eoe sub articles

EoE Sub Articles

All procedures involving human participants have been performed in compliance with the institutional, national, and international guidelines for human welfare and have been reviewed by the local institutional review board.
1. Device Fabrication and Soft Lithography
NOTE: Standard soft lithography techniques&#160;were used to create the polydimethylsiloxane (PDMS) microchannel.
<ol>
	<li>Mix the PDMS precursor in a 10:1 ratio of base and curing agent.</li>
	<li>Pour 30 g of the PDMS precursor mixture into the micro-machined aluminum mold (see&#160;Figure 1&#160;for dimensions) and 20 g of the PDMS precursor mixture into the 100 mm Petri dish.&#160;&#160; 
	NOTE: The Petri dish is used to make the thick film of PDMS (~3 mm) for the supporting layer. The supporting layer of PDMS provides uniform physical surface properties throughout the microfluidics. Alternatively, a thin PDMS film on the glass slide can be used. The master mold with specific channel dimensions was designed and fabricated by micro-milling on the aluminum sheet. The spiral channel used in this study was an 8-loop spiral microchannel with one inlet and two outlets, with the radius increasing from 8 mm to 24 mm for efficient size-based separation.</li>
	<li>Place the mold and the Petri dish into a vacuum desiccator to degas until no bubbles are visible on the surface, typically 5 - 10 min. Use a house vacuum for the desiccator.</li>
	<li>Release the vacuum and place the mold and the Petri dish in a 90 &#176;C oven for 1 h. 
	NOTE: A hotplate or other heating tools can be used instead of an oven.</li>
	<li>Remove the mold and the Petri dish from the oven and allow it to cool at room temperature for 10 min.</li>
	<li>Carefully cut out the outline and punch the fluid access holes on the device using a 2 mm puncher.&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160; 
	NOTE: The size of the punch can vary depending on the size of the tubing or fluid guide.</li>
	<li>Adhere a tape to the channel side of the device and a thick film of PDMS, and peel carefully with forceps to remove dust.</li>
	<li>Treat both the channel side of the device and plain PDMS with air plasma and bond with the prepared supporting layer of plain PDMS (Figure 1A).</li>
	<li>Place the chip on the 50 mm x 70 mm glass slide and place it in a 70 &#176;C oven for at least 30 min to enhance the bonding strength.</li>
</ol>
2. Tracheal Secretion Collection from Mechanically Ventilated Patients
NOTE: Tracheal secretions can be obtained from mechanically ventilated patients during normal routine airway care by using a protocol modified from conventional methods to accommodate the standard, adult ventilated patient. Samples were de-identified and sent immediately for processing.
<ol>
	<li>If tracheal aspiration is indicated, use a catheter to extract airway secretions.</li>
	<li>Advance the catheter carefully halfway into the endotracheal tube and instill 5 mL of 0.9% sterile normal saline from a pre-filled 10 mL syringe.</li>
	<li>When the catheter is advanced fully, or resistance is met, aspirate the secretions and collect them into a sterile sputum collection container.</li>
	<li>Collect 10 mL of tracheal secretions in a sterile sputum container and place it on ice. Send samples immediately for processing.</li>
</ol>
3. Tracheal Secretion Sample Preparation
NOTE: All experiments must be performed under a biosafety cabinet with the proper personal protective equipment.
<ol>
	<li>Disperse 1 mL of airway secretion samples in 9 mL of phosphate-buffered saline (PBS) using a plastic 10 mL syringe (for a 10x dilution). Use a blunt pipette to homogenize the mucus sample.</li>
	<li>Strain the diluent with a 40 &#181;m nylon cell strainer to remove large chunks or blood clots, which can block the microfluidics access hole or the channel. Place the sample on the ice after processing.</li>
	<li>Disperse the diluent of each sample using a 100x volume of PBS buffer, resulting in a 1,000x diluted suspension. Place the sample on the ice during the entire dissociation operation.</li>
</ol>
4. Experimental Setup
NOTE: All experiments must be performed under a biosafety cabinet with the proper personal protective equipment.
<ol>
	<li>Assemble the PDMS chip with the fluid guide to apply uniform flow to each of the four spiral microchannels (Figure 1B).&#160;&#160;&#160;&#160; 
	NOTE: Four channels were used to increase the throughput by parallelization, as well as optimization of the volume and cell density of the resulting suspension. The fluid guide is designed and made with a stereolithography-type 3D printer with clear resin. The inlet and the outlet port of the fluid guide use female Luer connectors for ease of connection and stable sealing during the operation.</li>
	<li>Connect a 1/16-inch male Luer connector to the inlet, the inner wall (IW) outlet, and the outer wall (OW) outlet port of the fluid guide and connect a silicone tubing to the sample suspension.</li>
	<li>Insert blunt tips to each end of the inlet and outlets to reach the bottom of the sample reservoir.</li>
	<li>Connect the peristaltic pump with the inlet tubing.</li>
	<li>Place the end of the inlet tubing and IW outlet tubing in the sample reservoir and place the end of the OW outlet tubing in the waste reservoir (Figure 1C, D).</li>
	<li>Place the 50 mL tube of filtered PBS without calcium and magnesium in the sample reservoir.</li>
	<li>Start pumping at a low flow rate (~1 mL/min) to prime the device. 
	NOTE: When bubbles are captured in the channel, push the top of the channel with the tweezer to destabilize and eliminate air bubbles. When the device is fully filled with buffer solution, change the PBS tube to prepare the airway secretion sample tube.</li>
	<li>When the sample is placed in the sample reservoir, switch on the peristaltic pump and set the flow rate at 4 mL/min (Figure 1C, D).</li>
	<li>When the sample volume reaches the designated volume (~1 mL), stop the operation and disconnect the silicone tubing.&#160;&#160;&#160; 
	NOTE: The proposed method is more efficient at reducing a large volume of diluent (&#62;50 mL) into a micro-centrifuge tube volume (~1 mL) (Figure 2).</li>
</ol>

<table><tbody><tr><td>PDMS precursor</td><td>Dow corning</td><td>184 SIL ELAST KIT 3.9KG</td><td>10:1 ratio of base and curing agent</td></tr><tr><td>VWR gravity convection oven</td><td>VWR</td><td>414005-128</td><td>PDMS precursor to be cured in 90 deg.</td></tr><tr><td>100mm petri dish</td><td>VWR</td><td>89000-324</td><td>Fabrication of PDMS Supporting layer</td></tr><tr><td>Harris Uni-core puncher</td><td>Sigma-aldrich</td><td>WHAWB100076</td><td>2mm diameter or other depending on the tubing size</td></tr><tr><td>Air plasma machine</td><td>Femto Science</td><td>Cute</td><td>Surface plasma treatment for PDMS device to bottom base.</td></tr><tr><td>2&quot; x 3&quot; glass slide</td><td>TED PELLA, INC.</td><td>2195</td><td>To support PDMS device</td></tr><tr><td>Masterflex spooled platinum-cured silicone tubing, L/S 14</td><td>Cole-Parmer</td><td>EW-96410-14</td><td>Tubing for microfluidics and peristlatic pump</td></tr><tr><td>1/16 inch Luer connector, male</td><td>Harvard apparatus</td><td>PC2 72-1443</td><td>Connector for fluid guide</td></tr><tr><td>50mL Falcon tube</td><td>Corning</td><td>21008-940</td><td>Sample collection &amp;amp; preparation</td></tr><tr><td>Phosphate-Buffered Saline, 1X Without Calcium and Magnesium</td><td>Corning</td><td>45000-446&amp;nbsp;</td><td>Buffer solution to dilute sample</td></tr><tr><td>Halyard Closed suction Catheter, Elbow, 14F/ channel 4.67mm</td><td>HALYARD HEALTH</td><td>22113</td><td>Tracheal seceation suction catheter</td></tr><tr><td>0.9% Sterile Normal saline, 10mL pre-filled syringe</td><td>BD PosiFlush</td><td>NHRIC: 8290-306547</td><td>For tracheal seceation collection from the patients</td></tr><tr><td>SecurTainer&amp;trade; III Specimen Containers, 20mL</td><td>Simport</td><td>1176R36</td><td>Sterile sputum (airway secretion) collection container</td></tr><tr><td>Syringe with Luer-Lok Tip, 10mL</td><td>BD</td><td>BD309604</td><td>To pipette homogenize the mucus sample and reach the bottom of sample tube</td></tr><tr><td>BD&amp;nbsp; Blunt Fill Needle, with BD Luer-Lok&amp;nbsp; Tip</td><td>BD</td><td></td><td>To pipette homogenize the mucus sample and reach the bottom of sample tube</td></tr><tr><td>40&amp;micro;m nylon cell strainer&amp;nbsp;</td><td>Falcon</td><td>21008-949</td><td>To remove large chunk or blood clots, which can block the microfluidics access hole or the channel.</td></tr><tr><td>Peristaltic pump (Masterflex L/S Digital Drive)</td><td>Cole-Parmer</td><td>HV-07522-30</td><td>&amp;nbsp;Operation of microfluidics</td></tr></tbody></table>

label-free neutrophil separation from tracheal secretion using spiral microfluidics channel

Source: Ryu, H., et al., <a href="https://appjove.unicartagenaproxy.elogim.com/v/57673">Label-free Neutrophil Enrichment from Patient-derived Airway Secretion Using Closed-loop Inertial Microfluidics.</a>&#160;J. Vis. Exp.&#160;(2018).
This video demonstrates separating neutrophils from tracheal secretions using a microfluidic device with spiral channels. The device achieves efficient separation based on cell size by utilizing varying thicknesses and trapezoidal-shaped channels. The interplay between forces results in large neutrophils accumulating near the inner wall while erythrocytes and mucin aggregates remain near the outer wall, ensuring effective neutrophil separation.

<img alt="Figure 1" src="/files/ftp_upload/21573/21573_Figure1.jpg" /> 
Figure 1: Spiral microfluidic device and experimental settings.&#160;Photograph images of (A) spiral microfluidics and (B) the device assembled with the fluidic adaptor. (C) Schematic diagram of closed-loop separation using spiral inertial microfluidics. By recirculating the particle/cell concentrated stream (IW outlet) back into the original sample reservoir, immune-related cells were concentrated in a small volume while the ba...

Label-Free Neutrophil Separation from Tracheal Secretion Using Spiral Microfluidics Channel

Source: Ryu, H., et al., Label-free Neutrophil Enrichment from Patient-derived Airway Secretion Using Closed-loop Inertial Microfluidics.&#160;J. Vis. ...

Neutrophils &#8212; immune cells with multilobed nuclei, regulate tracheal immunity by engulfing invading pathogens.
To separate neutrophils from tracheal secretion, begin with a spiral microfluidic channel.
The spiral channel originates from the central inlet, progressively extending and bifurcating into inner and outer wall outlets. The bifurcation channel has varying thicknesses, ensuring efficient separation. Each curved channel resembles a trapezoid, with the outer wall height greater than the inner wall&#39;s, generating a variable flow pattern.
Fill the inlet with a pre-filtered, diluted human tracheal secretion comprising mucin aggregates, neutrophils, and erythrocytes &#8212; as incidental contaminants.&#160; Flow the sample at a specific flow rate through the spiral microchannel leading to the dispersion of the cells and aggregates.
As cells travel through the trapezoidal channel, they experience Dean drag and inertial lift forces. The interplay between these two forces creates an equilibrium, separating cells by their sizes. As a result, larger-sized neutrophils accumulate near the channel&#39;s inner wall, while erythrocytes and mucin aggregates remain near the channel&#39;s outer wall.
Finally, neutrophils move through the broader channel and get collected in the inner wall outlet.
In contrast, the narrow channel collects erythrocytes and mucin aggregates in the outer wall outlet, ensuring efficient neutrophil separation.

label-free-neutrophil-separation-from-tracheal-secretion-using-spiral

Universidad de Cartagena UDEC

Research

JoVE Encyclopedia of Experiments

Immunology

Immune Systems and Components

Assays and Functional Profiling

82 ビュー. 出典:Ryu, H., et al., Label-free Neutrophil Enrichment from Patient-derived Airway Secretion Using Closed-loop Inertial Microfluidics.J. Vis. Exp.(2018年)。 このビデオは、スパイラルチャネルを備えたマイクロ流体デバイスを使用して、気管分泌物から好中球を分離する方法を示しています。このデバイスは、さまざまな厚さと台形のチャネルを利用することにより、細胞サイズに基づく効率的な分離を実?...

ビデオ: スパイラルマイクロ流体チャネルを用いた気管分泌物からのラベルフリー好中球分離 - 概念

Isolation and Characterization of Neutrophils with Anti-Tumor Properties

Neutrophils, the most abundant of all white blood cells in the human circulation, play an important role in the host defense against invading microorganisms. In addition, neutrophils play a central role in the immune surveillance of tumor cells. They have the ability to recognize tumor cells and induce tumor cell death either through a cell contact-dependent mechanism involving hydrogen peroxide or through antibody-dependent cell-mediated cytotoxicity (ADCC). Neutrophils with anti-tumor activity can be isolated from peripheral blood of cancer patients and of tumor-bearing mice. These neutrophils are termed tumor-entrained neutrophils (TEN) to distinguish them from neutrophils of healthy subjects or na&#239;ve mice that show no significant tumor cytotoxic activity. Compared with other white blood cells, neutrophils show different buoyancy making it feasible to obtain a &#62; 98% pure neutrophil population when subjected to a density gradient. However, in addition to the normal high-density neutrophil population (HDN), in cancer patients, in tumor-bearing mice, as well as under chronic inflammatory conditions, distinct low-density neutrophil populations (LDN) appear in the circulation. LDN co-purify with the mononuclear fraction and can be separated from mononuclear cells using either positive or negative selection strategies. Once the purity of the isolated neutrophils is determined by flow cytometry, they can be used for in vitro and in vivo functional assays. We describe techniques for monitoring the anti-tumor activity of neutrophils, their ability to migrate and to produce reactive oxygen species, as well as monitoring their phagocytic capacity ex vivo. We further describe techniques to label the neutrophils for in vivo tracking, and to determine their anti-metastatic capacity in vivo. All these techniques are essential for understanding how to obtain and characterize neutrophils with anti-tumor function.

Neutrophils play an important role not only in host defense against invading microorganisms, but are also involved in the immune surveillance of tumor cells. Here, we describe techniques related to the isolation of neutrophils with anti-tumor properties and methods for monitoring anti-tumor neutrophil function in vitro and in vivo.

抗腫瘍特性を有する好中球の単離とキャラクタリゼーション

Neutrophils, the most abundant of all white blood cells in the human circulation, play an important role in the host defense against invading ...

JoVE Journal

免疫・感染学

Preparation of Whole Bone Marrow for Mass Cytometry Analysis of Neutrophil-lineage Cells

In this article, we present a protocol that is optimized to preserve neutrophil-lineage cells in fresh BM for whole BM CyTOF analysis. We utilized a myeloid-biased 39-antibody CyTOF panel to evaluate the hematopoietic system with a focus on the neutrophil-lineage cells by using this protocol. The CyTOF result was analyzed with an open-resource dimensional reduction algorithm, viSNE, and the data was presented to demonstrate the outcome of this protocol. We have discovered new neutrophil-lineage cell populations based on this protocol. This protocol of fresh whole BM preparation may be used for 1), CyTOF analysis to discover unidentified cell populations from whole BM, 2), investigating whole BM defects for patients with blood disorders such as leukemia, 3), assisting optimization of fluorescence-activated flow cytometry protocols that utilize fresh whole BM.

Here, we present a protocol to process fresh bone marrow (BM) isolated from mouse or human for high-dimensional mass cytometry (Cytometry by Time-Of-Flight, CyTOF) analysis of neutrophil-lineage cells.

好中球系統細胞の質量細胞法解析に対する全骨髄の調製

In this article, we present a protocol that is optimized to preserve neutrophil-lineage cells in fresh BM for whole BM CyTOF analysis. We utilized a ...

Isolation of Human Neutrophils from Whole Blood and Buffy Coats

Neutrophils (PMNs) are the most abundant leukocytes in human circulation, ranging from 40 to 70% of total blood leukocytes. They are the first cells recruited at the site of inflammation via rapid extravasation through vessels. There, neutrophils perform an array of functions to kill invading pathogens and mediate immune signaling. Freshly purified neutrophils from human blood are the model of choice for study, as no cell line fully replicates PMN functions and biology. However, neutrophils are short-lived, terminally differentiated cells and are highly susceptible to activation in response to physical (temperature, centrifugation speed) and biological (endotoxin, chemo- and cytokines) stimuli. Therefore, it is crucial to follow a standardized, reliable, and fast method to obtain pure and non-activated cells. This protocol presents an updated protocol combining density gradient centrifugation, red blood cell (RBC) sedimentation, and RBC lysis to obtain high PMN purity and minimize cell activation. Furthermore, methods to assess neutrophil isolation quality, viability, and purity are also discussed.

This protocol details a method for the isolation of neutrophils from whole blood, buffy coats, or leukapheresis membranes, achieving good yield, high purity, and minimal cell activation. We utilize gradient purification, red blood cell (RBC) sedimentation, and RBC lysis to obtain a high-quality/purity neutrophil preparation.

全血とバフィーコートからのヒト好中球の分離

Neutrophils (PMNs) are the most abundant leukocytes in human circulation, ranging from 40 to 70% of total blood leukocytes. They are the first cells ...

Label-Free Neutrophil Separation from Tracheal Secretion Using Spiral Microfluidics Channel

記録

Label-Free Neutrophil Separation from Tracheal Secretion Using Spiral Microfluidics Channel