Imaging-Based Reporter Systems to Define CVB-Induced Membrane Remodeling in Living Cells

Enteroviruses manipulate host membranes to form replication organelles, which concentrate viral and host factors to allow for efficient replication. However, this process has not been well-studied in living cells throughout the course of infection. To define the dynamic process of enterovirus membrane remodeling of major secretory pathway organelles, we have developed plasmid-based reporter systems that utilize viral protease-dependent release of a nuclear-localized fluorescent protein from the endoplasmic reticulum (ER) membrane during infection, while retaining organelle-specific fluorescent protein markers such as the ER and Golgi. This system thus allows for the monitoring of organelle-specific changes induced by infection in real-time. Using long-term time-lapse imaging of living cells infected with coxsackievirus B3 (CVB), we detected reporter translocation to the nucleus beginning ~4 h post-infection, which correlated with a loss of Golgi integrity and a collapse of the peripheral ER. Lastly, we applied our system to study the effects of a calcium channel inhibitor, 2APB, on virus-induced manipulation of host membranes. We found that 2APB treatment had no effect on the kinetics of infection or the percentage of infected cells. However, we observed aberrant ER structures in CVB-infected cells treated with 2APB and a significant decrease in viral-dependent cell lysis, which corresponded with a decrease in extracellular virus titers. Thus, our system provides a tractable platform to monitor the effects of inhibitors, gene silencing, and/or gene editing on viral manipulation of host membranes, which can help determine the mechanism of action for antivirals.

Download Full-text

Visualization of Membrane Sorting and Fusion in Living Cells using Total Internal Reflection (TIR) and Multicolor Video Microscopy

Microscopy and Microanalysis ◽

10.1017/s1431927600026246 ◽

2001 ◽

Vol 7 (S2) ◽

pp. 34-35

Author(s):

Derek Toomre ◽

Patrick Keller ◽

Elena Diaz ◽

Jamie White ◽

Kai Simons

Keyword(s):

Plasma Membrane ◽

Total Internal Reflection ◽

Fluorescent Protein ◽

Time Lapse ◽

Living Cells ◽

Video Microscopy ◽

Internal Reflection ◽

Fast Time ◽

Cellular Polarity ◽

Microscopy Technique

Post-Golgi sorting of different classes of newly synthesized proteins and lipids is central to the generation and maintenance of cellular polarity. to directly visualize the dynamics and location of apical/basolateral sorting and trafficking we used fast time-lapse multicolor video microscopy in living cells. Specifically, green fluorescent protein color variants (cyan, CFP; yellow, YFP) of apical cargo (GPI-anchored) and basolateral cargo (vesicular stomatitis virus glycoprotein, VSVG) were generated; see FIG 1. Fast dual color fluorescence video microscopy allowed visualization with high temporal and spatial resolution. Our studies revealed that apical and basolateral cargo progressively segregated into large domains in Golgi/TGN structures, excluded resident proteins, and exited in separate transport containers. These carries remained distinct and did not merge with endocytic structures en route to the plasma membrane. Interestingly, our data suggest that the primary sorting occurs by lateral segregation in the Golgi, prior to budding (FIG 2). Further characterization of morphological differences of apical versus basolateral transport carriers was achieved using a specialized microscopy technique called total internal reflection (TIR) microscopy. with this approach only the bottom of the cell (<100 nm) was illuminated by an exponentially decaying evanescent “wave” of light. A series of images, taken at ∼1 second intervals, shows a bright “flash” of fluorescence when the vesicle fuse with the plasma membrane and the fluorophore diffuses into the plasma membrane (FIG 3).

Download Full-text

An Artificially Constructed De Novo Human Chromosome Behaves Almost Identically to Its Natural Counterpart during Metaphase and Anaphase in Living Cells

Molecular and Cellular Biology ◽

10.1128/mcb.00355-06 ◽

2006 ◽

Vol 26 (20) ◽

pp. 7682-7695 ◽

Cited By ~ 16

Author(s):

Tomohiro Tsuduki ◽

Megumi Nakano ◽

Nao Yasuoka ◽

Saeko Yamazaki ◽

Teruaki Okada ◽

...

Keyword(s):

Yeast Artificial Chromosome ◽

Fluorescent Protein ◽

De Novo ◽

Artificial Chromosome ◽

Time Lapse ◽

Living Cells ◽

Lac Repressor ◽

Host Chromosome ◽

Artificial Chromosomes ◽

Spindle Midzone

ABSTRACT Human artificial chromosomes (HACs) are promising reagents for the analysis of chromosome function. While HACs are maintained stably, the segregation mechanisms of HACs have not been investigated in detail. To analyze HACs in living cells, we integrated 256 copies of the Lac operator into a precursor yeast artificial chromosome (YAC) containing α-satellite DNA and generated green fluorescent protein (GFP)-tagged HACs in HT1080 cells expressing a GFP-Lac repressor fusion protein. Time-lapse analyses of GFP-HACs and host centromeres in living mitotic cells indicated that the HAC was properly aligned at the spindle midzone and that sister chromatids of the HAC separated with the same timing as host chromosomes and moved to the spindle poles with mobility similar to that of the host centromeres. These results indicate that a HAC composed of a multimer of input α-satellite YACs retains most of the functions of the centromeres on natural chromosomes. The only difference between the HAC and the host chromosome was that the HAC oscillated more frequently, at higher velocity, across the spindle midzone during metaphase. However, this provides important evidence that an individual HAC has the capacity to maintain tensional balance in the pole-to-pole direction, thereby stabilizing its position around the spindle midzone.

Download Full-text

The Equine Herpesvirus 1 US2 Homolog Encodes a Nonessential Membrane-Associated Virion Component

Journal of Virology ◽

10.1128/jvi.73.4.3430-3437.1999 ◽

1999 ◽

Vol 73 (4) ◽

pp. 3430-3437 ◽

Cited By ~ 27

Author(s):

Alexandra Meindl ◽

Nikolaus Osterrieder

Keyword(s):

Amino Acids ◽

Plasma Membrane ◽

Secretory Pathway ◽

Fluorescent Protein ◽

Viral Envelope ◽

Equine Herpesvirus ◽

Equine Herpesvirus 1 ◽

Amino Terminal ◽

Infected Cells ◽

Herpesvirus 1

ABSTRACT Experiments were conducted to analyze the equine herpesvirus 1 (EHV-1) gene 68 product which is encoded by the EHV-1 US2 homolog. An antiserum directed against the amino-terminal 206 amino acids of the EHV-1 US2 protein specifically detected a protein with an M r of 34,000 in cells infected with EHV-1 strain RacL11. EHV-1 strain Ab4 encodes a 44,000-M r Us2 protein, whereas vaccine strain RacH, a high-passage derivative of RacL11, encodes a 31,000-M r Us2 polypeptide. Irrespective of its size, the US2 protein was incorporated into virions. The EHV-1 US2 protein localized to membrane and nuclear fractions of RacL11-infected cells and to the envelope fraction of purified virions. To monitor intracellular trafficking of the protein, the green fluorescent protein (GFP) was fused to the carboxy terminus of the EHV-1 US2 protein or to a truncated US2 protein lacking a stretch of 16 hydrophobic amino acids at the extreme amino terminus. Both fusion proteins were detected at the plasma membrane and accumulated in the vicinity of nuclei of transfected cells. However, trafficking of either GFP fusion protein through the secretory pathway could not be demonstrated, and the EHV-1 US2 protein lacked detectable N- and O-linked carbohydrates. Consistent with the presence of the US2 protein in the viral envelope and plasma membrane of infected cells, a US2-negative RacL11 mutant (L11ΔUS2) exhibited delayed penetration kinetics and produced smaller plaques compared with either wild-type RacL11 or a US2-repaired virus. After infection of BALB/c mice with L11ΔUS2, reduced pathogenicity compared with the parental RacL11 virus and the repaired virus was observed. It is concluded that the EHV-1 US2 protein modulates virus entry and cell-to-cell spread and appears to support sustained EHV-1 replication in vivo.

Download Full-text

Transport Through the Secretory Pathway of VSVG Tagged With Green Fluorescent Protein: Role of Tubulovesicular Carriers and Microtubules

Microscopy and Microanalysis ◽

10.1017/s1431927600007583 ◽

1997 ◽

Vol 3 (S2) ◽

pp. 139-140

Author(s):

John Presley ◽

Koret Hirschberg ◽

Nelson Cole

Keyword(s):

Green Fluorescent Protein ◽

Membrane Transport ◽

G Protein ◽

Golgi Complex ◽

Secretory Pathway ◽

Fluorescent Protein ◽

Dynamic Properties ◽

Living Cells ◽

Morphological Properties ◽

Green Fluorescent

The ts045 mutant of VSV G protein has been used in numerous studies to identify biochemical and morphological properties of membrane transport, due to its reversible misfolding and retention in the ER at 40°C and ability to traffic out of the ER and into the Golgi complex upon temperature reduction to 32oC. The dynamic properties of membrane transport intermediates of the secretory pathway, including their lifetime and fate within cells, have not until now been explored due to the inability to follow transport in single living cells. Here, we attached green fluorescent protein to the cytoplasmic tail of VSV G protein in order to visualize ER-to-Golgi and Golgi-to-plasma membrane transport in living cells. VSVG-GFP expressed in Cos cells accumulated in the ER at 40°C and translocated to the Golgi complex when shifted to 32oC. Translocation of the protein was followed using time-lapse imaging of live cells on a confocal microscope. VSVG-GFP accumulated in tubulovesicular structures scattered throughout the cell upon shift from 40°C to 15°C for three hours.

Download Full-text

Development and Use of Fluorescent Protein Markers in Living Cells

Science ◽

10.1126/science.1082520 ◽

2003 ◽

Vol 300 (5616) ◽

pp. 87-91 ◽

Cited By ~ 685

Author(s):

J. Lippincott-Schwartz

Keyword(s):

Fluorescent Protein ◽

Living Cells ◽

Protein Markers

Download Full-text

Actin dynamics in living mammalian cells

Journal of Cell Science ◽

10.1242/jcs.111.12.1649 ◽

1998 ◽

Vol 111 (12) ◽

pp. 1649-1658 ◽

Cited By ~ 20

Author(s):

C. Ballestrem ◽

B. Wehrle-Haller ◽

B.A. Imhof

Keyword(s):

Actin Cytoskeleton ◽

Mammalian Cells ◽

Fluorescent Protein ◽

Leading Edge ◽

Time Lapse ◽

Living Cells ◽

Actin Dynamics ◽

Mammalian Cell Lines ◽

Cytoskeletal Dynamics ◽

Green Fluorescent

The actin cytoskeleton maintains the cellular architecture and mediates cell movements. To explore actin cytoskeletal dynamics, the enhanced green fluorescent protein (EGFP) was fused to human β-actin. The fusion protein was incorporated into actin fibers which became depolymerized upon cytochalasin B treatment. This functional EGFP-actin construct enabled observation of the actin cytoskeleton in living cells by time lapse fluorescence microscopy. Stable expression of the construct was obtained in mammalian cell lines of different tissue origins. In stationary cells, actin rich, ring-like structured ‘actin clouds’ were observed in addition to stress fibers. These ruffle-like structures were found to be involved in the reorganization of the actin cytoskeleton. In migratory cells, EGFP-actin was found in the advancing lamellipodium. Immobile actin spots developed in the lamellipodium and thin actin fibers formed parallel to the leading edge. Thus EGFP-actin expressed in living cells unveiled structures involved in the dynamics of the actin cytoskeleton.

Download Full-text

Faculty Opinions recommendation of Development and use of fluorescent protein markers in living cells.

Faculty Opinions – Post-Publication Peer Review of the Biomedical Literature ◽

10.3410/f.1013330.190053 ◽

2003 ◽

Author(s):

Atsushi Miyawaki

Keyword(s):

Fluorescent Protein ◽

Living Cells ◽

Protein Markers

Download Full-text

A spinning disk confocal microscope system for rapid high resolution, multimode, fluorescence speckle microscopy and GFP imaging in living cells

Microscopy and Microanalysis ◽

10.1017/s1431927600026118 ◽

2001 ◽

Vol 7 (S2) ◽

pp. 8-9

Author(s):

Paul Maddox ◽

Julie Canman ◽

Sonia Grego ◽

Wendy Salmon ◽

Clare Waterman-Storer ◽

...

Keyword(s):

High Resolution ◽

Fluorescent Protein ◽

Imaging System ◽

Ccd Camera ◽

High Sensitivity ◽

Time Lapse ◽

Living Cells ◽

High Signal ◽

High Quantum Efficiency ◽

Spinning Disk

High resolution fluorescent speckle microscopy (FSM) and green fluorescent protein (GFP) imaging in living cells can require image recording at low densities of fluorophores (10 or less/resolvable unit) with low light excitation to prevent photobleaching. This needs efficient optical components, a high quantum efficiency detector, and a digital image acquisition and display system for time-lapse recording of multiple channels. Recently, Shinya and Ted Inoue have described the advantages of the Yokogawa CSU-10 spinning-disk confocal scanning unit for obtaining high quality fluorescent images with brief exposures and low fluorescence bleaching. Based on their findings, we have combined the CSU-10 unit with a high sensitivity pan-chromatic CCD camera to facilitate high spatial and temporal resolution imaging of fluorescence in living cells. in addition, the high signal-to-noise in images obtained with this instrument provides the opportunity to obtain 3-D views of extraordinary resolution and image quality after iterative constrained de-convolution.Our imaging system is constructed around a Nikon TE300 inverted microscope equipped with either a 60X or 100X Plan Apochromat objective, and standard epi-fluorescence optics for visual inspection of the specimen to locate cells for recording.

Download Full-text

Connexin-specific distribution within gap junctions revealed in living cells

Journal of Cell Science ◽

10.1242/jcs.113.22.4109 ◽

2000 ◽

Vol 113 (22) ◽

pp. 4109-4120 ◽

Cited By ~ 7

Author(s):

M.M. Falk

Keyword(s):

High Resolution ◽

Gap Junctions ◽

Gap Junction ◽

Fluorescent Protein ◽

Three Dimensional ◽

Time Lapse ◽

Living Cells ◽

Dye Transfer ◽

Channel Distribution ◽

Specific Distribution

To study the organization of gap junctions in living cells, the connexin isotypes alpha(1)(Cx43), beta(1)(Cx32) and beta(2)(Cx26) were tagged with the autofluorescent tracer green fluorescent protein (GFP) and its cyan (CFP) and yellow (YFP) color variants. The cellular fate of the tagged connexins was followed by high-resolution fluorescence deconvolution microscopy and time-lapse imaging. Comprehensive analyses demonstrated that the tagged channels were functional as monitored by dye transfer, even under conditions where the channels were assembled solely from tagged connexins. High-resolution images revealed a detailed structural organization, and volume reconstructions provided a three-dimensional view of entire gap junction plaques. Specifically, deconvolved dual-color images of gap junction plaques assembled from CFP- and YFP-tagged connexins revealed that different connexin isotypes gathered within the same plaques. Connexins either codistributed homogeneously throughout the plaque, or each connexin isotype segregated into well-separated domains. The studies demonstrate that the mode of channel distribution strictly depends on the connexin isotypes. Based on previous studies on the synthesis and assembly of connexins I suggest that channel distribution is regulated by intrinsic connexin isotype specific signals.

Download Full-text

Motile Properties of Vimentin Intermediate Filament Networks in Living Cells

The Journal of Cell Biology ◽

10.1083/jcb.143.1.147 ◽

1998 ◽

Vol 143 (1) ◽

pp. 147-157 ◽

Cited By ~ 172

Author(s):

Miri Yoon ◽

Robert D. Moir ◽

Veena Prahlad ◽

Robert D. Goldman

Keyword(s):

Intermediate Filament ◽

Cell Shape ◽

Fluorescence Recovery After Photobleaching ◽

Fluorescent Protein ◽

Time Lapse ◽

Living Cells ◽

A Cell ◽

Filament Networks ◽

Green Fluorescent ◽

Vimentin Intermediate Filament

The motile properties of intermediate filament (IF) networks have been studied in living cells expressing vimentin tagged with green fluorescent protein (GFP-vimentin). In interphase and mitotic cells, GFP-vimentin is incorporated into the endogenous IF network, and accurately reports the behavior of IF. Time-lapse observations of interphase arrays of vimentin fibrils demonstrate that they are constantly changing their configurations in the absence of alterations in cell shape. Intersecting points of vimentin fibrils, or foci, frequently move towards or away from each other, indicating that the fibrils can lengthen or shorten. Fluorescence recovery after photobleaching shows that bleach zones across fibrils rapidly recover their fluorescence. During this recovery, bleached zones frequently move, indicating translocation of fibrils. Intriguingly, neighboring fibrils within a cell can exhibit different rates and directions of movement, and they often appear to extend or elongate into the peripheral regions of the cytoplasm. In these same regions, short filamentous structures are also seen actively translocating. All of these motile properties require energy, and the majority appear to be mediated by interactions of IF with microtubules and microfilaments.

Download Full-text