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Pyrosequencing

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Cover of 'Pyrosequencing'

Table of Contents

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    Book Overview
  2. Altmetric Badge
    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 11: HLA-B and HLA-C Supratyping by Pyrosequencing ®
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Chapter title
HLA-B and HLA-C Supratyping by Pyrosequencing ®
Chapter number 11
Book title
Pyrosequencing
Published in
Methods in molecular biology, January 2015
DOI 10.1007/978-1-4939-2715-9_11
Pubmed ID
Book ISBNs
978-1-4939-2714-2, 978-1-4939-2715-9
Authors

Irene Vanni, Elisabetta Ugolotti, Patrizia Larghero, Roberto Biassoni, Vanni, Irene, Ugolotti, Elisabetta, Larghero, Patrizia, Biassoni, Roberto

Abstract

Usually, HLA typing has been performed either by serology-based typing incubating a panel of known anti-HLA antibodies with viable lymphocytes of unknown HLA type or by molecular typing including medium-resolution HLA typing by Sequence Specific Oligonucleotide Probes (SSOP) or high-resolution HLA typing by Sequence Based Typing (SBT). Traditionally, HLA antigens have been defined using serological techniques, but these methods have several disadvantages, such as low resolution, the requirement for viable cells, and cell surface expression of HLA molecules. HLA type screening methods are categorized as low, medium, and high resolution, and only sequencing-based typing methods provide the highest resolution and are considered the gold standard for HLA typing.Among the HLA SBT based-methods, the Pyrosequencing(®) technique is an extremely versatile and accurate real-time sequencing technique with some advantages compared to classic Sanger method.Here, we describe a quick and inexpensive method that allows through the use of Pyrosequencing subtyping of HLA class I molecules, into HLA-Bw6, -Bw4 I80, or -Bw4 T80 and HLA-C1, or -C2 groups. In particular, this analysis is focused on the amino acids around residue 80. This method demonstrated good sensitivity, specificity, and reproducibility. Using a quantitative allele acquisition mode, the method provides accurate sequence information required for the definition of heterozygous and/or homozygous samples.

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Mendeley readers

The data shown below were compiled from readership statistics for 3 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 3 100%

Demographic breakdown

Readers by professional status Count As %
Researcher 2 67%
Unknown 1 33%
Readers by discipline Count As %
Immunology and Microbiology 2 67%
Unknown 1 33%