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US20120156679A1 - Methods for making transcription products - Google Patents

Methods for making transcription products
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Publication number
US20120156679A1
US20120156679A1US13/027,162US201113027162AUS2012156679A1US 20120156679 A1US20120156679 A1US 20120156679A1US 201113027162 AUS201113027162 AUS 201113027162AUS 2012156679 A1US2012156679 A1US 2012156679A1
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United States
Prior art keywords
transcription
promoter
sequence
sense
nucleic acid
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
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US13/027,162
Inventor
Gary A. Dahl
Jerome J. Jendrisak
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Illumina Inc
Cellscript Inc
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Epicentre Technologies Corp
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 Epicentre Technologies CorpfiledCriticalEpicentre Technologies Corp
Priority to US13/027,162priorityCriticalpatent/US20120156679A1/en
Assigned to EPICENTRE TECHNOLOGIES CORPORATIONreassignmentEPICENTRE TECHNOLOGIES CORPORATIONASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: JENDRISAK, JEROME J., DAHL, GARY A.
Assigned to CELLSCRIPT, INC.reassignmentCELLSCRIPT, INC.ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: EPICENTRE TECHNOLOGIES CORPORATION
Publication of US20120156679A1publicationCriticalpatent/US20120156679A1/en
Assigned to ILLUMINA, INC.reassignmentILLUMINA, INC.MERGER (SEE DOCUMENT FOR DETAILS).Assignors: EPICENTRE TECHNOLOGIES CORPORATION
Abandonedlegal-statusCriticalCurrent

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Abstract

The present invention provides methods, compositions and kits for using an RNA polymerase for making transcription products corresponding to a target sequence by obtaining circular single-stranded DNA transcription substrates using a promoter primer that encodes one strand of a double-stranded promoter. The invention has broad applicability for research, diagnostic and therapeutic applications, such as preparing cDNA corresponding to mRNA, making sense or anti-sense probes, detecting gene- or organism-specific sequences, or making RNAi.

Description

Claims (6)

1. A method for making a transcription product corresponding to a target sequence in a target nucleic acid, the method comprising:
(a) obtaining a target nucleic acid;
(b) obtaining a sense promoter primer, the sense promoter primer comprising a 5′-end portion comprising a sense transcription promoter and a 3′-end portion that is complementary to the target;
(c) annealing the sense promoter primer with the target nucleic acid so as to form a target nucleic acid-sense promoter primer complex;
(d) contacting the target nucleic acid-sense promoter primer complex with a DNA polymerase under polymerization reaction conditions so as to obtain first-strand cDNA that is complementary to the target sequence;
(e) obtaining first-strand cDNA;
(f) ligating the first-strand cDNA under ligation conditions so as to obtain circular sense promoter-containing first-strand cDNA;
(g) obtaining an anti-sense promoter oligo;
(h) annealing the anti-sense promoter oligo to the circular sense promoter-containing first-strand cDNA so as to obtain a circular transcription substrate;
(i) obtaining the circular transcription substrate; and
(j) contacting the circular transcription substrate with an RNA polymerase under transcription conditions, wherein a transcription product is obtained.
3. A method for detecting an analyte in or from a sample, the method comprising:
a) obtaining an analyte-binding substance-oligonucleotide (“ABS-oligo”), wherein the ABS-oligo comprises an ABS that is joined to a oligonucleotide comprising a sequence for an anti-sense promoter portion of a double-stranded promoter for an RNA polymerase that recognizes the promoter;
b) obtaining a Signal Probe, wherein the Signal Probe comprises a sense promoter that is joined to the 3′-end of a template, wherein the sense promoter is sufficiently complementary to the anti-sense promoter of the ABS-oligo to form a complex that can be used for transcription of the template using an RNA polymerase that binds to the complex;
c) contacting an ABS-oligo with a surface to which an analyte is bound if present in a sample under analyte-binding conditions that permit the ABS-oligo to bind the analyte if present on said surface;
d) washing the surface under conditions that permit removal of unbound ABS-oligo;
e) contacting the surface with a Signal Probe under complexing conditions that permit complexing of the Signal Probe with the ABS-oligo if present on the surface;
f) optionally, washing the surface under conditions that permit removal of unbound Signal Probe;
g) contacting the surface with an RNA polymerase under conditions that permit transcription of a product encoded by the template using the complex between the ABS-oligo and the Signal Probe; and
h) detecting a transcription product encoded by the template, if present.
4. A method for amplifying the amount of a template-complementary transcription product, the method comprising:
a) obtaining a transcription product;
b) obtaining a sense promoter primer comprising a 3′-end portion that is complementary to the 3′-end of the transcription product and optionally, a phosphate group or a topoisomerase moiety on its 5-end;
c) annealing the sense promoter primer to the transcription product;
d) primer-extending the promoter primer annealed to the transcription product with an RNA-dependent DNA polymerase under DNA synthesis conditions so as to obtain first-strand cDNA;
e) optionally, removing the RNA that is annealed to the first-strand cDNA;
f) ligating the first-strand cDNA, wherein the 5′-end is covalently joined to the 3′-end of the first-strand cDNA so as to obtain circular sense promoter-containing first-strand cDNA;
g) annealing an anti-sense promoter oligo to the circular sense promoter-containing first-strand cDNA so as to obtain a circular substrate for transcription;
h) contacting the circular substrate for transcription with an RNA polymerase under transcription conditions so as to obtain additional transcription product; and
i) obtaining the additional transcription product.
US13/027,1622002-11-212011-02-14Methods for making transcription productsAbandonedUS20120156679A1 (en)

Priority Applications (1)

Application NumberPriority DateFiling DateTitle
US13/027,162US20120156679A1 (en)2002-11-212011-02-14Methods for making transcription products

Applications Claiming Priority (3)

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US42801302P2002-11-212002-11-21
US10/719,913US20040197802A1 (en)2002-11-212003-11-21Methods for using primers that encode one strand of a double-stranded promoter
US13/027,162US20120156679A1 (en)2002-11-212011-02-14Methods for making transcription products

Related Parent Applications (1)

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US10/719,913ContinuationUS20040197802A1 (en)2002-11-212003-11-21Methods for using primers that encode one strand of a double-stranded promoter

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US20120156679A1true US20120156679A1 (en)2012-06-21

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Family Applications (4)

Application NumberTitlePriority DateFiling Date
US10/719,168Expired - LifetimeUS7413857B2 (en)2002-11-212003-11-21Methods for using riboprimers for strand displacement replication of target sequences
US10/719,913AbandonedUS20040197802A1 (en)2002-11-212003-11-21Methods for using primers that encode one strand of a double-stranded promoter
US12/186,127Expired - LifetimeUS7659072B2 (en)2002-11-212008-08-05Methods for using riboprimers for strand displacement replication of target sequences
US13/027,162AbandonedUS20120156679A1 (en)2002-11-212011-02-14Methods for making transcription products

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Application NumberTitlePriority DateFiling Date
US10/719,168Expired - LifetimeUS7413857B2 (en)2002-11-212003-11-21Methods for using riboprimers for strand displacement replication of target sequences
US10/719,913AbandonedUS20040197802A1 (en)2002-11-212003-11-21Methods for using primers that encode one strand of a double-stranded promoter
US12/186,127Expired - LifetimeUS7659072B2 (en)2002-11-212008-08-05Methods for using riboprimers for strand displacement replication of target sequences

Country Status (9)

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US (4)US7413857B2 (en)
EP (3)EP1567675A4 (en)
JP (1)JP4651386B2 (en)
CN (2)CN1738914A (en)
AT (1)ATE411400T1 (en)
AU (3)AU2003297557B2 (en)
CA (1)CA2506805A1 (en)
DE (1)DE60324188D1 (en)
WO (3)WO2004048593A2 (en)

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