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Chemotaxis

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Cover of 'Chemotaxis'

Table of Contents

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    Book Overview
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    Chapter 1 Chemotaxis
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    Chapter 2 Chemotaxis
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    Chapter 3 Chemotaxis
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    Chapter 4 Mitochondrial Stress Tests Using Seahorse Respirometry on Intact Dictyostelium discoideum Cells
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    Chapter 5 Studying Chemoattractant Signal Transduction Dynamics in Dictyostelium by BRET
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    Chapter 6 Wave Patterns in Cell Membrane and Actin Cortex Uncoupled from Chemotactic Signals
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    Chapter 7 Chemotactic Blebbing in Dictyostelium Cells
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    Chapter 8 Dissecting Spatial and Temporal Sensing in Dictyostelium Chemotaxis Using a Wave Gradient Generator
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    Chapter 9 Employing Dictyostelium as an Advantageous 3Rs Model for Pharmacogenetic Research
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    Chapter 10 Identification of Associated Proteins by Immunoprecipitation and Mass Spectrometry Analysis
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    Chapter 11 Biochemical Responses to Chemically Distinct Chemoattractants During the Growth and Development of Dictyostelium
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    Chapter 12 Chemotaxis
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    Chapter 13 shRNA-Induced Gene Knockdown In Vivo to Investigate Neutrophil Function
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    Chapter 14 Studying Neutrophil Migration In Vivo Using Adoptive Cell Transfer
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    Chapter 15 Intravital Two-Photon Imaging of Lymphocytes Crossing High Endothelial Venules and Cortical Lymphatics in the Inguinal Lymph Node
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    Chapter 16 Flow Cytometry-Based Quantification of HIV-Induced T Cell Chemotactic Response
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    Chapter 17 Visualizing Cancer Cell Chemotaxis and Invasion in 2D and 3D
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    Chapter 18 4D Tumorigenesis Model for Quantitating Coalescence, Directed Cell Motility and Chemotaxis, Identifying Unique Cell Behaviors, and Testing Anticancer Drugs
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    Chapter 19 An Experimental Model for Simultaneous Study of Migration of Cell Fragments, Single Cells, and Cell Sheets
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    Chapter 20 Chemotaxis
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    Chapter 21 Visualization of Actin Assembly and Filament Turnover by In Vitro Multicolor TIRF Microscopy
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    Chapter 22 Quantitative Monitoring Spatiotemporal Activation of Ras and PKD1 Using Confocal Fluorescent Microscopy
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    Chapter 23 Fluorescence Readout of a Patch Clamped Membrane by Laser Scanning Microscopy
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    Chapter 24 Chemotaxis
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    Chapter 25 Multi-State Transition Kinetics of Intracellular Signaling Molecules by Single-Molecule Imaging Analysis
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    Chapter 26 Mathematics of Experimentally Generated Chemoattractant Gradients
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    Chapter 27 Modeling Excitable Dynamics of Chemotactic Networks
Attention for Chapter 15: Intravital Two-Photon Imaging of Lymphocytes Crossing High Endothelial Venules and Cortical Lymphatics in the Inguinal Lymph Node
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Chapter title
Intravital Two-Photon Imaging of Lymphocytes Crossing High Endothelial Venules and Cortical Lymphatics in the Inguinal Lymph Node
Chapter number 15
Book title
Chemotaxis
Published in
Methods in molecular biology, January 2016
DOI 10.1007/978-1-4939-3480-5_15
Pubmed ID
Book ISBNs
978-1-4939-3478-2, 978-1-4939-3480-5
Authors

Chung Park, Il-Young Hwang, John H. Kehrl, Park, Chung, Hwang, Il-Young, Kehrl, John H.

Abstract

Lymphocyte recirculation through lymph nodes (LNs) requires their crossing of endothelial barriers present in blood vessels and lymphatics by means of chemoattractant-triggered cell migration. The chemoattractant-chemoattractant receptor axes that predominately govern the trafficking of lymphocytes into, and out of, LNs are CCL19/CCR7 and sphingosine 1-phosphate (S1P)/S1P receptor 1 (S1PR1), respectively. Blood-borne lymphocytes downregulate S1PR1 and use CCR7 signaling to adhere to high endothelial venules (HEVs) for transmigration. During their LN residency, recirculating lymphocytes reacquire S1PR1 and attenuate their sensitivity to chemokines. Eventually lymphocytes exit the LN by entering the cortical or medullary lymphatics, a process that depends upon S1PR1 signaling. Upon entering into the lymph, lymphocytes lose their polarity, downregulate their sensitivity to S1P due to the high concentration of S1P, and upregulate their sensitivity to chemokines. However, many of the details of lymphocyte transmigration across endothelial barriers remain poorly understood. Intravital two-photon imaging with advanced microscope technologies not only allows the real-time observation of immune cells in intact LN of a live mouse, but also provides a means to monitor the interactions between circulating lymphocytes and stromal barriers. Here, we describe procedures to visualize lymphocytes engaging and crossing HEVs, and approaching and crossing the cortical lymphatic endothelium to enter the efferent lymph in live mice.

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Mendeley readers

The data shown below were compiled from readership statistics for 10 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 10 100%

Demographic breakdown

Readers by professional status Count As %
Student > Postgraduate 3 30%
Student > Bachelor 2 20%
Student > Ph. D. Student 2 20%
Researcher 1 10%
Student > Doctoral Student 1 10%
Other 0 0%
Unknown 1 10%
Readers by discipline Count As %
Medicine and Dentistry 2 20%
Engineering 2 20%
Immunology and Microbiology 2 20%
Biochemistry, Genetics and Molecular Biology 1 10%
Neuroscience 1 10%
Other 1 10%
Unknown 1 10%