Amplification based polymorphism detection
First Claim
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1. A method for detecting a target nucleic acid sequence suspected of having single or large deletions or insertions in a test sample comprising the steps of:
- a) contacting the test sample with amplification reagents comprising a polymerase, a primer pair, and a probe to form a reaction mixture;
b) performing the following cycle comprising the steps of;
(i) maintaining the reaction mixture for a time and at temperature above 90°
C., sufficient to dissociate double stranded nucleic acid sequences,(ii) maintaining the reaction mixture for a time and at a temperature from 45°
C. to 65°
C. to allow the primers and probe to hybridize to the nucleic acid and thereby form primer hybrids and probe hybrids,(iii) maintaining the reaction mixture for a time and at a temperature at least 1°
C. above the temperature in (ii), sufficient to dissociate the probe hybrids, if the probe is not completely complementary to the nucleic acid, and(iv) raising the temperature of the reaction mixture to a temperature sufficient to activate the polymerase;
c) repeatedly performing the cycle of step b) to form an amplification product; and
d) detecting the amplification product as an indication of the presence of the nucleic acid sequence in the test sample.
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Abstract
An improved method of amplifying nucleic acids comprising the use of four discrete temperature steps in a thermocyclic amplification reaction, as well as, a method of detecting large nucleic acid insertions or deletions such as those that occur from gene duplication or deletion.
30 Citations
6 Claims
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1. A method for detecting a target nucleic acid sequence suspected of having single or large deletions or insertions in a test sample comprising the steps of:
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a) contacting the test sample with amplification reagents comprising a polymerase, a primer pair, and a probe to form a reaction mixture; b) performing the following cycle comprising the steps of; (i) maintaining the reaction mixture for a time and at temperature above 90°
C., sufficient to dissociate double stranded nucleic acid sequences,(ii) maintaining the reaction mixture for a time and at a temperature from 45°
C. to 65°
C. to allow the primers and probe to hybridize to the nucleic acid and thereby form primer hybrids and probe hybrids,(iii) maintaining the reaction mixture for a time and at a temperature at least 1°
C. above the temperature in (ii), sufficient to dissociate the probe hybrids, if the probe is not completely complementary to the nucleic acid, and(iv) raising the temperature of the reaction mixture to a temperature sufficient to activate the polymerase; c) repeatedly performing the cycle of step b) to form an amplification product; and d) detecting the amplification product as an indication of the presence of the nucleic acid sequence in the test sample. - View Dependent Claims (2)
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3. A method for determining whether a deletion or insertion of at least 50 base pairs is present in DNA in a test sample comprising the steps of
a) contacting the test sample with amplification reagents wherein the amplification reagents comprise amplification primers, a probe and a polymerase, to form a reaction mixture in which one of the amplification primers hybridize with the target nucleic acid and a standard nucleic acid sequence in the test sample; -
b) subjecting the reaction mixture to amplification conditions to form a target nucleic acid sequence amplification product and a standard nucleic acid amplification product, wherein the amplification conditions comprise performing the following cycle comprising the steps of; (i) maintaining the reaction mixture for a time and at temperature above 90°
C., sufficient to dissociate double stranded DNA sequences,(ii) maintaining the reaction mixture for a time and at a temperature from 45°
C. to 65°
C. to allow the amplification primers and probe to hybridize to the DNA and thereby form primer hybrids and probe hybrids,(iii) maintaining the reaction mixture for a time and at a temperature at least 1°
C. above the temperature in (ii) sufficient to dissociate the probe hybrids, if the probe is not completely complementary to the DNA,(iv) raising the temperature of the reaction mixture to a temperature sufficient to activate the polymerase; c) detecting a first signal that is proportional to the amount of the target nucleic acid sequence amplification product; d) detecting a second signal that is proportional to the amount of the standard nucleic acid amplification product; and e) comparing the first and second signal to determine whether a deletion or insertion of at least 50 base pairs is present in the DNA in the test sample. - View Dependent Claims (4, 5, 6)
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Specification
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Current AssigneeAbbott Laboratories Incorporated
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Original AssigneeAbbott Laboratories Incorporated
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InventorsKatz, David Aaron, Gentile-Davey, Maria C.
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Primary Examiner(s)Chunduru; Suryaprabha
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Application NumberUS09/747,538Publication NumberTime in Patent Office2,413 DaysField of Search435/6, 435/91.2, 536/24.32, 536/24.33, 536/24.31US Class Current435/6.11CPC Class CodesC12Q 1/6858 Allele-specific amplificationC12Q 1/6883 for diseases caused by alte...C12Q 2527/101 TemperatureC12Q 2537/143 Multiplexing, i.e. use of m...C12Q 2545/101 with an internal standard/c...C12Q 2600/156 Polymorphic or mutational m...
