Comparative genomic hybridization (CGH)

US 5,965,362 A
Filed: 11/27/1995
Issued: 10/12/1999
Est. Priority Date: 03/04/1992
Status: Expired due to Term

First Claim

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1. A method of detecting an amplification of unique sequences of at least one position selected from the group consisting of about position q24 of human chromosome 8, about position q13 of human chromosome 11 and about position q22-q24 on human chromosome 17, in a genome being tested, said method comprising the steps of:

(a) differently labelling DNA sequences from the test genome and a normal human genome;

(b) hybridizing said labelled DNA sequences from each of said genomes to a reference genome under the following conditions;

(i) either the labelled DNA sequences or the reference genome, or both, have their repetitive sequences blocked and/or removed; and

(ii) DNA unique sequences in the reference genome are retained; and

(c) comparing the intensities of the signals from the labelled DNA sequences as a function of position on the reference genome, thereby allowing detection of the presence or absence of the amplification in the test genome.

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Abstract

Disclosed are new methods comprising the use of in situ hybridization to detect abnormal nucleic acid sequence copy numbers in one or more genomes wherein repetitive sequences that bind to multiple loci in a reference chromosome spread are either substantially removed and/or their hybridization signals suppressed. The invention termed Comparative Genomic Hybridization (CGH) provides for methods of determining the relative number of copies of nucleic acid sequences in one or more subject genomes or portions thereof (for example, a tumor cell) as a function of the location of those sequences in a reference genome (for example, a normal human genome). The intensity(ies) of the signals from each labeled subject nucleic acid and/or the differences in the ratios between different signals from the labeled subject nucleic acid sequences are compared to determine the relative copy numbers of the nucleic acid sequences in the one or more subject genomes as a function of position along the reference chromosome spread. Amplifications, duplications and/or deletions in the subject genome(s) can be detected. Also provided is a method of determining the absolute copy numbers of substantially all RNA or DNA sequences in subject cell(s) or cell population(s).

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12 Claims

1. A method of detecting an amplification of unique sequences of at least one position selected from the group consisting of about position q24 of human chromosome 8, about position q13 of human chromosome 11 and about position q22-q24 on human chromosome 17, in a genome being tested, said method comprising the steps of:
- (a) differently labelling DNA sequences from the test genome and a normal human genome;
  
  (b) hybridizing said labelled DNA sequences from each of said genomes to a reference genome under the following conditions;
  
  (i) either the labelled DNA sequences or the reference genome, or both, have their repetitive sequences blocked and/or removed; and
  
  (ii) DNA unique sequences in the reference genome are retained; and
  
  (c) comparing the intensities of the signals from the labelled DNA sequences as a function of position on the reference genome, thereby allowing detection of the presence or absence of the amplification in the test genome.
- View Dependent Claims (2, 3, 4, 5, 6)
- - 2. The method of claim 1, wherein the step of comparing the intensities of the signals from the labelled DNA sequences comprises determining the ratio of the intensities of the signals as a function of position in the reference genome.
  - 3. The method of claim 1, wherein the amplification is detected at about position q24 of human chromosome 8 in the test genome.
  - 4. The method of claim 1, wherein the amplification is detected at about position q13 of human chromosome 11 in the test genome.
  - 5. The method of claim 1, wherein the amplification is detected at about position q22-q24 on human chromosome 17 in the test genome.
  - 6. The method of claim 1, wherein the reference genome comprises at least one metaphase chromosome.

7. A method of detecting an amplification of at least one chromosome arm selected from the group consisting of the q arm of human chromosome 1, the q arm of human chromosome 8 and the q arm of human chromosome 20, in a genome being tested, said method comprising the steps of:
- (a) differently labelling DNA sequences from the test genome and a normal human genome;
  
  (b) hybridizing said labelled DNA sequences from each of said genomes to a reference genome under the following conditions;
  
  (i) either the labelled DNA sequences or the reference genome, or both, have their repetitive sequences blocked and/or removed; and
  
  (ii) DNA unique sequences in the reference genome are retained; and
  
  (c) comparing the intensities of the signals from the labelled DNA sequences as a function of position on the reference genome, thereby allowing detection of the presence or absence of the amplification in the test genome.
- View Dependent Claims (8, 9, 10, 11, 12)
- - 8. The method of claim 7, wherein the step of comparing the intensities of the signals from the labelled DNA sequences comprises determining the ratio of the intensities of the signals as a function of position in the reference genome.
  - 9. The method of claim 7, wherein the amplification is of the q arm of human chromosome 1.
  - 10. The method of claim 7, wherein the amplification is of the q arm of human chromosome 8.
  - 11. The method of claim 7, wherein the amplification is of the q arm of human chromosome 20.
  - 12. The method of claim 7, wherein the reference genome comprises at least one metaphase chromosome.

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Current Assignee
Regents of the University of California (University of California)
Original Assignee
Regents of the University of California (University of California)
Inventors
Sakamoto, Masaru, Waldman, Frederic, Pinkel, Daniel, Gray, Joe W., Kallioniemi, Anne, Kallioniemi, Olli-Pekka
Primary Examiner(s)
Jones, W. Gary
Assistant Examiner(s)
FREDMAN, JEFFREY NORMAN

Application Number

US08/562,965
Time in Patent Office

1,415 Days
Field of Search

435/5, 435/6, 435/91.2, 536/22.1, 536/23.1, 536/24.3, 536/24.31, 536/24.32, 536/24.33, 424/9.1
US Class Current

435/6.14
CPC Class Codes

C12Q 1/6809   Methods for determination o...

C12Q 1/6841   In situ hybridisation

C12Q 1/6886   for cancer immunoassay for ...

C12Q 2537/157   A reaction step characteris...

C12Q 2545/114   involving a quantitation step

C12Q 2600/156   Polymorphic or mutational m...

G06F 15/025   adapted to a specific appli...

Y10S 436/813   Cancer

Comparative genomic hybridization (CGH)

First Claim

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Abstract

106 Citations

12 Claims

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Comparative genomic hybridization (CGH)

First Claim

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Abstract

106 Citations

12 Claims

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