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In Vitro Differentiation of T-Cells

Overview of attention for book
Cover of 'In Vitro Differentiation of T-Cells'

Table of Contents

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    Book Overview
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    Chapter 1 Flow Cytometry Analysis to Identify Human CD8 + T Cells
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    Chapter 2 Flow Cytometry Analysis to Identify Human CD4 + T Cell Subsets
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    Chapter 3 Gene Modification and Immunological Analyses for the Development of Immunotherapy Utilizing T Cells Redirected with Antigen-Specific Receptors
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    Chapter 4 In Vitro Conversion of Activated T Cells into Stem Cell Memory-Like T Cells
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    Chapter 5 Human iPSC Generation from Antigen-Specific T Cells
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    Chapter 6 In Vitro Differentiation of T Cells: From Human Embryonic Stem Cells and Induced Pluripotent Stem Cells
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    Chapter 7 Redifferentiation of Adaptive Naïve-Like CTL from T-Cell-Derived iPSC
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    Chapter 8 In Vitro Differentiation of T Cell: From Human iPS Cells in Feeder-Free Condition
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    Chapter 9 Differentiating CD8αβ T Cells from TCR-Transduced iPSCs for Cancer Immunotherapy
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    Chapter 10 In Vitro Differentiation of T Cell: From CAR-Modified T-iPSC
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    Chapter 11 In Vitro Differentiation of T Cells: From Nonhuman Primate-Induced Pluripotent Stem Cells
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    Chapter 12 An Improved Method to Produce Clinical-Scale Natural Killer Cells from Human Pluripotent Stem Cells.
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    Chapter 13 In Vitro Detection of Cellular Adjuvant Properties of Human Invariant Natural Killer T Cells.
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    Chapter 14 In Vitro Differentiation of T Cells from Murine Pluripotent Stem Cells
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    Chapter 15 Clonogenic Culture of Mouse Thymic Epithelial Cells.
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    Chapter 16 Single-Cell Transcriptome Analysis of T Cells.
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    Chapter 17 Structural Modeling of Lymphocyte Receptors and Their Antigens.
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    Chapter 18 Assessing T Lymphocyte Aging Using Telomere Length and Telomerase Activity Measurements in Low Cell Numbers
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    Chapter 19 Generation of Hematopoietic Stem and Progenitor Cells from Human Pluripotent Stem Cells
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    Chapter 20 Using the Inducible Caspase-9 Suicide-Safeguard System with iPSC and Bioluminescent Tracking
Attention for Chapter 12: An Improved Method to Produce Clinical-Scale Natural Killer Cells from Human Pluripotent Stem Cells.
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  • Above-average Attention Score compared to outputs of the same age and source (53rd percentile)

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Chapter title
An Improved Method to Produce Clinical-Scale Natural Killer Cells from Human Pluripotent Stem Cells.
Chapter number 12
Book title
In Vitro Differentiation of T-Cells
Published in
Methods in molecular biology, January 2019
DOI 10.1007/978-1-4939-9728-2_12
Pubmed ID
31396935
Book ISBNs
978-1-4939-9727-5, 978-1-4939-9728-2
Authors

Zhu, Huang, Kaufman, Dan S, Kaufman, Dan S.

Abstract

Human natural killer (NK) cell-based adoptive anticancer immunotherapy has gained intense interest with many clinical trials actively recruiting patients to treat a variety of both hematological malignancies and solid tumors. Most of these trials use primary NK cells isolated either from peripheral blood (PB-NK cells) or umbilical cord blood (UCB-NK cells), though these sources require NK cell collection for each patient leading to donor variability and heterogeneity in the NK cell populations. In contrast, NK cells derived human embryonic stem cells (hESC-NK cells) or induced pluripotent stem cells (hiPSC-NK cells) provide more homogeneous cell populations that can be grown at clinical scale, and genetically engineered if needed. These characteristics make hESC-/iPSC-derived NK cells an ideal cell population for developing standardized, "off-the-shelf" immunotherapy products. Additionally, production of NK cells from undifferentiated human pluripotent stem cells enables studies to better define pathways that regulate human NK cell development and function. Our group previously has established a stromal-free, two-stage culture system to derive NK cells from hESC/hiPSC in vitro followed by clinical-scale expansion of these cells using interleukin (IL)-21 expressing artificial antigen-presenting cells. However, prior to differentiation, this method requires single-cell adaptation of hESCs/hiPSCs which takes months. Recently we optimized this method by adapting the mouse embryonic fibroblast-dependent hESC/hiPSC to feeder-free culture conditions. These feeder-free hESCs/hiPSCs are directly used to form embryoid body (EB) to generate hemato-endothelial precursor cells. This new method produces mature, functional NK cells with higher efficiency to enable rapid production of an essentially unlimited number of homogenous NK cells that can be used for standardized, targeted immunotherapy for the treatment of refractory cancers and infectious diseases.

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X Demographics

The data shown below were collected from the profiles of 4 X users who shared this research output. Click here to find out more about how the information was compiled.
 Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 141 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 141 100%

Demographic breakdown

Readers by professional status Count As %
Student > Ph. D. Student 32 23%
Researcher 23 16%
Student > Master 12 9%
Student > Bachelor 10 7%
Other 6 4%
Other 9 6%
Unknown 49 35%
Readers by discipline Count As %
Biochemistry, Genetics and Molecular Biology 32 23%
Agricultural and Biological Sciences 15 11%
Immunology and Microbiology 15 11%
Medicine and Dentistry 11 8%
Engineering 9 6%
Other 13 9%
Unknown 46 33%
Attention Score in Context

Attention Score in Context

This research output has an Altmetric Attention Score of 3. This is our high-level measure of the quality and quantity of online attention that it has received. This Attention Score, as well as the ranking and number of research outputs shown below, was calculated when the research output was last mentioned on 11 August 2019.
All research outputs
#14,833,136
of 25,734,859 outputs
Outputs from Methods in molecular biology
#3,852
of 14,336 outputs
Outputs of similar age
#223,720
of 449,133 outputs
Outputs of similar age from Methods in molecular biology
#26
of 58 outputs
Altmetric has tracked 25,734,859 research outputs across all sources so far. This one is in the 41st percentile – i.e., 41% of other outputs scored the same or lower than it.
So far Altmetric has tracked 14,336 research outputs from this source. They receive a mean Attention Score of 3.4. This one has gotten more attention than average, scoring higher than 72% of its peers.
Older research outputs will score higher simply because they've had more time to accumulate mentions. To account for age we can compare this Altmetric Attention Score to the 449,133 tracked outputs that were published within six weeks on either side of this one in any source. This one is in the 49th percentile – i.e., 49% of its contemporaries scored the same or lower than it.
We're also able to compare this research output to 58 others from the same source and published within six weeks on either side of this one. This one has gotten more attention than average, scoring higher than 53% of its contemporaries.

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