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US20060223066A1 - Methods for normalizing and for identifying small nucleic acids - Google Patents

Methods for normalizing and for identifying small nucleic acids
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Publication number
US20060223066A1
US20060223066A1US11/093,587US9358705AUS2006223066A1US 20060223066 A1US20060223066 A1US 20060223066A1US 9358705 AUS9358705 AUS 9358705AUS 2006223066 A1US2006223066 A1US 2006223066A1
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United States
Prior art keywords
adapter
primer
species
nucleic acid
different
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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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US11/093,587
Inventor
Kai Lao
Neil Straus
John Burns
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Applied Biosystems LLC
Applied Biosystems Inc
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Applera Corp
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Priority to US11/093,587priorityCriticalpatent/US20060223066A1/en
Application filed by Applera CorpfiledCriticalApplera Corp
Priority to PCT/US2006/012025prioritypatent/WO2007044066A2/en
Assigned to APPLERA CORPORATIONreassignmentAPPLERA CORPORATIONASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: BURNS, JOHN W., LAO, KAI QIN, STRAUS, NEIL A.
Publication of US20060223066A1publicationCriticalpatent/US20060223066A1/en
Assigned to BANK OF AMERICA, N.A, AS COLLATERAL AGENTreassignmentBANK OF AMERICA, N.A, AS COLLATERAL AGENTSECURITY AGREEMENTAssignors: APPLIED BIOSYSTEMS, LLC
Assigned to APPLIED BIOSYSTEMS INC.reassignmentAPPLIED BIOSYSTEMS INC.CHANGE OF NAME (SEE DOCUMENT FOR DETAILS).Assignors: APPLERA CORPORATION
Assigned to APPLIED BIOSYSTEMS, LLCreassignmentAPPLIED BIOSYSTEMS, LLCMERGER (SEE DOCUMENT FOR DETAILS).Assignors: ATOM ACQUISITION, LLC & APPLIED BIOSYSTEMS INC.
Assigned to APPLIED BIOSYSTEMS, INC.reassignmentAPPLIED BIOSYSTEMS, INC.MERGER (SEE DOCUMENT FOR DETAILS).Assignors: ATOM ACQUISITION CORPORATION
Priority to US12/604,792prioritypatent/US8741569B2/en
Assigned to APPLIED BIOSYSTEMS INC.reassignmentAPPLIED BIOSYSTEMS INC.CHANGE OF NAME (SEE DOCUMENT FOR DETAILS).Assignors: APPLERA CORPORATION
Assigned to APPLIED BIOSYSTEMS, LLCreassignmentAPPLIED BIOSYSTEMS, LLCMERGER (SEE DOCUMENT FOR DETAILS).Assignors: APPLIED BIOSYSTEMS INC.
Assigned to APPLIED BIOSYSTEMS, INC.reassignmentAPPLIED BIOSYSTEMS, INC.LIEN RELEASEAssignors: BANK OF AMERICA, N.A.
Priority to US14/293,875prioritypatent/US20140349301A1/en
Assigned to APPLIED BIOSYSTEMS, LLCreassignmentAPPLIED BIOSYSTEMS, LLCCORRECTIVE ASSIGNMENT TO CORRECT THE RECEIVING PARTY NAME PREVIOUSLY RECORDED AT REEL: 030182 FRAME: 0677. ASSIGNOR(S) HEREBY CONFIRMS THE RELEASE OF SECURITY INTEREST.Assignors: BANK OF AMERICA, N.A.
Abandonedlegal-statusCriticalCurrent

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Abstract

The present teachings are generally directed to methods for normalizing at least one species of small nucleic acid that is present in a population of small nucleic acid species, wherein the relative concentration of at least one small nucleic acid species is substantially greater than the relative concentration of at least one other small nucleic acid species in the population. At least one small nucleic acid species is normalized using a multiplicity of primers comprising degenerate sequences. In some embodiments, a small nucleic acid species is identified by inserting at least part of an extension product from a normalized population into a vector and subsequently sequencing the insert. In some embodiments, a small nucleic acid species is identified by determining the sequence of at least part of an extension product.

Description

Claims (26)

26. A method for identifying a miRNA species in a population of different small nucleic acid species of varying abundance comprising,
ligating a 3′ adapter and a 5′ adapter to at least one end of at least some of the small nucleic acids in the population to form a multiplicity of double different adapter-modified molecules, wherein the adapters comprise a 3′ adapter comprising a first primer-binding site and a restriction enzyme cleavage site, a 5′ adapter comprising a second primer-binding site and a restriction enzyme cleavage site, wherein the 5′ adapter and the 3′ adapter comprise deoxyribonucleotides and ribonucleotides, and wherein at least the terminal nucleotide on the 3′-end of the 5′ adapter comprises a ribonucleotide and at least the terminal nucleotide on the 5′-end of the 3′ adapter comprises a ribonucleotide;
amplifying at least some of the multiplicity of different double adapter-modified molecules with a formulated relative concentration of primers to generate a normalized population, wherein the formulated relative concentration of primers comprises a multiplicity of primer species each comprising different degenerate sequences at their respective 3′-ends and a corresponding universal primer species, wherein at least one of the degenerate sequences comprises one, two, three, four, five, or six nucleotides, wherein the concentration of the universal primer species is at least ten times greater than the concentration of any one of the primer species comprising a degenerate sequence, and wherein the concentration of the universal primer is greater than the total concentration of the multiplicity of primers comprising different degenerate sequences, and wherein the amplifying comprises a polymerase chain reaction;
determining the nucleotide sequence of a normalized nucleic acid comprising: (a) inserting at least a portion of a normalized nucleic acid into a vector; (b) amplifying the vector comprising the insert in a host cell; and (c) sequencing at least part of the insert of the amplified vector or its complement.; and
identifying the corresponding miRNA species.
US11/093,5872005-03-292005-03-29Methods for normalizing and for identifying small nucleic acidsAbandonedUS20060223066A1 (en)

Priority Applications (4)

Application NumberPriority DateFiling DateTitle
US11/093,587US20060223066A1 (en)2005-03-292005-03-29Methods for normalizing and for identifying small nucleic acids
PCT/US2006/012025WO2007044066A2 (en)2005-03-292006-03-29Methods for normalizing and for identifying small nucleic acids
US12/604,792US8741569B2 (en)2005-03-292009-10-23Methods for normalizing and for identifying small nucleic acids
US14/293,875US20140349301A1 (en)2005-03-292014-06-02Methods for Normalizing and for Identifying Small Nucleic Acids

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US11/093,587US20060223066A1 (en)2005-03-292005-03-29Methods for normalizing and for identifying small nucleic acids

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US12/604,792ContinuationUS8741569B2 (en)2005-03-292009-10-23Methods for normalizing and for identifying small nucleic acids

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US20060223066A1true US20060223066A1 (en)2006-10-05

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US11/093,587AbandonedUS20060223066A1 (en)2005-03-292005-03-29Methods for normalizing and for identifying small nucleic acids
US12/604,792Active2027-04-14US8741569B2 (en)2005-03-292009-10-23Methods for normalizing and for identifying small nucleic acids
US14/293,875AbandonedUS20140349301A1 (en)2005-03-292014-06-02Methods for Normalizing and for Identifying Small Nucleic Acids

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US12/604,792Active2027-04-14US8741569B2 (en)2005-03-292009-10-23Methods for normalizing and for identifying small nucleic acids
US14/293,875AbandonedUS20140349301A1 (en)2005-03-292014-06-02Methods for Normalizing and for Identifying Small Nucleic Acids

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Cited By (8)

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US20070128621A1 (en)*2005-07-152007-06-07Applera CorporationAnalyzing messenger rna and micro rna in the same reaction mixture
US20070128620A1 (en)*2005-07-152007-06-07Applera CorporationHot start reverse transcription by primer design
US20080241831A1 (en)*2007-03-282008-10-02Jian-Bing FanMethods for detecting small RNA species
WO2009018449A1 (en)*2007-07-312009-02-05Verenium CorporationTailored multi-site combinatorial assembly
US20090137415A1 (en)*2005-08-052009-05-28Euclid Diagnostics LlcSUBTRACTIVE SEPARATION AND AMPLIFICATION OF NON-RIBOSOMAL TRANSCRIBED RNA (nrRNA)
US20130005594A1 (en)*2010-03-292013-01-03Dxterity Diagnostics IncorporatedMethods and compositions for detecting target nucleic acids
US20140227691A1 (en)*2010-05-142014-08-14Fluidigm, Inc.Nucleic acid isolation methods
USRE45349E1 (en)1999-06-142015-01-20Bp Corporation North America Inc.Synthetic ligation reassembly in directed evolution

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WO2009091719A1 (en)2008-01-142009-07-23Applera CorporationCompositions, methods, and kits for detecting ribonucleic acid
ES2586153T3 (en)*2010-11-302016-10-11Yafeng Dong Prediction of spontaneous premature birth by measuring free nucleic acids from cells in maternal blood
US10954564B2 (en)2010-11-302021-03-23Yafeng DongCombinations of cell free nucleic acids
US12319966B2 (en)2010-11-302025-06-03Rosetta Signaling Laboratories, LlcCombinations of cell free nucleic acids
CN111793621B (en)2012-11-022024-12-10生命技术公司 Novel compositions, methods and kits for enhancing PCR specificity
ES2890776T3 (en)2015-03-132022-01-24Life Technologies Corp Methods, compositions and kits for the capture, detection and quantification of small RNA
US20240401121A1 (en)*2021-09-302024-12-05The University Of ChicagoUniversal hairpin primer system for quantification of microrna

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US6017702A (en)*1996-12-052000-01-25The Perkin-Elmer CorporationChain-termination type nucleic acid sequencing method including 2'-deoxyuridine-5'-triphosphate
US20030113781A1 (en)*2000-06-062003-06-19Susan BortolinCapture moieties for nucleic acids and uses thereof
US20020197616A1 (en)*2000-10-302002-12-26Gabriel NunezNod2 nucleic acids and proteins
US20030207279A1 (en)*2002-04-252003-11-06Crothers Donald M.Amplification of DNA to produce single-stranded product of defined sequence and length

Cited By (19)

* Cited by examiner, † Cited by third party
Publication numberPriority datePublication dateAssigneeTitle
USRE45349E1 (en)1999-06-142015-01-20Bp Corporation North America Inc.Synthetic ligation reassembly in directed evolution
US20100221790A1 (en)*2005-07-152010-09-02Applied Biosystems, Llc.Analyzing Messenger RNA and Micro RNA in the Same Reaction Mixture
US8487085B2 (en)2005-07-152013-07-16Applied Biosystems, LlcAnalyzing messenger RNA and micro RNA in the same reaction mixture
US9422603B2 (en)2005-07-152016-08-23Applied Biosystems, LlcAnalyzing messenger RNA and micro RNA in the same reaction mixture
US7745122B2 (en)2005-07-152010-06-29Applied Biosystems, LlcAnalyzing messenger RNA and micro RNA in the same reaction mixture
US8962254B2 (en)2005-07-152015-02-24Applied Biosystems, LlcAnalyzing messenger RNA and micro RNA in the same reaction mixture
US20070128621A1 (en)*2005-07-152007-06-07Applera CorporationAnalyzing messenger rna and micro rna in the same reaction mixture
US20070128620A1 (en)*2005-07-152007-06-07Applera CorporationHot start reverse transcription by primer design
US20090137415A1 (en)*2005-08-052009-05-28Euclid Diagnostics LlcSUBTRACTIVE SEPARATION AND AMPLIFICATION OF NON-RIBOSOMAL TRANSCRIBED RNA (nrRNA)
EP2140032A1 (en)*2007-03-282010-01-06Illumina, Inc.Methods for detecting small rna species
US20080241831A1 (en)*2007-03-282008-10-02Jian-Bing FanMethods for detecting small RNA species
CN101821402B (en)*2007-07-312015-03-04Bp法人北美有限公司 pruned multilocus combinatorial assembly
US20100216192A1 (en)*2007-07-312010-08-26Xuqiu TanTailored multi-site combinatorial assembly
EP3031919A1 (en)*2007-07-312016-06-15BP Corporation North America Inc.Tailored multi-site combinational assembly
WO2009018449A1 (en)*2007-07-312009-02-05Verenium CorporationTailored multi-site combinatorial assembly
US9476078B2 (en)2007-07-312016-10-25Basf Enzymes LlcTailored multi-site combinatorial assembly
US20130005594A1 (en)*2010-03-292013-01-03Dxterity Diagnostics IncorporatedMethods and compositions for detecting target nucleic acids
US10066257B2 (en)*2010-03-292018-09-04Dxterity Diagnostics IncorporatedMethods and compositions for detecting target nucleic acids
US20140227691A1 (en)*2010-05-142014-08-14Fluidigm, Inc.Nucleic acid isolation methods

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US20100112581A1 (en)2010-05-06
WO2007044066A2 (en)2007-04-19
WO2007044066A3 (en)2008-01-10
US8741569B2 (en)2014-06-03
US20140349301A1 (en)2014-11-27

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Owner name:APPLERA CORPORATION, CALIFORNIA

Free format text:ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:LAO, KAI QIN;STRAUS, NEIL A.;BURNS, JOHN W.;REEL/FRAME:017524/0163;SIGNING DATES FROM 20050720 TO 20051026

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