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US20020006617A1 - Nucleic acid detection methods using universal priming - Google Patents

Nucleic acid detection methods using universal priming
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Publication number
US20020006617A1
US20020006617A1US09/779,376US77937601AUS2002006617A1US 20020006617 A1US20020006617 A1US 20020006617A1US 77937601 AUS77937601 AUS 77937601AUS 2002006617 A1US2002006617 A1US 2002006617A1
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United States
Prior art keywords
target
probe
probes
sequence
detection position
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Abandoned
Application number
US09/779,376
Inventor
Jian-Bing Fan
Mark Chee
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Illumina Inc
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Illumina Inc
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First worldwide family litigation filedlitigationCriticalhttps://patents.darts-ip.com/?family=26876658&utm_source=google_patent&utm_medium=platform_link&utm_campaign=public_patent_search&patent=US20020006617(A1)"Global patent litigation dataset” by Darts-ip is licensed under a Creative Commons Attribution 4.0 International License.
Priority to US09/779,376priorityCriticalpatent/US20020006617A1/en
Application filed by Illumina IncfiledCriticalIllumina Inc
Priority to US09/915,231prioritypatent/US6890741B2/en
Assigned to ILLUMINA, INC.reassignmentILLUMINA, INC.ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: CHEE, MARK S., FAN, JIAN-BING
Publication of US20020006617A1publicationCriticalpatent/US20020006617A1/en
Priority to US10/155,550prioritypatent/US20030003490A1/en
Priority to US10/177,727prioritypatent/US7955794B2/en
Priority to PCT/US2002/038672prioritypatent/WO2003048732A2/en
Priority to US10/309,803prioritypatent/US7611869B2/en
Priority to US10/620,852prioritypatent/US20040121364A1/en
Priority to US10/537,204prioritypatent/US8076063B2/en
Priority to US10/864,935prioritypatent/US20040224352A1/en
Priority to US10/864,937prioritypatent/US20040224353A1/en
Priority to US11/036,886prioritypatent/US20050214825A1/en
Priority to US12/032,581prioritypatent/US8003354B2/en
Priority to US12/507,022prioritypatent/US20100015626A1/en
Priority to US12/790,757prioritypatent/US8288103B2/en
Priority to US13/604,872prioritypatent/US8906626B2/en
Priority to US14/540,832prioritypatent/US9850536B2/en
Priority to US15/827,141prioritypatent/US10837059B2/en
Abandonedlegal-statusCriticalCurrent

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Abstract

The present invention is directed to providing sensitive and accurate assays for genotyping with a minimum or absence of target-specific amplification.

Description

Claims (29)

We claim:
1. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising:
a) providing a first probe comprising:
i) an upstream universal priming site (UUP);
ii) an adapter sequence;
iii) a first target-specific sequence comprising a first base at a readout position; and
iv) a downstream universal priming site (DUP);
b) contacting said first probe with said target sequence under conditions whereby only if said first base is perfectly complementary to a nucleotide at said detection position is a first hybridization complex formed;
c) removing non-hybridized first probes;
d) denaturing said hybridization complex;
e) amplifying said first probe to generate a plurality of amplicons;
f) contacting said amplicons with an array of capture probes; and
g) determining the nucleotide at said detection position.
2. A method according toclaim 1 wherein said amplicons comprise a label.
3. A method according toclaim 1 further comprising:
a) providing a second probe comprising:
i) an upstream universal priming site (UUP);
ii) an adapter sequence;
iii) a second target-specific sequence comprising a second base at said readout position; and
iv) a downstream universal priming site (DUP);
b) contacting said second probe with said target sequence under conditions whereby only if said second base is perfectly complementary to a nucleotide at said detection position is a second hybridization complex formed;
c) removing non-hybridized second probes;
d) denaturing said second hybridization complex;
e) amplifying said second probe to generate a plurality of amplicons;
f) contacting said amplicons with an array of capture probes; and
g) determining the nucleotide at said detection position.
4. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising:
a) providing a plurality of readout probes each comprising:
i) an upstream universal priming site (UUP);
ii) an adapter sequence;
iii) a target-specific sequence comprising a unique base at a readout position; and
iv) a downstream universal priming site (DUP);
b) contacting said detection probes with said target sequence under conditions whereby only if said base at said readout position is perfectly complementary to a nucleotide at said detection position is a first hybridization complex formed;
c) removing non-hybridized first probes;
d) denaturing said first hybridization complex;
e) amplifying said detection probes to generate a plurality of amplicons;
f) contacting said amplicons with an array of capture probes; and
g) determining the nucleotide at said detection position.
5. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) hybridizing a first ligation probe to said first target domain, said first ligation probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence; and
b) hybridizing a second ligation probe to said second target domain, said second ligation probe comprising:
i) a downstream universal priming site (DUP); and
ii) a second target-specific sequence comprising a first base at an interrogation position;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed and wherein at least one of said first and second ligation probes comprises an adapter sequence;
c) removing non-hybridized first probes;
d) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
e) amplifying said ligated probe to generate a plurality of amplicons;
f) contacting said amplicons with an array of capture probes; and
g) determining the nucleotide at said detection position.
6. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) hybridizing a first ligation probe to said first target domain, said first ligation probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence; and
b) hybridizing a second ligation probe to said second target domain, said second ligation probe comprising:
i) a downstream universal priming site (DUP); and
ii) a second target-specific sequence comprising a first base at an interrogation position;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed and wherein at least one of said first and second ligation probes comprises an adapter sequence;
c) removing non-hybridized first probes;
d) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
e) hybridizing said ligated probe to a rolling circle (RC) sequence comprising:
i) an upstream priming sequence; and
ii) a downstream priming sequence;
f) providing a ligase that ligates said upstream and downstream priming sites to form a circular ligated probe;
g) amplifying said circular ligated probe to generate a plurality of amplicons;
f) contacting said amplicons with an array of capture probes; and
g) determining the nucleotide at said detection position.
7. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) hybridizing a rolling circle (RC) probe to said target sequence, said RC probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence;
iii) a second target-specific sequence comprising a first base at an interrogation position; and
iv) an adapter sequence;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed;
c) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
d) amplifying said ligated probe to generate a plurality of amplicons;
e) contacting said amplicons with an array of capture probes; and
f) determining the nucleotide at said detection position.
8. A method according toclaim 7, further comprising removing non-hybridized RC probe.
9. A method according toclaim 1,4,5,6 or8 wherein said removing comprises:
a) enzymatically adding a binding ligand to said target sequence;
b) binding a hybridization complex comprising said target sequence comprising said binding ligand to a binding partner immobilized on a solid support;
c) washing away unhybridized probes; and
d) eluting said probe off said solid support.
10. A method according toclaim 1,4,5,6 or8 wherein said removing is done using a double-stranded specific moiety.
11. A method according toclaim 10 wherein said double-stranded specific moiety is an intercalator attached to a support.
12. A method according toclaim 9 wherein said support is a bead.
13. A method according toclaim 1,4,5,6 or7 wherein said amplifying is done by:
a) hybridizing a first universal primer to said UUP;
b) providing a polymerase and dNTPs such that said first universal primer is extended;
c) hybridizing a second universal primer to said DUP;
d) providing a polymerase and dNTPs such that said second universal primer is extended; and
e) repeating steps a) through d).
14. A method according toclaim 1,4,5,6 or7 wherein said array comprises:
a) a substrate with a patterned surface comprising discrete sites; and
b) a population of microspheres comprising at least a first subpopulation comprising a first capture probe and a second subpopulation comprising a second capture probe.
15. A method according toclaim 14 wherein said discrete sites comprise wells.
16. A method according toclaim 14 or15 wherein said substrate comprises a fiber optic bundle.
17. A method of determining the identification of a nucleotide at a detection position in a genomic target sequence comprising:
a) attaching a library of genomic target sequences to a solid support;
b) adding at least one probe and an enzyme to form an extended primer;
c) denaturing said extended primer from said target sequence;
d) hybridizing said extended primer to an array comprising capture probes; and
e) determining said nucleotide at said detection position.
18. A method according toclaim 17, further comprising removing unhybridized probes.
19. A method according toclaim 1,4,5,6 or7, further comprising providing a support on which the target sequence is immobilized.
20. A method according toclaim 19, wherein said non-hybridized first probes are removed without removing said target sequence from said support.
21. A method according toclaim 1,4,5,6 or7, further comprising attaching said target sequence to a support.
22. A method according toclaim 21, wherein said target sequence is attached to said support by a method selected from the group consisting of labeling said target sequence with a functional attachment moiety, absorption of said target sequence on a charged support, direct chemical attachment of said target sequence to said support and photocrosslinking said target sequence to said support.
23. A method according toclaim 1,4,5,6 or7, wherein said support is selected from the group consisting of paper, plastic and tubes.
24. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising:
a) providing a support on which the target sequence is immobilized;
b) providing a first probe comprising:
i) an upstream universal priming site (UUP);
ii) an adapter sequence;
iii) a first target-specific sequence comprising a first base at a readout position; and
iv) a downstream universal priming site (DUP);
c) contacting said first probe with said target sequence under conditions whereby only if said first base is perfectly complementary to a nucleotide at said detection position is a first hybridization complex formed;
d) removing non-hybridized first probes;
e) denaturing said hybridization complex;
f) amplifying said first probe to generate a plurality of amplicons;
g) contacting said amplicons with an array of capture probes; and
h) determining the nucleotide at said detection position
25. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising:
a) providing a support on which the target sequence is immobilized;
b) providing a plurality of readout probes each comprising:
i) an upstream universal priming site (UUP);
ii) an adapter sequence;
iii) a target-specific sequence comprising a unique base at a readout position; and
iv) a downstream universal priming site (DUP);
c) contacting said detection probes with said target sequence under conditions whereby only if said base at said readout position is perfectly complementary to a nucleotide at said detection position is a first hybridization complex formed;
d) removing non-hybridized first probes;
e) denaturing said first hybridization complex;
f) amplifying said detection probes to generate a plurality of amplicons;
g) contacting said amplicons with an array of capture probes; and
h) determining the nucleotide at said detection position.
26. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) providing a support on which the target sequence is immobilized;
b) hybridizing a first ligation probe to said first target domain, said first ligation probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence; and
c) hybridizing a second ligation probe to said second target domain, said second ligation probe comprising:
i) a downstream universal priming site (DUP); and
ii) a second target-specific sequence comprising a first base at an interrogation position;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed and wherein at least one of said first and second ligation probes comprises an adapter sequence;
d) removing non-hybridized first probes;
e) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
f) amplifying said ligated probe to generate a plurality of amplicons;
g) contacting said amplicons with an array of capture probes; and
h) determining the nucleotide at said detection position.
27. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) providing a support on which the target sequence is immobilized;
b) hybridizing a first ligation probe to said first target domain, said first ligation probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence; and
c) hybridizing a second ligation probe to said second target domain, said second ligation probe comprising:
i) a downstream universal priming site (DUP); and
ii) a second target-specific sequence comprising a first base at an interrogation position;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed and wherein at least one of said first and second ligation probes comprises an adapter sequence;
d) removing non-hybridized first probes;
e) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
f) hybridizing said ligated probe to a rolling circle (RC) sequence comprising:
i) an upstream priming sequence; and
ii) a downstream priming sequence;
g) providing a ligase that ligates said upstream and downstream priming sites to form a circular ligated probe;
h) amplifying said circular ligated probe to generate a plurality of amplicons;
i) contacting said amplicons with an array of capture probes; and
j) determining the nucleotide at said detection position.
28. A method of determining the identification of a nucleotide at a detection position in a target sequence comprising a first target domain comprising said detection position and a second target domain adjacent to said detection position, wherein said method comprises:
a) providing a support on which the target sequence is immobilized;
b) hybridizing a rolling circle (RC) probe to said target sequence, said RC probe comprising:
i) an upstream universal priming site (UUP); and
ii) a first target-specific sequence;
iii) a second target-specific sequence comprising a first base at an interrogation position; and
iv) an adapter sequence;
wherein if said first base is perfectly complementary to said nucleotide at said detection position a ligation complex is formed;
c) providing a ligase that ligates said first and second ligation probes to form a ligated probe;
d) amplifying said ligated probe to generate a plurality of amplicons;
e) contacting said amplicons with an array of capture probes; and
f) determining the nucleotide at said detection position.
29. A method according toclaim 28, further comprising removing unhybridized RC probe.
US09/779,3762000-02-072001-02-07Nucleic acid detection methods using universal primingAbandonedUS20020006617A1 (en)

Priority Applications (17)

Application NumberPriority DateFiling DateTitle
US09/779,376US20020006617A1 (en)2000-02-072001-02-07Nucleic acid detection methods using universal priming
US09/915,231US6890741B2 (en)2000-02-072001-07-24Multiplexed detection of analytes
US10/155,550US20030003490A1 (en)2000-02-072002-05-24Nucleic acid detection methods using universal priming
US10/177,727US7955794B2 (en)2000-09-212002-06-20Multiplex nucleic acid reactions
PCT/US2002/038672WO2003048732A2 (en)2001-02-072002-12-03Multiplexed methylation detection methods
US10/309,803US7611869B2 (en)2000-02-072002-12-03Multiplexed methylation detection methods
US10/620,852US20040121364A1 (en)2000-02-072003-07-15Multiplex nucleic acid reactions
US10/537,204US8076063B2 (en)2000-02-072003-12-03Multiplexed methylation detection methods
US10/864,937US20040224353A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming
US10/864,935US20040224352A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming
US11/036,886US20050214825A1 (en)2000-02-072005-01-14Multiplex sample analysis on universal arrays
US12/032,581US8003354B2 (en)2000-02-072008-02-15Multiplex nucleic acid reactions
US12/507,022US20100015626A1 (en)2000-02-072009-07-21Multiplex nucleic acid reactions
US12/790,757US8288103B2 (en)2000-02-072010-05-28Multiplex nucleic acid reactions
US13/604,872US8906626B2 (en)2000-02-072012-09-06Multiplex nucleic acid reactions
US14/540,832US9850536B2 (en)2000-02-072014-11-13Multiplex nucleic acid reactions
US15/827,141US10837059B2 (en)2000-02-072017-11-30Multiplex nucleic acid reactions

Applications Claiming Priority (3)

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US18081000P2000-02-072000-02-07
US23473200P2000-09-222000-09-22
US09/779,376US20020006617A1 (en)2000-02-072001-02-07Nucleic acid detection methods using universal priming

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US09/915,231Continuation-In-PartUS6890741B2 (en)2000-02-072001-07-24Multiplexed detection of analytes
US09/931,285Continuation-In-PartUS6913884B2 (en)2000-02-072001-08-16Compositions and methods for repetitive use of genomic DNA

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US09/915,231Continuation-In-PartUS6890741B2 (en)2000-02-072001-07-24Multiplexed detection of analytes
US09/915,231ContinuationUS6890741B2 (en)2000-02-072001-07-24Multiplexed detection of analytes
US09/931,285Continuation-In-PartUS6913884B2 (en)2000-02-072001-08-16Compositions and methods for repetitive use of genomic DNA
US10/155,550DivisionUS20030003490A1 (en)2000-02-072002-05-24Nucleic acid detection methods using universal priming
US10/177,727Continuation-In-PartUS7955794B2 (en)2000-02-072002-06-20Multiplex nucleic acid reactions
US10/309,803ContinuationUS7611869B2 (en)2000-02-072002-12-03Multiplexed methylation detection methods
US10/864,935ContinuationUS20040224352A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming
US10/864,937ContinuationUS20040224353A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming

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US09/779,376AbandonedUS20020006617A1 (en)2000-02-072001-02-07Nucleic acid detection methods using universal priming
US09/915,231Expired - LifetimeUS6890741B2 (en)2000-02-072001-07-24Multiplexed detection of analytes
US10/155,550AbandonedUS20030003490A1 (en)2000-02-072002-05-24Nucleic acid detection methods using universal priming
US10/864,937AbandonedUS20040224353A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming
US10/864,935AbandonedUS20040224352A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming

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US10/155,550AbandonedUS20030003490A1 (en)2000-02-072002-05-24Nucleic acid detection methods using universal priming
US10/864,937AbandonedUS20040224353A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming
US10/864,935AbandonedUS20040224352A1 (en)2000-02-072004-06-09Nucleic acid detection methods using universal priming

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