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US20020012933A1 - Method of sequencing a nucleic acid - Google Patents

Method of sequencing a nucleic acid
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Publication number
US20020012933A1
US20020012933A1US09/826,141US82614101AUS2002012933A1US 20020012933 A1US20020012933 A1US 20020012933A1US 82614101 AUS82614101 AUS 82614101AUS 2002012933 A1US2002012933 A1US 2002012933A1
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United States
Prior art keywords
nucleic acid
substrate
approximately
sequencing
sequence
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Abandoned
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US09/826,141
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Jonathan Rothberg
Joel Bader
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CuraGen Corp
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CuraGen Corp
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Priority to US09/826,141priorityCriticalpatent/US20020012933A1/en
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Abstract

Disclosed herein are methods and apparatuses for sequencing a nucleic acid. The method includes annealing a population of circular nucleic acid molecules to a plurality of anchor primers linked to a solid support, and amplifying those members of the population of circular nucleic acid molecules which anneal to the target nucleic acid, and then sequencing the amplified molecules by detecting the presence of a sequence byproduct.

Description

Claims (62)

What is claimed is:
1. A method for sequencing a nucleic acid, the method comprising:
providing one or more or more nucleic acid anchor primers linked to a solid support;
providing a plurality of circular nucleic acid templates;
annealing an effective amount of the nucleic acid anchor primer to at least one of the single-stranded circular templates to yield a primed anchor primer-circular template complex;
combining the primed anchor primer-circular template complex with a polymerase to generate multiple copies of the circular nucleic acid template;
annealing an effective amount of a sequencing primer to the circular nucleic acid template to yield a primed sequencing primer-circular nucleic acid template complex;
extending the sequencing primer with a polymerase and a predetermined nucleotide triphosphate to yield a sequencing product and a sequencing reaction byproduct; and
identifying the sequencing reaction byproduct, thereby determining the sequence of the nucleic acid.
2. The method ofclaim 1, wherein the circular nucleic acid template is single-stranded DNA.
3. The method ofclaim 1, wherein the circular nucleic acid template is an open circle nucleic acid.
4. The method ofclaim 1, wherein the circular nucleic acid template is a closed circle nucleic acid.
5. The method ofclaim 1, wherein the circular nucleic acid template is genomic DNA.
6. The method ofclaim 1, wherein the circular nucleic acid template is cDNA.
7. The method ofclaim 1, wherein the circular nucleic acid is 10-200 nucleotides in length.
8. The method ofclaim 1, wherein the circular nucleic acid is 10-100 nucleotides in length.
9. The method ofclaim 1, wherein the circular nucleic acid is 10-50 nucleotides in length.
10. The method ofclaim 1, wherein the multiple copies are generated by a polymerase chain reaction.
11. The method ofclaim 1, wherein the primed circular template is extended by rolling circle amplification to yield a single-stranded concatamer of the annealed circular nucleic acid template.
12. The method ofclaim 11, further comprising:
annealing a reverse primer to the single-stranded concatamer to yield a primed concatamer template, and
combining the primed concatamer template with a polymerase enzyme to generate multiple copies of the concatamer template.
13. The method ofclaim 1, wherein the sequencing byproduct is pyrophosphate.
14. The method ofclaim 13, wherein the pyrophosphate is detected by contacting the sequencing byproduct with ATP sulfurylase under conditions sufficient to form ATP.
15. The method ofclaim 14, wherein the ATP is detected with luciferase.
16. The method ofclaim 13, further comprising apyrase.
17. The method ofclaim 13, further comprising washing the sequencing product with a wash buffer.
18. The method ofclaim 17, wherein the wash buffer includes apyrase.
19. The method ofclaim 1, wherein the anchor primer sequence includes a biotin group.
20. The method ofclaim 19, wherein the biotin group on the anchor primer is linked to an avidin group on the solid support.
21. The method ofclaim 1, wherein the anchor primer is conjugated to a biotin-BSA moiety.
22. The method ofclaim 21, wherein the biotin-BSA moiety on the anchor primer is linked to an avidin-biotin group on the solid support.
23. The method ofclaim 21, wherein the biotin-BSA moiety on the anchor primer is linked to a BSA group on the solid support in the presence of silane.
24. The method ofclaim 1, wherein the solid support includes at least one optical fiber.
25. The method ofclaim 1, wherein the sequencing primer is extended in the presence of a dATP analog.
26. The method ofclaim 25, wherein the dATP analog is adenosine 5′-phosphosulfate (APS).
27. The method ofclaim 1, wherein the solid substrate includes two or more anchoring primers separated by approximately 10 μm to approximately 200 μm.
28. The method ofclaim 27, wherein the solid substrate includes two or more anchoring primers separated by approximately 50 μm to approximately 150 μm.
29. The method ofclaim 27, wherein the solid substrate includes two or more anchoring primers separated by approximately 100 μm to approximately 150 μm.
30. The method ofclaim 1, wherein the solid support matrix comprises of a plurality of anchor pads that are covalently linked to the solid support.
31. The method ofclaim 30, wherein the surface area of each anchor pad is approximately 10 μm2.
32. The method ofclaim 30, wherein and each pad is separated from one another by a distance ranging from approximately 50 μm to approximately 150 μm.
33. A substrate for analyzing a nucleic acid, the substrate comprising:
a cavitated fiber optic surface; and
a nucleic acid sequence linked to the fiber optic surface.
34. The substrate ofclaim 33, wherein the substrate comprises a plurality of fiber optic surfaces.
35. The substrate ofclaim 33, wherein the nucleic acid sequence is an anchor primer.
36. The substrate ofclaim 33, wherein the fiber optic surface includes two or more anchoring primers separated by approximately 10 μm to approximately 200 μm.
37. The substrate ofclaim 33, wherein the fiber optic surface includes two or more anchoring primers separated by approximately 100 μm to approximately 150 μm.
38. The substrate ofclaim 33, wherein the fiber optic surface includes two or more anchoring primers separated by approximately 150 μm.
39. The substrate ofclaim 33, wherein the fiber optic surface includes two or more anchor pads separated by approximately 100 μm to approximately 150 μm.
40. The substrate ofclaim 39, wherein the surface area of each pad is approximately 10 μm2.
41. A substrate with a cavitated surface comprising 103or more groups of oligonucleotides covalently attached to the surface in discrete known regions, the 103or more groups of oligonucleotides occupying a total area of less than 1 cm2on said substrate, said groups of oligonucleotides having different nucleotide sequences.
42. The substrate as recited inclaim 41 wherein said substrate comprises 104or more different groups of sequences in discrete known regions.
43. The substrate as recited inclaim 1 wherein said substrate comprises 105or more different groups of oligonucleotides with known sequences in discrete known regions.
44. The substrate as recited inclaim 1 wherein the groups of oligonucleotides are attached to the surface by a linker.
45. An array of more than 1,000 different groups of oligonucleotide molecules with known sequences covalently coupled to a surface of a cavitated substrate, said groups of oligonucleotide molecules each in discrete known regions and differing from other groups of oligonucleotide molecules in monomer sequence, each of said discrete known regions being an area of less than about 0.01 cm2and each discrete known region comprising oligonucleotides of known sequence, said different groups occupying a total area of less than 1 cm2.
46. The array as recited inclaim 45 wherein said area is less than 10,000 microns2.
47. The array as recited inclaim 46 made by the process of:
exposing a first region of said substrate to light to remove photoremovable group from nucleic acids in said first region, and not exposing a second region of said surface to light;
covalently coupling a first nucleotide to said nucleic acids on said part of said substrate exposed to light, said first nucleotide covalently coupled to said photoremovable group;
exposing a part of said first region of said substrate to light, and not exposing another part of said first region of said substrate to light to remove said photoremovable groups; covalently coupling a second nucleotide to said part of said first region exposed to light; and
repeating said steps of exposing said substrate to light and covalently coupling nucleotides until said more than 500 different groups of nucleotides are formed on said surface.
48. The array as recited inclaim 46 comprising more than 10,000 groups of oligonucleotides of known sequences.
49. An apparatus for analyzing a nucleic acid sequence, the apparatus comprising:
a perfusion chamber, wherein the chamber includes a nucleic acid substrate;
a conduit in communication with the perfusion chamber;
an imaging system in communication with the perfusion chamber; and
a data collection system in communication with the imaging system.
50. The apparatus ofclaim 49, wherein the substrate is a planar substrate.
51. The apparatus ofclaim 49, wherein the imaging system is a fiber optic system.
52. The apparatus ofclaim 49, wherein the substrate comprises
a cavitated fiber optic surface in communication with said imaging system; and
a nucleic acid sequence linked to the fiber optic surface.
53. The apparatus ofclaim 49, wherein the substrate comprises a plurality of fiber optic surfaces, said fiber optic surfaces being in communication with said imaging system.
54. The apparatus ofclaim 49, wherein the fiber optic surface includes two or more anchoring primers separated by approximately 100 μm to approximately 150 μm.
55. The apparatus ofclaim 49, wherein the fiber optic surface includes two or more anchoring primers separated by approximately 150 μm.
56. The apparatus ofclaim 49, wherein the fiber optic surface includes two or more anchor pads separated by approximately 100 μm to approximately 150 μm.
57. The apparatus ofclaim 49, wherein the surface area of each pad is approximately 5 μm2to approximately 20 μm2.
58. The apparatus ofclaim 49, wherein the surface area of each pad is approximately 10 μm2.
59. An apparatus for processing a plurality of analyses, the apparatus comprising:
a flow chamber having disposed therein a substrate comprising a plurality of cavitated surfaces, said cavitated surfaces having disposed thereon nucleic acid molecules;
fluid means for delivering processing reagents from one or more reservoirs to the flow chamber so that the analytes anchored to the plurality of microparticles are exposed to the reagents; and
detection means for detecting a sequence of optical signals from each microparticle of the plurality, each optical signal of the sequence being indicative of an interaction between a processing reagent and the analyte anchored thereto, wherein said detection means is in communication with the cavitated surfaces.
60. The apparatus ofclaim 59, wherein said detection means further comprises signal tracking means for correlating said optical signals from each of said microparticles in each of said digital images to form for each said microparticle of said plurality a sequence of said optical signals.
61. The apparatus ofclaim 60, wherein said signal tracking means is a CCD camera.
62. The apparatus ofclaim 59, wherein said analyte is DNA.
US09/826,1411999-09-162001-04-04Method of sequencing a nucleic acidAbandonedUS20020012933A1 (en)

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US09/398,833US6274320B1 (en)1999-09-161999-09-16Method of sequencing a nucleic acid
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EP (1)EP1212467A2 (en)
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