Detection of Mitochondria Membrane Potential to Study CLIC4 Knockdown-induced HN4 Cell Apoptosis In Vitro

Jinsen Lu; Lele Wu; Xiaoke Wang; Jinhang Zhu; Juan Du; Bing Shen

doi:10.3791/56317

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Method Article

Detection of Mitochondria Membrane Potential to Study CLIC4 Knockdown-induced HN4 Cell Apoptosis In Vitro

DOI:

10.3791/56317

⸱

July 17th, 2018

Jinsen Lu¹, Lele Wu², Xiaoke Wang², Jinhang Zhu², Juan Du², Bing Shen²

¹School of Basic Medical Sciences, Anhui Medical University, ²Department of Orthopedics, Anhui Provincial Hospital, Anhui Medical University

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Podsumowanie

Here we present a detailed protocol for the application of rhodamine 123 to identify the mitochondrial membrane potential (MMP) and study CLIC4 knockdown-induced HN4 cell apoptosis in vitro. Under common fluorescence microscope and confocal laser scanning fluorescence microscope, the real-time change of the MMP was recorded.

Streszczenie

Depletion of the mitochondrial membrane potential (MMP, ΔΨm) is considered the earliest event in the apoptotic cascade. It even occurs ahead of nuclear apoptotic characteristics, including chromatin condensation and DNA breakage. Once the MMP collapses, cell apoptosis will initiate irreversibly. A series of lipophilic cationic dyes can pass through the cell membrane and aggregate inside the matrix of mitochondrion, and serve as fluorescence marker to evaluate MMP change. As one of the six members of the Cl^- intracellular channel (CLIC) family, CLIC4 participates in the cell apoptotic process mainly through the mitochondrial pathway. Here we describe a detailed protocol to measure MMP via monitoring the fluorescence fluctuation of Rhodamine 123 (Rh123), through which we study apoptosis induced by CLIC4 knockdown. We discuss the advantages and limitations of the application of confocal laser scanning and normal fluorescence microscope in detail, and also compare it with other methods.

Wprowadzenie

Rh123 is a cationic fluorescence dye, which serves as an indicator for transmembrane potential. Rh123 is capable of penetrating the cell membrane and entering the mitochondrial matrix depending on the potential difference of inside and outside the membrane¹. Apoptosis leads to damage of mitochondrial membrane integrity. The mitochondrion permeability transition pore (MPTP) will open and lead to collapse of the MMP, which in turn results in the release of Rh123 to the outside of the mitochondria. Finally, stronger green fluorescence signal will be detected under fluorescence microscope. It is well documented that depletion of the MMP and elevated membrane permeability are early signs of cell apoptosis². Therefore, Rh123 may be applied to the detection of MMP change and the occurrence of cell apoptosis.

As the 6th most common carcinoma in the world, head and neck cancer severely deteriorates a person's health³. Although many approaches were developed in recent years, clinical outcome of treatment for patients suffering from head and neck squamous cell carcinoma (HNSCC) is still not ideal⁴. Exploring new therapeutic methods can improve the treatment for HNSCC⁵. Ion channels involving numerous biological processes display an important role in the development of different cancers⁶. Partial or total participation of Cl^- channels are highly involved in various properties of neoplastic transformation including active migration, high rate of proliferation and invasiveness. In light of this, the CLIC, a novel protein family, has been listed as a promising class of therapeutic targets for cancer treatment⁶^,⁷. Recent studies have revealed that members of the CLIC family including CLIC1, CLIC4, and CLIC5, localize to cardiac mitochondrial and the reactive oxygen species (ROS) level is upregulated by CLIC5, indicating the functional role of mitochondrial-located Cl^- channels in the apoptotic response⁸. CLIC4, one members of the CLIC family (also known as mtCLIC, P64H1, and RS43), has been most extensively studied for its apoptotic regulation properties in cancer cells and subcellular location including Golgi, endoplasmic reticulum, and mitochondrion in human keratinocytes⁷^,⁹^,¹⁰. The expression profile of CLIC4 was regulated by tumor necrosis factor-α (TNF-α), P53, and external stimulus. Overexpression and downregulation of CLIC4 trigger an apoptotic response mainly through the mitochondrial pathway accompanied with the imbalance of Bcl-2 family members, activation of caspase cascade, and release of cytochrome C¹¹^,¹²^,¹³. Therefore, MMP measurement is crucial to explore CLIC4-related apoptosis, and Rh123 serves as an ideal fluorescence indicator.

The present study describes a detailed protocol for the detection of MMP to study CLIC4 knockdown-induced apoptosis in HN4 cells. Rh123 is used as a fluorescence probe to observe the change of the MMP. Under common fluorescence microscope and confocal laser scanning fluorescence microscope, the real-time fluctuation of the MMP may be resolved. We discuss the advantages and limitations of the application of confocal laser scanning fluorescence microscope in detail, and also compare it with other methods. This protocol also can be applied to other apoptosis-related studies.

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Protokół

1. Cell Culture and Transfection

Cell culture
Note: HN4, an HNSCC cell line, was derived from patients with HNSCC¹⁴.
1. Culture HN4 cells in Dulbecco's modified Eagle medium (DMEM, 4.5 g/L glucose) supplemented with 10% fetal bovine serum and antibiotics (100 U/mL penicillin and 100 µg/mL streptomycin). Incubate cells at 37 °C with 5% CO₂.
Cell transfection
1. One day before transfection, plate 5 x 10⁵ cells in 2 mL/well of culture medium without antibiotics in 6-well plates.
2. Dilute 100 pmol CLIC4 siRNA or scrambled SiRNA in 250 µL of reduced serum media, gently. Dilute 5 µL liposome reagent in 250 µL of reduced serum media and incubate for 5 min. Combine the diluted siRNA with the diluted liposome reagent, mix gently, and incubate for 20 min at room temperature.
3. Add the mixture to each well containing cells and medium. Mix gently by rocking the plate back-and-forth. Incubate the cells at 37 °C in a CO₂ incubator for 24 h before proceeding with the following Rh123 labeling procedure. Replace the medium with normal growth medium 4 h after transfection.

2. Rh123 Labeling

Note: Rh123 was utilized to measure the MMP in HN4 cells¹.

After CLIC4 siRNA treatment (Section 1), use HN4 cells in 6-well plates for the following treatment. The amount of HN4 cells in each well is enough to repeat the experiment 10 times on coverslips.
Use tweezers to put circular coverslips on the bottom of new 12-well plates. The number of plates is set according to the experimental design (Figure 1A).
Put 150 µL of 100 µg/mL polylysine on the middle of every coverslip inside the 12-well plates and wait 2 min. Pay attention to not put polylysine outside the coverslips. Then remove the polylysine by pipettor thoroughly (Figure 1B).
Remove the culture medium of the HN4 cells inside the dish and add 1 mL 0.25% trypsin to detach the cells. After 6 min, add 2 mL culture medium to neutralize the trypsin. Gently mix the HN4 cells by pipettor for 5 times and seed 2 - 6 х 10⁴cells on the circular coverslips. Place in an incubator at 37 °C with 5% CO₂ (Figure 1C).
After 8 h incubation, incubate the HN4 cells with 2 µmol/L Rh123 for 40 min at 37 °C. Gently mix the medium up-and-down several times to ensure even distribution of Rh123 in the medium (Figure 1D).
Prepare enough normal physiological saline solution (NPSS); to make NPSS (in mmol/L): 140 NaCl, 5 KCl, 1 MgCl₂, 1 CaCl₂, 10 glucose, and 5 HEPES, pH 7.4). Preheat to 37 °C in a water bath.
Use tweezers to remove the coverslips and wash the remaining liquid via briefly placing the coverslips into the preheated NPBS buffer (Figure 1E).
Place the coverslips on the bottom of the 500 µL stainless steel chamber (see Table of Materials) with a replaceable 25 mm glass coverslip bottom sealed in place by an o-ring. Fix it by tightening the lid of the chamber (Figure 1E).
Add 450 µL preheated NPSS buffer to the assembled chamber and put the bath under the visual field of the fluorescence microscope or confocal laser scanning fluorescence microscope (Figure 1E).

3. Detection of the MMP

Common fluorescence microscope
1. Turn on the fluorescence microscope following the manufacturer's instructions.
  NOTE: Common fluorescence microscope was accomplished with a mercury lamp fiberoptic light source, a FITC filter set for Rh123 (480/40 excitation filter, 505 LP dichroic mirror and 535/40 emission filter) at room temperature. 20X objective was used to perform live-cell imaging.
2. Open the imaging system software and select the "New" button from the command bar to begin a new experiment (Figure 2A).
3. Adjust the visual field and focus to find the location of the cells in white light.
4. Turn off the light and push the button to close white light. Click the "Focus" button from the Command bar and select "Start Focusing" to switch on the fluorescence. Find the location of the cells again via microscope with a 507 nm excitation and 529 nm long pass emission wavelength (Set before the experiment). Adjust the visual field and focus again if needed (Figure 2B).
5. Select a visual field containing only 20 to 30 separated HN4 cells. The change of intracellular fluorescence signal for each cell will be recorded accurately.
6. Once a clear visual field is achieved, click "Close Focusing" from the Focus bar. Click "Acq One" from the Command Bar to acquire one set of images. Click "Regions" from the Command Bar and click the "OK" button to edit measurement regions.
  NOTE: From the Edit Region bar, different region shapes can be used depending on the study.
7. To fit for different shapes of individual cells, select the "Trace Region" tool and circle the region of one single cell and double click when finished. Repeat the procedure until all cells are circled (Figure 2C). Click "Done" and select "Save Images" to find the saved location.
8. Click "Zeroclock "and quickly push F4 to start monitoring the change of fluorescence intensity. Record the real-time change of fluorescence intensity once every 5 s for 5 min (Figure 2D).
9. When the baseline becomes stable, add 50 µL NPSS mixed with 0.5 µL of 100 mmol/L ATP to the chamber via pipettor. Remember to not touch the chamber to avoid removing the visual field (Figure 2E).
  NOTE: The fluorescence image will be recorded for 20 min and then the experiment can end via manual operation. The time duration is routinely settled for 20 min in order to observe the entire fluorescence change. However, manual operation to stop capture is applied when unexpected factors influence the stability of the curve or when the entire process takes less than 20 min.
Confocal laser scanning fluorescence microscope
1. Turn on the confocal laser scanning fluorescence microscope following the manufacturer's instructions, and open the bundled software.
  NOTE: Here, Rh123 was excited by an Argon laser set at 488 nm and the emitted signal was recorded over the range of 545 - 700 nm via application of the TD488/543/633 filter.
2. Click "Objective" under the "Acquire" menu to select 63X/1.4 N.A. oil objective lens. Observe the specimen and find a clear visual field under the light field.
3. Push the "TL/IL" button to switch to fluorescence mode and select the correct fluorescence filters to find the location of the cell under darkness via microscope. Push "SHUTTER" to protect the specimen when observation is finished.
4. Under the "Acquire" menu, adjust suitable PMT channel and click "Achieve" to activate the settled optical path (Figure 3A). Click on the "Configuration" menu and choose "Laser" to determine the needed laser type. "Argon" is recommended for this protocol (Figure 3B).
5. Click "Live" to get real-time image and make sure the visual field contains only 20 to 30 separated HN4 cells. The change of intracellular fluorescence signal for each cell will be recorded accurately.
6. Select "xyt" in Acquisition Mode in the "Acquisition" submenu under the "Acquire" menu (Figure 3C). Set 5 s and 20 min for time interval and duration, respectively. Click" Apply" when all parameters are settled.
7. Under the "Quantify" menu, use the "Draw Polyline" tool to circle the recording area of each cell. Select "Line Profile" and choose "Start" to conduct observation. Record the real-time change of fluorescence intensity for 5 min (Figure 3D - E).
8. When the baseline becomes stable, add 50 µL NPSS mixed with 0.5 µL of 100 mmol/L ATP to the chamber via pipettor. Remember to not touch the chamber to avoid removing the visual field.
  NOTE: The fluorescence image will be recorded for 20 min and then the experiment is completed.

4. Statistical Analysis

Common fluorescence microscope
1. Turn on the fluorescence microscope routinely following the operator's manual. Open the imaging system software and select the "Open" button from the command bar to open a saved experiment. Click "Regions" from the 'Command Bar' and click "OK" button to edit measurement regions.
2. Select the "Trace region" tool and circle the region of one single cell and double click when done. Repeat the procedure until all cells have been circled. Click "Done" and select the "F4: forward" button to obtain a trace showing fluorescence intensity.
3. Once finished, click the down arrow button located on the lower right corner of the graph and click "Show Graph Data" (Figure 2F). Click "OK" twice and choose the "Log Data" button to open the interface of data processing software. Click "Log Data" again and find the records of real time fluctuation of fluorescence intensity appear on the spreadsheet.
  NOTE: For each cell, changes in MMP were displayed as the ratio of fluorescence relative to the intensity before the application of ATP or TG (F1/F0). Each fluorescence intensity data were the average of 20 - 30 cells. Data for Rh123 are presented as mean ± SE. Results from 2 groups were tested by the two-tailed independent t test and P value <0.05 was considered as statistical significance. Statistical analysis software was applied to conduct the statistical analyses in this experiment.
Confocal laser scanning fluorescence microscope
1. Turn on the confocal laser microscope and log into the bundled software following the manufacturer's instructions.
2. Select "Fire" to open a recorded experiment.
3. Select the "Stack profile" tool under the "Quantify" menu, choose "All in one" from "Sort charts by Channels and ROIs."
4. Use the "Draw polygon" tool to circle cell regions for observation.
5. Select the "Graph" menu and click the right mouse button, and choose "Export to excel" to add the values of fluorescent intensity to a spreadsheet. The following analysis is consistent with normal fluorescence microscopes (Figure 3F).

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Wyniki

In the present study, Rh123 was applied to detect the MMP. Initially, HN4 cells were cultured for the following fluorescence staining experiments. Tweezers were used to put circular coverslips on the bottom of 6-well plates (Figure 1A). The coverslips were coated with polylysine for 5 min and then the polylysine removed via pipettor (Figure 1B). Then HN4 cells were trypsinized and seeded on the c...

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Dyskusje

It is well documented that Cl⁻ channels are essential in maintaining the hemostasis of the internal environment and play important roles in cell proliferation and apoptosis¹⁵^,¹⁶. Therefore, understanding the relationship between ion channel-targeted intervention and apoptosis is of great need and significance to find a better therapeutic approach for various cancers¹⁷. Mitochondria maintain the normal biological state of a...

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Ujawnienia

The authors have nothing to disclose.

Podziękowania

We kindly thank Mr. Chao Fang for cell culture. This work was supported by grants from the Natural Science Foundation of China (Grant No. 81570403, 81371284); Anhui Provincial Natural Science Foundation (Grant No. 1408085MH158); Outstanding Young Investigator of Anhui Medical University; Supporting Program for Excellent Young Talents in Universities of Anhui Province.

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Materiały

Name	Company	Catalog Number	Comments
HNSCC cells	ATCC	CRL-3241
Polylysine	Thermo Fisher Scientific	P4981
Specific siRNA for human CLIC4	Biomics	NM_013943	(accession numbers, NM_013943; corresponding to the cDNA sequence 5-GCTGAAGGAGGAGGACAAAGA-3) and scrambled siRNA (5 ACGCGUAACGCGGGAAUUU-3) were designed and obtained from Biomics Company
Lipofectamine 2000 Transfection Reagent	Thermo Fisher Scientific	L3000-015
Opti-MEM I Reduced Serum Medium, GlutaMAX	Thermo Fisher Scientific	51985-042
Rhodamine 123, FluoroPure grede	Thermo Fisher Scientific	R22420
Dulbecco’smodified Eagle medium (DMEM, 4.5 g/L glucose)	Gibco	11965-084
Fetal Bovine Serum, Qualified, Australia Origin	Gibco	10099141
Trypsin-EDTA Solution	Beyotime	C0201
Antibiotic-Antimycotic, 100X	Gibco	15240062
Laser Scanning Confocal Microscopy	Leica Microsystems GmbH	LEICA.SP5-DMI6000-DIC
Nikon Eclipse TE300 Inverted Microscope	Nikon	N/A
Metaflour, V7.5.0.0	Universal Imaging Corporation	N/A
Leica application suite, v2.6.0.7266	Leica Microsystems GmbH	N/A
Microsoft office Excel 2007	Microsoft	N/A
Sigma Plot 12.5	Systat Software	N/A
Attofluor Cell Chamber	Thermo Fisher Scientific	A7816

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