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Natural Killer Cells

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Cover of 'Natural Killer Cells'

Table of Contents

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    Book Overview
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    Chapter 1 Natural Killer Cells
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    Chapter 2 Natural Killer Cells
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    Chapter 3 Assessment of NK Cell Metabolism.
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    Chapter 4 Genotyping Single Nucleotide Polymorphisms and Copy Number Variability of the FCGRs Expressed on NK Cells.
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    Chapter 5 Measurement of Average Telomere Length in Ex Vivo Expanded Natural Killer Cells by Fluorescence In Situ Hybridization (FISH) and Flow Cytometry.
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    Chapter 6 In Vitro Assessment of Human Natural Killer Cell Migration and Invasion.
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    Chapter 7 Natural Killer Cells
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    Chapter 8 Microwell-Based Live Cell Imaging of NK Cell Dynamics to Assess Heterogeneity in Motility and Cytotoxic Response.
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    Chapter 9 Assessment of Natural Killer Cell Cytotoxicity Using Image Cytometry Method.
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    Chapter 10 Natural Killer Cells
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    Chapter 11 Using NK Cell Lipid Raft Fractionation to Understand the Role of Lipid Rafts in NK Cell Receptor Signaling.
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    Chapter 12 Natural Killer Cells
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    Chapter 13 The Planar Lipid Bilayer System Serves as a Reductionist Approach for Studying NK Cell Immunological Synapses and Their Functions.
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    Chapter 14 Natural Killer Cells
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    Chapter 15 Natural Killer Cells
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    Chapter 16 Large-Scale Culture and Genetic Modification of Human Natural Killer Cells for Cellular Therapy.
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    Chapter 17 Gene Modification of Human Natural Killer Cells Using a Retroviral Vector.
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    Chapter 18 Modification of Expanded NK Cells with Chimeric Antigen Receptor mRNA for Adoptive Cellular Therapy.
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    Chapter 19 mRNA Transfection to Improve NK Cell Homing to Tumors.
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    Chapter 20 Natural Killer Cells
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    Chapter 21 Engineering Receptor Expression on Natural Killer Cells Through Trogocytosis.
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    Chapter 22 Natural Killer Cells
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    Chapter 23 Natural Killer Cells
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    Chapter 24 Natural Killer Cells
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    Chapter 25 Natural Killer Cells
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    Chapter 26 Noninvasive In Vivo Fluorescence Imaging of NK Cells in Preclinical Models of Adoptive Immunotherapy.
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    Chapter 27 Natural Killer Cells
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    Chapter 28 Generation of BiKEs and TriKEs to Improve NK Cell-Mediated Targeting of Tumor Cells.
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    Chapter 29 Natural Killer Cells
Attention for Chapter 4: Genotyping Single Nucleotide Polymorphisms and Copy Number Variability of the FCGRs Expressed on NK Cells.
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Chapter title
Genotyping Single Nucleotide Polymorphisms and Copy Number Variability of the FCGRs Expressed on NK Cells.
Chapter number 4
Book title
Natural Killer Cells
Published in
Methods in molecular biology, January 2016
DOI 10.1007/978-1-4939-3684-7_4
Pubmed ID
Book ISBNs
978-1-4939-3682-3, 978-1-4939-3684-7
Authors

Amy K. Erbe Ph.D., Wei Wang, Mikayla Gallenberger, Jacquelyn A. Hank, Paul M. Sondel, Amy K. Erbe

Editors

Srinivas S. Somanchi

Abstract

Natural killer (NK) cells are one of the main effector immune cells involved in antibody-dependent cell-mediated cytotoxicity (ADCC). Upon recognition of cell-bound IgG antibodies, which occurs through Fc gamma receptors (FCGRs) expressed on the cell surface of NK cells, NK cells become activated and lyse target tumor or infected cells. The FCGRs, FCGR3A and FCGR2C, expressed on the surface of NK cells have single nucleotide polymorphisms (SNPs) that result in differential activity of NK cells. In addition to SNP genetic variation within each of these genes, the FCGRs are subject to copy number variation (CNV), which leads to variable protein expression levels on the cell surface. Studies have found that FCGR genotype for FCGR3A and FCGR2C is associated with variation in the response to immunotherapy.Due to high sequence homology within FCGR3 and FCGR2 families, there are difficulties associated with genotyping these specific receptors related to cross-amplification of non-targeted FCGRs. To improve specificity for both FCGR3A and FCGR2C, Rnase-H (RH) primers were designed to amplify specifically FCGR3A (while not co-amplifying FCGR3B) and FCGR2C (while not co-amplifying FCGR2B). In addition, fluorescently labeled locked nucleic acid (LNA) probes provide additional precision for determination of the SNPs within both FCGR3A and FCGR2C. For CNV determination, separate fluorescently labeled probes for FCGR3A, and for FCGR2C, can be used with the same RH primers for each gene. These probes can be combined in the same well with control primers/probe for a known diploid gene and used to calculate the copy number of both FCGR3A and FCGR2C. Here we provide new detailed methodology that allows for the specific amplification of these FCGRs in a single PCR reaction, allowing for genotyping of both the SNPs and CNVs using real-time PCR.

Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 49 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 49 100%

Demographic breakdown

Readers by professional status Count As %
Student > Ph. D. Student 13 27%
Researcher 10 20%
Student > Bachelor 3 6%
Student > Postgraduate 2 4%
Student > Master 2 4%
Other 4 8%
Unknown 15 31%
Readers by discipline Count As %
Immunology and Microbiology 11 22%
Biochemistry, Genetics and Molecular Biology 9 18%
Medicine and Dentistry 5 10%
Agricultural and Biological Sciences 5 10%
Neuroscience 2 4%
Other 2 4%
Unknown 15 31%