Literature DB >> 21111699

Design, construction, and validation of a modular library of sequence diversity standards for polymerase chain reaction.

Paul D Baum1, Jennifer J Young, Qianjun Zhang, Zeljka Kasakow, Joseph M McCune.   

Abstract

Methods to measure the sequence diversity of polymerase chain reaction (PCR)-amplified DNA lack standards for use as assay calibrators and controls. Here we present a general and economical method for developing customizable DNA standards of known sequence diversity. Standards ranging from 1 to 25,000 sequences were generated by directional ligation of oligonucleotide "words" of standard length and GC content and then amplified by PCR. The sequence accuracy and diversity of the library were validated using AmpliCot analysis (DNA hybridization kinetics) and Illumina sequencing. The library has the following features: (i) pools containing tens of thousands of sequences can be generated from the ligation of relatively few commercially synthesized short oligonucleotides; (ii) each sequence differs from all others in the library at a minimum of three nucleotide positions, permitting discrimination between different sequences by either sequencing or hybridization; (iii) all sequences have identical length, GC content, and melting temperature; (iv) the identity of each standard can be verified by restriction digestion; and (v) once made, the ends of the library may be cleaved and replaced with sequences to match any PCR primer pair. These standards should greatly improve the accuracy and reproducibility of sequence diversity measurements.
Copyright © 2010 Elsevier Inc. All rights reserved.

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Year:  2010        PMID: 21111699      PMCID: PMC3073996          DOI: 10.1016/j.ab.2010.11.035

Source DB:  PubMed          Journal:  Anal Biochem        ISSN: 0003-2697            Impact factor:   3.365


  26 in total

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2.  Direct measurement of lymphocyte receptor diversity.

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3.  In vitro selection of RNA molecules that bind specific ligands.

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4.  Searching for peptide ligands with an epitope library.

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Journal:  Science       Date:  1990-07-27       Impact factor: 47.728

5.  DNA recombination during PCR.

Authors:  A Meyerhans; J P Vartanian; S Wain-Hobson
Journal:  Nucleic Acids Res       Date:  1990-04-11       Impact factor: 16.971

6.  A ligase-mediated gene detection technique.

Authors:  U Landegren; R Kaiser; J Sanders; L Hood
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Authors:  Hamilton O Smith; Clyde A Hutchison; Cynthia Pfannkoch; J Craig Venter
Journal:  Proc Natl Acad Sci U S A       Date:  2003-12-02       Impact factor: 11.205

8.  A microfluidic oligonucleotide synthesizer.

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9.  DNA display I. Sequence-encoded routing of DNA populations.

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Journal:  PLoS Biol       Date:  2004-06-22       Impact factor: 8.029

10.  Multi-line split DNA synthesis: a novel combinatorial method to make high quality peptide libraries.

Authors:  Ichiro Tabuchi; Sayaka Soramoto; Shingo Ueno; Yuzuru Husimi
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  4 in total

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2.  Blood T-cell receptor diversity decreases during the course of HIV infection, but the potential for a diverse repertoire persists.

Authors:  Paul D Baum; Jennifer J Young; Diane Schmidt; Qianjun Zhang; Rebecca Hoh; Michael Busch; Jeffrey Martin; Steven Deeks; Joseph M McCune
Journal:  Blood       Date:  2012-02-27       Impact factor: 22.113

3.  Microarray generation of thousand-member oligonucleotide libraries.

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Journal:  PLoS One       Date:  2011-09-23       Impact factor: 3.240

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Journal:  PLoS One       Date:  2014-10-15       Impact factor: 3.240

  4 in total

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