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US20090286286A1 - Methods for controlling amplification - Google Patents

Methods for controlling amplification
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Publication number
US20090286286A1
US20090286286A1US12/290,813US29081308AUS2009286286A1US 20090286286 A1US20090286286 A1US 20090286286A1US 29081308 AUS29081308 AUS 29081308AUS 2009286286 A1US2009286286 A1US 2009286286A1
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United States
Prior art keywords
beads
nucleic acid
bead
template
primers
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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
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US12/290,813
Inventor
Mark J. Lim
Kenneth J. Rothschild
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Ambergen Inc
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Ambergen Inc
Priority date (The priority date 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 date listed.)
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Publication date
Application filed by Ambergen IncfiledCriticalAmbergen Inc
Priority to US12/290,813priorityCriticalpatent/US20090286286A1/en
Assigned to AMBERGEN, INC.reassignmentAMBERGEN, INC.ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: LIM, MARK J., ROTHSCHILD, KENNETH J.
Publication of US20090286286A1publicationCriticalpatent/US20090286286A1/en
Priority to US12/779,493prioritypatent/US9334530B2/en
Priority to US12/779,616prioritypatent/US20100317542A1/en
Assigned to NATIONAL INSTITUTES OF HEALTH (NIH), U.S. DEPT. OF HEALTH AND HUMAN SERVICES (DHHS), U.S. GOVERNMENTreassignmentNATIONAL INSTITUTES OF HEALTH (NIH), U.S. DEPT. OF HEALTH AND HUMAN SERVICES (DHHS), U.S. GOVERNMENTCONFIRMATORY LICENSE (SEE DOCUMENT FOR DETAILS).Assignors: AMBERGEN INCORPORATED
Abandonedlegal-statusCriticalCurrent

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Abstract

Methods of amplifying nucleic acid on a solid support are described. Beads and template, each in known concentrations, are employed so a range of template to bead ratios can be exploited. Where the beads contain primers, the template can be amplified. After amplification, non-covalently bound template is removed, so as to leave beads with extended primers (or beads with primers that were not extended).

Description

Claims (53)

1. A method of amplifying nucleic acid on a solid support, comprising:
(a) providing i) a population of beads, each bead comprising one or more amplification primers, ii) a solution of amplification reagents comprising a thermostable polymerase, and iii) a population of nucleic acid template molecules,
(b) mixing said beads and said template molecules in a first aliquot of said solution of amplification reagents so as to create a mixture;
(c) treating the mixture under conditions such that at least a portion of said template molecules non-covalently bind to at least a portion of said beads to create bound template, and at least a portion of said primers on at least a portion of said beads are extended by said polymerase, so as to create treated beads;
(d) manipulating said treated beads so as to remove at least a portion of said bound template so as to create manipulated beads; and
(e) contacting said manipulated beads with a second aliquot of said solution of amplification reagents under conditions such that at least a portion of said extended primers is amplified to create loaded beads comprising immobilized amplified nucleic acid and unloaded beads lacking amplified nucleic acid.
15. A method of amplifying nucleic acid on a solid support, comprising:
a) providing i) a population of beads, each bead comprising forward and reverse PCR primers primers, ii) a solution of amplification reagents comprising a thermostable polymerase, and iii) a population of nucleic acid template molecules,
b) mixing said beads and said template molecules in a first aliquot of said solution of amplification reagents so as to create a mixture;
c) treating the mixture under conditions such that at least a portion of said template molecules non-covalently bind to at least a portion of said beads to create bound template, and at least a portion of said primers on at least a portion of said beads are extended by said polymerase, so as to create treated beads;
d) washing said treated beads with a denaturing solution so as to create manipulated beads; and
e) contacting said manipulated beads with a second aliquot of said solution of amplification reagents under conditions such that at least a portion of said extended primers is amplified to create loaded beads comprising immobilized amplified nucleic acid and unloaded beads lacking amplified nucleic acid.
29. A method of amplifying nucleic acid on a solid support, comprising: a) providing i) a population of a known concentration of beads, each bead comprising one or more amplification primers, ii) a solution of amplification reagents comprising a thermostable polymerase, and iii) a population of a known concentration of nucleic acid template molecules; b) mixing said beads and said template molecules in a first aliquot of said solution of amplification reagents so as to create a mixture under the conditions such that the ratio of the number of nucleic acid template molecules to the number of beads is between 1:1 and 10,000:1; c) treating the mixture under conditions such that at least a portion of said template molecules non-covalently bind to at least a portion of said beads to create bound template, and at least a portion of said primers on at least a portion of said beads are extended by said polymerase, so as to create treated beads; d) manipulating said treated beads so as to remove at least a portion of said bound template so as to create manipulated beads; and e) contacting said manipulated beads with a second aliquot of said solution of amplification reagents under conditions such that at least a portion of said extended primers is amplified to create loaded beads comprising immobilized amplified nucleic acid and unloaded beads lacking amplified nucleic acid.
45. A method of amplifying nucleic acid on a solid support, comprising:
a) providing i) a population of a known concentration of beads, each bead comprising one or more amplification primers, ii) a solution of amplification reagents comprising a thermostable polymerase, and iii) a population of a known concentration of nucleic acid template molecules,
b) mixing said beads and said template molecules in a first aliquot of said solution of amplification reagents so as to create a mixture under the conditions such that the ratio of the number of nucleic acid template molecules to the number of beads is between 0.1:1 and 2:1;
c) treating the mixture under conditions such that at least a portion of said template molecules non-covalently bind to at least a portion of said beads to create bound template, and at least a portion of said primers on at least a portion of said beads are extended by said polymerase, so as to create treated beads;
d) exposing said treated beads to a denaturing solution so as to create manipulated beads; and
e) contacting said manipulated beads with a second aliquot of said solution of amplification reagents under conditions such that at least a portion of said extended primers is amplified to create loaded beads comprising immobilized amplified nucleic acid and unloaded beads lacking amplified nucleic acid.
US12/290,8132007-11-062008-11-04Methods for controlling amplificationAbandonedUS20090286286A1 (en)

Priority Applications (3)

Application NumberPriority DateFiling DateTitle
US12/290,813US20090286286A1 (en)2007-11-062008-11-04Methods for controlling amplification
US12/779,493US9334530B2 (en)2007-11-062010-05-13Methods for making and imaging arrays that comprise a plurality of different biomolecules
US12/779,616US20100317542A1 (en)2007-11-062010-05-13Methods For Detecting Biomarkers

Applications Claiming Priority (2)

Application NumberPriority DateFiling DateTitle
US208307P2007-11-062007-11-06
US12/290,813US20090286286A1 (en)2007-11-062008-11-04Methods for controlling amplification

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US12/779,493ContinuationUS9334530B2 (en)2007-11-062010-05-13Methods for making and imaging arrays that comprise a plurality of different biomolecules
US12/779,616ContinuationUS20100317542A1 (en)2007-11-062010-05-13Methods For Detecting Biomarkers

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US20090286286A1true US20090286286A1 (en)2009-11-19

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US12/290,813AbandonedUS20090286286A1 (en)2007-11-062008-11-04Methods for controlling amplification
US12/779,493ActiveUS9334530B2 (en)2007-11-062010-05-13Methods for making and imaging arrays that comprise a plurality of different biomolecules
US12/779,616AbandonedUS20100317542A1 (en)2007-11-062010-05-13Methods For Detecting Biomarkers

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US12/779,493ActiveUS9334530B2 (en)2007-11-062010-05-13Methods for making and imaging arrays that comprise a plurality of different biomolecules
US12/779,616AbandonedUS20100317542A1 (en)2007-11-062010-05-13Methods For Detecting Biomarkers

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Cited By (31)

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US10329544B2 (en)2009-05-132019-06-25Life Technologies CorporationNucleic acid amplification
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US10113195B2 (en)2010-12-172018-10-30Life Technologies CorporationNucleic acid amplification
US9334531B2 (en)*2010-12-172016-05-10Life Technologies CorporationNucleic acid amplification
US9371557B2 (en)*2010-12-172016-06-21Life Technologies CorporationNucleic acid amplification
US9476080B2 (en)2010-12-172016-10-25Life Technologies CorporationClonal amplification of nucleic acid on solid surface with template walking
US9309566B2 (en)2010-12-172016-04-12Life Technologies CorporationMethods, compositions, systems, apparatuses and kits for nucleic acid amplification
US9309557B2 (en)*2010-12-172016-04-12Life Technologies CorporationNucleic acid amplification
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US20100317542A1 (en)2010-12-16
US20100256015A1 (en)2010-10-07

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ASAssignment

Owner name:AMBERGEN, INC., MASSACHUSETTS

Free format text:ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:LIM, MARK J.;ROTHSCHILD, KENNETH J.;REEL/FRAME:023010/0279

Effective date:20090209

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Owner name:NATIONAL INSTITUTES OF HEALTH (NIH), U.S. DEPT. OF

Free format text:CONFIRMATORY LICENSE;ASSIGNOR:AMBERGEN INCORPORATED;REEL/FRAME:028291/0845

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