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Pyrosequencing

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Cover of 'Pyrosequencing'

Table of Contents

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    Book Overview
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    Chapter 1 The History of Pyrosequencing ®
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    Chapter 2 PyroMark(®) Instruments, Chemistry, and Software for Pyrosequencing(®) Analysis.
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    Chapter 3 Software-Based Pyrogram ® Evaluation
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    Chapter 4 Quantitative Validation and Quality Control of Pyrosequencing ® Assays
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    Chapter 5 Extended KRAS and NRAS Mutation Profiling by Pyrosequencing ®
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    Chapter 6 Universal BRAF State Detection by the Pyrosequencing ® -Based U-BRAF V600 Assay
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    Chapter 7 Pyrosequencing
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    Chapter 8 Analysis of Mutational Hotspots in Routinely Processed Bone Marrow Trephines by Pyrosequencing ®
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    Chapter 9 Analysis of Copy Number Variation by Pyrosequencing(®) Using Paralogous Sequences.
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    Chapter 10 Prenatal Diagnosis of Chromosomal Aneuploidies by Quantitative Pyrosequencing(®).
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    Chapter 11 HLA-B and HLA-C Supratyping by Pyrosequencing ®
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    Chapter 12 Allele Quantification Pyrosequencing(®) at Designated SNP Sites to Detect Allelic Expression Imbalance and Loss-of-Heterozygosity.
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    Chapter 13 Quantitative DNA Methylation Analysis by Pyrosequencing(®).
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    Chapter 14 Quantitative Methylation Analysis of the PCDHB Gene Cluster.
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    Chapter 15 Assessment of Changes in Global DNA Methylation Levels by Pyrosequencing(®) of Repetitive Elements.
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    Chapter 16 Global Analysis of DNA 5-Methylcytosine Using the Luminometric Methylation Assay, LUMA.
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    Chapter 17 Limiting Dilution Bisulfite Pyrosequencing(®): A Method for Methylation Analysis of Individual DNA Molecules in a Single or a Few Cells.
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    Chapter 18 Detection of Loss of Imprinting by Pyrosequencing(®).
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    Chapter 19 Analysis of DNA Methylation Patterns in Single Blastocysts by Pyrosequencing(®).
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    Chapter 20 Allele-Specific DNA Methylation Detection by Pyrosequencing(®).
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    Chapter 21 SNP-Based Quantification of Allele-Specific DNA Methylation Patterns by Pyrosequencing ®
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    Chapter 22 DNA Methylation Analysis of ChIP Products at Single Nucleotide Resolution by Pyrosequencing(®).
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    Chapter 23 Multiplex Pyrosequencing ® : Simultaneous Genotyping Based on SNPs from Distant Genomic Regions
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    Chapter 24 Pyrosequencing
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    Chapter 25 Application of Pyrosequencing ® in Food Biodefense
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    Chapter 26 Pyrosequencing
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    Chapter 27 Tissue-Specific DNA Methylation Patterns in Forensic Samples Detected by Pyrosequencing(®).
Attention for Chapter 12: Allele Quantification Pyrosequencing(®) at Designated SNP Sites to Detect Allelic Expression Imbalance and Loss-of-Heterozygosity.
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Chapter title
Allele Quantification Pyrosequencing(®) at Designated SNP Sites to Detect Allelic Expression Imbalance and Loss-of-Heterozygosity.
Chapter number 12
Book title
Pyrosequencing
Published in
Methods in molecular biology, January 2015
DOI 10.1007/978-1-4939-2715-9_12
Pubmed ID
Book ISBNs
978-1-4939-2714-2, 978-1-4939-2715-9
Authors

Kwok, Chau-To, Hitchins, Megan P, Chau-To Kwok, Megan P. Hitchins, Hitchins, Megan P.

Abstract

Pyrosequencing(®) is able to quantitate the level of a nucleotide at a designated germ-line or somatic variant, including single nucleotide polymorphisms (SNPs). SNPs within a gene of interest may be used to distinguish between the two genetic alleles and study their behavior in heterozygous individuals. With regard to cancer etiology and development, identification of alleles and the detection of allelic imbalances, such as transcriptional loss from one allele or loss-of-heterozygosity (due to deletion of one allele), within a tumor are particularly useful. Lynch syndrome, the most common form of hereditary bowel and uterine cancer, is caused by heterozygous germ-line mutations within the DNA mismatch repair genes and tumors develop following inactivation of the remaining functional allele within somatic tissues, usually by acquired loss-of-heterozygosity. MLH1 is the most frequently mutated gene in Lynch syndrome; however, some cases whose tumors display immunohistochemical loss of the MLH1 protein have no apparent mutation within the coding region of MLH1. Allelic loss of expression or reduced function of MLH1 can also result in the propensity to develop Lynch syndrome associated cancers. In this chapter we describe allele quantification Pyrosequencing assays designed at a common benign SNP within the MLH1 coding region for application to either DNA or mRNA (cDNA) templates, which enabled us to detect pathological allelic imbalances in such cases with suspected Lynch syndrome. Our allele quantification Pyrosequencing assays at the MLH1 c.655A > G (rs1799977) exonic SNP were applied to clinical specimens and detected both constitutional allelic expression loss and tumor loss-of-heterozygosity in some cases, facilitating the identification of the mechanistic cause underlying their cancer development. We provide detailed protocols for implementing these Pyrosequencing assays and illustrative examples of their application in patients.

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Mendeley readers

The data shown below were compiled from readership statistics for 9 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 9 100%

Demographic breakdown

Readers by professional status Count As %
Student > Doctoral Student 2 22%
Student > Ph. D. Student 2 22%
Student > Bachelor 1 11%
Researcher 1 11%
Professor > Associate Professor 1 11%
Other 1 11%
Unknown 1 11%
Readers by discipline Count As %
Biochemistry, Genetics and Molecular Biology 4 44%
Medicine and Dentistry 2 22%
Agricultural and Biological Sciences 1 11%
Unknown 2 22%