Complexity management of genomic DNA

US 7,202,039 B2
Filed: 11/03/2004
Issued: 04/10/2007
Est. Priority Date: 07/25/2001
Status: Expired due to Fees

First Claim

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1. A method for analyzing a first nucleic acid sample comprising:

obtaining a second nucleic acid sample by;

fragmenting the first nucleic acid sample to produce double stranded fragments;

ligating one or more adaptors to the double stranded fragments;

digesting the adaptor ligated double stranded fragments to produce single stranded half molecules;

adding a homopolymeric tail to the 3′

end of the single stranded half molecules, hybridizing a primer to the homopolymeric tail and extending the primer to generate double stranded half fragments from the single stranded half molecules; and

amplifying a plurality of the double stranded half fragments by a polymerase chain reaction (PCR) wherein the size of the amplified fragments is modulated by varying one or more reaction conditions or reagents to reduce the complexity of the first nucleic acid sample;

providing a nucleic acid array;

hybridizing the second nucleic acid sample to the array; and

analyzing a hybridization pattern resulting from the hybridization.

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Abstract

The presently claimed invention provides for novel methods and kits for reducing the complexity of a nucleic acid sample by providing non-gel based methods for size fractionation. In a preferred embodiment, size fractionation can be accomplished by varying conditions or reagents of a PCR reaction to amplify fragments of specific size ranges. The invention further provides for analysis of the above sample by hybridization to an array, which may be specifically designed to interrogate the desired fragments for particular characteristics, such as, for example, the presence or absence of a polymorphism.

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15 Claims

1. A method for analyzing a first nucleic acid sample comprising:
- obtaining a second nucleic acid sample by;
  
  fragmenting the first nucleic acid sample to produce double stranded fragments;
  
  ligating one or more adaptors to the double stranded fragments;
  
  digesting the adaptor ligated double stranded fragments to produce single stranded half molecules;
  
  adding a homopolymeric tail to the 3′
  
  end of the single stranded half molecules, hybridizing a primer to the homopolymeric tail and extending the primer to generate double stranded half fragments from the single stranded half molecules; and
  
  amplifying a plurality of the double stranded half fragments by a polymerase chain reaction (PCR) wherein the size of the amplified fragments is modulated by varying one or more reaction conditions or reagents to reduce the complexity of the first nucleic acid sample;
  
  providing a nucleic acid array;
  
  hybridizing the second nucleic acid sample to the array; and
  
  analyzing a hybridization pattern resulting from the hybridization.
- View Dependent Claims (2, 3, 4, 5, 6, 7)
- - 2. The method of claim 1 wherein the reaction condition or reagent varied is chosen from the group consisting of:
    - extension time, annealing time, primer concentration, primer length, presence or absence of 3′
      
      to 5′
      
      exonuclease activity, and concentration of nucleotide analogues.
  - 3. The method of claim 1 wherein the method for analyzing a first nucleic acid sample comprises determining whether the first nucleic acid sample contains sequence variations.
  - 4. The method of claim 3 wherein the sequence variations are single nucleotide polymorphisms (SNPs).
  - 5. The method of claim 1 wherein the nucleic acid array is designed to query DNA fragments which have been produced by the procedures used to obtain the second nucleic acid sample.
  - 6. The method of claim 1 wherein a substantial amount of the sequences predicted to be contained in the second nucleic acid sample are predetermined.
  - 7. The method of claim 1 wherein a substantial amount of the sequences predicted to be contained in the second nucleic acid sample are first determined by a computer system.

8. A method of screening for DNA sequence variations in an individual comprising:
- providing a first nucleic acid sample from the individual;
  
  obtaining a second nucleic acid sample by;
  
  fragmenting the first nucleic acid sample to produce double stranded fragments;
  
  ligating adaptor sequences to the double stranded fragments;
  
  digesting the adaptor ligated double stranded fragments to produce single stranded half molecules;
  
  adding a homopolymeric tail to the 3′
  
  end of the single stranded half molecules, hybridizing a primer to the homopolymeric tail and extending the primer to generate double stranded half fragments from the single stranded half molecules; and
  
  ,amplifying a subset of the double stranded half fragments by a polymerase chain reaction (PCR) wherein one or more reaction conditions or reagents are varied to favor amplification of a subset of fragments of a specific size range;
  
  providing a nucleic acid array wherein the array comprises probes designed to interrogate for DNA sequence variations;
  
  hybridizing the second nucleic acid sample to the array;
  
  generating a hybridization pattern resulting from the hybridization; and
  
  determining the presence or absence of DNA sequence variations in the individual based upon an analysis of the hybridization pattern.
- View Dependent Claims (9, 10, 11)
- - 9. The method of claim 8 wherein the sequence variation is a single nucleotide polymorphism (SNP).
  - 10. The method of claim 8 wherein the SNP is associated with a disease.
  - 11. The method of claim 8 wherein the SNP is associated with the efficacy of a drug.

12. A method for screening for DNA sequence variations in a population of individuals comprising:
- providing a first nucleic acid sample from each of the individuals;
  
  providing a second nucleic acid sample by;
  
  fragmenting the first nucleic acid sample to produce double stranded fragments;
  
  ligating adaptor sequences to the double stranded fragments;
  
  digesting the adaptor ligated double stranded fragments to produce single stranded half molecules;
  
  adding a homopolymeric tail to the 3′
  
  end of the single stranded half molecules, hybridizing a primer to the homopolymeric tail and extending the primer to generate double stranded half fragments from the single stranded half molecules;
  
  amplifying a subset of the double stranded half fragments by a polymerase chain reaction (PCR) wherein one or more reaction conditions or reagents are varied to favor amplification of a subset of fragments of a specific size range; and
  
  providing a plurality of nucleic acid arrays wherein the arrays comprise probes designed to interrogate for DNA sequence variations;
  
  hybridizing each of the second nucleic acid samples to one of the plurality of arrays;
  
  generating a plurality of hybridization patterns resulting from the hybridizations; and
  
  analyzing the hybridization patterns to determine the presence or absence of sequence variation in the population of individuals.
- View Dependent Claims (13, 14)
- - 13. The method of claim 12 wherein the sequence variation is a single nucleotide polymorphism (SNP).
  - 14. The method of claim 12 further comprising the steps of diluting the product of the PCR and amplifying the diluted product by a second round of PCR.

15. A method of genotyping an individual comprising:
- identifying a collection of SNPs that are found on fragments of a selected size range resulting from digestion with one or more selected restriction enzymes;
  
  designing an array to interrogate the collection of SNPs;
  
  providing a first nucleic acid sample from the individual;
  
  fragmenting the first nucleic acid sample with the one or more selected restriction enzymes to produce double stranded fragments;
  
  ligating adaptor sequences to the double stranded fragments;
  
  digesting the adaptor ligated double stranded fragments to produce single stranded half molecules;
  
  adding a homopolymeric tail to the 3′
  
  end of the single stranded half molecules, hybridizing a primer to the homopolymeric tail and extending the primer to generate double stranded half fragments from the single stranded half molecules;
  
  amplifying the double stranded half fragments by PCR wherein a subset of fragments of the selected size range are preferentially amplified to obtain a PCR product;
  
  hybridizing the PCR product to an array; and
  
  analyzing the hybridization pattern to determine the presence or absence of the collection of SNPs.

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Current Assignee
Affymetrix, Inc. (Thermo Fisher Scientific Incorporated)
Original Assignee
Affymetrix, Inc. (Thermo Fisher Scientific Incorporated)
Inventors
Su, Xing
Primary Examiner(s)
Fredman; Jeffrey
Assistant Examiner(s)
BERTAGNA, ANGELA MARIE

Application Number

US10/981,222
Publication Number

US 20050079536A1
Time in Patent Office

888 Days
Field of Search

None
US Class Current

435/6.12
CPC Class Codes

C12Q 1/6855   Ligating adaptors

C12Q 2527/113   Time

C12Q 2527/143   Concentration of primer or ...

Complexity management of genomic DNA

First Claim

4 Assignments

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Abstract

Citations

15 Claims

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Complexity management of genomic DNA

First Claim

4 Assignments

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Abstract

Citations

15 Claims

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