Reducing chimera formation during PCR amplification to ensure accurate genotyping

Redmond P Smyth; Timothy E Schlub; Andrew J Grimm; Vanessa Venturi; Abha Chopra; Simon Mallal; Miles P Davenport; Johnson Mak

doi:10.1016/j.gene.2010.08.009

Reducing chimera formation during PCR amplification to ensure accurate genotyping

Redmond P Smyth, Timothy E Schlub, Andrew J Grimm, Vanessa Venturi, Abha Chopra, Simon Mallal, Miles P Davenport, Johnson Mak

Biochemistry & Molecular Biology

Research output: Contribution to journal › Article › Research › peer-review

82 Citations (Scopus)

Abstract

Measurements of population diversity are fundamental to the reconstruction of the evolutionary and epidemiological history of organisms. Commonly used protocols to measure population diversity using the polymerase chain reaction (PCR) are prone to the introduction of artificial chimeras. These are often difficult to detect and can confound the correct interpretation of results due to the false generation of recombinants when the underlying DNA sample contains multiple distinct templates. This study presents a standardised procedure to suppress the formation of artificial chimeras during PCR amplification. The solution is based on the accurate determination of the efficiency and end point of the log-linear phase of a PCR. This procedure will facilitate the generation of data sets that more accurately reflect the underlying population diversity rather than artifacts introduced by the process itself.

Original language	English
Pages (from-to)	45 - 51
Number of pages	7
Journal	Gene
Volume	469
Issue number	1-2
DOIs	https://doi.org/10.1016/j.gene.2010.08.009
Publication status	Published - 2010

Access to Document

10.1016/j.gene.2010.08.009

Cite this

@article{78f489d2b1d54aeea4497c3326ec1793,

title = "Reducing chimera formation during PCR amplification to ensure accurate genotyping",

abstract = "Measurements of population diversity are fundamental to the reconstruction of the evolutionary and epidemiological history of organisms. Commonly used protocols to measure population diversity using the polymerase chain reaction (PCR) are prone to the introduction of artificial chimeras. These are often difficult to detect and can confound the correct interpretation of results due to the false generation of recombinants when the underlying DNA sample contains multiple distinct templates. This study presents a standardised procedure to suppress the formation of artificial chimeras during PCR amplification. The solution is based on the accurate determination of the efficiency and end point of the log-linear phase of a PCR. This procedure will facilitate the generation of data sets that more accurately reflect the underlying population diversity rather than artifacts introduced by the process itself.",

author = "Smyth, {Redmond P} and Schlub, {Timothy E} and Grimm, {Andrew J} and Vanessa Venturi and Abha Chopra and Simon Mallal and Davenport, {Miles P} and Johnson Mak",

year = "2010",

doi = "10.1016/j.gene.2010.08.009",

language = "English",

volume = "469",

pages = "45 -- 51",

journal = "Gene",

issn = "0378-1119",

publisher = "Elsevier",

number = "1-2",

}

TY - JOUR

T1 - Reducing chimera formation during PCR amplification to ensure accurate genotyping

AU - Smyth, Redmond P

AU - Schlub, Timothy E

AU - Grimm, Andrew J

AU - Venturi, Vanessa

AU - Chopra, Abha

AU - Mallal, Simon

AU - Davenport, Miles P

AU - Mak, Johnson

PY - 2010

Y1 - 2010

N2 - Measurements of population diversity are fundamental to the reconstruction of the evolutionary and epidemiological history of organisms. Commonly used protocols to measure population diversity using the polymerase chain reaction (PCR) are prone to the introduction of artificial chimeras. These are often difficult to detect and can confound the correct interpretation of results due to the false generation of recombinants when the underlying DNA sample contains multiple distinct templates. This study presents a standardised procedure to suppress the formation of artificial chimeras during PCR amplification. The solution is based on the accurate determination of the efficiency and end point of the log-linear phase of a PCR. This procedure will facilitate the generation of data sets that more accurately reflect the underlying population diversity rather than artifacts introduced by the process itself.

AB - Measurements of population diversity are fundamental to the reconstruction of the evolutionary and epidemiological history of organisms. Commonly used protocols to measure population diversity using the polymerase chain reaction (PCR) are prone to the introduction of artificial chimeras. These are often difficult to detect and can confound the correct interpretation of results due to the false generation of recombinants when the underlying DNA sample contains multiple distinct templates. This study presents a standardised procedure to suppress the formation of artificial chimeras during PCR amplification. The solution is based on the accurate determination of the efficiency and end point of the log-linear phase of a PCR. This procedure will facilitate the generation of data sets that more accurately reflect the underlying population diversity rather than artifacts introduced by the process itself.

UR - http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&dopt=Citation&list_uids=20833233

U2 - 10.1016/j.gene.2010.08.009

DO - 10.1016/j.gene.2010.08.009

M3 - Article

SN - 0378-1119

VL - 469

SP - 45

EP - 51

JO - Gene

JF - Gene

IS - 1-2

ER -

Reducing chimera formation during PCR amplification to ensure accurate genotyping

Abstract

Access to Document

Other files and links

Cite this