A Comparison Between Denaturing Gradient Gel Electrophoresis and Denaturing High Performance Liquid Chromatography in Detecting Mutations in Genes Associated with Hereditary Non-Polyposis Colorectal Cancer (HNPCC) and the Identification of 9 New Mutations Previously Unidentified by DGGE
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作者:
Cliff J. Meldrum
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机构:John Hunter Hospital,Hunter Area Pathology Service
Cliff J. Meldrum
Mary McPhillips
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机构:John Hunter Hospital,Hunter Area Pathology Service
Mary McPhillips
Renee Crooks
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机构:John Hunter Hospital,Hunter Area Pathology Service
Renee Crooks
Lesley Thomas
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机构:John Hunter Hospital,Hunter Area Pathology Service
Lesley Thomas
Ted Edkins
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机构:John Hunter Hospital,Hunter Area Pathology Service
Ted Edkins
Rohanna Creegan
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机构:John Hunter Hospital,Hunter Area Pathology Service
Rohanna Creegan
Ewan Miller
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机构:John Hunter Hospital,Hunter Area Pathology Service
Ewan Miller
Michael Agrez
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机构:John Hunter Hospital,Hunter Area Pathology Service
Michael Agrez
Rodney J. Scott
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机构:John Hunter Hospital,Hunter Area Pathology Service
Rodney J. Scott
机构:
[1] John Hunter Hospital,Hunter Area Pathology Service
[2] Princess Margaret Children's Hospital,Discipline of Surgical Science
[3] University of Newcastle,Newcastle Bowel Research Collaborative
[4] University of Newcastle and the Hunter Medical Research Institute,Discipline of Medical Genetics, Faculty of Health
DGGE;
DHPLC;
hereditary non-polyposis colorectal cancer mutation detection;
D O I:
10.1186/1897-4287-1-1-39
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摘要:
Denaturing high performance liquid chromatography is a relatively new method by which heteroduplex structures formed during the PCR amplification of heterozygote samples can be rapidly identified. The use of this technology for mutation detection in hereditary non-polyposis colorectal cancer (HNPCC) has the potential to appreciably shorten the time it takes to analyze genes associated with this disorder. Prior to acceptance of this method for screening genes associated with HNPCC, assessment of the reliability of this method should be performed. In this report we have compared mutation and polymorphism detection by denaturing gradient gel electrophoresis (DGGE) with denaturing high performance liquid chromatography (DHPLC) in a set of 130 families. All mutations/polymorphisms representing base substitutions, deletions, insertions and a 23 base pair inversion were detected by DHPLC whereas DGGE failed to identify four single base substitutions and a single base pair deletion. In addition, we show that DHPLC has been used for the identification of 5 different mutations in exon 7 of hMSH2 that could not be detected by DGGE.