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1. Gene Delivery and Analysis of Optogenetic Induction of Lytic Cell Death

   https://doi.org/10.1002/cpz1.1023  

   Oh, Teak‐Jung; Gworek, Bryan; Mehfooz, Amna; Zhang, Kai (April 2024, Current Protocols)

   Abstract Necroptosis is a form of inflammatory lytic cell death involving active cytokine production and plasma membrane rupture. Progression of necroptosis is tightly regulated in time and space, and its signaling outcomes can shape the local inflammatory environment of cells and tissues. Pharmacological induction of necroptosis is well established, but the diffusive nature of chemical death inducers makes it challenging to study cell‐cell communication precisely during necroptosis. Receptor‐interacting protein kinase 3, or RIPK3, is a crucial signaling component of necroptosis, acting as a crucial signaling node for both canonical and non‐canonical necroptosis. RIPK3 oligomerization is crucial to the formation of the necrosome, which regulates plasma membrane rupture and cytokine production. Commonly used necroptosis inducers can activate multiple downstream signaling pathways, confounding the signaling outcomes of RIPK3‐mediated necroptosis. Opsin‐free optogenetic techniques may provide an alternative strategy to address this issue. Optogenetics uses light‐sensitive protein‐protein interaction to modulate cell signaling. Compared to chemical‐based approaches, optogenetic strategies allow for spatiotemporal modulation of signal transduction in live cells and animals. We developed an optogenetic system that allows for ligand‐free optical control of RIPK3 oligomerization and necroptosis. This article describes the sample preparation, experimental setup, and optimization required to achieve robust optogenetic induction of RIPK3‐mediated necroptosis in colorectal HT‐29 cells. We expect that this optogenetic system could provide valuable insights into the dynamic nature of lytic cell death. © 2024 The Authors. Current Protocols published by Wiley Periodicals LLC. Basic Protocol 1: Production of lentivirus encoding the optogenetic RIPK3 system Support Protocol: Quantification of the titer of lentivirus Basic Protocol 2: Culturing, chemical transfection, and lentivirus transduction of HT‐29 cells Basic Protocol 3: Optimization of optogenetic stimulation conditions Basic Protocol 4: Time‐stamped live‐cell imaging of HT‐29 lytic cell death Basic Protocol 5: Quantification of HT‐29 lytic cell death 

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2. Magnetic Stimulation of Dissociated Cortical Neurons on a Planar Mulitelectrode Array

   Mukesh, S; Zeller-Townson, R; Butera, R; Bhatti, P (March 2019, International IEEE/EMBS Conference on Neural Engineering)

   We perform experiments to study the magnetic stimulus-induced changes in neural activity in dissociated cortical neurons with different stimulation parameters. The goal of performing these studies is to build on the results from our previous work that suggested magnetic stimulation may lead to improved performance of cochlear implants. A magnetic stimulator is assembled using a micro-scale coil. To detect small changes in activity, we use glass substrate MEAs to measure culture-wide synaptically-mediated response to stimulation, rather than the direct activation of individual neurons. Our initial findings show magnetic stimulation is associated with changes in network-wide firing rates, beyond those expected by spontaneous drift in activity. This suggests that the magnetic stimulation parameters we used were able to evoke neural activity. However, we observe substantial differences in the type of change induced in neural activity in different cultures and with different stimulation parameters, some showing increases in activity and others showing decreases in activity. This may be due to differences in the number and type of neurons (inhibitory or excitatory) activated by stimulation in different experiments, which in turn may be affected by differences in stimulator location and alignment, differences in stimulus pulse waveform and amplitudes, or differences in culture density or cell morphology. We also compare the power consumption and heating of this stimulation technique with that of electrical stimulation. Finally, a need to optimize the experimental setup to allow longer experiments is identified, to reach definite conclusions. 

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3. Agarose‐based 3D Cell Confinement Assay to Study Nuclear Mechanobiology

   https://doi.org/10.1002/cpz1.847  

   Elpers, Margaret A; Varlet, Alice‐Anais; Agrawal, Richa; Lammerding, Jan (July 2023, Current Protocols)

   Abstract Cells in living tissues are exposed to substantial mechanical forces and constraints imposed by neighboring cells, the extracellular matrix, and external factors. Mechanical forces and physical confinement can drive various cellular responses, including changes in gene expression, cell growth, differentiation, and migration, all of which have important implications in physiological and pathological processes, such as immune cell migration or cancer metastasis. Previous studies have shown that nuclear deformation induced by 3D confinement promotes cell contractility but can also cause DNA damage and changes in chromatin organization, thereby motivating further studies in nuclear mechanobiology. In this protocol, we present a custom‐developed, easy‐to‐use, robust, and low‐cost approach to induce precisely defined physical confinement on cells using agarose pads with micropillars and externally applied weights. We validated the device by confirming nuclear deformation, changes in nuclear area, and cell viability after confinement. The device is suitable for short‐ and long‐term confinement studies and compatible with imaging of both live and fixed samples, thus presenting a versatile approach to studying the impact of 3D cell confinement and nuclear deformation on cellular function. This article contains detailed protocols for the fabrication and use of the confinement device, including live cell imaging and labeling of fixed cells for subsequent analysis. These protocols can be amended for specific applications. © 2023 Wiley Periodicals LLC. Basic Protocol 1: Design and fabrication of the confinement device wafer Basic Protocol 2: Cell confinement assay Support Protocol 1: Fixation and staining of cells after confinement Support protocol 2: Live/dead staining of cells during confinement 

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4. Methods for Discerning the Impact of Mucus on Host Defenses Against Viral Infection

   https://doi.org/10.1002/cpz1.70201  

   Corkran, Maria; Boboltz, Allison; Duncan, Gregg A; Scull, Margaret A (September 2025, Current Protocols)

   Abstract Mucus is an important component of airway host defenses that acts by enabling the trapping and clearance of infectious materials such as bacteria and viruses. It can be difficult, however, to design experiments that independently determine the extent to which mucus contributes to innate barrier functions in the lung. Here, we provide detailed protocols to collect mucus from human airway epithelial cultures and evaluate how the properties of mucus impact mucociliary transport and protection from viral infection. We include recommended test parameters depending on the specific research question as it relates to respiratory infectious diseases. © 2025 The Author(s). Current Protocols published by Wiley Periodicals LLC. Basic Protocol 1: Analysis of mucociliary transport and ciliary beat frequency in HAE cultures Basic Protocol 2: Collection of mucus from HAE cultures Basic Protocol 3: Transplantation of mucus to HAE cultures and infection with virus 

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5. Measuring Cytoskeletal Mechanical Fluctuations and Rheology with Active Micropost Arrays

   https://doi.org/10.1002/cpz1.433  

   Shi, Yu; Sivarajan, Shankar; Crocker, John C.; Reich, Daniel H. (May 2022, Current Protocols)

   Abstract The dynamics of the cellular actomyosin cytoskeleton are crucial to many aspects of cellular function. Here, we describe techniques that employ active micropost array detectors (AMPADs) to measure cytoskeletal rheology and mechanical force fluctuations. The AMPADS are arrays of flexible poly(dimethylsiloxane) (PDMS) microposts with magnetic nanowires embedded in a subset of microposts to enable actuation of those posts via an externally applied magnetic field. Techniques are described to track the magnetic microposts’ motion with nanometer precision at up to 100 video frames per second to measure the local cellular rheology at well‐defined positions. Application of these high‐precision tracking techniques to the full array of microposts in contact with a cell also enables mapping of the cytoskeletal mechanical fluctuation dynamics with high spatial and temporal resolution. This article describes (1) the fabrication of magnetic micropost arrays, (2) measurement protocols for both local rheology and cytoskeletal force fluctuation mapping, and (3) special‐purpose software routines to reduce and analyze these data. © 2022 The Authors. Current Protocols published by Wiley Periodicals LLC. Basic Protocol 1: Fabrication of magnetic micropost arrays Basic Protocol 2: Data acquisition for cellular force fluctuations on non‐magnetic micropost arrays Basic Protocol 3: Data acquisition for local cellular rheology measurements with magnetic microposts Basic Protocol 4: Data reduction: determining microposts’ motion Basic Protocol 5: Data analysis: determining local rheology from magnetic microposts Basic Protocol 6: Data analysis for force fluctuation measurements Support Protocol 1: Fabrication of magnetic Ni nanowires by electrodeposition Support Protocol 2: Configuring Streampix for magnetic rheology measurements 

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