The Cdc42 and Rac1 GTPases are required for capillary lumen formation in three-dimensional extracellular matrices

Here we show a requirement for the Cdc42 and Rac1 GTPases in endothelial cell (EC) morphogenesis in three-dimensional extracellular matrices. Cdc42 and Rac1 specifically regulate EC intracellular vacuole and lumen formation in both collagen and fibrin matrices. Clostridium difficile toxin B(which blocks all three Rho GTPases) completely inhibited the ability of ECs to form both vacuoles and lumens, whereas C3 transferase, a selective inhibitor of Rho, did not. Expression of either dominant-negative (N17) or constitutively active (V12) Cdc42 using recombinant adenoviruses dramatically inhibited EC vacuole and lumen formation in both collagen and fibrin matrices. Both vacuole and lumen formation initiated in ECs expressing dominant-negative(N17) Rac1 but later collapsed, indicating a role for Rac1 during later stages of vessel development. Analysis of cultures using confocal microscopy revealed green fluorescent protein-V12Rac1, -Rac1 wild-type and -Cdc42 wild-type chimeric proteins targeted to intracellular vacuole membranes during the lumen formation process. Also, expression of the verprolin-cofilin-acidic domain of N-WASP, a downstream Cdc42 effector, in ECs completely interfered with vacuole and lumen formation. These results collectively reveal a novel role for Cdc42 and Rac1 in the process of EC vacuole and lumen formation in three-dimensional extracellular matrices.

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Differential Localization of Rho Gtpases in Live Cells

The Journal of Cell Biology ◽

10.1083/jcb.152.1.111 ◽

2001 ◽

Vol 152 (1) ◽

pp. 111-126 ◽

Cited By ~ 472

Author(s):

David Michaelson ◽

Joseph Silletti ◽

Gretchen Murphy ◽

Peter D'Eustachio ◽

Mark Rush ◽

...

Keyword(s):

Rho Gtpases ◽

Fluorescent Protein ◽

Essential Feature ◽

Hypervariable Region ◽

Dominant Negative ◽

Live Cells ◽

Rho Proteins ◽

Guanine Nucleotide Dissociation Inhibitor ◽

Membrane Compartment ◽

Green Fluorescent

Determinants of membrane targeting of Rho proteins were investigated in live cells with green fluorescent fusion proteins expressed with or without Rho-guanine nucleotide dissociation inhibitor (GDI)α. The hypervariable region determined to which membrane compartment each protein was targeted. Targeting was regulated by binding to RhoGDIα in the case of RhoA, Rac1, Rac2, and Cdc42hs but not RhoB or TC10. Although RhoB localized to the plasma membrane (PM), Golgi, and motile peri-Golgi vesicles, TC10 localized to PMs and endosomes. Inhibition of palmitoylation mislocalized H-Ras, RhoB, and TC10 to the endoplasmic reticulum. Although overexpressed Cdc42hs and Rac2 were observed predominantly on endomembrane, Rac1 was predominantly at the PM. RhoA was cytosolic even when expressed at levels in vast excess of RhoGDIα. Oncogenic Dbl stimulated translocation of green fluorescent protein (GFP)-Rac1, GFP-Cdc42hs, and GFP-RhoA to lamellipodia. RhoGDI binding to GFP-Cdc42hs was not affected by substituting farnesylation for geranylgeranylation. A palmitoylation site inserted into RhoA blocked RhoGDIα binding. Mutations that render RhoA, Cdc42hs, or Rac1, either constitutively active or dominant negative abrogated binding to RhoGDIα and redirected expression to both PMs and internal membranes. Thus, despite the common essential feature of the CAAX (prenylation, AAX tripeptide proteolysis, and carboxyl methylation) motif, the subcellular localizations of Rho GTPases, like their functions, are diverse and dynamic.

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Rac1 GTPases control filopodia formation, cell motility, endocytosis, cytokinesis and development in Dictyostelium

Journal of Cell Science ◽

10.1242/jcs.113.12.2253 ◽

2000 ◽

Vol 113 (12) ◽

pp. 2253-2265 ◽

Cited By ~ 12

Author(s):

M. Dumontier ◽

P. Hocht ◽

U. Mintert ◽

J. Faix

Keyword(s):

Green Fluorescent Protein ◽

Actin Cytoskeleton ◽

Cell Motility ◽

Fluorescent Protein ◽

Colony Growth ◽

Dominant Negative ◽

Related Protein ◽

Wild Type ◽

Equal Capacity ◽

Green Fluorescent

The function of the highly homologous Rac1A, Rac1B, and Rac1C GTPases of the Dictyostelium Rac1 group was investigated. All three GTPases bound with an equal capacity to the IQGAP-related protein DGAP1, with a preference for the activated GTP-bound form. Strong overexpression of wild-type Rac1 GTPases N-terminally tagged with green fluorescent protein (GFP), predominantly induced the formation of numerous long filopodia. Remarkably, expression of the constitutively-activated GTPases resulted in dominant-negative phenotypes: these Rac1-V12 mutants completely lacked filopodia but formed numerous crown shaped structures resembling macropinosomes. Moreover, these mutants were severely impaired in cell motility, colony growth, phagocytosis, pinocytosis, cytokinesis and development. Transformants expressing constitutively-inactivated Rac1-N17 proteins were similar to wild-type cells, but displayed abundant and short filopodia and exhibited a moderate defect in cytokinesis. Taken together, our results indicate that the three GTPases play an identical role in signaling pathways and are key regulators of cellular activities that depend on the re-organization of the actin cytoskeleton in Dictyostelium.

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A Novel In Vivo Assay Reveals Inhibition of Ribosomal Nuclear Export in Ran-Cycle and Nucleoporin Mutants

The Journal of Cell Biology ◽

10.1083/jcb.144.3.389 ◽

1999 ◽

Vol 144 (3) ◽

pp. 389-401 ◽

Cited By ~ 118

Author(s):

Ed Hurt ◽

Stefan Hannus ◽

Birgit Schmelzl ◽

Denise Lau ◽

David Tollervey ◽

...

Keyword(s):

Nuclear Export ◽

Fluorescent Protein ◽

Dominant Negative ◽

Nuclear Accumulation ◽

Wild Type ◽

Ribosomal Subunits ◽

In Vivo Assay ◽

Green Fluorescent ◽

Transport Factors

To identify components involved in the nuclear export of ribosomes in yeast, we developed an in vivo assay exploiting a green fluorescent protein (GFP)-tagged version of ribosomal protein L25. After its import into the nucleolus, L25-GFP assembles with 60S ribosomal subunits that are subsequently exported into the cytoplasm. In wild-type cells, GFP-labeled ribosomes are only detected by fluorescence in the cytoplasm. However, thermosensitive rna1-1 (Ran-GAP), prp20-1 (Ran-GEF), and nucleoporin nup49 and nsp1 mutants are impaired in ribosomal export as revealed by nuclear accumulation of L25-GFP. Furthermore, overexpression of dominant-negative RanGTP (Gsp1-G21V) and the tRNA exportin Los1p inhibits ribosomal export. The pattern of subnuclear accumulation of L25-GFP observed in different mutants is not identical, suggesting that transport can be blocked at different steps. Thus, nuclear export of ribosomes requires the nuclear/cytoplasmic Ran-cycle and distinct nucleoporins. This assay can be used to identify soluble transport factors required for nuclear exit of ribosomes.

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Probing the domain structure of FtsZ by random truncation and insertion of GFP

Microbiology ◽

10.1099/mic.0.28219-0 ◽

2005 ◽

Vol 151 (12) ◽

pp. 4033-4043 ◽

Cited By ~ 22

Author(s):

Masaki Osawa ◽

Harold P. Erickson

Keyword(s):

Fluorescent Protein ◽

Dynamic Instability ◽

Yellow Fluorescent Protein ◽

Dominant Negative ◽

Wild Type ◽

Negative Effects ◽

Terminal Domain ◽

Z Ring ◽

Green Fluorescent

Random transposon-mediated mutagenesis has been used to create truncations and insertions of green fluorescent protein (GFP), and Venus-yellow fluorescent protein (YFP), in Escherichia coli FtsZ. Sixteen unique insertions were obtained, and one of them, in the poorly conserved C-terminal spacer, was functional for cell division with the Venus-YFP insert. The insertion of enhanced GFP (eGFP) at this same site was not functional; Venus-YFP was found to be superior to eGFP in other respects too. Testing the constructs for dominant negative effects led to the following general conclusion. The N-terminal domain, aa 1–195, is an independently folding domain that can poison Z-ring function when expressed without a functional C-terminal domain. The effects were weak, requiring expression of the mutant at 3–5 times the level of wild-type FtsZ. The C-terminal domain, aa 195–383, was also independently folding, but had no activity in vivo. The differential activity of the N- and C-terminal domains suggests that FtsZ protofilament assembly is directional, with subunits adding primarily at the bottom of the protofilament. Directional assembly could occur by either a treadmilling or a dynamic instability mechanism.

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Duration of fusion pore opening and the amount of hormone released are regulated by myosin II during kiss-and-run exocytosis

Biochemical Journal ◽

10.1042/bj20091839 ◽

2010 ◽

Vol 429 (3) ◽

pp. 497-504 ◽

Cited By ~ 30

Author(s):

Ryo Aoki ◽

Tetsuya Kitaguchi ◽

Manami Oya ◽

Yu Yanagihara ◽

Mai Sato ◽

...

Keyword(s):

Fluorescent Protein ◽

Release Kinetics ◽

Myosin Ii ◽

Ph Sensor ◽

Secretory Vesicle ◽

Dominant Negative ◽

Fusion Pore ◽

Wild Type ◽

Pore Opening ◽

Green Fluorescent

Since the fusion pore of the secretory vesicle is resealed before complete dilation during ‘kiss-and-run’ exocytosis, their cargoes are not completely released. Although the transient fusion pore is kept open for several seconds, the precise mechanisms that control fusion pore maintenance, and their physiological significance, are not well understood. Using dual-colour TIRF (total internal reflection fluorescence) microscopy in neuroendocrine PC12 cells, we show that myosin II regulates the fusion pore dynamics during kiss-and-run exocytosis. The release kinetics of mRFP (monomeric red fluorescent protein)-tagged tPA (tissue plasminogen activator) and Venus-tagged BDNF (brain-derived neurotrophic factor), which show slower release kinetics than NPY (neuropeptide Y)–mRFP and insulin–mRFP, were prolonged by the overexpression of a wild-type form of the RLC (myosin II regulatory light chain). In contrast, overexpression of a dominant-negative form of RLC shortened the release kinetics. Using spH (synapto-pHluorin), a green fluorescent protein-based pH sensor inside the vesicles, we confirmed that the modulation of the release kinetics by myosin II is due to changes in the duration of fusion pore opening. In addition, we revealed that the amount of hormone released into the extracellular space upon stimulation was increased by overexpression of wild-type RLC. We propose that the duration of fusion pore opening is regulated by myosin II to control the amount of hormone released from a single vesicle.

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Coxiella burnetii Localizes in a Rab7-Labeled Compartment with Autophagic Characteristics

Infection and Immunity ◽

10.1128/iai.70.10.5816-5821.2002 ◽

2002 ◽

Vol 70 (10) ◽

pp. 5816-5821 ◽

Cited By ~ 161

Author(s):

Walter Berón ◽

Maximiliano G. Gutierrez ◽

Michel Rabinovitch ◽

Maria I. Colombo

Keyword(s):

Phase Ii ◽

Coxiella Burnetii ◽

Fluorescent Protein ◽

Q Fever ◽

Small Gtpases ◽

Dominant Negative ◽

Dominant Negative Mutant ◽

Wild Type ◽

Green Fluorescent

ABSTRACT The obligate intracellular bacterium Coxiella burnetii, the agent of Q fever in humans and of coxiellosis in other animals, survives and replicates within large, acidified, phagolysosome-like vacuoles known to fuse homo- and heterotypically with other vesicles. To further characterize these vacuoles, HeLa cells were infected with C. burnetii phase II; 48 h later, bacteria-containing vacuoles were labeled by LysoTracker, a marker of acidic compartments, and accumulated monodansylcadaverine and displayed protein LC3, both markers of autophagic vacuoles. Furthermore, 3-methyladenine and wortmannin, agents known to inhibit early stages in the autophagic process, each blocked Coxiella vacuole formation. These autophagosomal features suggest that Coxiella vacuoles interact with the autophagic pathway. The localization and role of wild-type and mutated Rab5 and Rab7, markers of early and late endosomes, respectively, were also examined to determine the role of these small GTPases in the trafficking of C. burnetii phase II. Green fluorescent protein (GFP)-Rab5 and GFP-Rab7 constructs were overexpressed and visualized by fluorescence microscopy. Coxiella-containing large vacuoles were labeled with wild-type Rab7 (Rab7wt) and with GTPase-deficient mutant Rab7Q67L, whereas no colocalization was observed with the dominant-negative mutant Rab7T22N. The vacuoles were also decorated by GFP-Rab5Q79L but not by GFP-Rab5wt. These results suggest that Rab7 participates in the biogenesis of the parasitophorous vacuoles.

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Molecular Mechanisms Controlling Vascular Lumen Formation in Three-Dimensional Extracellular Matrices

Cells Tissues Organs ◽

10.1159/000331410 ◽

2012 ◽

Vol 195 (1-2) ◽

pp. 122-143 ◽

Cited By ~ 57

Author(s):

Anastasia Sacharidou ◽

Amber N. Stratman ◽

George E. Davis

Keyword(s):

Molecular Mechanisms ◽

Three Dimensional ◽

Extracellular Matrices ◽

Lumen Formation ◽

Vascular Lumen

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Mechanism of Aurora-B Degradation and Its Dependency on Intact KEN and A-Boxes: Identification of an Aneuploidy-Promoting Property

Molecular and Cellular Biology ◽

10.1128/mcb.25.12.4977-4992.2005 ◽

2005 ◽

Vol 25 (12) ◽

pp. 4977-4992 ◽

Cited By ~ 100

Author(s):

Hao G. Nguyen ◽

Dharmaraj Chinnappan ◽

Takeshi Urano ◽

Katya Ravid

Keyword(s):

Chromosome Segregation ◽

Fluorescent Protein ◽

Point Mutations ◽

Degradation Pathway ◽

Aurora B ◽

Stable Form ◽

Wild Type ◽

Green Fluorescent ◽

Critical Regions

ABSTRACT The kinase Aurora-B, a regulator of chromosome segregation and cytokinesis, is highly expressed in a variety of tumors. During the cell cycle, the level of this protein is tightly controlled, and its deregulated abundance is suspected to contribute to aneuploidy. Here, we provide evidence that Aurora-B is a short-lived protein degraded by the proteasome via the anaphase-promoting cyclosome complex (APC/c) pathway. Aurora-B interacts with the APC/c through the Cdc27 subunit, Aurora-B is ubiquitinated, and its level is increased upon treatment with inhibitors of the proteasome. Aurora-B binds in vivo to the degradation-targeting proteins Cdh1 and Cdc20, the overexpression of which accelerates Aurora-B degradation. Using deletions or point mutations of the five putative degradation signals in Aurora-B, we show that degradation of this protein does not depend on its D-boxes (RXXL), but it does require intact KEN boxes and A-boxes (QRVL) located within the first 65 amino acids. Cells transfected with wild-type or A-box-mutated or KEN box-mutated Aurora-B fused to green fluorescent protein display the protein localized to the chromosomes and then to the midzone during mitosis, but the mutated forms are detected at greater intensities. Hence, we identified the degradation pathway for Aurora-B as well as critical regions for its clearance. Intriguingly, overexpression of a stable form of Aurora-B alone induces aneuploidy and anchorage-independent growth.

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Microvascular Sprouting, Extension, and Creation of New Capillary Connections with Adaptation of the Neighboring Astrocytes in Adult Mouse Cortex under Chronic Hypoxia

Journal of Cerebral Blood Flow & Metabolism ◽

10.1038/jcbfm.2013.201 ◽

2013 ◽

Vol 34 (2) ◽

pp. 325-331 ◽

Cited By ~ 19

Author(s):

Kazuto Masamoto ◽

Hiroyuki Takuwa ◽

Chie Seki ◽

Junko Taniguchi ◽

Yoshiaki Itoh ◽

...

Keyword(s):

Adult Mouse ◽

Fluorescent Protein ◽

Vascular Endothelial Cells ◽

Three Dimensional ◽

Vascular Endothelial ◽

Two Photon Microscopy ◽

Two Photon ◽

Mouse Cortex ◽

Hypoxia Adaptation ◽

Green Fluorescent

The present study aimed to determine the spatiotemporal dynamics of microvascular and astrocytic adaptation during hypoxia-induced cerebral angiogenesis. Adult C57BL/6J and Tie2-green fluorescent protein (GFP) mice with vascular endothelial cells expressing GFP were exposed to normobaric hypoxia for 3 weeks, whereas the three-dimensional microvessels and astrocytes were imaged repeatedly using two-photon microscopy. After 7 to14 days of hypoxia, a vessel sprout appeared from the capillaries with a bump-like head shape (mean diameter 14 μm), and stagnant blood cells were seen inside the sprout. However, no detectable changes in the astrocyte morphology were observed for this early phase of the hypoxia adaptation. More than 50% of the sprouts emerged from capillaries 60 μm away from the center penetrating arteries, which indicates that the capillary distant from the penetrating arteries is a favored site for sprouting. After 14 to 21 days of hypoxia, the sprouting vessels created a new connection with an existing capillary. In this phase, the shape of the new vessel and its blood flow were normalized, and the outside of the vessels were wrapped with numerous processes from the neighboring astrocytes. The findings indicate that hypoxia-induced cerebral angiogenesis provokes the adaptation of neighboring astrocytes, which may stabilize the blood–brain barrier in immature vessels.

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Targeting of Protein Kinase C-ϵ during Fcγ Receptor-dependent Phagocytosis Requires the ϵC1B Domain and Phospholipase C-γ1

Molecular Biology of the Cell ◽

10.1091/mbc.e04-12-1100 ◽

2006 ◽

Vol 17 (2) ◽

pp. 799-813 ◽

Cited By ~ 35

Author(s):

Keylon L. Cheeseman ◽

Takehiko Ueyama ◽

Tanya M. Michaud ◽

Kaori Kashiwagi ◽

Demin Wang ◽

...

Keyword(s):

Protein Kinase C ◽

Protein Kinase ◽

Phospholipase C ◽

Phospholipase D ◽

Fluorescent Protein ◽

Wild Type ◽

Fcγ Receptor ◽

Kinase C ◽

Green Fluorescent

Protein kinase C-ϵ (PKC-ϵ) translocates to phagosomes and promotes uptake of IgG-opsonized targets. To identify the regions responsible for this concentration, green fluorescent protein (GFP)-protein kinase C-ϵ mutants were tracked during phagocytosis and in response to exogenous lipids. Deletion of the diacylglycerol (DAG)-binding ϵC1 and ϵC1B domains, or the ϵC1B point mutant ϵC259G, decreased accumulation at phagosomes and membrane translocation in response to exogenous DAG. Quantitation of GFP revealed that ϵC259G, ϵC1, and ϵC1B accumulation at phagosomes was significantly less than that of intact PKC-ϵ. Also, the DAG antagonist 1-hexadecyl-2-acetyl glycerol (EI-150) blocked PKC-ϵ translocation. Thus, DAG binding to ϵC1B is necessary for PKC-ϵ translocation. The role of phospholipase D (PLD), phosphatidylinositol-specific phospholipase C (PI-PLC)-γ1, and PI-PLC-γ2 in PKC-ϵ accumulation was assessed. Although GFP-PLD2 localized to phagosomes and enhanced phagocytosis, PLD inhibition did not alter target ingestion or PKC-ϵ localization. In contrast, the PI-PLC inhibitor U73122 decreased both phagocytosis and PKC-ϵ accumulation. Although expression of PI-PLC-γ2 is higher than that of PI-PLC-γ1, PI-PLC-γ1 but not PI-PLC-γ2 consistently concentrated at phagosomes. Macrophages from PI-PLC-γ2-/-mice were similar to wild-type macrophages in their rate and extent of phagocytosis, their accumulation of PKC-ϵ at the phagosome, and their sensitivity to U73122. This implicates PI-PLC-γ1 as the enzyme that supports PKC-ϵ localization and phagocytosis. That PI-PLC-γ1 was transiently tyrosine phosphorylated in nascent phagosomes is consistent with this conclusion. Together, these results support a model in which PI-PLC-γ1 provides DAG that binds to ϵC1B, facilitating PKC-ϵ localization to phagosomes for efficient IgG-mediated phagocytosis.

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