Current Biology, Volume 19
Supplemental Data
VE-Cadherin-Mediated Cell-Cell Interaction Suppresses Sprouting via Signaling to MLC2 Phosphorylation
Sabu Abraham, Margaret Yeo, Mercedes Montero-Balaguer, Hugh Paterson, Elisabetta Dejana, Christopher J. Marshall, and Georgia Mavria
Experimental Procedures
Cells, Antibodies, Plasmids, and siRNA
Angiokit-validated HDF and HUVEC were from TCS CellWorks (Buckingham, UK)
and were cultured in DMEM 10% FCS and Large Vessel Endothelial Cell Medium
(TCS CellWorks), respectively. HUVEC-EGFP were generated by retroviral infection
as previously described [7]. HUVEC were used to passage 6, and tube-forming ability
was assessed in the co-culture assay [7]. Antibodies against mono-phosphorylated
(Ser-19) and di-phosphorylated (Thr 18/Ser 19) MLC2 were from Cell Signalling
Technology. Antibodies against total MLC2 used for immunofluorescence or
immunobloting were from Cell Signalling Technology and Santa Cruz respectively.
Antibodies against total and phosphorylated VEGFR2 were from Cell Signalling
Technology. Antibodies against VE-cadherin (goat polyclonal for
immunofluorescence and mouse monoclonal used for immunoblotting) were from
Santa Cruz. VE-cadherin blocking antibody (Cadherin 5) and control IgG1 were from
BD Biosciences, BV9 was from HyCult Biotechnology (Uden, the Netherlands).
pEF-Myc-RhoC containing human RhoC and pEF-Myc empty vector have been
previously described [30]. VE-cadherin, Rho-kinase I and II, Rac1 and p120 catenin
pools of siRNA oligonucleotide duplexes were from Dharmacon (Lafayette, USA)
and scrambled siRNA was as previously described [7]. Oligonucleotide sequences are
listed in Figure S6. Levels of knockdown for VE-cadherin were determined using the
LI-COR Odyssey system. Knockdown of Rho-kinases I and II was determined by
quantitative RT-PCR, using QuantiTect Primer Assays (Qiagen, GmbH) and the
7900HT Fast Real-Time PCR System (Applied Biosystems). HUVEC were
transfected in 6-well plates at a density of 1.5x105 using GeneFECTORTM (Venn
Nova, Inc.) according to the manufacturer’s recommendations.
Inhibitors, Immunoblotting, and Rac1 Pull-Down Assay
Y27632 was from Tocris (Southampton, UK), H1152 (Ikenoya et al., 2002),
blebbistatin (Straight et al., 2003), VEGFR2 inhibitor SU1498 and Rac1 inhibitor
NSC23766 were from Calbiochem, AvastinTM was from the Royal Marsden Hospital
pharmacy. For VE-cadherin immunoblotting cell lysates were prepared as previously
described [31]. For phospho-MLC2 immunoblotting whole-cell extracts were
harvested in Laemmli sample buffer supplemented with 10mM sodium fluoride, 1mM
sodium vanadate, 10mM sodium β-glycerophosphate, 0.5mM PMSF and Complete-
EDTA free protease (Roche, Diagnostics GmbH) and sonicated for 15s prior to
centrifugation. Western Blotting was performed using ECL Plus detection System
(GE Healthcare-Amersham) with horseradish peroxidase-conjugated secondary
antibodies (Sigma). MLC2 quantifications were performed using the Scion image
software (http://www.scioncorp.com) unless otherwise stated. For Rac1 pull-down
assays HUVEC were grown on fibronectin coated plates (10μg/ml; Sigma) in the
presence of VEGF (10ng/ml; TCS CellWorks). Whole-cell extracts were harvested in
Rac1 lysis buffer [32] and the pull-down assays were performed using GST-PAK as
previously described [32]. Immunoblotting for Rac1 was performed using anti-Rac1,
clone 23A8 (Upstate). The Li-COR Odyssey system (Li-COR Biosciences) was used
for quantifications.
Immunofluorescence and Microscopy
Immunofluorescence was performed using standard methods. Fixation was in 3.7%
paraformaldehyde, and permeabilization was in 0.1% Triton X-100. The phospho-
MLC2 (Ser 19) antibody was applied at 1:50 dilution at 4oC overnight. Confocal
sections were obtained using a BioRad MRC1024 confocal laser controlled by
Lasersharp (v3.4) acquisition software attached to a Nikon E600 upright fluorescence
microscope, using Nikon 20x (0.75 n.a.) PlanFluor multi-immersion, and Nikon Fluor
60x (1.00 n.a) water-dipping objectives. Phase contrast images of CD31-stained co-
cultures and loop formation were obtained using a 4x objective. Multisite time-lapse
microscopy was performed in a humidified CO2-equilibrated chamber using a
Diaphot inverted microscope (Nikon, Kingston upon Thames, UK) equipped with a
motorized stage Prior Scientific, Oxford, UK) controlled by Simple PCI software
(Compix, Cranberry Township, PA). Cells were imaged using 10x objective. Movies
were exported from Simple PCI software as uncompressed .AVI files. Adobe
Premiere v6.0 was used to compress movie files using the MPEG codec, and to export
compressed files in the .MOV (Quicktime) format.
Tissue Culture Angiogenesis Assays
Co-cultures of HUVEC with HDF (TCS Angiokit) were purchased from TCS
CellWorks, co-cultures of HUVEC-EGFP with HDF were set up as previously
described [7]. Treatments were performed in Optimized Medium (TCS CellWorks).
Tube formation was assessed using mouse anti-human CD31 Tubule Staining Kit
(TCS CellWorks). Automated analysis was performed using the AngioSys software.
Number of tubules, total tubule length and number of branch points were measured in
9 microscopic fields from triplicate wells at x4 magnification. For siRNA experiments
HUVEC (4x104 per 12-well) were seeded on fibroblasts that had reached confluency
over a period of 7 days, and cultured in 1:1 Large Vessel Endothelial Cell medium,
DMEM 10% FCS. Matrigel assays were performed in 60mm plates using growth
factor reduced matrigel (BD Biosciences; concentration 12.3mg/ml) diluted 1:1 with
PBS. HUVEC (5x105) were plated on matrigel (0.6ml) in Optimized Medium (TCS
CellWorks). Tranfected HUVEC were plated on matrigel or confluent fibroblasts
24hrs after transfection.
Morpholino-Mediated Knockdown of cdh5 in Zebrafish
Zebrafish were raised and kept at 28°C according to standard protocols [33]. The
Tg(fli1:EGFP)y1 transgenic zebrafish line has been previously described [8]. Two
morpholino antisense oligonucleotides (Cdh5-MO2 and Cdh5-MO3) were designed to
complement splicing donor sites of the zebrafish VE-cdh gene (cdh5; Ensembl
accession ENSDARG00000046128) in order to block proper splicing (Cdh5-MO2
5’-TACAAGACCGTCTACCTTTCCAATC-3’, Cdh5-MO3 5’-
ATTTGAGATGAACCTACCCAGGATG-3’). A 5 pb mismatch morpholino was
used as control (Cont-MO2 5’-TAgAAcACgGTCTAgCTTTCgAATC-3’). For a
diagram of exon/intron structure of zebrafish cdh5 see Figure S1B. Morpholinos were
reconstituted in nuclease free water, and the volume of the injected drop was
estimated with a micrometer scale. Embryos at 1- to 4-cell stage were injected with
8ng of morpholino into the yolk immediately below the blastomeres. This dose
delivers a fully penetrant phenotype in 95% of the embryos. The efficiency of the
morpholino was assessed by RT-PCR using Superscript One-step RT-PCR system
(Invitrogen) and using total RNA from wild type or morpholino injected pooled
embryos as template. The primers used are: e1F2 5’ -
TGTATGCGTATGAGGAAACAC, VE3R 5’-AGGCAGAACAGGATGGAGAC
(Figure S1B available online). For imaging zebrafish vessels, live embryos were
dechorionated manually with forceps and mounted in low melting agarose. Image
acquisition was performed with 20x or 40x objective on a Leica TCS SP2 confocal
microscope. Confocal stacks were processed for maximum intensity projection with
Leica LCS software and movies were assembled using ImageJ (MacBiophotonics).
Supplemental References
30. Sahai, E., and Marshall, C.J. (2002). ROCK and Dia have opposing effects on
adherens junctions downstream of Rho. Nat. Cell Biol. 4, 408–415.
31. Nawroth, R., Poell, G., Ranft, A., Kloep, S., Samulowitz, U., Fachinger, G.,
Golding, M., Shima, D.T., Deutsch, U., and Vestweber, D. (2002). VE-PTP and VE-
cadherin ectodomains interact to facilitate regulation of phosphorylation and cell
contacts. EMBO J. 21, 4885–4895.
32. Vial, E., Sahai, E., and Marshall, C.J. (2003). ERK-MAPK signaling coordinately
regulates activity of Rac1 and RhoA for tumor cell motility. Cancer Cell 4, 67–79.
33. Akimenko, M.A., Johnson, S.L., Westerfield, M., and Ekker, M. (1995).
Differential induction of four msx homeobox genes during fin development and
regeneration in zebrafish. Development 121, 347–357.
34. Larson, J.D., Wadman, S.A., Chen, E., Kerley, L., Clark, K.J., Eide, M., Lippert,
S., Nasevicius, A., Ekker, S.C., Hackett, P.B., et al. (2004). Expression of VE-
cadherin in zebrafish embryos: a new tool to evaluate vascular development. Dev.
Dyn. 231, 204–213.
Supplemental Figures
Figure S1
(A) HUVEC-HDF co-cultures were treated with VEGF (20ng/ml) for 48hrs starting at
6 days (migratory) or 12 days (established) after co-culture. The cultures were fixed
after a further 5 days and tube formation was visualized by CD31 staining. Branch
points are represented as mean ±SEM (n=9 microscopic fields from triplicate wells).
Scale bar, 100 μm.
(B) Diagram of the exon/intron structure of zebrafish VE-cadherin gene (cdh5)
indicating the position of the splice blocking morpholinos (Cdh5-MO2 and Cdh5-
MO3) used to down-regulate VE-cadherin. The cdh5 gene was identified through
Ensembl database searches as ENSDARG00000046128. The cdh transcript has been
previously described [34]. Bottom inset shows the confirmation of the efficiency of
the morpholinos by RT-PCR, lack of amplification of endogenous VE-cadherin
transcript upon cdh5-MO2 injection and the truncated splicing induced by cdh5-MO3.
Figure S2
(A) Schematic representation of VE-cadherin blockade in co-culture.
(B) Long-term Cad 5 treatment results in disassembly and endothelial cell rounding.
Tubules treated with 5μg/ml Cad5 or control IgG were followed by timelapse
microscopy. Video stills are at 24hr intervals over 3 days. Closed arrows show
sprouting points; open arrows rounding cells and disassembly. Scale bar, 50μm.
(C) Partial VE-cadherin blockade with BV9 increases tube formation. Established
tubules treated with 10μg/ml BV9 [5] or control IgG were visualized by CD31
staining 3 days after the end of treatment. Scale bar, 100μm.
(D) Treatment with Cad 5 alters the localization of VE-cadherin. Established tubules
treated with 10μg/ml Cad5 or control IgG for 4hrs, or 10μM Y27632 for 30min were
fixed and stained for VE-cadherin. Note the diffuse appearance of VE-cadherin in
Cad 5 treated tubules. Scale bar, 50 μm. Western blot shows VE-cadherin blockade or
Rho-kinase inhibition in the matrigel assay does not alter VE-cadherin expression
levels.
(E) VE-cadherin knockdown increases tube formation. HUVEC transfected with VE-
cadherin siRNA or scrambled control were seeded on confluent fibroblasts. After 5
days the cultures were fixed and stained for CD31. The number of branch points are
represented as mean ±SEM (n=9 microscopic fields from triplicate wells). Scale bar,
100μm.
Figure S3
(A) Schematic representation of treatments in matrigel.
(B) Rho-kinase inhibition increases cord formation. 24 hours after plating on matrigel
HUVEC were treated with Y27632 for 24 hrs. Loops were counted at the end of
treatment and are represented as mean ±SEM (n=9 microscopic fields). Western blot
shows reduced levels of mono-phosphorylated (S19) and di-phosphorylated (T18S19)
MLC2 following Y27632 treatment for 30 min.
(C) VE-cadherin blockade with BV9 down-regulates MLC2 phosphorylation and
increases cord formation. 24 hrs after plating on matrigel HUVEC were treated with
25μg/ml BV9 or control IgG for 24 hrs. Loops counted at the end of treatment are
represented as in (B). Western blot shows levels of phosphorylated MLC2 (T18S19)
with BV9 treatment (50μg/ml) for 2 hrs. Average phospho-MLC2 downregulation
27.8% ±6.7% (p=0.01 n=6).
(D) Knockdown of p120 catenin down-regulates MLC2 phosphorylation and
increases cord formation. HUVEC were transfected with p120 or control siRNAs.
Loops counted 48hrs after plating are represented as in (B). Scale bar, 50 μm.
Western blot shows phosphorylated MLC2 (T18S19) in HUVEC transfected with
p120 or scrambled siRNAs. Levels of p120 protein were quantified using the Licor
system.
(E) The effect of inhibition of actomyosin contractility on cord formation is dose
dependent. HUVEC were plated on matrigel and after 24 hours the cultures were
treated with blebbistatin at 10, 50 or 100μM for 24 hrs. Loops counted at the end of
treatment are represented as in (B). Scale bar 100μm.
(F) VE-cadherin blockade does not alter the localization of MLC2. 48 hrs after plating
on matrigel HUVEC were treated with Cad 5 (10μg/ml) or control IgG for 15min and
stained for VE-cadherin and total MLC2. Images were obtained using 60x objective.
Scale bar, 50 μm.
(G) VE-cadherin knockdown down-regulates MLC2 phosphorylation at cell junctions.
HUVEC were transfected with VE-cadherin or scrambled siRNAs. 24 hrs after plating
on matrigel the cultures were stained for VE-cadherin and phosphorylated (Ser19)
MLC2. Images were obtained using 60x objective. Scale bar, 50 μm.
Figure S4
(A) Schematic representation of inhibition of Rho-kinase and actomyosin contractility
in co-culture.
(B) MLC2 phosphorylation at endothelial cell junctions is Rho-kinase dependent and
is regulated by VE-cadherin. Established tubules were treated with Y27632 (10μM)
for 30mins or Cad 5 (10μg/ml) for 5 hrs, fixed and stained for VE-cadherin and
phospho-MLC2 (Ser19). Images were obtained using a 60x objective. Scale bar, 20
μm.
(C) The effect of inhibition of actomyosin contractility is dose dependent. Established
tubules treated with blebbistatin 5, 10, 20, or 50μM for 48 hrs were visualized by
CD31 staining 3 days after the end of treatment. Scale bar, 100μm.
Figure S5
E
(A-C) VE-cadherin blockade or Rho-kinase inhibition result in increases in Rac1-
GTP. HUVEC were grown to confluency in the presence of VEGF (20ng/ml) and
Rac1 activity was assayed by pulldown assays. Quantifications were performed using
the Licor system.
(A) HUVEC were treated with 10μg/ml Cad 5 or control IgG for 30 mins. Rac1-GTP
levels in treated HUVEC are shown as fraction of Rac1-GTP in IgG treated controls
after normalization for total Rac1.
(B) HUVEC were treated with the Rho-kinase inhibitor Y27632 (10μM) in the
absence or presence of the VEGFR2 inhibitors SU1498 (10 μM), BAY 43-9006
(1μM) or Avastin (5μg/ml). Rac1-GTP levels in treated HUVEC are shown as
fraction of Rac1-GTP in untreated controls after normalization for total Rac1.
(C) HUVEC were treated with the Rho-kinase inhibitor Y27632 (10μM) for 15, 30 or
60 mins. Western blot shows levels of phosphorylated VEGFR2. Rac1-GTP levels in
treated cells are shown as fraction of Rac1-GTP in untreated controls after
normalization for total Rac1.
(D) Treatment with the Rac1 inhibitor NSC23766 reduces CDC42-GTP levels.
HUVEC were treated with the Rac1 inhibitor NSC23766 (100μM) for 4, 8, 24 or 30
hrs. Levels of CDC42-GTP are shown as percentage of CDC42-GTP in untreated
controls after normalization for total CDC42.
(E) The sprouting response to VE-cadherin blockade is not augmented by addition of
exogenous VEGF. Established tubules treated with 5μg/ml Cad 5 or control IgG in
the presence or absence of VEGF (20 or 50ng/ml) were followed by timelapse
microscopy. Video stills are shown at 12 hr intervals over 36 hrs. Arrows show
sprouting points. Scale bar 50μm.
Figure S6. Sequences of siRNA Oligonucleotide Duplexes