Serial analysis of ribosomal and other microbial sequence tags

US 20070003924A1
Filed: 06/20/2005
Published: 01/04/2007
Est. Priority Date: 06/18/2004
Status: Abandoned Application

First Claim

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1. A method for genetic analysis in complex microbial communities, comprising the steps of:

amplifying a sample containing polynucleotides isolated from a microbial community to provide amplified polynucleotide products using one or more primer pairs, each of said primer pairs having sequences that are complementary to a targeted sequence, wherein each of the primers comprise extensions having restriction endonuclease recognition sites, which, upon digestion of the amplified polynucleotide products with corresponding restriction endonuclease reagents, provide polynucleotide ribosomal sequence tags comprising overhangs that are complementary at their 3′ and

5′

ends;

isolating the amplified polynucleotide products;

digesting the amplified polynucleotide products with the corresponding restriction endonuclease reagents to provide polynucleotide ribosomal sequence tags;

separating the tags from the primers;

concatenating the tags in a head to tail orientation.

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Abstract

A simple and robust method for genetic analysis of complex microbial communities involves the steps of PCR amplification of V1 region of rrs genes in the community DNA sample using two universal primers, followed by cleavage by BsgI and removal of dual-biotinylated primers using streptavidin-coated magnetic beads to purify RSTs, and concatemerization of the RSTs and size selection of resultant concatemers by agarose gel electrophoresis. The isolated concatamers are then cloned and sequenced and subjected to sequence analyses to enable identification of the members of the microbial community.

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20 Claims

1. A method for genetic analysis in complex microbial communities, comprising the steps of:
- amplifying a sample containing polynucleotides isolated from a microbial community to provide amplified polynucleotide products using one or more primer pairs, each of said primer pairs having sequences that are complementary to a targeted sequence, wherein each of the primers comprise extensions having restriction endonuclease recognition sites, which, upon digestion of the amplified polynucleotide products with corresponding restriction endonuclease reagents, provide polynucleotide ribosomal sequence tags comprising overhangs that are complementary at their 3′ and
  
  5′
  
  ends;
  
  isolating the amplified polynucleotide products;
  
  digesting the amplified polynucleotide products with the corresponding restriction endonuclease reagents to provide polynucleotide ribosomal sequence tags;
  
  separating the tags from the primers;
  
  concatenating the tags in a head to tail orientation.
- View Dependent Claims (2, 3, 4, 5, 6)
- - 2. The method according to claim 1 wherein the concatenated tags are subjected to sequence analysis.
  - 3. The method according to claim 1 wherein the primers are complementarity to the V1 region of 16S rrs gene.
  - 4. The method according to claim 3 wherein the restriction endonuclease recognition sites of the primers are BsgI restriction endonuclease sites.
  - 5. The method according to claim 4, wherein the primers each have a dual biotin label.
  - 6. The method according to claim 5, wherein the primers comprise a first primer having the sequence 5′
    - -TTT GAC CGT GCA GCY TAA YRC ATG CAA GTC G-3′
      
      (SEQ ID NO;
      
      1) and a second primer having the sequence 5′
      
      -TTT GAC CGT GCA GYY CAC GYG TTA CKC ACC CGT-3′
      
      (SEQ ID NO;
      
      2).

7. A method for genetic analysis of complex microbial communities, comprising the steps of:
- amplifying a DNA sample from a microbial community to provide amplified polynucleotide products using primer pairs having sequences that are complementary to one of the V1 through V9 regions of the ribosomal genes, wherein each of the primers comprise extensions having restriction endonuclease recognition sites, which, upon digestion of the amplified polynucleotide products with corresponding restriction endonuclease reagents, provide polynucleotide ribosomal sequence tags comprising overhangs that are complementary at their 3′ and
  
  5′
  
  ends;
  
  isolating the amplified polynucleotide products;
  
  digesting the amplified polynucleotide products with the corresponding restriction endonuclease reagents to provide polynucleotide ribosomal sequence tags;
  
  separating the tags from the primers;
  
  concatenating the tags in a head to tail orientation.
- View Dependent Claims (8, 9, 10, 11)
- - 8. The method according to claim 7 wherein the concatenated tags are subjected to sequence analysis.
  - 9. The method according to claim 7 wherein the restriction endonuclease recognition sites of the primers are BsgI restriction endonuclease sites.
  - 10. The method according to claim 9, wherein the primers each have a dual biotin label.
  - 11. The method according to claim 10, wherein the primers are complementarity to the V1 region of 16S rrs gene and comprise a first primer having the sequence 5′
    - -TTT GAC CGT GCA GCY TAA YRC ATG CAA GTC G-3′
      
      (SEQ ID NO;
      
      1) and a second primer having the sequence 5′
      
      -TTT GAC CGT GCA GYY CAC GYG TTA CKC ACC CGT-3′
      
      (SEQ ID NO;
      
      2).

12. A method for genetic analysis of complex microbial communities, comprising the steps of:
- amplifying a DNA sample from a microbial community to provide amplified polynucleotide products using primer pairs having sequences that are complementary to one or more antibiotic or antimicrobial resistance genes, wherein each of the primers comprise extensions having restriction endonuclease recognition sites, which, upon digestion of the amplified polynucleotide products with corresponding restriction endonuclease reagents, provide polynucleotide ribosomal sequence tags comprising overhangs that are complementary at their 3′ and
  
  5′
  
  ends;
  
  isolating the amplified polynucleotide products;
  
  digesting the amplified polynucleotide products with the corresponding restriction endonuclease reagents to provide polynucleotide ribosomal sequence tags;
  
  separating the tags from the primers;
  
  concatenating the tags in a head to tail orientation.
- View Dependent Claims (13, 14, 15)
- - 13. The method according to claim 12 wherein the concatenated tags are subjected to sequence analysis.
  - 14. The method according to claim 12 wherein the restriction endonuclease recognition sites of the primers are BsgI restriction endonuclease sites.
  - 15. The method according to claim 14, wherein the primers each have a dual biotin label.

16. Isolated polynucleotide primers for amplifying and isolating DNA tags located within a targeted genetic region from one or more microbial organisms, comprising polynucleotides having sequences that are complementary to sequences within the targeted genetic region and extensions designed to enable direct concatenation of two or more isolated tags in a head to tail orientation without the need for intermediate linkers.
- View Dependent Claims (17)
- - 17. Isolated polynucleotide primers according to claim 16, wherein the primers comprise a first and a second primer, each primer comprising a dual biotin label and a BsgI restriction endonuclease site, said first primer having the sequence 5′
    - -TTT GAC CGT GCA GCY TAA YRC ATG CAA GTC G-3′
      
      (SEQ ID NO;
      
      1), and said second primer having the sequence 5′
      
      -TTT GAC CGT GCA GYY CAC GYG TTA CKC ACC CGT-3′
      
      (SEQ ID NO;
      
      2).

18. A kit for evaluating microbial populations, comprising one or more primer sets used to provide amplified polynucleotide products in appropriate containers, each of said one or more primer sets comprising primer pairs for targeting specific genetic regions in a microbial genome, each of said primers having extension sequences encoding for restriction endonuclease recognition sites which, upon digestion of the to provide amplified polynucleotide products with corresponding restriction endonuclease reagents, produce isolated polynucleotide tags from within the targeted region of DNA, said tags comprising overhangs that are complementary at their 3′
- and 5′
  
  ends;
  
  reaction components in appropriate containers comprising restriction endonucleases corresponding to and specific for the restriction endonuclease recognition sites on the one or more primer sets;
  
  at least one ligase for producing concatemers, such as T4 ligase, in an appropriate container;
  
  DNA polymerase, such as T4 DNA polymerase, in an appropriate container; and
  
  a cloning vector in an appropriate container.
- View Dependent Claims (19, 20)
- - 19. A kit according to claim 18 wherein the primers have complementarity to one of the V1 through V9 regions of the ribosomal genes or to one or more antibiotic or antimicrobial resistance genes, or combinations thereof.
  - 20. A kit according to claim 19, comprising a first and a second primer, each primer having complementarity to the V1 region of 16S rrs gene, a BsgI restriction endonuclease recognition site, and a dual biotin label, the first primer having the sequence 5′
    - -TTT GAC CGT GCA GCY TAA YRC ATG CAA GTC G-3′
      
      (SEQ ID NO;
      
      1), and the second primer having the sequence 5′
      
      -TTT GAC CGT GCA GYY CAC GYG TTA CKC ACC CGT-3′
      
      (SEQ ID NO;
      
      2).

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Current Assignee
The Ohio State University Research Foundation
Original Assignee
The Ohio State University Research Foundation
Inventors
Morrison, Mark, Yu, Zhongtang, Yu, Marie

Application Number

US11/157,072
Publication Number

US 20070003924A1
Time in Patent Office

Days
Field of Search
US Class Current

435/5
CPC Class Codes

C12Q 1/6809   Methods for determination o...

C12Q 1/689   for bacteria

C12Q 2521/313   Type II endonucleases, i.e....

C12Q 2525/131   incorporating a restriction...

C12Q 2539/103   Serial analysis of gene exp...

Serial analysis of ribosomal and other microbial sequence tags

First Claim

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Abstract

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Serial analysis of ribosomal and other microbial sequence tags

First Claim

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Abstract

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