Arrays comprising background features that provide for a measure of a non-specific binding and methods for using the same
First Claim
Patent Images
1. A hybridization assay comprising:
- (a) contacting a sample of target nucleic acids with a collection of substrate bound probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature that is an empirically observed inactive probe that does not hybridize to a fully complementary fluorescently labeled target nucleic acid as determined in an assay wherein said probe is provided in an array that is contacted with said fluorescently labeled fully complementary target under said hybridization conditions, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted collection are 50% melted;
(b) separating unbound target nucleic acids/label from said collection of probe nucleic acid features;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c).
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Abstract
Methods for substantially improved detection and analysis in nucleic acid hybridization assays are described. The methods provide the reliable estimation of background signal which derives primarily from nonspecific hybridization. The invention is useful in chemical, biological, medical and diagnostic techniques, as well as for drug discovery.
70 Citations
26 Claims
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1. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with a collection of substrate bound probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature that is an empirically observed inactive probe that does not hybridize to a fully complementary fluorescently labeled target nucleic acid as determined in an assay wherein said probe is provided in an array that is contacted with said fluorescently labeled fully complementary target under said hybridization conditions, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted collection are 50% melted;
(b) separating unbound target nucleic acids/label from said collection of probe nucleic acid features;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c). - View Dependent Claims (2, 3, 4, 5, 6)
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7. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with a collection of substrate bound probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid selected from the group consisting of SEQ ID NOS;
05 to 18 and 24 to 32, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted collection are 50% melted;
b) separating unbound target nucleic acids/label from said collection of probe nucleic acid features;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from at said least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c).
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8. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with a collection of substrate bound probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid that is chosen from;
(i) a probe nucleic acid that forms a stable intramolecular structure;
(ii) a probe nucleic acid that comprises reverse polarity nucleotide analogs; and
(iii) a probe nucleic acid that comprises abasic phosphodiesters, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted collection are 50% melted;
b) separating unbound target nucleic acids/label from said collection of probe nucleic acid features;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c). - View Dependent Claims (9, 10)
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11. A hybridization assay comprising:
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(a) contacting a sample of detectably labeled target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature that is an empirically observed inactive probe that does not hybridize to a fully complementary fluorescently labeled target nucleic acid as determined in an assay wherein said probe is provided in an array that is contacted with said fluorescently labeled fully complementary target under said hybridization conditions, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids/label from said array;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c).
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12. A hybridization assay comprising:
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(a) contacting a sample of detectably labeled target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid selected from the group consisting of SEQ ID NOS;
05 to 18 and 24 to 32, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids from said array;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature.
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13. A hybridization assay comprising:
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(a) contacting a sample of detectably labeled target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid that is chosen from;
(i) a probe nucleic acid that forms a stable intramolecular structure;
(ii) a probe nucleic acid that comprises reverse polarity nucleotide analogs; and
(iii) a probe nucleic acid that comprises abasic phosphodiesters, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids from said array;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature. - View Dependent Claims (14, 15)
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16. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature that is an empirically observed inactive probe that does not hybridize to its fully complementary target nucleic acid as determined in an assay wherein said probe is provided in an array that is contacted with said fluorescently labeled fully complementary target under said hybridization conditions, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids, of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids from said array;
(c) detectably labeling target nucleic acids hybridized to said array of probe nucleic acid features;
(d) separating unbound label from said array;
(e) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(f) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature.
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17. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid selected from the group consisting of SEQ ID NOS;
05 to 18 and 24 to 32, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids from said array;
(c) detectably labeling target nucleic acids hybridized to said array of probe nucleic acid features;
(d) separating unbound label from said array;
(e) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(f) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature.
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18. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with an array of probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature, wherein said at least one background feature is made up of a probe nucleic acid that is chosen from;
(i) a probe nucleic acid that forms a stable intramolecular structure;
(ii) a probe nucleic acid that comprises reverse polarity nucleotide analogs; and
(iii) a probe nucleic acid that comprises abasic phosphodiesters, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted array are 50% melted;
(b) separating non-hybridized target nucleic acids from said array;
(c) detectably labeling target nucleic acids hybridized to said array of probe nucleic acid features;
(d) separating unbound label from said array;
(e) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(f) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature. - View Dependent Claims (19, 20)
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21. A hybridization assay comprising:
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(a) contacting a sample of target nucleic acids with a collection of substrate bound probe nucleic acid features that includes at least one hybridization nucleic acid feature and at least one background nucleic acid feature made up of background probes that do not selectively bind to any of said target nucleic acids, wherein said contacting occurs between 10-25°
C. below the average temperature (Tm) at which nucleotide hybrids of the contacted collection are 50% melted;
(b) washing said contacted array to remove unbound target nucleic acids/label from said array;
(c) detecting a signal, if present, from said at least one background feature and said at least one hybridization nucleic acid feature; and
(d) subtracting a detected signal from said at least one background nucleic acid feature from signal detected from said at least one hybridization nucleic acid feature;
wherein said method is further characterized by including a target nucleic acid labeling step prior to said detecting step(c). - View Dependent Claims (22, 23, 24, 25, 26)
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Specification