Analytical methods and materials for nucleic acid detection
First Claim
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1. A method for determining the presence or absence of a predetermined nucleic acid target sequence in a nucleic acid sample that comprises the steps of:
- (A) providing a treated sample that may contain said predetermined nucleic acid target sequence hybridized with a nucleic acid probe that includes an identifier nucleotide in the 3′
-terminal region;
(B) admixing the treated sample with a depolymerizing amount of an enzyme whose activity is to release one or more nucleotides from the 3′
-terminus of a hybridized nucleic acid probe to form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(C) maintaining the treated reaction mixture for a time period sufficient to permit the enzyme to depolymerize hybridized nucleic acid and release identifier nucleotide therefrom; and
(D) analyzing for the presence of released identifier nucleotides to obtain an analytical output obtained by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy, the analytical output indicating the presence or absence of said nucleic acid target sequence.
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Abstract
Mass spectrometric, absorbance spectroscopic and fluorescence spectroscopic processes are disclosed to detect the depolymerization of a nucleic acid hybrid in order to qualitatively and quantitatively assay for the presence of a predetermined nucleic acid target. Applications of those processes include the detection of single nucleotide polymorphisms, identification of single base changes, speciation, determination of viral load, genotyping, medical marker diagnostics, and the like, including multiplexed assays.
234 Citations
36 Claims
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1. A method for determining the presence or absence of a predetermined nucleic acid target sequence in a nucleic acid sample that comprises the steps of:
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(A) providing a treated sample that may contain said predetermined nucleic acid target sequence hybridized with a nucleic acid probe that includes an identifier nucleotide in the 3′
-terminal region;
(B) admixing the treated sample with a depolymerizing amount of an enzyme whose activity is to release one or more nucleotides from the 3′
-terminus of a hybridized nucleic acid probe to form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(C) maintaining the treated reaction mixture for a time period sufficient to permit the enzyme to depolymerize hybridized nucleic acid and release identifier nucleotide therefrom; and
(D) analyzing for the presence of released identifier nucleotides to obtain an analytical output obtained by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy, the analytical output indicating the presence or absence of said nucleic acid target sequence. - View Dependent Claims (2, 3, 4, 5, 6, 7, 8)
(A) admixing a sample to be assayed with one or more nucleic acid probes to form a hybridization composition, wherein the 3′ - -terminal region of said nucleic acid probes (i) hybridize with partial or total complementarity to said nucleic acid target sequence when that sequence is present in the sample and (ii) include an identifier nucleotide;
(B) maintaining said hybridization composition for a time period sufficient to form a treated sample that may contain said one predetermined nucleic acid target sequence hybridized with a nucleic acid probe.
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9. A method for determining the presence or absence of at least one predetermined nucleic acid target sequence in a nucleic acid sample that comprises the steps of:
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(A) admixing a sample to be assayed with one or more nucleic acid probes to form a hybridization composition, wherein the 3′
-terminal region of said nucleic acid probes (i) hybridizes with partial or total complementarity to at least one said predetermined nucleic acid target sequence when that sequence is present in the sample and (ii) includes an identifier nucleotide;
(B) maintaining said hybridization composition for a time period sufficient to form a treated sample that may contain said predetermined nucleic acid target sequence hybridized with a nucleic acid probe;
(C) admixing the treated sample with a depolymerizing amount of an enzyme whose activity is to release one or more nucleotides from the 3′
-terminus of a hybridized nucleic acid probe to form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(D) maintaining the treated reaction mixture for a time period sufficient to permit the enzyme to depolymerize hybridized nucleic acid and release identifier nucleotide therefrom; and
(E) analyzing for the presence of released identifier nucleotides to obtain an analytical output obtained by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy, the analytical output indicating the presence or absence of at least one said nucleic acid target sequence. - View Dependent Claims (10, 11, 12, 13, 14, 15)
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16. A method for determining the presence or absence of a specific base in a nucleic acid target sequence in a sample to be assayed that comprises the steps of:
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(A) admixing a sample to be assayed with one or more nucleic acid probes to form a hybridization composition, wherein the 3′
-terminal region of at least one of said nucleic acid probes (i) is substantially complementary to said nucleic acid target sequence and comprises at least one predetermined nucleotide at an interrogation position, and (ii) includes an identifier nucleotide, and wherein said nucleic acid target sequence comprises at least one specific base whose presence or absence is to be determined(B) maintaining said hybridization composition for a time period sufficient to form a treated sample, wherein said interrogation position of the probe is a nucleotide that is aligned with said specific base to be identified in said target sequence, when present, so that base pairing can occur;
(C) admixing the treated sample with an enzyme whose activity is to release one or more nucleotides from the 3′
-terminus of a hybridized nucleic acid probe to depolymerize the hybrid and form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(D) maintaining the treated reaction mixture for a time period sufficient to release an identifier nucleotide therefrom; and
(E) analyzing for the presence or absence of released identifier nucleotide to obtain an analytical output by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy that indicates the presence or absence of said specific base to be identified. - View Dependent Claims (17, 18, 19, 20, 21, 22)
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23. A method for determining the presence or absence of a first nucleic acid target in a nucleic acid sample containing that target or a substantially identical second target that comprises the steps of:
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(A) admixing said sample to be assayed with one or more nucleic acid probes to form a hybridization composition, wherein said first and second nucleic acid targets comprise a region of sequence identity except for at least a single nucleotide at a predetermined position that differs between the targets, and wherein said nucleic acid probe (i) is substantially complementary to said nucleic acid target region of sequence identity and comprises at least one nucleotide at an interrogation position, said interrogation position of the probe being aligned with said predetermined position of a target when a target and probe are hybridized and (ii) includes an identifier nucleotide in the 3′
-terminal region;
(B) maintaining said hybridization composition for a time period sufficient to form a treated sample wherein the nucleotide at said interrogation position of said probe is aligned with the nucleotide at said predetermined position of said target in said region of identity;
(C) admixing the treated sample with a depolymerizing amount an enzyme whose activity is to release one or more nucleotides from the 3′
-terminus of a hybridized nucleic acid probe to form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(D) maintaining the treated reaction mixture for a time period sufficient to depolymerize said hybridized nucleic acid probe and release identifier nucleotide therefrom; and
(E) analyzing for the presence of released identifier nucleotide to obtain an analytical output obtained by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy, said analytical output indicating the presence or absence of said nucleotide at said predetermined region and thereby the presence or absence of a first or second nucleic acid target. - View Dependent Claims (24, 25, 26, 27, 28)
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29. A method for selectively detecting a poly(A)+ RNA that comprises the steps of:
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(A) admixing a sample to be assayed with an oligo(dT) probe to form a hybridization composition, wherein said oligo(dT) probe includes an identifier nucleotide in the 3′
-terminal region;
(B) maintaining said hybridization composition for a time period sufficient to form a treated sample wherein said poly(A)+ RNA hybridizes to said oligo(dT) probe;
(C) admixing the treated sample with an enzyme whose activity is to release of one or more nucleotides from the 3′
-terminus of a nucleic acid hybrid, including the identifier nucleotide, to form a treated reaction mixture, wherein said enzyme catalyzes pyrophosphorolysis;
(D) maintaining the treated reaction mixture for a time period sufficient to depolymerize hybridized nucleic acid probe and release identifier nucleotides therefrom; and
(E) analyzing for the presence of released identifier nucleotide to obtain an analytical output obtained by fluorescence spectroscopy, mass spectrometry or absorbance spectroscopy, said analytical output indicating the presence of said poly(A)+ RNA. - View Dependent Claims (30, 31, 32, 33, 34, 35, 36)
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Specification