an immunofluorescence technique for viral protein localization in infected cells

An Immunofluorescence Technique for Viral Protein Localization in Infected Cells

20 to 24 hours before the virus infection, seed 5 x 104 human embryonic lung or HEL fibroblast cells per well onto a 4-well 11-millimeter staggered slide in growth medium for overnight incubation at 37 degrees Celsius, with 5% carbon dioxide.
It is important to rock the slide thoroughly to ensure an even distribution of the cells while taking care to avoid spilling the culture medium. The next day, replace the supernatants of the 70% to 80% confluent cultures with Medium-199 containing 4-10 plaque-forming units per cell, and place the slide at 37 degrees Celsius with shaking for 1 hour.
At the end of the incubation, replace the supernatants with fresh growth medium, and return the cells to the incubator for the appropriate experimental infection period. For immunofluorescence staining of the virus-infected cells, quickly wash the cells three times with PBS, followed by an 8 to 10-minute incubation in 200 microliters of 4% paraformaldehyde in PBS per well. At the end of the fixation, wash the cells three times with 200 microliters of PBS per wash and permeabilize the cells with 100 microliters of 0.2% nonionic surfactant per well for 5 to 10 minutes.
Wash the permeabilized cells three times in PBS as demonstrated, and add 200 microliters of blocking buffer to each well for a 1-hour incubation at room temperature. Next, add the appropriate concentration of the primary antibody of interest to each well for a 2-hour room-temperature incubation.
At the end of the incubation, remove any unbound primary antibody with three 10-minute washes in fresh blocking buffer, and add an appropriate secondary antibody to each well for a 1-hour incubation at room temperature, protected from light.
At the end of the incubation, wash the cells three times in a blocking buffer as demonstrated, followed by one wash in PBS, and add one drop of anti-fade mounting medium, supplemented with DAPI to each well. Then place a coverslip over the slide, and seal the coverslip with transparent nail polish.
Applying gentle pressure while mounting the coverslip will remove any excess mounting medium, helping to ensure the acquisition of high-quality images.
To analyze the nuclear and cytoplasmic distribution of ICP0, open the project in the confocal application software and select an image. Open the Quantity tab and select Sort Regions of Interest from the Tools menu. Select Draw Line, and draw a longitudinal line across the cell to be analyzed. A histogram will appear showing the fluorescence intensity along the line for both the protein of interest and DAPI.
Based on the background staining, set up a constant threshold for the intensity of the protein of interest for analysis of the subcellular distribution of the protein in each experiment. If the protein signal, on average, is below the threshold in the nuclear region, but is above the threshold beyond the DAPI boundary, categorize the protein signal as predominantly located within the cytoplasm.
If the protein signal is above the threshold throughout the nucleus and beyond the boundary of the DAPI signal, group the protein signal as a nucleus plus cytoplasmic localization. If the protein signal is above the threshold in the nucleus, but on average is below the threshold outside the boundary of the DAPI signal, group the protein signal as a nuclear localization.

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Immunology

Antibody-Based Technologies

Antibody-Based Imaging and Detection Methods

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1. Cell Seeding and Virus Infection
<ol>
	<li>At 20&#8211;24 h before the virus infection, seed 5 x 104&#160;of human embryonic lung (HEL) fibroblast cells or other cells to be examined on a 4-well 11 mm staggered slide in growth medium (Dulbecco&#39;s Modified Eagle Medium (DMEM) supplemented with 10% fetal bovine serum (FBS)). Incubate the cells at 37 &#176;C with 5% carbon dioxide (CO2). 
	NOTE: Each well should have 70-80% cell confluency at the time of infection.</li>
	<li>On the next day, remove the growth medium and infect the cells with viruses in Medium-199 at a range of 4&#8211;10 pfu/cell. Incubate virus-infected cells for 1 h at 37 &#176;C. Keep shaking the slide during the incubation period.</li>
	<li>After the 1 h incubation, remove Medium-199 and supplement with growth medium. 
	NOTE: Drugs that interfere with different infection phases can be added at this step or prior to viral absorption.</li>
	<li>Incubate the virus-infected cells at 37 &#176;C with 5% CO2&#160;for various lengths of infection period.</li>
</ol>
2. Fixation and Permeabilization
<ol>
	<li>At proper infection time, quickly wash the infected cells with phosphate-buffered saline (PBS) 3 times and add 200 &#956;L of 4% paraformaldehyde freshly prepared in PBS. Incubate the cells with paraformaldehyde for 8&#8211;10 min at room temperature to fix the cells in each well.</li>
	<li>Aspirate paraformaldehyde and wash the wells with 200 &#956;L of PBS for 3 times. Completely aspirate PBS after the 3rd&#160;wash.</li>
	<li>Add 100 &#956;L of 0.2% non-ionic surfactant to each well to permeabilize the cells for 5&#8211;10 min.</li>
	<li>Aspirate the non-ionic surfactant and wash the wells with 200 &#956;L of PBS for 3 times.</li>
</ol>
3. Immunofluorescent Staining
<ol>
	<li>Completely aspirate PBS and add 200 &#956;L of blocking buffer (1% bovine serum albumin (BSA) and 5% horse serum in PBS) in each well and incubate at room temperature for 1 h or at 4 &#176;C overnight.</li>
	<li>Add experimentally determined concentration of primary antibody against infected cell protein 0 (rabbit anti-ICP0 polyclonal antibody) in blocking buffer and incubate primary antibody at room temperature for 2 h or at 4 &#176;C overnight.</li>
	<li>Wash with blocking buffer 3 times with 10 min incubation. Add Alexa 594-conjugated goat anti-rabbit secondary antibody (1:400 diluted in blocking buffer) and incubate the slides at room temperature for 1 h. Then wash the slides 3 times with blocking buffer at 10 min intervals.</li>
	<li>Finally wash the slide once with PBS to remove residual BSA and horse serum.</li>
	<li>Add one drop of antifade mounting medium with 4&#39;,6-diamidino-2-phenylindole (DAPI) to mount the slide and seal it with coverslip using transparent nail polish.</li>
</ol>
4. Confocal Imaging
<ol>
	<li>With a confocal microscope, set the wavelength at 590&#8211;650 nm for Alexa 594 and 410&#8211;520 nm for DAPI. Select image format at 1024 x 1024 and line average of 8 to acquire high resolution images.</li>
	<li>Analyze each well on the 4-well slide under a confocal microscope. Acquire representative cell images under the 100X objective, as shown in&#160;Figure&#160;1&#160;and&#160;Figure&#160;2.</li>
	<li>For counting large numbers of cells, take images of consecutive fields under the 40X objective. 
	NOTE: It requires 5&#8211;10 images to accumulate over 200 infected cells from each time point of each infection.</li>
	<li>In each experiment, take pictures with constant confocal parameters for all samples that need to be compared.</li>
</ol>
5. Analyzing Nuclear&#160;vs.&#160;Cytoplasmic Distribution
<ol>
	<li>Open project with the confocal application software. Select an image from which cells need to be tabulated for nuclear&#160;vs.&#160;cytoplasmic distribution of ICP0.</li>
	<li>Click the tab &#34;Quantity&#34; from top menu and select &#34;sort ROIs&#34; from tools menu.</li>
	<li>Draw a longitudinal line across the cell to be analyzed by selecting &#34;Draw line&#34; from top menu.&#160;&#160;&#160;&#160; 
	NOTE: Histogram will appear showing the fluorescence intensity along the line for both ICP0 and DAPI. In the histogram, blue line represents DAPI pixels and marks the boundary of the nucleus whereas the red line represents ICP0 pixels.</li>
	<li>Based on background staining, set up a constant threshold for ICP0 intensity to analyze ICP0 subcellular distribution in each experiment.
	<ol>
		<li>As exemplified in&#160;Figure 2, if the red signal on average is below the threshold in the nuclear region but is above the threshold beyond the blue boundary, categorize the red signal as predominantly located in the cytoplasm.</li>
		<li>If the red signal is above the threshold throughout the nucleus and beyond the boundary of blue signal, group the red signal as nucleus plus cytoplasmic localization.</li>
		<li>If the red signal is above the threshold in the nucleus but on average is below it outside the boundary of blue signal, group the red signal as nuclear localization.</li>
	</ol>
	</li>
	<li>Tabulate more than 200 infected cells from each sample at different infection time and plot in bar graph to illustrate ICP0 movement according to time (Figure 3).</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Cells and viruses</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Human Embryonic Lung fibroblasts (HEL Cells)</td>
			<td>Dr. Thomas E. Shenk (Princeton University)</td>
			<td></td>
			<td>HEL cells were grown in DMEM supplemented with 10% FBS</td>
		</tr>
		<tr>
			<td>HSV-1 viral Stock (Strain F)</td>
			<td>Dr. Bernard Roizman Lab</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Medium</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Dulbecco&#39;s modified Eagle&#39;s medium (DMEM)</td>
			<td>Invitrogen</td>
			<td>&#160;11965-092</td>
			<td></td>
		</tr>
		<tr>
			<td>Fetal Bovine Serum (FBS)</td>
			<td>Sigma</td>
			<td>F0926-500ml</td>
			<td></td>
		</tr>
		<tr>
			<td>Medium-199 (10X)</td>
			<td>Gibco</td>
			<td>11825-015</td>
			<td></td>
		</tr>
		<tr>
			<td>Reagents</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>4- well 11 mm staggered slide</td>
			<td>Cel-Line/Thermofisher Scientific</td>
			<td>&#160;30-149H-BLACK</td>
			<td></td>
		</tr>
		<tr>
			<td>16% Paraformaldehyde solution(w/v) Methanol free</td>
			<td>Thermo Scientific</td>
			<td>28908</td>
			<td></td>
		</tr>
		<tr>
			<td>Triton X-100</td>
			<td>Fisher reagents</td>
			<td>BP151-1C0</td>
			<td></td>
		</tr>
		<tr>
			<td>Bovine Serum Abumin (BSA)</td>
			<td>Calbiochem</td>
			<td>CAS 9048-46-8</td>
			<td></td>
		</tr>
		<tr>
			<td>Horse Serum</td>
			<td>Sigma</td>
			<td>H1270</td>
			<td></td>
		</tr>
		<tr>
			<td>Phosphate Buffered Saline (PBS) (137 mM NaCl, 2.7 mM KCl, 10 mM Na2HPO4, pH7.4)</td>
			<td>Dr. Haidong Gu lab</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>NaCl&#160;&#160;&#160;&#160;&#160;&#160;</td>
			<td>Fisher Bioreagent</td>
			<td>BP358-212</td>
			<td></td>
		</tr>
		<tr>
			<td>KH2PO4&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;</td>
			<td>Fisher Bioreagent</td>
			<td>BP362-500</td>
			<td></td>
		</tr>
		<tr>
			<td>KCl&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;</td>
			<td>Fisher Scientific&#160;</td>
			<td>BP366-500</td>
			<td></td>
		</tr>
		<tr>
			<td>Na2HPO4&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;</td>
			<td>Fisher Bioreagent</td>
			<td>BP332-500</td>
			<td></td>
		</tr>
		<tr>
			<td>Blocking buffer (PBS with 1% BSA and 5% Horse serum )</td>
			<td>Dr. Haidong Gu lab</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Rabiit Anti-ICP0 antibody</td>
			<td>Dr. Haidong Gu lab</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>PML (PG-M3)-Mouse monoclonal IgG</td>
			<td>santa Cruz Biotechnology</td>
			<td>SC-966</td>
			<td></td>
		</tr>
		<tr>
			<td>Alexa Fluor 594-goat anti-rabbit IgG</td>
			<td>invitrogen</td>
			<td>A11012</td>
			<td></td>
		</tr>
		<tr>
			<td>Alexa Fluor 488-goat anti-mouse IgG</td>
			<td>invitrogen</td>
			<td>A11001</td>
			<td></td>
		</tr>
		<tr>
			<td>Vectashield Mouting medium with DAPI</td>
			<td>Vector laboratories</td>
			<td>H-1200</td>
			<td></td>
		</tr>
		<tr>
			<td>Pasteur pipette</td>
			<td>Fisher Brand</td>
			<td>13-678-20D</td>
			<td></td>
		</tr>
		<tr>
			<td>Nail Polish</td>
			<td>Sally Hansen</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Equipment</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Confocal Microscope</td>
			<td>Leica SP8</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Confocal Software</td>
			<td>Leica LAS X Application suite</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Excel software</td>
			<td>Microsoft Excel</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>HERAcell 150i CO2&#160;incubator</td>
			<td>Thermo Scientific</td>
			<td>Order code 51026282</td>
			<td></td>
		</tr>
	</tbody>
</table>

Source: Samrat, S. K. et al., <a href="https://app.jove.com/v/58504">Temporal Analysis of the Nuclear-to-cytoplasmic Translocation of a Herpes Simplex Virus 1 Protein by Immunofluorescent Confocal Microscopy.</a>&#160;J. Vis. Exp.&#160;(2018)
This video demonstrates a method for monitoring infected cell protein 0, ICP0 trafficking in herpes simplex virus-1 infection. Post-de novo synthesis, ICP0 translocates to the nucleus, later moving to the cytoplasm during infection progression. Immunofluorescence microscopy reveals and analyzes the protein&#39;s subcellular localization, offering insights into its trafficking across infection phases.

<img alt="Figure 1" src="/files/ftp_upload/22140/22140_Figure1.jpg" /> 
Figure 1: Dynamic trafficking of ICP0 during HSV-1 infection.&#160;HEL cells grown on 4-well slides were infected with prototype HSV-1 (strain F) at 10 pfu/cell. At 1, 5, and 9 h post infection (hpi), cells were fixed, permeabilized, and reacted to rabbit anti-ICP0 and mouse anti-PML primary antibodies, and then reacted to Alexa 594-conjugated anti-rabbit and Alexa 488-cojugated anti-mouse second...

1. Cell Seeding and Virus Infection

	At 20&#8211;24 h before the virus infection, seed 5 x 104&#160;of human embryonic lung (HEL) fibroblast cells or ...

Begin with a slide containing adhered host cells.
Add viruses and allow them to enter the host cells.
Remove the spent medium. Add fresh medium to enable viral protein synthesis and transport.
Use paraformaldehyde to preserve cell morphology and protein location.
Add detergent molecules to make the cells permeable.
Apply a blocking buffer to block non-target binding sites.
Add primary antibodies that bind target viral proteins. Remove unbound antibodies.
Overlay with red fluorophore-conjugated secondary antibodies for fluorescently tagging the viral proteins. Remove unbound antibodies.
Add a fluorescent nuclear dye-containing mounting medium to stain the nuclei.
Using confocal microscopy, observe the location of red-fluorescent viral proteins and blue-fluorescent host nuclei.
A stronger red signal around the blue area indicates cytoplasmic localization, while a stronger signal on the inside suggests nuclear localization.
Equal signal levels in and around the blue area indicate that proteins are located in both the nucleus and cytoplasm.

68 ビュー. 感染細胞におけるウイルスタンパク質の局在化のための免疫蛍光法

ビデオ: 感染細胞におけるウイルスタンパク質の局在化のための免疫蛍光法 - 実験

Subcellular Fractionation of Primary Chronic Lymphocytic Leukemia Cells to Monitor Nuclear/Cytoplasmic Protein Trafficking

Nuclear export of macromolecules is often deregulated in cancer cells. Tumor suppressor proteins, such as p53, can be rendered inactive due to aberrant cellular localization disrupting their mechanism of action. The survival of chronic lymphocytic leukaemia (CLL) cells, among other cancer cells, is assisted by the deregulation of nuclear to cytoplasmic shuttling, at least in part through deregulation of the transport receptor XPO1 and the constitutive activation of PI3K-mediated signaling pathways. It is essential to understand the role of individual proteins in the context of their intracellular location to gain a deeper understanding of the role of such proteins in the pathobiology of the disease. Furthermore, identifying processes that underlie cell stimulation and the mechanism of action of specific pharmacological inhibitors, in the context of subcellular protein trafficking, will provide a more comprehensive understanding of the mechanism of action. The protocol described here enables the optimization and subsequent efficient generation of nuclear and cytoplasmic fractions from primary chronic lymphocytic leukemia cells. These fractions can be used to determine changes in protein trafficking between the nuclear and cytoplasmic fractions upon cell stimulation and drug treatment. The data can be quantified and presented in parallel with immunofluorescent images, thus providing robust and quantifiable data.

This protocol enables the optimization and subsequent efficient generation of nuclear and cytoplasmic fractions from primary chronic lymphocytic leukemia cells. These samples are used to determine protein localization as well as changes in protein trafficking that take place between the nuclear and cytoplasmic compartments upon cell stimulation and drug treatment.

核/細胞質タンパク質の密売を監視する原発性慢性リンパ球性白血病細胞の細胞分画

Nuclear export of macromolecules is often deregulated in cancer cells. Tumor suppressor proteins, such as p53, can be rendered inactive due to aberrant ...

JoVE Journal

がん研究

Ex Vivo Infection of Murine Epidermis with Herpes Simplex Virus Type 1

To enter its human host, herpes simplex virus type 1 (HSV-1) must overcome the barrier of mucosal surfaces, skin, or cornea. HSV-1 targets keratinocytes during initial entry and establishes a primary infection in the epithelium, which is followed by latent infection of neurons. After reactivation, viruses can become evident at mucocutaneous sites that appear as skin vesicles or mucosal ulcers. How HSV-1 invades skin or mucosa and reaches its receptors is poorly understood. To investigate the invasion route of HSV-1 into epidermal tissue at the cellular level, we established an ex vivo infection model of murine epidermis, which represents the site of primary and recurrent infection in skin. The assay includes the preparation of murine skin. The epidermis is separated from the dermis by dispase II treatment. After floating the epidermal sheets on virus-containing medium, the tissue is fixed and infection can be visualized at various times postinfection by staining infected cells with an antibody against the HSV-1 immediate early protein ICP0. ICP0-expressing cells can be observed in the basal keratinocyte layer already at 1.5 hr postinfection. With longer infection times, infected cells are detected in suprabasal layers, indicating that infection is not restricted to the basal keratinocytes, but the virus spreads to other layers in the tissue. Using epidermal sheets of various mouse models, the infection protocol allows determining the involvement of cellular components that contribute to HSV-1 invasion into tissue. In addition, the assay is suitable to test inhibitors in tissue that interfere with the initial entry steps, cell-to-cell spread and virus production. Here, we describe the ex vivo infection protocol in detail and present our results using nectin-1- or HVEM-deficient mice.

Ex Vivo Infection of Murine Epidermis with Herpes Simplex Virus Type 1

The skin is one target tissue of the human pathogen herpes simplex virus type 1 (HSV-1). To explore the invasion route of HSV-1 into tissue, we established an ex vivo infection model of murine epidermal sheets which represent the outermost layer of skin.

単純ヘルペスウイルス1型を持つマウス表皮の ex vivo 感染

To enter its human host, herpes simplex virus type 1 (HSV-1) must overcome the barrier of mucosal surfaces, skin, or cornea. HSV-1 targets keratinocytes ...

免疫・感染学

Tyramide Signal Amplification for the Immunofluorescent Staining of ZBP1-Dependent Phosphorylation of RIPK3 and MLKL After HSV-1 Infection in Human Cells

The kinase Receptor-interacting serine/threonine protein kinase 3 (RIPK3) and its substrate mixed lineage kinase domain-like (MLKL) are critical regulators of necroptosis, an inflammatory form of cell death with important antiviral functions. Autophosphorylation of RIPK3 induces phosphorylation and activation of the pore-forming executioner protein of necroptosis MLKL. Trafficking and oligomerization of phosphorylated MLKL at the cell membrane results in cell lysis, characteristic of necroptotic cell death. The nucleic acid sensor ZBP1 is activated by binding to left-handed Z-form double-stranded RNA (Z-RNA) after infection with RNA and DNA viruses. ZBP1 activation restricts virus infection by inducing regulated cell death, including necroptosis, of infected host cells. Immunofluorescence microscopy permits the visualization of different signaling steps downstream of ZBP1-mediated necroptosis on a per-cell basis. However, the sensitivity of standard fluorescence microscopy, using current commercially available phospho-specific antibodies against human RIPK3 and MLKL, precludes reproducible imaging of these markers. Here, we describe an optimized staining procedure for serine (S) phosphorylated RIPK3 (S227) and MLKL (S358) in human HT-29 cells infected with herpes simplex virus 1 (HSV-1). The inclusion of a tyramide signal amplification (TSA) step in the immunofluorescent staining protocol allows the specific detection of S227 phosphorylated RIPK3. Moreover, TSA greatly increases the sensitivity of the detection of S358 phosphorylated MLKL. Together, this method enables the visualization of these two critical signaling events during the induction of ZBP1-induced necroptosis.

Tyramide signal amplification during immunofluorescent staining enables the sensitive detection of phosphorylated RIPK3 and MLKL during ZBP1-induced necroptosis after HSV-1 infection.

An Immunofluorescence Technique for Viral Protein Localization in Infected Cells

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An Immunofluorescence Technique for Viral Protein Localization in Infected Cells