isolation of lipids from human blood-derived neutrophils by biphasic separation

Isolation of Lipids from Human Blood-Derived Neutrophils by Biphasic Separation

To isolate the lipids from the human peripheral blood-derived neutrophils, take the prepared neutrophils and place them on ice. Pipette the neutrophils to a 15-milliliter screw cap glass tube with a PTFE seal, and homogenize them by shaking for one minute. Then, add 2 milliliters of methanol, followed one minute later by 1 milliliter of chloroform. After shaking for another one minute, rotate the glass tubes at room temperature and 50 RPM for 30 minutes.
Next, pellet the protein fraction by centrifuging the solution at 7 degrees Celsius and 1952 times g for 10 minutes. Carefully decant the supernatant into a new 15-milliliter glass screw cap tube leaving the protein-containing pellet behind. Store the pellet at minus 20 degrees Celsius for future quantification.
Add 1 milliliter of chloroform and wait one minute. Then, add 1 milliliter of double distilled water and invert the glass screw cap tube with the sample for 30 seconds. After centrifuging the sample as before, remove and discard the upper phase down to but not including the cloudy layer. Dry the samples in a vacuum concentrator at 60 degrees Celsius and store them at minus 20 degrees Celsius until required.

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1. Lipid Isolation and Analysis of Human Blood-derived Neutrophils
<ol>
	<li>Take neutrophils and place them on ice.</li>
	<li>On the ice, pipette the neutrophils (present in methanol and chloroform solution) to a 15 mL screw-cap glass tube with a polytetrafluoroethylene (PTFE) seal and homogenize them by shaking for 1 min. Use glass tubes to prevent the lipids from binding to plastic surfaces. Use PTFE caps to prevent contamination from rubber/plastic.</li>
	<li>Add 2 mL of methanol followed 1 min later by 1 mL of chloroform. Shake again for 1 min.</li>
	<li>Rotate the glass tubes at RT and 50 rpm for 30 min.</li>
	<li>Pellet the protein fraction by centrifuging the solution at 7 &#176;C and 1,952 x g for 10 min.</li>
	<li>Carefully decant the supernatant into a new 15 mL glass screw-cap tube, leaving the protein-containing pellet behind. Store the pellet at -20 &#176;C for future quantification.</li>
	<li>Add 1 mL of chloroform, wait 1 min, add 1 mL of double-distilled water, and invert the glass screw-cap tube with the sample for 30 s.</li>
	<li>Centrifuge at 7 &#176;C and 1,952 x g for 10 min and discard the upper phase, down to, but not including the cloudy layer.</li>
	<li>If required, perform an optional further purification step by repeating step 1.1.8.</li>
	<li>Dry the samples in a vacuum concentrator at 60 &#176;C and store them at -20 &#176;C until required.</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>10 &#181;l syringe</td>
			<td>Hamilton</td>
			<td>701 NR 10 &#181;l</td>
			<td></td>
		</tr>
		<tr>
			<td>Cannula 26G</td>
			<td>Braun</td>
			<td>4657683</td>
			<td></td>
		</tr>
		<tr>
			<td>Chloroform</td>
			<td>Carl Roth</td>
			<td>7331.1</td>
			<td></td>
		</tr>
		<tr>
			<td>Methanol</td>
			<td>Carl Roth</td>
			<td>7342.1</td>
			<td></td>
		</tr>
		<tr>
			<td>Water</td>
			<td>Carl Roth</td>
			<td>3255.1</td>
			<td>Endotoxin-free</td>
		</tr>
	</tbody>
</table>

Source: Brogden, G., et al. <a href="https://app.jove.com/v/54667">Methods to Study Lipid Alterations in Neutrophils and the Subsequent Formation of Neutrophil Extracellular Traps.</a> J. Vis. Exp. (2017)
This video demonstrates lipid isolation from human neutrophils by a biphasic solvent system using methanol and chloroform.

1. Lipid Isolation and Analysis of Human Blood-derived Neutrophils

	Take neutrophils and place them on ice.
	On the ice, pipette the neutrophils (present ...

Take a glass tube containing neutrophil homogenate with released intracellular components.
&#160;Add methanol, a polar solvent, that disrupts lipid-lipid and lipid-protein interactions. The inherent polarity of methanol evenly distributes polar lipids, solubilizing them. Next, add chloroform, a nonpolar organic solvent, that interacts with nonpolar lipids, causing them to disperse and solubilize.
Centrifuge to separate the protein-containing pellet from the supernatant containing lipids, polysaccharides, and cell debris. Transfer the supernatant to a fresh glass tube. Add chloroform and distilled water. Centrifuge the sample.
Water addition spontaneously forms a biphasic system, partitioning biomolecules within the lower chloroform and the upper water-methanol layers.
The chloroform layer comprises dissolved nonpolar lipids, while the upper layer contains non-lipid contaminants and more polar lipids. Remove the upper water-methanol layer without disturbing the lipid-containing layer.
Use a vacuum concentrator to remove the solvent from the lipids. Store at lower temperatures until further use.

35 조회수. Biphasic Separation에 의한 인간 혈액 유래 호중구에서 지질의 분리

비디오: Biphasic Separation에 의한 인간 혈액 유래 호중구에서 지질의 분리 - 실험

Development and Identification of a Novel Subpopulation of Human Neutrophil-derived Giant Phagocytes In Vitro

Neutrophils (PMN) are best known for their phagocytic functions against invading pathogens and microorganisms. They have the shortest half-life amongst leukocytes and in their non-activated state are constitutively committed to apoptosis. When recruited to inflammatory sites to resolve inflammation, they produce an array of cytotoxic molecules with potent antimicrobial killing. Yet, when these powerful cytotoxic molecules are released in an uncontrolled manner they can damage surrounding tissues. In recent years however, neutrophil versatility is increasingly evidenced, by demonstrating plasticity and immunoregulatory functions. We have recently identified a new neutrophil-derived subpopulation, which develops spontaneously in standard culture conditions without the addition of cytokines/growth factors such as granulocyte colony-stimulating factor (GM-CSF)/interleukin (IL)-4. Their phagocytic abilities of neutrophil remnants largely contribute to increase their size immensely; therefore they were termed giant phagocytes (G&#981;). Unlike neutrophils, G&#981; are long lived in culture. They express the cluster of differentiation (CD) neutrophil markers CD66b/CD63/CD15/CD11b/myeloperoxidase (MPO)/neutrophil elastase (NE), and are devoid of the monocytic lineage markers CD14/CD16/CD163 and the dendritic CD1c/CD141 markers. They also take-up latex and zymosan, and respond by oxidative burst to stimulation with opsonized-zymosan and PMA. G&#981; also express the scavenger receptors CD68/CD36, and unlike neutrophils, internalize oxidized-low density lipoprotein (oxLDL). Moreover, unlike fresh neutrophils, or cultured monocytes, they respond to oxLDL uptake by increased reactive oxygen species (ROS) production. Additionally, these phagocytes contain microtubule-associated protein-1 light chain 3B (LC3B) coated vacuoles, indicating the activation of autophagy. Using specific inhibitors it is evident that both phagocytosis and autophagy are prerequisites for their development and likely NADPH oxidase dependent ROS. We describe here a method for the preparation of this new subpopulation of long-lived, neutrophil-derived phagocytic cells in culture, their identification and their currently known characteristics. This protocol is essential for obtaining and characterizing G&#981; in order to further investigate their significance and functions.

Development and Identification of a Novel Subpopulation of Human Neutrophil-derived Giant Phagocytes In Vitro

We describe here a method for obtaining and identifying a newly characterized subpopulation of neutrophil-derived giant phagocytes. These cells develop in culture from fresh human blood neutrophils, and are characterized by phagocytosis, autophagy, immensely large size, and extended lifespan. This method is essential to further investigate this unique neutrophil-derived subpopulation.

인간 호중구 유래 거 식세포의 소설 모집단의 개발 및 식별<em&gt; 체외</em

Neutrophils (PMN) are best known for their phagocytic functions against invading pathogens and microorganisms. They have the shortest half-life amongst ...

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A High-throughput Assay to Assess and Quantify Neutrophil Extracellular Trap Formation

Neutrophil extracellular traps (NETs) are immunogenic extracellular DNA structures that can be released by neutrophils upon a wide variety of triggers. NETs have been demonstrated to serve as an important host defense mechanism that traps and kills microorganisms. On the other hand, they have been implicated in diverse systemic autoimmune diseases. NETs are immunogenic and toxic structures that contain a pool of relevant autoantigens including anti-neutrophil cytoplasmic antibodies (ANCA)-associated vasculitis (AAV) and systemic lupus erythematosus (SLE). Different forms of NETs can be induced depending on the stimulus. The amount of NETs can be quantified using different techniques including measuring DNA release in supernatants, measuring DNA-complexed with NET-molecules like myeloperoxidase (MPO) or neutrophil elastase (NE), measuring the presence of citrullinated histones by fluorescence microscopy, or flow cytometric detection of NET-components which all have different features regarding their specificity, sensitivity, objectivity, and quantity. Here is a protocol to quantify ex vivo NET formation in a highly-sensitive, high-throughput manner by using three-dimensional immunofluorescence confocal microscopy. This protocol can be applied to address various research questions about NET formation and degradation in health and disease.

This protocol describes a highly sensitive and high throughput neutrophil extracellular trap (NET) assay for the semi-automated quantification of ex vivo NET formation by immunofluorescence three-dimensional confocal microscopy. This protocol can be used to evaluate NET formation and degradation after different stimuli and can be used to study potential NET-targeted therapies.

평가 하 고 호 중구 Extracellular 함정 대형 계량 높은 처리량 분석 결과

Neutrophil extracellular traps (NETs) are immunogenic extracellular DNA structures that can be released by neutrophils upon a wide variety of triggers. ...

Morphological and Compositional Analysis of Neutrophil Extracellular Traps Induced by Microbial and Chemical Stimuli

Neutrophils function as the first line of cellular defense in an innate immune response by employing diverse mechanisms, such as the formation of neutrophil extracellular traps (NETs). This study analyzes the morphological and compositional changes in NETs induced by microbial and chemical stimuli using standardized in vitro methodologies for NET induction and characterization with human cells. The procedures described here allow the analysis of NET morphology (lytic or non-lytic) and composition (DNA-protein structures and enzymatic activity), and the effect of soluble factors or cellular contact on such characteristics. Additionally, the techniques described here could be modified to evaluate the effect of exogenous soluble factors or cellular contact on NET composition.
The applied techniques include the purification of polymorphonuclear cells from human peripheral blood using a double density gradient (1.079-1.098 g/mL), guaranteeing optimal purity and viability (&#8805; 95%) as demonstrated by Wright's staining, trypan blue exclusion, and flow cytometry, including FSC versus SSC analysis and 7AAD staining. NET formation is induced with microbial (Pseudomonas aeruginosa, Staphylococcus aureus, and Candida albicans) and chemical (phorbol myristate acetate, HOCl) stimuli, and the NETs are characterized by DNA-DAPI staining, immunostaining for the antimicrobial peptide cathelicidin (LL37), and quantification of enzymatic activity (neutrophil elastase, cathepsin G, and myeloperoxidase). The images are acquired through fluorescence microscopy and analyzed with ImageJ.

Presented here is a protocol for the induction and analysis of in vitro neutrophil extracellular traps (NETs). Quantification of DNA, cathelicidin (LL37), and enzyme activity yielded data that show the variability in the composition and morphology of NETs induced by microbial and chemical stimuli under similar controlled conditions.

Isolation of Lipids from Human Blood-Derived Neutrophils by Biphasic Separation

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Isolation of Lipids from Human Blood-Derived Neutrophils by Biphasic Separation