From MEFs to Matrigel 3: Passaging hESCs from Matrigel onto Matrigel

This video demonstrates how to maintain the growth of human embryonic stem cells (hESCs) in feeder cell-free conditions and how to continuously passage hESCs in feeder cell-free conditions. Confirmation of hESC pluripotency grown in feeder cell-free conditions by immunofluorescence microscopy is also demonstrated.Open in a separate windowClick here to view.^{(24M, flv)}     

Using Bioluminescent Imaging to Investigate Synergism Between Streptococcus pneumoniae and Influenza A Virus in Infant Mice

During the 1918 influenza virus pandemic, which killed approximately 50 million people worldwide, the majority of fatalities were not the result of infection with influenza virus alone. Instead, most individuals are thought to have succumbed to a secondary bacterial infection, predominately caused by the bacterium Streptococcus pneumoniae (the pneumococcus). The synergistic relationship between infections caused by influenza virus and the pneumococcus has subsequently been observed during the 1957 Asian influenza virus pandemic, as well as during seasonal outbreaks of the virus (reviewed in ^{1, 2}). Here, we describe a protocol used to investigate the mechanism(s) that may be involved in increased morbidity as a result of concurrent influenza A virus and S. pneumoniae infection. We have developed an infant murine model to reliably and reproducibly demonstrate the effects of influenza virus infection of mice colonised with S. pneumoniae. Using this protocol, we have provided the first insight into the kinetics of pneumococcal transmission between co-housed, neonatal mice using in vivo imaging ³.Download video file.^{(66M, mov)}     

The Preparation of Primary Hematopoietic Cell Cultures From Murine Bone Marrow for Electroporation

It is becoming increasingly apparent that electroporation is the most effective way to introduce plasmid DNA or siRNA into primary cells. The Gene Pulser MXcell electroporation system and Gene Pulser electroporation buffer were specifically developed to transfect nucleic acids into mammalian cells and difficult-to-transfect cells, such as primary and stem cells.This video demonstrates how to establish primary hematopoietic cell cultures from murine bone marrow, and then prepare them for electroporation in the MXcell system. We begin by isolating femur and tibia. Bone marrow from both femur and tibia are then harvested and cultures are established. Cultured bone marrow cells are then transfected and analyzed.Download video file.^{(51M, flv)}     

In Vitro Nuclear Assembly Using Fractionated Xenopus Egg Extracts

Nuclear membrane assembly is an essential step in the cell division cycle; this process can be replicated in the test tube by combining Xenopus sperm chromatin, cytosol, and light membrane fractions. Complete nuclei are formed, including nuclear membranes with pore complexes, and these reconstituted nuclei are capable of normal nuclear processes.Open in a separate windowClick here to view.^{(28M, flv)}     

Freezing and Thawing Human Embryonic Stem Cells

Since James Thomson et al developed a technique in 1998 to isolate and grow hES in culture, freezing cells for later use and thawing and expanding cells from a frozen stock have become important procedures performed in routine hES cell culture. Since hES cells are very sensitive to the stresses of freezing and thawing, special care must taken. Here we demonstrate the proper technique for rapidly thawing hES cells from liquid nitrogen stocks, plating them on mouse embryonic feeder cells, and slowly freezing them for long-term storage.Download video file.^{(102M, mp4)}     

Studying Membrane Biogenesis with a Luciferase-Based Reporter Gene Assay

To study the coordination of different lipid synthesis pathways during membrane biogenesis it is useful to work with an experimental system where membrane biogenesis occurs rapidly and in an inducible manner. We have found that phagocytosis of latex beads is practical for these purposes as cells rapidly synthesize membrane lipids to replenish membrane pools lost as wrapping material during particle engulfment. Here, we describe procedures for studying changes in phagocytosis-induced gene expression with a luciferase-based reporter gene approach using the Dual-Glo Luciferase Assay System from Promega.Open in a separate windowClick here to view.^{(86M, flv)}     

From MEFs to Matrigel 2: Splitting hESCs from MEFs onto Matrigel

This video demonstrates how to grow human embryonic stem cells (hESCs) on mouse embryonic fibroblast (MEF) feeder cells, how to passage hESCs from MEF plates to feeder cell-free Matrigel plates. Download video file.^{(134M, mov)}     

Protocols for Oral Infection of Lepidopteran Larvae with Baculovirus

Baculoviruses are widely used both as protein expression vectors and as insect pest control agents. This video shows how lepidopteran larvae can be infected with polyhedra by droplet feeding and diet plug-based bioassays. This accompanying Springer Protocols section provides an overview of the baculovirus lifecycle and use of baculoviruses as insecticidal agents, including discussion of the pros and cons for use of baculoviruses as insecticides, and progress made in genetic enhancement of baculoviruses for improved insecticidal efficacy.Open in a separate windowClick here to view.^{(52M, flv)}     

Spinal Cord Electrophysiology

The neonatal mouse spinal cord is a model for studying the development of neural circuitries and locomotor movement. We demonstrate the spinal cord dissection and preparation of recording bath artificial cerebrospinal fluid used for locomotor studies. Once dissected, the spinal cord ventral nerve roots can be attached to a recording electrode to record the electrophysiologic signals of the central pattern generating circuitry within the lumbar cord.Open in a separate windowClick here to view.^{(19M, flv)}     

Alphavirus Transducing System: Tools for Visualizing Infection in Mosquito Vectors

Alphavirus transducing systems (ATSs) are important tools for expressing genes of interest (GOI) during infection. ATSs are derived from cDNA clones of mosquito-borne RNA viruses (genus Alphavirus; family Togaviridae). The Alphavirus genus contains about 30 different mosquito-borne virus species. Alphaviruses are enveloped viruses and contain single-stranded RNA genomes (~11.7 Kb). Alphaviruses transcribe a subgenomic mRNA that encodes the structural proteins of the virus required for encapsidation of the genome and maturation of the virus. Alphaviruses are usually highly lytic in vertebrate cells, but persistently infect susceptible mosquito cells with minimal cytopathology. These attributes make them excellent tools for gene expression in mosquito vectors. The most common ATSs in use are derived from Sindbis virus (SINV). The broad species tropism of SINV allows for infection of insect, avian, and mammalian cells8. However, ATSs have been derived from other alphaviruses as well^9,10,20. Foreign gene expression is made possible by the insertion of an additional viral subgenomic RNA initiation site or promoter. ATSs in which an exogenous gene sequence is positioned 5'' to the viral structural genes is used for stable protein expression in insects. ATSs, in which a gene sequence is positioned 3'' to the structural genes, is used to trigger RNAi and silence expression of that gene in the insect.ATSs have proven to be valuable tools for understanding vector-pathogen interactions, molecular details of viral replication and maintenance infectious cycles^3,4,11,19,21. In particular, the expression of fluorescent and bioluminescent reporters has been instrumental tracking the viral infection in the vector and virus transmission^5,14-16,18. Additionally, the vector immune response has been described using two strains of SINV engineered to express GFP^2,9.Here, we present a method for the production of SINV containing a fluorescent reporter (GFP) from the cDNA infectious clone. Infectious, full-length RNA is transcribed from the linearized cDNA clone. Infectious RNA is introduced into permissive target cells by electroporation. Transfected cells generate infectious virus particles expressing the GOI. Harvested virus is used to infect mosquitoes, as described here, or other host species (not shown herein). Vector competence is assessed by detecting fluorescence outside the midgut or by monitoring virus transmission⁷. Use of a fluorescent reporter as the GOI allows for convenient estimation of virus spread throughout a cell culture, for determination of rate of infection, dissemination in exposed mosquitoes, virus transmission from the mosquito and provides a rapid gauge of vector competence.Download video file.^{(46M, mov)}     

Peptides from Phage Display Library Modulate Gene Expression in Mesenchymal Cells and Potentiate Osteogenesis in Unicortical Bone Defects

Two novel synthetic peptides accelerate bone formation and can be delivered using a collagen matrix. The aim of this study was to investigate the effects on bone repair in a unicortical defect model. Treatment of mesenchymal cells produced an increase in alkaline phosphatase activity, showed nodule formation by the cells, and increased the expression of genes for runx2, osterix, bone sialoprotein, and osteocalcin. A collagen sponge soaked with peptide promoted repair of bone defects, whereas the control was less effective. The results from this study demonstrated that mesenchymal cells treated with peptide in vitro differentiate towards osteogenesis, and, that peptides delivered in vivo using a collagen sponge promote the repair of unicortical defects.Download video file.^{(49M, mov)}     

Single-Particle Tracking Demonstrates that Actin Coordinates the Movement of the Ebola Virus Matrix Protein

The Ebola virus causes severe hemorrhagic fever and has a mortality rate that can be as high as 90%, yet no vaccines or approved therapeutics, to our knowledge, are available. To replicate and egress the infected host cell the Ebola virus uses VP40, its major matrix protein to assemble at the inner leaflet of the plasma membrane. The assembly and budding of VP40 from the plasma membrane of host cells seem still poorly understood. We investigated the assembly and egress of VP40 at the plasma membrane of human cells using single-particle tracking. Our results demonstrate that actin coordinates the movement and assembly of VP40, a critical step in viral egress. These findings underscore the ability of single-molecule techniques to investigate the interplay of VP40 and host proteins in viral replication.The actin cortex below the plasma membrane of mammalian cells is essential for maintenance of cell shape and for cell movement. This cortex has also been found to play an essential role in the replication process of a number of viruses including West Nile virus (1), respiratory syncytial virus (2), influenza (3), and vaccinia virus (4). Additionally, actin has been found to play a central role in the assembly and budding of HIV-1 (5) whereas Marburg virus has been shown to use actin-enriched filopodia to exit the host cell (6). Actin has also been found to be packaged into Ebola-virus-like particles (VLPs) (7). Ebola virus, which causes severe hemorrhagic fever, harbors a single-stranded negative-sense RNA genome encoding seven proteins. Of these seven proteins, VP40 is the most abundantly expressed and has been found to play a central role in the budding of the virus from the plasma membrane (8). Whereas actin has been found in Ebola VLPs (7), the role of actin in Ebola VP40 assembly is still seemingly unknown. Here, we have used Raster image correlation spectroscopy (RICS) (9) and three-dimensional single-particle tracking (see Fig. S1 in the Supporting Material) (10) to investigate the dynamics of Ebola VP40 and actin. We report that preassembled VLPs (pVLPs) of Ebola VP40 require actin for directed movement and assembly.Ebola VP40 has been demonstrated to colocalize with actin and actin is found in VP40 VLPs (7), suggesting an important role for actin in the replication cycle of the virus. To confirm the colocalization between VP40 and actin in HEK293 and CHO-K1 cells, we used confocal microscopy to examine the distribution of EGFP-VP40 and mCherry-actin. EGFP-VP40 and mCherry-actin displayed colocalization at the plasma membrane of HEK293 and CHO-K1 cells (see Fig. S2 A), which was markedly reduced in response to treatment with LAT-A (see Fig. S2 B and Fig. S3 A), an actin polymerization inhibitor. VP40 plasma membrane localization was not disrupted by LAT-A treatment (not unexpected, as VP40 is a lipid-binding protein (11) where high affinity for the PM drives its cellular localization (E. Adu-Gyamfi and R. V. Stahelin, unpublished)). To test whether this VP40-actin interaction is important to viral egress, we detected EGFP-VP40 with an anti-EGFP antibody used to measure VLPs formed from cells expressing EGFP-VP40. This was also performed to assess the effect of pharmacological treatment on EGFP-VP40-expressing cells with LAT-A or with the microtubule polymerization inhibitor nocodazole (see Fig. S3 B). LAT-A treatment led to a significant reduction in VLP formation whereas nocodazole did not display detectable effects.To test whether the VP40 and actin are engaged in synchronized movement, we performed time-lapse imaging in both the green and red channels. We observed that the pVLPs move with actin fibers extending from the plasma membrane (see Movie S1 in the Supporting Material). The movement was rapid, and caused smaller particles to merge into larger filamentous forms. To further demonstrate that the motion of actin and VP40 spatially overlapped, we used RICS to obtain correlation maps of EGFP-VP40 and mCherry-actin (Fig. 1). The spatial cross-correlation map indicated significant overlap of VP40 and actin movement (Fig. 2, A–C) at the plasma membrane (Fig. 1 and see Fig. S6), but not in the cytosol (see Fig. S5 and Fig. S7). In contrast, EGFP-VP40 and mCherry-α-tubulin (see Fig. S8, Fig. S9, and Fig. S10) displayed no significant spatial cross-correlation at the plasma membrane (Fig. S11) or other regions of the cell (see Fig. S12), supporting the VLP egress data where inhibition of microtubule polymerization did not influence viral egress.Open in a separate windowFigure 1EGFP-VP40 and mCherry-actin RICS analysis at the membrane. (A) HEK293 cells expressing EGFP-VP40 and mCherry-actin were imaged for 100 frames at 256 × 256 pixels. (White scale bar = 2 μm.) (B) Average intensity image of EGFP-VP40 across the 100 collected frames. (Pink box) Used to select a region of interest to yield the (C) average EGFP-VP40 intensity image. (D) Average intensity image of mCherry-actin taken for 100 frames at 256 × 256 pixels was used to select the same region of interest as in panel B (pink box) to yield the (E) average intensity image of the mCherry-actin signal in this region. (F) The two-dimensional spatial cross-correlation analysis of panels C and E demonstrates significant cross-correlation of VP40 and actin signals.Open in a separate windowFigure 2Three-dimensional RICS correlation maps of VP40 and actin cross-correlate at the plasma membrane. (A) EGFP-VP40 and (B) mCherry-actin (Fig. 1 and see Fig. S6 in the Supporting Material) RICS autocorrelation functions. (C) Appreciable cross-correlation is observed for EGFP-VP40 and mCherry-actin at the plasma membrane.To test whether the motion of the pVLPs is directed by actin, we applied the three-dimensional orbital tracking method first introduced by Levi et. al. (10). Tracking of isolated particles (Fig. 3 A) in five different cells allowed determination of the pVLPs trajectories (Fig. 3 D), which suggested that the VP40 particles undergo a directed motion. To verify this, we plotted the mean-square displacement (MSD) curves for the pVLPs (Fig. 3 C), which confirmed the trajectory was characteristic of directed motion. Analysis of the intensity profile of the dynamic VP40 particles suggested that the intensity of the particle changes with respect to time. Bleaching is expected if the molecule is exposed to the laser beam for an extended period of time; however, an increase in intensities was observed along the trajectory of the green channel due to addition of VP40 molecules. This suggests that the movement of the particles along actin fibers promote multimerization and maturation of the pVLPs. When actin polymerization was inhibited in four different cells with LAT-B, the rapid movement (see Fig. S13) and the directed trajectories of the pVLPs were lost (Fig. 3, E and F). This was reflected in a change from directed motion to movement indicative of random then constrained diffusion (Fig. 3, E and F).Open in a separate windowFigure 3Actin directs the movement of VP40 particles. HEK293 cells transfected with EGFP-VP40 were imaged with an electronic zoom of 2000 mV, corresponding to 72 nm/pixel in both X and Y. (A) An isolated and representative VP40 particle (highlighted by white box, inset) was tracked as described in the Supporting Material. (B) Intensity profile of the pVLP in A demonstrates increases in EGFP-VP40 intensity along the trajectory. (C) MSD of the pVLP, which follows a ballistic motion with a velocity of 0.067 ± 0.01 μm² s⁻¹. (D) The three-dimensional trajectory of the particle shown in panels A–C. (E) MSD curve of VP40 particles yields random then constrained diffusion after LAT-B treatment with a mean velocity of 0.017 ± 0.006 μm² s⁻¹ (p < 0.001). (F) Three-dimensional trajectory of the same particle shown in panel E displays a random then constrained diffusion.Taken together, our findings demonstrate that the movement of the pVLPs is driven by actin. Analysis of the pVLPs trajectories also suggests that the motion of pVLPs on actin enables further addition of VP40 molecules. These findings raise important questions regarding contemporary understanding of Ebola assembly and egress. VP40 lacks a consensus actin-binding motif, suggesting an adaptor protein such as an actin motor protein may function in this process. For instance, Myo10 has been found to be essential to Marburg virus release (6); however, Marburg VP40-Myo10 direct interactions were not observed, suggesting other cellular adaptor proteins may function in this process. Given the pathogenic nature of the Ebola virus and the necessity of VP40 to the assembly and egress of the virus (8), the VP40-actin coordination represents, to us, a novel target for therapeutic development.     

Titration of Human Coronaviruses Using an Immunoperoxidase Assay

Calculation of infectious viral titers represents a basic and essential experimental approach for virologists. Classical plaque assays cannot be used for viruses that do not cause significant cytopathic effects, which is the case for strains 229E and OC43 of human coronavirus (HCoV). An alternative indirect immunoperoxidase assay (IPA) is herein described for the detection and titration of these viruses. Susceptible cells are inoculated with serial logarithmic dilutions of samples in a 96-well plate. After viral growth, viral detection by IPA yields the infectious virus titer, expressed as "Tissue Culture Infectious Dose" (TCID50). This represents the dilution of a virus-containing sample at which half of a series of laboratory wells contain replicating virus. This technique is a reliable method for the titration of HCoV in biological samples (cells, tissues or fluids).Download video file.^{(92M, mov)}     

Measuring Caenorhabditis elegans Life Span on Solid Media

Aging is a degenerative process characterized by a progressive deterioration of cellular components and organelles resulting in mortality. The nematode Caenorhabditis elegans has emerged as a principal model used to study the biology of aging. Because virtually every biological subsystem undergoes functional decline with increasing age, life span is the primary endpoint of interest when considering total rate of aging. In nematodes, life span is typically defined as the number of days an animal remains responsive to external stimuli. Nematodes can be propagated either in liquid media or on solid media in plates, and techniques have been developed for measuring life span under both conditions. Here we present a generalized protocol for measuring life span of nematodes maintained on solid nematode growth media and fed a diet of UV-killed bacteria. These procedures can easily be adapted to assay life span under various common conditions, including a diet consisting of live bacteria, dietary restriction, and RNA interference.Open in a separate windowClick here to view.^{(78M, flv)}