted aryl and heteroaryl moieties of the invention are single ring systems or they are fused ring systems including more than one aryl moiety fused into a poly cyclic system, more than one heteroaryl moiety fused into a poly cyclic system or a combination of at least one aryl ring fused to at least one heteroaryl ring to form a poly cyclic system.
  • nucleobase mimetics e.g., those in which a nitrogen is missing from the five-membered ring of a purine. Such mimetics fall within the scope of the term "nucleobase”.
  • the conjugate of the invention includes a naturally occurring nucleobase, which is other than uridine.
  • the present invention provides a conjugate as described above having a structure according to Formula I:
  • R a , R and R c are independently selected water-solubilizing moieties, e.g., sulfonate, carboxylate, phosphate, phosphonate, charged amine (e.g., quaternized), hydroxy, oligohydroxy, ether.
  • the indices a and b are independently selected from 0, 1 , 2, 3, 4, and 5.
  • L is a linker as that term is defined herein.
  • B is a nucleobase.
  • R 2 is the oligophosphate moiety, in which O is attached to the 5' carbon of the ribose moiety.
  • R a and R b are independently selected from H and OH.
  • the invention provides a quencher conjugate according to Formula II:
  • the invention provides a quencher conjugate according to Formula III:
  • a residue of a compound of the invention is incorporated into an oligonucleotide through a phosphate moiety derived from the oligophosphate.
  • an exemplary compound of the invention has the formula:
  • R 4 is an oligonucleotide.
  • the structure in Formula IV can be located at an internal position of the oligonucleotide, or it can be on the terminus.
  • Formula IV includes a dideoxy ribose structure, it is a chain terminating nucleic acid, and at the 3 '-terminus of the oligonucleotide.
  • R 2 is selected from H, and alkyl or heteroalkyl.
  • the alkyl and heteroalkyl moiety is optionally substituted at one or more positions other than where it is joined to the nitrogen.
  • L 1 is selected from a bond, substituted or unsubstituted alkylene, substituted or unsubstitued alkenylene, substituted or unsubstituted alkynylene, substituted or unsubstituted cycloalkylene, substituted or unsubstituted heteroalkylene, and substituted or unsubstituted heterocycloalkylene.
  • L 1 is covalently bonded to the nucleobase through an alkenyl carbon or an alkynyl carbon.
  • nucleic acid oligophosphate quencher conjugates of the invention include:
  • L 2 is Ci-Cig alkyl, e.g, C2-C1 0 alkyl, e.g., C3-C6 alkyl, or heteroalkyl including 1-5 heteroatoms interrupting a carbon chain, e.g., Ci-Cig alkyl, e.g, C 2 - C1 0 alkyl, e.g., C3-C6 alkyl.
  • L 2 is optionally substituted at one or more position in addition to the attachment points to the carbonyl carbon and the nitrogen of quencher, Q.
  • the compounds of the invention are displayed in their charged form, it will be apparent to those of skill in the art that the compounds also exist in various forms of protonation. Moreover, the charged species of the invention can be associated with any useful counterion. Thus, as will be readily appreciated, those species shown without a counterion can include any useful counterion and those displayed with a counterion exist in forms in which the displayed counterion is replaced by another useful ion.
  • nucleic acid oligomer e.g., a probe, prepared using a quencher of the invention and including components of the quencher from which it is synthesized.
  • the oligomer optionally further includes one or more fluorophore, minor groove binder, or intercalator.
  • Exemplary oligomers include oligonucleotides, oligonucleosides,
  • oligodeoxyribonucleotides containing 2'-deoxy-D-ribose or modified forms thereof), i.e., DNA, oligoribonucleotides (containing D-ribose or modified forms thereof), i.e., RNA, and any other type of polynucleotide which is an N-glycoside or C-glycoside of a purine or pyrimidine nucleobase, or modified purine or pyrimidine nucleobase.
  • Oligomer as used herein also includes compounds where adjacent nucleomonomers are linked via amide linkages as previously described (Nielsen et al, Science (1991) 254: 1497-1500).
  • Oligomers can be replaced with any suitable functionally equivalent element.
  • "Oligomer” is thus intended to include any structure that serves as a scaffold or support for the nucleobases wherein the scaffold permits binding to target nucleic acids in a sequence-dependent manner.
  • Exemplary groups linking nucleomonomers in an oligomer of the invention include (i) phosphodiester and phosphodiester modifications (phosphorothioate, methylphosphonate, etc), (ii) substitute linkages that contain a non-phosphorous isostere (formacetal, riboacetal, carbamate, etc), (iii) morpholino residues, carbocyclic residues or other furanose sugars, such as arabinose, or a hexose in place of ribose or deoxyribose and (iv) nucleomonomers linked via amide bonds or acyclic nucleomonomers linked via any suitable substitute linkage.
  • the oligomers of the invention can be formed using modified and conventional nucleomonomers and synthesized using standard solid phase (or solution phase) oligomer synthesis techniques, which are now commercially available.
  • the oligomers can be synthesized by a method comprising the steps of: synthesizing a nucleomonomer or oligomer synthon having a protecting group and a nucleobase and a coupling group capable of coupling to a nucleomonomer or oligomer; coupling the nucleomonomer or oligomer synthon to an acceptor nucleomonomer or an acceptor oligomer; removing the protecting group; and repeating the cycle as needed until the desired oligomer is synthesized.
  • the oligomers of the present invention can be of any length including those of greater than 40, 50 or 100 nucleomonomers. In various embodiments, oligomers contain 2- 100 nucleomonomers. Lengths of greater than or equal to about 10 to 40 nucleomonomers are useful for therapeutic or diagnostic applications. Short oligomers containing 2, 3, 4 or 5 nucleomonomers are specifically included in the present invention and are useful, e.g., as synthons.
  • Oligomers having a randomized sequence and containing fewer than 20, fewer thanl5 or fewer than 10 nucleomonomers are useful for primers, e.g., in cloning or amplification protocols that use random sequence primers, provided that the oligomer contains residues that can serve as a primer for polymerases or reverse transcriptases.
  • Oligomers can contain conventional phosphodiester linkages or can contain phosphodiester modification such as phosphoramidate linkages. These substitute linkages include, but are not limited to, embodiments wherein a moiety of the formula -0-P(0)(S)-0- ("phosphorothioate"), -0-P(S)(S)-0- ("phosphorodithioate”), -O-P(O)- (NR° 2 )-X-,
  • the substitute linkages for use in the oligomers of the present invention include phosphodiester, phosphorothioate, methylphosphonate and thionomethylphosphonate linkages.
  • Phosphorothioate and methylphosphonate linkages confer added stability to the oligomer in physiological environments. While not all such linkages in the same oligomer need be identical, particularly preferred oligomers of the invention contain uniformly phosphorothioate linkages or uniformly methylphosphonate linkages.
  • Oligomers or the segments thereof are conventionally synthesized, and can be prepared using a compound of the invention.
  • the synthetic methods known in the art and described herein can be used to synthesize oligomers containing compounds of the invention, as well as other nucleobases known in the art, using appropriately protected
  • the invention provides "conjugates" of oligomers, which are formed using a quencher of the invention.
  • the oligomers can be covalently linked to various functional components such as, stabilizing moieties, fluorophores, quenchers, intercalators, and substances which interact specifically with the minor groove of the DNA double helix (minor groove binders, "MGB").
  • Other chosen conjugate moieties can be labels such as radioactive, fluorescent, enzyme, or moieties which facilitate cell association using cleavage linkers and the like.
  • Suitable radiolabels include 2 P, 5 S, H and 14 C; and suitable fluorescent labels include fluorescein, resorufin, rhodamine, BODIPY (Molecular Probes) and texas red; suitable enzymes include alkaline phosphatase and horseradish peroxidase.
  • oligomers can be derivatized through any convenient linkage.
  • minor groove binders, fluorophores, quenchers and intercalators such as acridine or psoralen can be linked to the oligomers of the invention through any available -OH or -SH, e.g., at the terminal 5'-position of the oligomer, the 2'-positions of RNA, or an OH, NH 2 , COOH or SH incorporated into the 5-position of pyrimi dines.
  • a derivatized form which contains, for example, -CH 2 CH 2 NH 2 ,
  • Conjugates including polylysine or lysine can be synthesized as described and can further enhance the binding affinity of an oligomer to its target nucleic acid sequence (Lemaitre, M. et al, Proc Natl Acad Sci (1987) 84:648-652; Lemaitre, M. et al, Nucleosides and
  • a wide variety of substituents can be attached, including those bound through linkages or substitute linkages.
  • the -OH moieties in the phosphodiester linkages of the oligomers can be replaced by phosphate groups, protected by standard protecting groups, or coupling groups to prepare additional linkages to other nucleomonomers, or can be bound to the conjugated substituent.
  • the 5 '-terminal OH can be phosphorylated; the 2'-OH or OH substituents at the 3'-terminus can also be phosphorylated.
  • the hydroxyls can also be derivatized to standard protecting groups.
  • Oligomers of the invention can be covalently derivatized to moieties that facilitate cell association using cleavable linkers.
  • Linkers used for such conjugates can include disulfide linkages that are reduced after the oligomer-transport agent conjugate has entered a cell.
  • Disulfi de-containing linkers of this type have a controllable half life. Such linkers are stable under extracellular conditions relative to intracellular conditions due to the redox potential of the disulfide linkage.
  • One of the advantages of the compounds of the invention is that a wide range of energy donor molecules can be used in conjunction with the quencher of the invention and oligonucleotides incorporating the quencher.
  • a vast array of fluorophores is known to those of skill in the art. See, for example, Cardullo et al. , Proc. Natl. Acad. Sci. USA 85: 8790- 8794 (1988); Dexter, D.L., J. of Chemical Physics 21: 836- 850 (1953); Hochstrasser et al , Biophysical Chemistry 45: 133-141 (1992); Selvin, P., Methods in Enzymology 246: 300-334 (1995); Steinberg, I. Ann. Rev.
  • Reactive Red 4 (CibacronTM Brilliant Red 3B-A)
  • TAMRA N,N,N',N'-tetramethyl-6-carboxyrhodamine
  • TRITC tetramethyl rhodamine isothiocyanate
  • metal chelates e.g., lanthanide chelates (e.g.,europium terbium chelates), ruthenium chelates
  • an energy exchange pair for a particular application and to conjugate the members of this pair to a probe molecule, such as, for example, a nucleic acid, peptide or other polymer.
  • a probe molecule such as, for example, a nucleic acid, peptide or other polymer.
  • an absorbance band of the quencher substantially overlap the fluorescence emission band of the donor.
  • the donor fluorescent moiety and the quencher (acceptor) of the invention are preferably selected so that the donor and acceptor moieties exhibit donor-acceptor energy transfer when the donor moiety is excited.
  • the efficiency of donor-acceptor energy transfer between them is the efficiency of donor-acceptor energy transfer between them.
  • the efficiency of FRET between the donor and acceptor moieties is at least 10%, more preferably at least 50% and even more preferably at least 80%.
  • the efficiency of FRET can easily be empirically tested using the methods both described herein and known in the art.
  • the efficiency of energy transfer between the donor-acceptor pair can also be adjusted by changing the ability of the donor and acceptor groups to dimerize or closely associate. If the donor and acceptor moieties are known or determined to closely associate, an increase or decrease in association can be promoted by adjusting the length of a linker moiety, or of the probe itself, between the donor and acceptor.
  • the ability of donor-acceptor pair to associate can be increased or decreased by tuning the hydrophobic or ionic interactions, or the steric repulsions in the probe construct.
  • intramolecular interactions responsible for the association of the donor-acceptor pair can be enhanced or attenuated.
  • the association between the donor-acceptor pair can be increased by, for example, utilizing a donor bearing an overall negative charge and an acceptor with an overall positive charge.
  • a ligand molecule e.g., biotin
  • a ligand molecule is generally covalently bound to the probe species.
  • the ligand then binds to another molecules (e.g., streptavidin) molecule, which is either inherently detectable or covalently bound to a signal system, such as a fluorescent compound, or an enzyme that produces a fluorescent compound by conversion of a non-fluorescent compound.
  • Useful enzymes of interest as labels include, for example, hydrolases, particularly phosphatases, esterases and glycosidases, hydrolases, peptidases or oxidases, particularly peroxidases, and .
  • Fluorescent compounds include fluorescein and its derivatives, rhodamine and its derivatives, dansyl, umbelliferone, etc., as discussed above.
  • Donors of use in conjunction with the quenchers of the invention include, for example, xanthene dyes, including fluoresceins, cyanine dyes and rhodamine dyes.
  • Another group of fluorescent compounds of use in conjunction with the quenchers of the invention are the naphthylamines, having an amino group in the alpha or beta position. Included among such naphthylamino compounds are l-dimethylaminonaphthyl-5-sulfonate, l-anilino-8-naphthalene sulfonate and 2-p- touidinyl-6-naphthalene sulfonate.
  • Other donors include 3-phenyl-7-isocyanatocoumarin, acridines, such as 9-isothiocyanatoacridine and acridine orange; N-(p-(2- benzoxazolyl)phenyl)maleimide; benzoxadiazoles, stilbenes, pyrenes, and the like.
  • quenchers and fluorophores For clarity of illustration, the discussion below focuses on attaching quenchers and fluorophores to nucleic acids. The focus on nucleic acid probes is not intended to limit the scope of probe molecules to which quenchers can be attached. Those of skill in the art will appreciate that quenchers can also be attached to small molecules, proteins, peptides, synthetic polymers, solid supports and the like using standard synthetic chemisty.
  • the fluorophore is a Quasar ® dye (Biosearch Technologies, Inc.).
  • the fluorophore is preferably attached to either the 3'- or the 5'-terminus of the nucleic acid, although internal sites are also accessible and have utility for selected purposes. Whichever terminus the fluorophore is attached to, the quencher will generally be attached to its antipode, or at a position internal to the nucleic acid chain.
  • Donor groups are preferably introduced using an amidite derivative of the donor. Alternatively, donor groups comprising reactive functional groups (e.g.
  • isothiocyanates, active esters, etc. can be introduced via reaction with a reactive functional group on a tether or linker arm attached to the nucleic acid (e.g., hexyl amine).
  • the donor moiety can be attached at the 3'- terminus of a nucleic acid by the use of a derivatized synthesis support.
  • TAMRA tetramethylrhodamine carboxylic acid
  • an analogue of this fluorophore Biosearch Technologies, Inc.
  • linker moieties and methodologies for attaching groups to the 5'- or 3 '-termini of nucleic acids are many linker moieties and methodologies for attaching groups to the 5'- or 3 '-termini of nucleic acids, as exemplified by the following references: Eckstein, editor, Nucleic acids and Analogues: A Practical Approach (IRL Press, Oxford, 1991); Zuckerman et al, Nucleic Acids Research, 15: 5305-5321 (1987) (3'-thiol group on nucleic acid); Sharma ei a/., Nucleic Acids Research, 19: 3019 (1991) (3'-sulfhydryl); Giusti et al, PCRMethods and Applications , 2: 223-227 (1993) and Fung et al , U.S. Pat. No.
  • fluorescent labels can be detected by exciting the fluorophore with the appropriate wavelength of light and detecting the resulting fluorescence.
  • the fluorescence can be detected visually, by means of photographic film, by the use of electronic detectors such as charge coupled devices (CCDs) or photomultipliers and the like.
  • enzymatic labels may be detected by providing the appropriate substrates for the enzyme and detecting the resulting reaction product.
  • the components of the compounds of the invention may be linked through linkage sites formed by reaction of a first and a second reactive functional group.
  • the reactive functional groups are of complementary reactivity, and they react to form a covalent link between two components of the compounds, referred to herein as a linkage site.
  • the formulae set forth herein can be prepared by reacting the amine at the terminus of a precursor to linker L with an activated carbonyl derivative of the quencher under conditions forming an amide between the two reactive functional groups. See, Example 1.
  • a reactive functional group can be reacted with a reactive functional group of complementary reactivity on another component (such as a linker, nucleoside, nucleotide, oligonucleotide, nucleic acid, carrier molecule, and solid support) to covalently join the components through the resulting linkage site.
  • the reactive functional group of complementary reactivity can be located at any position of the other component (linker, nucleoside etc.), e.g., an alkyl or heteroalkyl an aryl or heteroaryl nucleus or a substituent on an aryl or heteroaryl nucleus.
  • the reactive group when the reactive group is attached to an alkyl (or heteroalkyl), or substituted alkyl (or heteroalkyl) chain, the reactive group is preferably located at a terminal position of the chain.
  • Reactive groups and classes of reactions useful in practicing the present invention are generally those that are well known in the art of bioconjugate chemistry.
  • Currently favored classes of reactions available with reactive precursors of the oligomers of the invention are those which proceed under relatively mild conditions. These include, but are not limited to nucleophilic substitutions (e.g. , reactions of amines and alcohols with acyl halides, active esters), electrophilic substitutions (e.g. , enamine reactions) and additions to carbon-carbon and carbon-heteroatom multiple bonds (e.g., Michael reaction, Diels-Alder addition). These and other useful reactions are discussed in, for example, March,
  • reactive functional groups of use in the present invention include, but are not limited to olefins, acetylenes, alcohols, phenols, ethers, oxides, halides, aldehydes, ketones, carboxylic acids, esters, amides, cyanates, isocyanates, thiocyanates, isothiocyanates, amines, hydrazines, hydrazones, hydrazides, diazo, diazonium, nitro, nitriles, mercaptans, sulfides, disulfides, sulfoxides, sulfones, sulfonic acids, sulfinic acids, acetals, ketals, anhydrides, sulfates, sulfenic acids isonitriles, amidines, imides, imidates, nitrones, hydroxylamines, oximes, hydroxamic acids thiohydroxamic acids, allen
  • Reactive functional groups also include those used to prepare bioconjugates, e.g., N- hydroxysuccinimide esters, maleimides and the like. Methods to prepare each of these functional groups are well known in the art and their application to or modification for a particular purpose is within the ability of one of skill in the art (see, for example, Sandler and Karo, eds. ORGANIC FUNCTIONAL GROUP PREPARATIONS, Academic Press, San Diego, 1989).
  • Useful reactive functional group conversions include, for example:
  • carboxyl groups which are readily converted to various derivatives including, but not limited to, active esters (e.g., N-hydroxysuccinimide esters, N- hydroxybenztriazole esters, thioesters, p-nitrophenyl esters), acid halides, acyl imidazoles, alkyl, alkenyl, alkynyl and aromatic esters;
  • active esters e.g., N-hydroxysuccinimide esters, N- hydroxybenztriazole esters, thioesters, p-nitrophenyl esters
  • acid halides e.g., N-hydroxysuccinimide esters, N- hydroxybenztriazole esters, thioesters, p-nitrophenyl esters
  • acid halides e.g., N-hydroxysuccinimide esters, N- hydroxybenztriazole esters, thioesters, p-nitrophenyl esters
  • acyl imidazoles al
  • haloalkyl groups wherein the halide can be later displaced with a nucleophilic group such as, for example, an amine, a carboxylate anion, thiol anion, carbanion, or an alkoxide ion, thereby resulting in the covalent attachment of a new group at the site of the halogen atom;
  • a nucleophilic group such as, for example, an amine, a carboxylate anion, thiol anion, carbanion, or an alkoxide ion
  • dienophile groups which are capable of participating in Diels-Alder reactions such as, for example, maleimido groups;
  • aldehyde or ketone groups such that subsequent derivatization is possible via formation of carbonyl derivatives such as, for example, imines, hydrazones, semicarbazones or oximes, or via such mechanisms as Grignard addition or alkyllithium addition;
  • amine or sulfhydryl groups which can be, for example, acylated, alkylated or oxidized;
  • alkenes which can undergo, for example, cycloadditions, acylation, Michael addition, etc
  • epoxides which can react with, for example, amines and hydroxyl compounds
  • the reactive functional groups are members selected from:
  • R 31 and R 32 are members independently selected from substituted or unsubstituted alkyl, substituted or unsubstituted heteroalkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted heterocycloalkyl, substituted or unsubstituted aryl, substituted or unsubstituted heteroaryl. Also of note are tetrazines and alkenes.
  • the reactive functional groups can react with a corresponding functional group on a target molecule, or the same fluorescent compound, in order to create a fluorescent molecule.
  • target molecules can be polymers or biomolecules, which include, but are not limited to the group consisting of antibody, lipid, protein, peptide, carbohydrate, nucleotides which contain or are derivatized to contain one or more of an amino, sulphydryl, carbonyl, hydroxyl and carboxyl, phosphate and thiophosphate groups, and oxy or deoxy polynucleic acids which contain or are derivatized to contain one or more of an amino, sulphydryl, carbonyl, hydroxyl and carboxyl, phosphate and thiophosphate groups, microbial materials, drugs, toxins, particles, plastics or glass surfaces and polymers.
  • Succinimidyl esters primary amino, secondary amino, hydroxyl
  • exemplary reactive functional groups include, succinimidyl esters, anhydrides, isothiocyantes, thiocyanates, sulfonyl chlorides, sulfonyl fluorides, acid halides, haloacetamides, maleimides and phosphoramidites.
  • the reactive functional groups can be chosen such that they do not participate in, or interfere with, the reactions necessary to assemble the compound of the invention.
  • a reactive functional group can be protected from participating in the reaction by the presence of a protecting group.
  • a protecting group Those of skill in the art understand how to protect a particular functional group such that it does not interfere with a chosen set of reaction conditions.
  • useful protecting groups see, for example, Greene et al,
  • the reactive functional groups can be chosen such that they do not participate in, or interfere with, the reactions necessary to assemble the oligomer of the invention.
  • a reactive functional group can be protected from participating in the reaction by the presence of a protecting group.
  • a protecting group Those of skill in the art understand how to protect a particular functional group such that it does not interfere with a chosen set of reaction conditions.
  • useful protecting groups see, for example, Greene et al.,
  • oligomers of the invention include a reactive functional group moiety which is capable of effecting at least one covalent bond between the oligomer and a target sequence. Multiple covalent bonds can also be formed by providing a multiplicity of such moieties.
  • the covalent bond is preferably to a nucleobase residue in the target strand, but can also be made with other portions of the target, including the sugar or phosphodiester.
  • the reaction nature of the moiety which effects crosslinker determines the nature of the target in the duplex.
  • Preferred crosslinker moieties include acylating and alkylating agents, and, in particular, those positioned relative to the sequence specificity-conferring portion so as to permit reaction with the target location in the strand.
  • the crosslinker moiety can conveniently be placed as an analogous pyrimidine or purine residue in the sequence of the oligomer.
  • the placement can be at the 5'- and/or 3'- ends, the internal portions of the sequence, or combinations of the above. Placement at the termini to permit enhanced flexibility is preferred.
  • Analogous moieties can also be attached to peptide backbones.
  • Exemplary of alkylating moieties that are useful in the invention include N 4 ,N 4 - ethanocytosine and N 6 ,N 6 -ethanoadenine.
  • nucleobase need not be a purine or pyrimidine; indeed the moiety to which the reactive function is attached need not be a nucleobase at all and may be a sugar, a linker, a quencher, a stabilizing moiety a fluorophore or some combination of these components of the oligomers of the invention. Any means of attaching the reactive group is satisfactory so long as the positioning is correct.
  • phosphoramidites and oligomers of the invention or the segments thereof) are generally conventionally synthesized. See, for example, U.S. Patent No. 7,019,129; U.S. Patent No. 8,466,266; and U.S. Patent No. 7,879,986.
  • the synthetic methods known in the art and described herein can be used to synthesize oligomers containing compounds of the invention, as well as other nucleobases known in the art, using appropriately protected
  • Example 1 An exemplary synthesis of various compounds of the invention is set forth in Example 1.
  • nucleomonomers are directly incorporated into oligomers or a convenient fragment thereof using standard synthesis conditions and reagents.
  • Exemplary linkages made by this method include phosphodiester, phosphorothioate, phosphoroamidate, methylphosphonate, phosphorodithioate, carbonate, morpholino carbamate and sulfonate.
  • synthesis involves synthesis of short synthons (dimers, trimers, etc.) starting with an appropriate precursor. This approach is suitable for synthesis of linkages including N-methylhydroxylamine, dimethylhydrazo, sulfamate, carbamate, sulfonate, sulfonamide, formacetal thioformacetal and carbonate.
  • Oligomers of the invention can be synthesized by any suitable chemistry including amidite, triester or hydrogen phosphonate coupling methods and conditions. The oligomers are preferably synthesized from appropriate starting synthons which are preferably protected at the 5'-position with DMT, MMT, FMOC (9-fluorenylmethoxycarbonyl), PACO
  • phenoxyacetyl a silyl ether such as TBDMS (t-butyldiphenylsilyl) or TMS (trimethylsilyl) and activated at the 3 '-position is an ester, H-phosphonate, an amidite such as ⁇ - cyanoethylphosphoramidite, a silyl ether such as TBDMS or TMS or t-butyldiphenyl.
  • appropriate uridine or cytidine precursors such as blocked 5-iodo-2'- deoxyuridine, 5-iodo-2'-0-alkyluridine, 5 -bromo-2'-deoxy uridine, 5- trifluoromethanesulfonate-2'-deoxyuridine, 5-bromo-2'-0-alkyluridine or blocked and protected 5-iodo-2'-deoxy cytidine, 5-bromo-2'-deoxy cytidine, 5-trifluoromethanesulfonate-2'- deoxy cytidine, 5-iodo-2'-0-alkylcytidine, 5-bromo-2'-0-alkylcytidine can be conveniently incorporated into short oligomers such as dimer, trimer, tetramer, pentamer or longer synthons that are subsequently derivatized to yield suitable synthons and longer oligomers.
  • Exemplary synthesis of oligomers containing about 4 or more nucleomonomer residues are accomplished using synthons such as monomers, dimers or trimers that carry a coupling group suitable for use with amidite, H-phosphonate or triester chemistries.
  • the synthon can be used to link the components of the oligomer via a phosphodiester or phosphorous-containing linkage other than phosphodiester (e.g., phosphorothioate, methylphosphonate, thionomethylphosphonate, phosphoramidate and the like).
  • the desired nucleic acid is synthesized, it is preferably cleaved from the solid support on which it was synthesized and treated, by methods known in the art, to remove any protecting groups present (e.g., 60 °C, 5h, concentrated ammonia).
  • the deprotection will preferably use milder conditions (e.g., butylamine: water 1 :3, 8 hours, 70 °C).
  • the nucleic acid is purified by any method known in the art, including chromatography, extraction and gel purification. In a preferred embodiment, the nucleic acid is purified using HPLC. The concentration and purity of the isolated nucleic acid is preferably determined by measuring the optical density at
  • the present invention provides quenchers and an oligomers including one or more of these quenchers, or formed from one or more of these quenchers, which are of use in one or more assay formats.
  • the oligomer participates in the generation of a detectable signal upon association with or dissociation from its target.
  • the oligomeric probes of the invention are not limited in use to any particular assay format. Accordingly, the following description is intended to illustrate exemplary assays formats in which the oligomers of the invention find use, and is not intended to be limiting of the assay formats in which the oligomers are of use.
  • a target molecule such as, for example, a nucleic acid of unknown quantity
  • the intensity of fluorescence emission from each of the reference mixtures is used to derive a graph or standard curve, in which the unknown concentration is compared to the intensity of the known standards.
  • a probe that: a) hybridizes to a sequence within the target nucleic acid; b) has fluorophore and quencher modifications upon the 5' and 3' termini being the sites of labeling; and c) has fluorogenic character that is quenched in an unbound conformation and then releases signal upon binding to the target nucleic acid, can be used to obtain such reference data.
  • a probe gives a characteristic fluorescence emission in which the signal increases as the concentration of target nucleic acid increases. Then, a sample with an unknown quantity of target is contacted with the probe, and the fluorescence intensity from the mixture is determined. The intensity of fluorescence emission is then compared with the reference standards to obtain the concentration of the target in the test mixture.
  • the solid supports and oligomers of the invention are utilized as a probe or a component of one or more probes used in a multiplex assay for detecting one or more species in a mixture.
  • Probes based on the solid supports or oligomers of the invention are particularly useful in performing multiplex-type analyses and assays. In a typical multiplex analysis, two or more distinct species (or regions of one or more species) are detected using two or more probes, wherein each of the probes is labeled with a different fluorophore.
  • Preferred species used in multiplex analyses relying on donor-acceptor energy transfer meet at least two criteria: the fluorescent species is bright and spectrally well-resolved; and the energy transfer between the fluorescent species and the quencher is efficient.
  • the solid supports and oligomers of the invention allow for the design of multiplexed assays in which more than one fluorescent reporter is partnered with one or more quencher structures.
  • a number of different multiplexed assays using the solid supports or oligomers of the invention will be apparent to one of skill in the art.
  • each of at least two distinct fluorescent reporters are paired with the same type of quencher structure on their respective oligomers, to modulate the signal through either FRET or contact quenching.
  • an assay can be practiced in which at least two distinct fluorescent reporters are partnered with distinct quencher structures, to which the fluorescent properties are better "matched."
  • the fluorophores can be bound to the same molecule as the quencher or to a different molecule.
  • the carrier molecules of use in a particular assay system such as the oligo sequence that covelently tethers the fluorophore and quencher, can either be the same or different.
  • the present invention also provides a qualitative method for detecting the presence a particular molecular species.
  • the method includes: (a) contacting the species with a mixture containing a solid support or oligomer of the invention; and (b) detecting a change in a fluorescent property of one or more component of the resulting mixture, thereby detecting the presence the molecular species.
  • the quenchers of the present invention can be used in multiplex assays designed to detect and/or quantify substantially any species, including, for example, whole cells, viruses, proteins (e.g., enzymes, antibodies, receptors), glycoproteins, lipoproteins, subcellular particles, organisms (e.g., Salmonella), nucleic acids (e.g., DNA, RNA, and analogues thereof), polysaccharides, lipopolysaccharides, lipids, fatty acids, non-biological polymers and small molecules (e.g., toxins, drugs, pesticides, metabolites, hormones, alkaloids, steroids).
  • proteins e.g., enzymes, antibodies, receptors
  • glycoproteins e.g., lipoproteins, subcellular particles
  • organisms e.g., Salmonella
  • nucleic acids e.g., DNA, RNA, and analogues thereof
  • polysaccharides e.g., lipopolysaccharides, lipids
  • nucleic Acid Probes [00149]
  • the solid supports and oligomers of the invention are useful nucleic-acid probes and they can be used as components of detection agents in a variety of DNA
  • amplification/quantification strategies including, for example, 5 '-nuclease assay, Strand Displacement Amplification (SDA), Nucleic Acid Sequence-Based Amplification (NASBA), Rolling Circle Amplification (RCA), as well as for direct detection of targets in solution phase or solid phase (e.g., array) assays.
  • the solid supports and oligomers can be used in probes of substantially any format, including, for example, format selected from molecular beacons, Scorpion probesTM, Sunrise probesTM, conformationally assisted probes, light up probes, Invader Detection probes, and TaqManTM probes. See, for example, Cardullo, R, et al. , Proc. Natl. Acad. Sci.
  • the present invention provides a method for detecting a nucleic acid target sequence.
  • the method includes: (a) contacting the target sequence with a detector nucleic acid (e.g., an oligomer of the invention); (b) hybridizing the target binding sequence to the target sequence, thereby altering the conformation of the detector nucleic acid, causing a change in a fluorescence parameter; and (c) detecting the change in the fluorescence parameter, thereby detecting the nucleic acid target sequence.
  • a detector nucleic acid e.g., an oligomer of the invention
  • a preferred detector nucleic acid includes a single-stranded target binding sequence.
  • the binding sequence has linked thereto: i) a fluorophore; and ii) a quencher.
  • the binding sequence has optionally further linked thereto a stabilizing moiety.
  • the detector nucleic acid prior to its hybridization to a complementary sequence, is preferably in a conformation that allows donor-acceptor energy transfer between the fluorophore and the quencher when the fluorophore is excited.
  • a change in fluorescence is detected as an indication of the presence of the target sequence. The change in fluorescence is preferably detected in-real time.
  • the detector nucleic acid can assume substantially any intramolecularly associated secondary structure, but this structure is preferably a member selected from hairpins, stem-loop structures, pseudoknots, triple helices and conformationally assisted structures.
  • the intramolecularly base-paired secondary structure preferably comprises a portion of the target binding sequence.
  • the invention provides a method for detecting amplification of a target sequence.
  • the method involves the use of an amplification reaction such as PCR.
  • An exemplary amplification reaction includes one or more of the following steps:
  • a single stranded target binding sequence that is complementary to at least a portion of the sense or antisense strand of the target sequence in the PCR product, and hybridizes to a region between the PCR primers;
  • the detector nucleic acid is in a conformation allowing donor-acceptor energy transfer between the fluorophore and the quencher when the fluorophore is excited;
  • the conformation of the detector nucleic acid for example, linearizing any secondary structure or random coil conformations that contribute to the quenching efficiency, causing a change in a fluorescence parameter (such as the signal intensity); and (d) measuring the change in the fluorescence parameter to detect the target sequence and its amplification.
  • the change in the fluorescence parameter can be made permanent if the polymerase encounters the hybridized detector nucleic acid during primer extension (step (b) above) and hydrolyzes the oligomer tethering the fluorophore and quencher, such as through a secondary nuclease activity of the polymerase.
  • the invention provides a method of ascertaining whether a first nucleic acid and a second nucleic acid hybridize.
  • the first nucleic acid is an oligomer (in solution or attached to a solid support) according to the invention.
  • the method includes: (a) contacting the first nucleic acid with the second nucleic acid; (b) detecting an alteration in a fluorescent property of a member selected from the first nucleic acid, the second nucleic acid and a combination thereof, thereby ascertaining whether the hybridization occurs.
  • the present invention provides probes and methods of use in detecting polymorphism in nucleic acid target sequences.
  • Polymorphism refers to the occurrence of two or more genetically determined alternative sequences or alleles in a population.
  • a polymorphic marker or site is the locus at which divergence occurs.
  • Preferred markers have at least two alleles, each occurring at frequency of greater than 1 %, and more preferably greater than 10% or 20% of a selected population.
  • a polymorphic locus may be as small as one base pair.
  • Polymorphic markers include restriction fragment length
  • allelic form is arbitrarily designated as the reference form and other allelic forms are designated as alternative or variant alleles.
  • allelic form occurring most frequently in a selected population is sometimes referred to as the wildtype form. Diploid organisms may be homozygous or heterozygous for allelic forms.
  • a diallelic polymorphism has two forms.
  • a triallelic polymorphism has three forms.
  • a probe of the invention is utilized to detect a single nucleotide polymorphism.
  • a single nucleotide polymorphism occurs at a polymorphic site occupied by a single nucleotide, which is the site of variation between allelic sequences. The site is usually preceded by and followed by highly conserved sequences of the allele (e.g., sequences that vary in less than 1/100 or 1/1000 members of the populations).
  • a single nucleotide polymorphism usually arises due to substitution of one nucleotide for another at the polymorphic site.
  • a transition is the replacement of one purine by another purine or one pyrimidine by another pyrimidine.
  • a transversion is the replacement of a purine by a pyrimidine or vice versa.
  • Single nucleotide polymorphisms can also arise from a deletion of a nucleotide or an insertion of a nucleotide relative to a reference allele.
  • An oligomer of the invention bearing both a quencher and a fluorophore can be used or, alternatively, one or more of the nucleic acids can be singly labeled with a single member of an energy transfer pair (e.g. a quencher or fluorophore).
  • a nucleic acid singly labeled with a quencher is the probe, the interaction between the first and second nucleic acids can be detected by observing the interaction between the quencher and the nucleic acid or, more preferably, the quenching by the quencher of the fluorescence of a fluorophore attached to the second nucleic acid.
  • compositions and methods of the invention are of use for mutation
  • a diallelic organism contains two copies of each gene.
  • Genotyping involves the determination of whether a diallelic organism contains two copies of the reference allele (a reference-type homozygote), one copy each of the reference and variant allele (i.e., a heterozygote), or contains two copies of the variant allele (i.e., a variant-type homozygote).
  • the methods of the invention can be utilized to determine a single variant site (e.g., a SNP or a tandem repeat).
  • the methods can also be used to determine allelic frequency in a group of individuals, as well as the genotype of an individual in many different DNA loci, either on the same gene, different genes or combinations thereof.
  • SNPs consist of two allelic forms, i.e., the variant site includes one of two different nucleotides.
  • the sample can contain nucleic acids representative of the two copies of the target nucleic acid of interest. Analyses can be conducted with a single labeled nucleotide, but more typically labeled nucleotides complementary to both nucleotides potentially at the site of variation are utilized.
  • the amplification of the allele containing a complementary nucleotide at the variation site would produce a labeled amplified product, while the other allele not containing a complementary nucleotide at the variation site would not produce a labeled amplification product. Therefore, if the polynucleotide template is from a homozygote, it will give rise to a determinable level of label incorporation (i.e., if both allele containing a complementary nucleotide at the variation site), or no incorporation at all (i.e., if both allele not containing a complementary nucleotide at the variation site).
  • An intermediate level of label incorporation would indicate that the nucleotide template is derived from a heterozygote. If two labeled nucleotides are used in the reaction mixture (i.e., each labeled nucleotide may be incorporated into a different allele), the formation of a single labeled amplified product (i.e., reflected by the incorporation frequency) indicates that the sample is from a homozygote. The particular label signifies whether the sample is from a reference-type or variant-type homozygote. The existence of two labeled amplified products indicates that the sample is from a heterozygote.
  • Reactions can be conducted separately such that each labeled nucleotide is added to a different reaction mix, or reactions can be conducted in a single reaction mixture containing both labeled nucleotides. If reactions are conducted in a single reaction vessel, the labeled nucleotides are differentially labeled so that the different allelic forms can be distinguished. If different reactions are conducted with each labeled nucleotide, the labels for each labeled nucleotide can be the same or different since the particular nucleotide added to each reaction is tracked.
  • nucleotides that include more than two allelic forms
  • additional labeled nucleotides can be used.
  • three differentially labeled nucleotides can be used.
  • four differentially labeled nucleotides can be employed.
  • all the nucleotides can be added to a single reaction mixture or to separate reaction mixtures.
  • any additional nucleotides are provided as mixtures of labeled and unlabeled forms.
  • the ability to use the methods of the invention to make rapid genotyping determinations provides a powerful tool in genetic analysis and ascertaining the susceptibility of an individual to a disease. Individuals that are mutant homozygotes for an allele associated with a particular disease are at higher risk of having the disease than a
  • the invention provides a method for determining a sequence difference between a region of interest in a polynucleotide and a reference sequence.
  • the method includes: a) incubating the polynucleotide in a reaction mixture comprising a nucleotide labeled with a detectable label and/or a quencher of the invention to produce a polynucleotide product from the polynucleotide; b) determining an incorporation frequency of the labeled nucleotide and/or the quencher of the invention for the
  • step (b) comparing the incorporation frequency determined in step (b) with a known frequency for the reference sequence, wherein a difference in the two frequencies is indicative of a sequence difference between the region of interest of the polynucleotide and the reference sequence.
  • step (b) comprises detecting the incorporation of said labeled nucleotide into the polynucleotide product.
  • step (b) comprises measuring the signal from incorporated labeled nucleotides and measuring the amount of the polynucleotide product.
  • step (b) comprises measuring the signal from incorporated labeled nucleotides, measuring the amount of the polynucleotide product, and expressing the resulting values as a ratio of signal from incorporated nucleotides over the amount of the polynucleotide product.
  • the step of determining a relative incorporation frequency comprises computing the ratio of the signal generated by the incorporated labeled nucleotide and the signal generated by said polynucleotide stain.
  • the labeled nucleotide comprises a signal generating moiety and a quencher of the invention, wherein the quencher quenches the signal from the signal generating moiety when both these moieties are present on the labeled nucleotide.
  • the quencher of the invention is separated from the labeled nucleotide upon incorporation of the labeled nucleotide into said polynucleotide product.
  • the invention also provides a method for determining the presence of a mutation in a region of interest in a polynucleotide.
  • the method includes: a) incubating the
  • polynucleotide in a reaction mixture comprising a nucleotide labeled with a detectable label and/or a quencher of the invention, to produce a polynucleotide product from the
  • step (b) determining an incorporation frequency of the labeled nucleotide for the polynucleotide product; and c) comparing the incorporation frequency determined in step (b) with a known frequency for a reference wild-type sequence, wherein a difference in the two frequencies is indicative of the presence of a mutation in a region of interest in a
  • the invention further provides a method for genotyping comprising: a) incubating in a reaction mixture a first nucleic acid sample comprising a region of interest, the reaction mixture comprising a nucleotide labeled with a detectable label and a quencher of the invention to produce a polynucleotide product from the nucleic acid sample; and b) determining an incorporation frequency of the labeled nucleotide for said polynucleotide product, wherein the ascertained incorporation frequency is indicative of the genotype of the organism from which the nucleic acid sample was obtained.
  • a ground state complex between a quencher of the invention and a fluorophore is formed.
  • both the quencher and fluorophore are conjugated to the same nucleic acid oligomer.
  • the present solid supports and oligomers can be used in substantially any nucleic acid probe format now known or later discovered.
  • the solid supports and oligomers of the invention can be incorporated into probe motifs, such as TaqmanTM probes (Held et al., Genome Res. 6: 986- 994 (1996), Holland et al, Proc. Nat. Acad. Sci. USA 88: 7276-7280 (1991), Lee et al., Nucleic Acids Res. 21: 3761-3766 (1993)), molecular beacons (Tyagi et al., Nature
  • the oligomers for use in the probes of the invention can be any suitable size, and are preferably in the range of from about 2 to about 100 nucleotides, more preferably from about 10 to about 80 nucleotides and more preferably still, from about 10 to about 40 nucleotides.
  • the donor moiety is preferably separated from the quencher by at least about 6, preferably at least about 8, preferably at least about 10 nucleotides, and more preferably by at least about 15 nucleotides.
  • donor moiety is preferably attached to either the 3'- or 5 '-terminal nucleotides of the probe.
  • the quencher moiety is also preferably attached to either the 3'- or 5 '-terminal nucleotides of the probe. More preferably, the donor and acceptor moieties are attached to the 3'- and 5'- or 5'- and 3'-terminal nucleotides of the probe, respectively, although internal placement is also useful.
  • nucleic acid probe of the invention depends in part on the nature of the target polynucleotide to which it binds.
  • the binding location and length may be varied to achieve appropriate annealing and melting properties for a particular embodiment.
  • Guidance for making such design choices can be found in many art-recognized references.
  • the 3'-terminal nucleotide of the nucleic acid probe is blocked or rendered incapable of extension by a nucleic acid polymerase. Such blocking is conveniently carried out by the attachment of a donor or acceptor moiety to the terminal 3'- position of the nucleic acid probe, either directly or by a linker moiety.
  • the nucleic acid can comprise DNA, RNA or chimeric mixtures or derivatives or modified versions thereof. Both the probe and target nucleic acid can be present as a single strand, duplex, triplex, etc. Moreover, the nucleic acid can be modified at the nucleobase moiety, sugar moiety, or phosphate backbone with other groups such as radioactive labels, minor groove binders, intercalating agents, acetylinically unsaturated hydrocarbons, fluoralkyl groups, donor and/or acceptor moieties and the like.
  • the oligomers of the invention are useful as primers that are discrete sequences or as primers with a random sequence.
  • Random sequence primers are generally about 6 or 7 nucleomonomers in length.
  • Such primers can be used in various nucleic acid amplification protocols (PCR, ligase chain reaction, etc) or in cloning protocols. Substitutions on the 5' end of the invention generally do not interfere with the capacity of the oligomer to function as a primer.
  • Oligomers of the invention having 2'-modifications at sites other than the 3' terminal residue, other modifications that render the oligomer RNase H incompetent or otherwise nuclease stable can be advantageously used as probes or primers for RNA or DNA sequences in cellular extracts or other solutions that contain nucleases.
  • the oligomers can be used in protocols for amplifying nucleic acid in a sample by mixing the oligomer with a sample containing target nucleic acid, followed by hybridization of the oligomer with the target nucleic acid and amplifying the target nucleic acid by PCR, LCR or other suitable methods.
  • oligomers derivatized with chelating agents such as EDTA, DTP A or analogs of 1,2-diaminocyclohexane acetic acid can be utilized in various in vitro diagnostic assays as described (U. S. Pat. Nos. 4,772,548, 4,707,440 and 4,707,352).
  • oligomers of the invention can be derivatized with crosslinker agents such as 5-(3-iodoacetamidoprop-l - yl)-2'-deoxyuridine or 5-(3-(4-bromobutyramido)prop-l -yl)-2'-deoxyuridine and used in various assay methods or kits as described (International Publication No.
  • WO 90/14353 the ability of the oligomers to inhibit gene expression can be verified in in vitro systems by measuring the levels of expression in subject cells or in recombinant systems, by any suitable method (Graessmann, M., et al, Nucleic Acids Res. (1991) 19:53-59).
  • Conditions that favor hybridization between oligomer of the present invention and target nucleic acid molecules can be determined empirically by those skilled in the art, and can include optimal incubation temperatures, salt concentrations, length and nucleobase compositions of oligonucleotide analogue probes, and concentrations of oligomer and nucleic acid molecules of the sample.
  • hybridization is performed in the presence of at least one millimolar magnesium and at a pH that is above 6.0.
  • incorporating nonstandard nucleotide analogs into the oligomer of the present invention can increase or decrease the salt dependence of hybridization.
  • This modulation can be used to advantage in the methods of the present invention where it can in some aspects be desirable to be able to increase the stringency of hybridization by changing salt conditions, for example, or release a hybridized nucleic acid by reducing the salt concentration.
  • oligomers of the present invention in binding to target nucleic acid molecules allow the practitioner to select hybridization conditions that can favor discrimination between nucleic acid sequences that comprise a stretch of sequence that is completely complementary to at least a portion of one or more oligomer and target nucleic acid molecules that comprise a stretch of sequence that comprises a small number of non- complementary nucleobases within a substantially complementary sequence.
  • hybridization or wash temperatures can be selected that permit stable hybrids between oligomer of the present invention and target nucleic acid molecules that are completely complementary along a stretch of sequence but promote dissociation of hybrids between oligomer of the present invention and target nucleic acid molecules that are not completely complementary, including those that comprise one or two nucleobase mismatches along a stretch of complementary sequence.
  • the selection of a temperature for hybridization and washes can be dependent, at least in part, on other conditions, such as the salt concentration, the concentration of oligomer and target nucleic acid molecules, the relative proportions of oligomer to target nucleic acid molecules, the length of the oligomers to be hybridized, the nucleobase composition of the oligomer and target nucleic acid molecules, the monomer composition of the oligonucleotide analogue molecules, etc.
  • additional conditions can be taken into account, and, where desirable, altered, including but not limited to, the length of the oligonucleotide analogue to be hybridized, the length of the stretch of sequence of complementarity between oligomer and target nucleic acid molecules, the number of non-complementary nucleobases within a stretch of sequence of complementarity, the identity of mismatched nucleobases, the identity of nucleobases in the vicinity of the mismatched nucleobases, and the relative position of any mismatched nucleobases along a stretch of complementarity.
  • “Favorable conditions” can be those favoring stable hybrids between oligomer and target nucleic acid molecules that are, at least in part, substantially complementary, including those that comprise one or more mismatches. [00181] "Favorable conditions” can be those favoring stable hybrids between oligomer and target nucleic acid molecules that are, at least in part, completely complementary and disfavor or destabilized hybrids between molecules that are not completely complementary.
  • the melting temperature of oligomer of the present invention hybridized to target nucleic acid molecules of different sequences can be determined and can be used in determining favorable conditions for a given application. It is also possible to empirically determine favorable hybridization conditions by, for example, hybridizing target nucleic acid molecules to oligomer that are attached to a solid support and detecting hybridized complexes.
  • Target nucleic acid molecules that are bound to solid supports or oligomeric probes of the present invention can be conveniently and efficiently separated from unbound nucleic acid molecules of the survey population by the direct or indirect attachment of oligomer probes to a solid support.
  • a solid support can be washed at high stringency to remove nucleic acid molecules that are not bound to oligomer probes.
  • the attachment of oligomer probes to a solid support is not a requirement of the present invention.
  • bound and unbound nucleic acid molecules can be separated by centrifugation through a matrix or by phase separation or some by other forms of separation (for example, differential precipitation) that can optionally be aided by chemical groups incorporated into the oligomer probes (see, for example, U.S. Pat. No. 6,060,242 issued May 9, 2000, to Nie et al).
  • an immobilized nucleic acid comprising a quencher is used as a capture probe.
  • the immobilized nucleic acid optionally further comprises a stabilizing moiety.
  • the nucleic acid probe can be attached directly to a solid support, for example by attachment of the 3'- or 5 '-terminal nucleotide of the probe to the solid support. More preferably, however, the probe is attached to the solid support by a linker ⁇ supra).
  • the linker serves to distance the probe from the solid support.
  • the linker is most preferably from about 5 to about 30 atoms in length, more preferably from about 10 to about 50 atoms in length.
  • the solid support is also used as the synthesis support in preparing the oligomer (probe).
  • the length and chemical stability of the linker between the solid support and the first 3 '-unit of nucleic acid play an important role in efficient synthesis and hybridization of support bound nucleic acids.
  • the linker arm is preferably sufficiently long so that a high yield (> 97%) can be achieved during automated synthesis.
  • the required length of the linker will depend on the particular solid support used. For example, a six atom linker is generally sufficient to achieve a > 97% yield during automated synthesis of nucleic acids when high cross-linked polystyrene is used as the solid support.
  • the linker arm is preferably at least 20 atoms long in order to attain a high yield ( > 97%) during automated synthesis when CPG is used as the solid support.
  • Hybridization of a probe immobilized on a solid support generally requires that the probe be separated from the solid support by at least 30 atoms, more preferably at least 50 atoms.
  • the linker generally includes a spacer positioned between the linker and the 3 '-terminus.
  • the linker arm is usually attached to the 3'-OH of the 3 '-terminus by an ester linkage which can be cleaved with basic reagents to free the nucleic acid from the solid support.
  • linkers are known in the art, which may be used to attach the nucleic acid probe to the solid support.
  • the linker may be formed of any compound, which does not significantly interfere with the hybridization of the target sequence to the probe attached to the solid support.
  • the linker may be formed of, for example, a homopolymeric nucleic acid, which can be readily added on to the linker by automated synthesis.
  • polymers such as functionalized polyethylene glycol can be used as the linker.
  • Such polymers are presently preferred over homopolymeric nucleic acids because they do not significantly interfere with the hybridization of probe to the target nucleic acid.
  • Polyethylene glycol is particularly preferred because it is commercially available, soluble in both organic and aqueous media, easy to functionalize, and completely stable under nucleic acid synthesis and post-synthesis conditions.
  • linkages sites between the solid support, the linker and the probe are preferably not cleaved during synthesis or removal of nucleobase protecting groups under basic conditions at high temperature. These linkages can, however, be selected from groups that are cleavable under a variety of conditions. Examples of presently preferred linkages include carbamate, ester and amide linkages.
  • Quenchers and oligomers of the present invention can be used for detection of nucleic acids. Such detection methods include: providing a sample, contacting at least one oligonucleotide analogue of the present invention with the sample under conditions that allow hybridization of oligomer to nucleic acid molecules, and detecting one or more nucleic acid molecules of the sample that have hybridized to one or more oligomer of the present invention.
  • a sample can be from any source, and can be a biological sample, such as a sample from an organism or a group of organisms from the same or different species.
  • a biological sample can be a sample of bodily fluid, for example, a blood sample, serum sample, lymph sample, a bone marrow sample, ascites fluid, pleural fluid, pelvic wash fluid, ocular fluid, urine, semen, sputum, or saliva.
  • a biological sample can also be an extract from cutaneous, nasal, throat, or genital swabs, or extracts of fecal material.
  • Biological samples can also be samples of organs or tissues, including tumors.
  • Biological samples can also be samples of cell cultures, including both cell lines and primary cultures of both prokaryotic and eukaryotic cells.
  • a sample can be from the environment, such as from a body of water or from the soil, or from a food, beverage, or water source, an industrial source, workplace area, public area, or living area.
  • a sample can be an extract, for example a liquid extract of a soil or food sample.
  • a sample can be a solution made from washing or soaking, or suspending a swab from, articles such as tools, articles of clothing, artifacts, or other materials.
  • a sample can be an unprocessed or a processed sample; processing can involve steps that increase the purity, concentration, or accessibility of components of the sample to facilitate the analysis of the sample.
  • processing can include steps that reduce the volume of a sample, remove or separate components of a sample, solubilize a sample or one or more sample components, or disrupt, modify, expose, release, or isolate components of a sample.
  • Nonlimiting examples of such procedures are centrifugation, precipitation, filtration, homogenization, cell lysis, binding of antibodies, cell separation, etc.
  • the sample is a blood sample that is at least partially processed, for example, by the removal of red blood cells, by concentration, by selection of one or more cell or virus types (for example, white blood cells or pathogenic cells), or by lysis of cells, etc.
  • Exemplary samples include a solution of at least partially purified nucleic acid molecules.
  • the nucleic acid molecules can be from a single source or multiple sources, and can comprise DNA, RNA, or both.
  • a solution of nucleic acid molecules can be a sample that was subjected to any of the steps of cell lysis, concentration, extraction, precipitation, nucleic acid selection (such as, for example, poly A RNA selection or selection of DNA sequences comprising Alu elements), or treatment with one or more enzymes.
  • the sample can also be a solution that comprises synthetic nucleic acid molecules.
  • An oligomer or solid support of the present invention can be any oligomer format disclosed herein, or any oligomer comprising a monomer, dimer or non nucleic acid component (e.g., linker, fluorophore, quencher, stabilizing moiety) disclosed herein.
  • An oligonucleotide analogue used in the methods of the present invention can be of any length and of any nucleobase composition, and can comprise one or more nucleic acid moieties, peptides, proteins lipids, carbohydrates, steroids, and other biochemical and chemical moieties.
  • An oligonucleotide analogue of the present invention can be provided in solution or bound to a solid support. In some preferred embodiments of the present invention, the oligomer comprise non-standard nucleotide analogues.
  • Detection methods for bound nucleic acids are well known in the art, and can include the use of a detectable label that is attached to or incorporated into nucleic acid molecules of the survey population or that becomes bound to or incorporated into a hybridized target nucleic acid molecule or hybridized target nucleic acid molecule complex.
  • Detectable labels for nucleic acid molecules are well-known in the art, and comprise fluorescent molecules such as fluorophores (including those set forth herein), radioisotopes, mass-altered chemical groups, specific binding members such as biotin that can be detected by signal-generating molecules, and the like.
  • Detectable labels can also be incorporated into or attached to oligomer of the present invention, for example, in cases where sandwich hybridization using a signal oligomer is used for detection, or detection is performed using a specific binding member such as an antibody that recognizes oligomer/target nucleic acid molecule complexes.
  • Solid supports can be scanned, exposed to film, visually inspected, etc. to determine the presence of a detectable label and thereby determine the binding of a target nucleic acid molecule to an oligomer immbolized on a solid support such as those of the invention.
  • kits that facilitate the practice of syntheses using the compounds of the invention (such as solid supports of the invention or monomers of the invention) and assays using quenchers of the invention and oligomers of the invention, as described above.
  • the kits of the invention typically comprise a compound of the invention (such as a solid support of the invention or an oligomer of the invention), either present as a chemically reactive species useful for preparing conjugates, or present as a completed oligomer where the oligomer is a specific binding pair member.
  • the kit optionally further comprises one or more buffering agents, typically present as an aqueous solution.
  • kits of the invention optionally further comprise additional detection reagents, a purification medium for purifying the resulting labeled substance, luminescence standards, enzymes, enzyme inhibitors, organic solvent, or instructions for carrying out an assay of the invention.
  • additional detection reagents e.g., a labeled substance
  • purification medium for purifying the resulting labeled substance
  • luminescence standards e.g., luminescence standards
  • enzymes e.g., enzyme inhibitors, organic solvent, or instructions for carrying out an assay of the invention.
  • Other formats for kits will be apparent to those of skill in the art and are within the scope of the present invention.
  • the materials and methods of the present invention are further illustrated by the examples which follow. These examples are offered to illustrate, but not to limit the claimed invention.
  • BHQIO-dUTP 1.3 umol (65%) yield.
  • BHQlO-dCTP 1.4 umol (70%) yield.
  • BHQIO-ddCTP 1.6 umol (80%) yield.
  • BHQIO-dATP 1.3 umol (65%) yield.
  • BHQIO-ddATP 1.5 umol (74%) yield.
  • BHQIO-dGTP 1.5 umol (74%) yield.
  • BHQIO-UTP 0.9 umol (45%) yield.
  • M13 Forward Primer (5'- GTTTTCCCAGTCACGAC-3') and M13 Reverse Primer (5'- GGAAAC AGCTATGACC ATG-3 ' ) were diluted to 10 ⁇ working concentration each.
  • the M13 Forward and M13 Reverse primers bind to the circular plasmid DNA template to amplify a 388 bp double stranded DNA product of sequence 5'- GGAAACAGCTATGACCATGATTACGCCAAGCGCGCAATTAACCCTCACTAAAGG GAACAAAAGCTGGAGCTGCGGCCGCGAGCTTTGACAAAGTCGGTTATCCAGACT TTGTCAGCGTACCGAGCTCTGGGATTTAGGTGACACTATAGGGCAACTACAAGAC CCGCGCCGGTTTTAGAGCTAGAAATAGCAAGTTAAAATAAGGCTAGTCCGTTATC AACTTGAAAAAGTGGCACCGAGTCGGTGCTTTTTACGTAGGCCTCCTCCAGGT ACCAGCGGCCGCGTCGACAAGCTTATGC
  • PCR reactions in a 50 ⁇ final volume each contained a final concentration of IX PCR Buffer, supplemented with 1.5 mM MgCl 2 , 0.2 ⁇ M13 Forward Primer, 0.2 ⁇ M13 Reverse Primer, 10 ng plasmid DNA, 2.5 Units Taq DNA Polymerase, and 200 ⁇ of each dNTPs except as indicated in Table 3 below.
  • PCR Cycle Conditions are as follow: Initial Denature 95°C 2 minutes; 25 cycles of Denature 95°C 30 seconds, Anneal 42°C 30 seconds, Extension 68°C 30 seconds; Final Extension 68°C 5 minutes.
  • FIG. 8 shows the capillary gel electrophoresis analysis of the desalted PCR products. Reaction 1, 5, 9, and 13 are the controls of unlabeled double stranded DNA
  • dsDNA dsDNA PCR product.
  • BHQIO-dNTPs were tested at 0% (control), 10%, 5%, and 1% of their corresponding dNTP's final concentration.
  • Taq DNA Polymerase is able to incorporate various BHQIO-dNTP into the full length product.
  • BHQ10 labeled dsDNA has a higher molecular weight than unlabeled dsDNA, and thus migrates slower in capillary gel electrophoresis than unlabeled dsDNA (control reactions). Since each dsDNA fragment from the reactions with BHQIO-dNTP has a variable content of BHQIO-dNMP, a blurred band is expected, and was indeed observed.
  • Higher concentrations of BHQIO-dNTPs in the PCR reaction leads to a higher incorporation rate with a subsequent slower migration of the product in the capillary gel electrophoresis.
  • Taq DNA Polymerase with supplied 10 X PCR Buffer (New England Biolabs Cat. No. M0320L) was used for all DNA Polymerase linear amplification reactions.
  • the following dilutions were performed with molecular grade water (Fisher
  • Each BHQIO-dUTP, BHQIO-dATP, BHQIO-dCTP, and BHQIO-dGTP was diluted to a working concentration 100 ⁇ .
  • Individual dATP, dTTP, dGTP, and dCTP (Fermentas Cat No. R0182) were diluted to both 2.5 mM and 1.0 mM working solutions.
  • Plasmid DNA Template (Biosearch Lot No. GST205_4c-SP6) was diluted to 10 ng / ⁇ .
  • Ml 3 Forward Primer (5'- GTTTTCCC AGTC ACGAC-3 ') and Ml 3 Reverse Primer (5'- GGAAAC AGCTATGACC ATG-3 ' ) were diluted to 10 ⁇ working concentration each.
  • the Ml 3 Forward primer anneals to the circular plasmid DNA template to primer the amplification of a single-stranded DNA product, terminated as a BHQIO-ddATP or BHQIO-ddCTP is incorporated.
  • the M13 Reverse primer anneals to the plasmid DNA template to prime the amplification of a single-stranded DNA product, terminated as a BHQIO-ddATP or BHQ10- ddCTP is incorporated.
  • Linear amplification reactions (with a single primer) in a 50 ⁇ final volume each contained a final concentration of IX PCR Buffer, 1.5 mM MgCl 2 , 0.2 ⁇ M13 primer
  • reactions were desalted using the Qiagen DyeEx 2.0 Spin Kit (Qiagen Cat No. 63206), and reaction product separated by using a Qiagen QIAxcel with a QIAxcel DNA High Resolution Cartridge (Qiagen Cat No. 1050450), running module OM500 with a QX Alignment Marker 15 bp/3 kb (Qiagen Cat No. 929522).
  • DNA quantification was performed on aNano-Drop Spectrophotometer ND- 1000, Nucleic Acid DNA-50 analysis.
  • FIG. 9 shows the capillary gel electrophoresis analysis of a representative of the desalted linear amplified products.
  • Reaction 13 (lane 4) is the Ml 3 Reverse Primer control of un-labeled single stranded DNA (ssDNA) product.
  • BHQIO-ddATP or BHQIO-ddCTP is tested at 0% (control), 10%, 5%, and 1% of the corresponding dATP or dCTP final concentration.
  • Taq DNA Polymerase is able to incorporate BHQIO-ddATP or BHQ10- ddCTP into the linear product.
  • Successful incorporation of BHQIO-ddATP or BHQ10- ddCTP by Taq DNA Polymerase yields sDNA products of varying lengths.
  • EXAMPLE 3 EXAMPLE 3
  • BHQIO-rUTP is at a stock concentration of 3.67 mM.
  • Plasmid DNA Template (Biosearch Lot No. GST205_4c-SP6) for SP6 RNA Transcription was digested with Stul (New England Biolabs Cat. No. R0187S), desalted using the Qiagen QIAquick PCR Purification Kit (Qiagen Cat No. 28106), eluted with 40 ⁇ of Molecular Grade Water (Fisher Scientific Cat No. SH30538.03). Desalted digested plasmid was quantitated with aNano-Drop Spectrophotometer ND-1000 and 41.47 ng / ⁇ was obtained.
  • SP6 RNA Polymerase yields a transcript length of 111 nucleotides of sequence 5'- GGGCAACUACAAGACCCGCGCCGGUUUUAGAGCUAGAAAUAGCAAGUUAAAA UAAGGCUAGUCCGUUAUCAACUUGAAAAAGUGGCACCGAGUCGGUGCUUUUU ACGUAGG-3'.
  • T7 RNA Polymerase yields a transcript length of 111 nucleotides of sequence 5'- GGGAGCACGGGGCCGUCGCCGAUGUUUUAGAGCUAGAAAUAGCAAGUUAAAA UAAGGCUAGUCCGUUAUCAACUUGAAAAAGUGGCACCGAGUCGGUGCUUUUU ACGUAGG-3'.
  • SP6 transcription reactions at 20 ⁇ final volume each contained a final
  • Reactions were incubated at 37 °C for 15 hours, then 1 ⁇ of DNase (supplied with the SP6 RNA Polymerase kit) was added into each reaction, and incubated at 37 °C for an additional 15 minutes.
  • Reactions were desalted using the Qiagen RNeasy MinElute Cleanup Kit (Qiagen Cat No. 74204), eluted with 32 ⁇ of 0.05 N Triethylammonium acetate (TEAA) pH 7.0, and analyzed on a Qiagen QIAxcel with a QIAxcel DNA High Resolution Cartridge (Qiagen Cat No.
  • running module OH700 with a QX Alignment Marker 15/500 bp (Qiagen Cat No. 929520) and QX DNA Size Marker 25-500bp v2.0 (Qiagen Cat No. 929560).
  • Quantitation was performed on a Nano-Drop Spectrophotometer ND- 1000, Nucleic Acid RNA-40 analysis.
  • FIG. 10 shows the absorbance of the product RNA in Elution Buffer at 260 nm and absorbance of the BHQIO-rUTP at 517 nm.
  • Control reaction 4 and 8 has a 517 nm absorbance of 0.005 and 0.003, respectively.
  • the absorbance at 517 nm shows incorporation of the BHQ 10-rUTP within the RNA transcript.

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Abstract

La présente invention concerne des extincteurs d'énergie à l'état excité, des sondes et d'autres conjugués comprenant ces extincteurs, ainsi que leurs procédés d'utilisation.
PCT/US2016/051976 2015-09-15 2016-09-15 Extincteurs non-fluorescents oligophosphates et leurs utilisations WO2017048982A1 (fr)

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Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20140194611A1 (en) * 2008-04-01 2014-07-10 Biosearch Technologies, Inc. Stabilized nucleic acid dark quencher-fluorophore probes
US20150197792A1 (en) * 2000-05-09 2015-07-16 Biosearch Technologies, Inc. Dark quenchers for donor-acceptor energy transfer

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20150197792A1 (en) * 2000-05-09 2015-07-16 Biosearch Technologies, Inc. Dark quenchers for donor-acceptor energy transfer
US20140194611A1 (en) * 2008-04-01 2014-07-10 Biosearch Technologies, Inc. Stabilized nucleic acid dark quencher-fluorophore probes

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