Microscopy & Microtechniques

New Method for Real-Time Autophagy Studies

Feb 11 2014

Author: Cindy Chen, Terry Gaige, Paul Hung on behalf of Merck KGaA. The life science business of Merck operates as MilliporeSigma in the U.S. and Canada

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Autophagy is an intracellular process leading to the lysosomal degradation of cytosolic components and organelles. Its best understood role is in cellular housekeeping; this activity directs the removal of damaged or unwanted products [1]. However, autophagy can also be induced in response to cancer therapies, when autophagy functions as a survival mechanism and thus potentially limits drug efficacy [2,3]. In established tumours, malignant progression and tumour maintenance have been linked to physiological adaptations resulting in upregulated or constitutively active autophagic pathways [2]. In addition, there are many stimuli that have been shown to activate autophagy, including nutrient starvation, reactive oxygen species [4], stress on the endoplasmic reticulum, and ammonia [5].
Once stimulated, unwanted cytosolic proteins and aging organelles are sequestered by a double-membrane vesicle known as an autophagosome (Figure 1). Protein complexes coordinate vesicle formation and enable the recruitment of LC3 into the inner and outer membranes of the autophagosome. LC3-labelled vesicles are trafficked to the lysosome. During this last phase, autophagosomes fuse with lysosomes to form autolysosomes, where unwanted nutrients are reduced to basic molecular building blocks and ultimately released back into the cytoplasm.
Measurement and tracking of autophagy are essential for elucidating this process. Many newer autophagy assays rely on the expression of stably transfected green fluorescence protein (GFP)-LC3 fusion proteins; in this case, autophagosome activity is visually identified by changes in GFP puncta [6]. Lysosomal inhibitors, such as chloroquine (CQ), have also been invaluable in determining the relative autophagic response to cellular stress. CQ blocks the last step of autophagy, lysosomal degradation; the resulting buildup of intermediates can serve as a quantifiable marker of autophagic activity [7]. By combining the use of live cell imaging with transduction of a GFP-tagged autophagosome marker (LC-3) in the presence of CQ, researchers can monitor the autophagosome formation process on a fluorescent microscope in real time. However, little is known about the latter stages of autophagy and the dynamics of lysosomal degradation.
In this article, we demonstrate the use of a microfluidic live cell imaging platform (the CellASIC® ONIX Microfluidic Platform, EMD Millipore) to develop a dynamic cell-based assay for monitoring the whole autophagy process. This platform offers temperature and gas control as well as media perfusion for precise environmental control. Using this system, LC3-GFP CHO reporter cells were subjected to nutrient starvation or hypoxic stresses for a designated time period followed by reintroduction of normal growth conditions. The time course of autophagy was visualised in real time under a fluorescent microscope, providing quantitative information on both autophagosome formation and lysosomal degradation machinery.

Assay Validation
To validate the media exchange capability of the CellASIC® ONIX platform as well as the ability to monitor and quantify autophagy through autophagosome counting, LC3-GFP CHO cells (70% confluent) were perfused with EBSS + 50 µM CQ for 100 minutes followed by regular culture medium for 200 minutes. As shown in Figures 2 and 3, the dynamic changes of autophagy in both the stress and recovery phase could be quantified through autophagosome counting.
Assessment of CQ Dose Response
Once the assay was validated, profiling of the CQ dose response in CHO cell lines was conducted. Once established in the microchamber, exposure conditions involved three phases: standard culture medium for 135 minutes, continuous CQ (10 µM, 100 µM, or 1 mM) perfusion for 255 minutes, and culture medium for the final 240 minutes to permit visual capture of the lysosomal degradation process. Images were taken every 15 minutes. Overall, the rate of autophagosome formation was proportional to the CQ concentration applied. However, at 1 mM, cells ceased committing to the autophagy pathway, and the number of autophagosomes stayed constant for the rest of the experiment. We also observed more dead cells in this treated group, indicating either that the maximal levels of autophagy in this cell line had been achieved, or that the cells committed to apoptosis or necrosis at the high CQ dose. Furthermore, degradation of autophagosomes occurred at a faster rate than the accumulation (Figure 4).


Hypoxia Studies
To further explore the dynamics of stress-induced autophagy, we exploited the CellASIC® ONIX system’s ability to regulate gaseous microenvironments to introduce severely hypoxic conditions within the cell chamber. Prior to analysis, the system’s control of oxygen content was validated. For gas flow rates of 20 mL/min and 3 mL/min, we consistently found that the switch time from normoxic to hypoxic gas environment occurred in less than one hour. For these two gas flow rates, steady-state concentrations were achieved with less than 2% and 10% deviation from the supplied gas, respectively.
In traditional static cultures, achieving equilibrium following defined gas switching is impractical due to incubator size and differences between the measured pericellular oxygen tension (within the flask) and that in the ambient air [8,9]. However, the new platform features a significantly reduced culture vessel size (10,000 cells per chamber) and restricted fluid volume (a few nanolitres), together leading to a faster gas exchange during our hypoxia studies.
Results from initial hypoxia experiments supported this fact; specifically, we found that, compared to the typical hypoxic response of cells cultured in traditional petri dishes [8-12], LC3-GFP CHO reporter cells in the microfluidic perfusion environment were far more sensitive to gas switching, demonstrating autophagosome formation within three hours of hypoxic treatment [10-12]. Following six-hour exposure, a large percentage of cells failed to recover and underwent apoptosis.
Profiling Autophagosome Formation
Based on these preliminary results, we performed dynamic profiling of autophagosome formation in reporter cells in response to CQ (10 µM, 100 µM, or 1 mM) under hypoxia conditions. Similar to results of starvation-induced autophagy, the rate of autophagosome appearance accelerated with respect to increasing CQ dose. As for the recovery phase, cells treated with 100 µM of the CQ responded almost instantaneously, while those treated with the highest dose (1 mM) demonstrated a far more protracted recovery profile (Figure 5 and 6).
To simultaneously monitor the two most important organelles involved in autophagy, we further transduced the LC3-GFP reporter CHO cells with a fluorescently tagged, lysosome-specific fusion protein construct, LAMP1-RFP. Transduced cells were incubated under mildly hypoxic conditions (3% O2) in the presence of CQ at various concentrations for 180 minutes, followed by prolonged 660-minute culture under normoxia in the presence of standard medium.
The data indicate that autophagogome formation started immediately after the switch to hypoxic conditions and lasted for three hours in the cells treated with 1 mM of CQ. In these cultures, lysosome degradation did not occur until almost 11 hours after gas exchange (Figure 7). However, we did not observe any conclusive response in the lysosomal activity during either autophagy or recovery phases except for the observation that lysosomes were instantly condensed under the hypoxic stress.
We speculate that the LAMP1-RFP transduction process (or the LAMP1-RFP construct itself) might be another source of cellular stress, hence affecting overall autophagic activity. We are currently exploring alternative labelling methods for dual-colour assays for hypoxia-induced autophagy.

Conclusion
The CellASIC® ONIX live cell imaging platform was used to create a dynamic assay that not only has the potential to simultaneously monitor multiple intracellular components throughout the entire autophagic process without disruption but also allows precise manipulation of culture parameters, thus exposing cells to more physiologically relevant conditions. This platform may be capable of simulating conditions of pulse exposure to drug compounds, and could provide additional information on dose response for compound profiling by revealing rates of autophagosome formation and degradation. It therefore has the potential to help in the discovery of new targets and therapeutic compounds in cancer as well as other diseases.
References
1. Cuervo, A. et al. (2004). Autophagy: in sickness and in health. Trends in Cell Biology; 14(2); 70-77.
2. Kimmelman, A. et al. (2011). The dynamic nature of autophagy in cancer. Genes and Development 25: 1999-2010.
3. Amaravadi, R. et al. (2011). Principles and current strategies for targeting autophagy for cancer treatment. Clinical Cancer Research 17: 654-666.
4. Neufeld, T. et al. (2010). TOR-dependent control of autophagy: biting the hand that feeds. Current Opinions of Cell Biology 22: 157-168.
5. Cheong, H. et al. (2011). Ammonia-induced autophagy is independent of ULK1/ULK2 kinase. Proc Natl Acad Sci 108: 11121-11126.
6. Mizushima, N. et al. (2010). Methods in mammalian autophagy research. Cell 140 (3): 313-326.
7. Yamamoto A. et al. (1998). Bafilomycin A1 prevents maturation of autophagic vacuoles by inhibiting fusion between autophagosomes and lysosomes in rat hepatoma cell line, H-4-II-E cells. Cell Structure and Function 23: 33-42.
8. Baumgardner, J. et al. (2003). In vitro intermittent hypoxia: challenges for creating hypoxia in cell cultures. Respiratory Physiology and Neurobiology 136: 131-139.
9. Bambrick, L. et al. (2011). In vitro cell culture pO2 is significantly different from incubator pO2. Biotechnology Progress 27: 1185-1189
10. Song Y. et al. (2013). Autophagy contributes to the survival of CD133+ liver cancer stem cell in the hypoxic and nutrient-deprived tumor microenvironment. Cancer Letters (in press)
11. Grkovic S. et al. (2013). IGFBP-3 binds GRP78, stimulates autophagy and promotes the survival of breast cancer cells exposed to adverse microenvironments. Oncogene 32: 2412-2420.
12. Hubbi M. et al. (2013). Chaperone-mediated autophagy targets hypoxia-inducible factor-1(HIF-1) for lysosomal degradation. The Journal of Biological Chemistry 288: 10703-10714

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