Contribution of MT1-MMP and of human laminin-5 
2 chain degradation to mammary epithelial cell migration
Christine Gilles1,*,
,
Myriam Polette2,*,
Christelle Coraux2,
Jean-Marie Tournier2,
Guerrino Meneguzzi3,
Carine Munaut1,
Laure Volders1,
Patricia Rousselle4,
Philippe Birembaut2 and
Jean-Michel Foidart1
1
Laboratory of Tumor and Developmental Biology, University of
Liège, C.H.U. Sart-Tilman, B23,
Liège, Belgium
2
Unité INSERM U.514, Laboratoire Pol Bouin, IFR
53, C.H.U. Maison Blanche, Reims, France
3
Unité INSERM U.385, Faculty of Medicine, Nice,
France
4
Institut de Biologie et de Chimie des
Protéines, CNRS, U.P.R. 412, Lyon,
France
*
These authors contributed equally to this research
Author for correspondence (e-mail:
cgilles{at}ulg.ac.be
)
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Fig. 1. In vitro migration assay. MCF10A cells were plated inside a glass ring and
were allowed to migrate as an outgrowth after the ring removal. (A) Sequential
video images of a migratory culture of MCF10A cells, taken immediately, 24, 48
or 72 hours after the removal of the ring and showing the expansion of the
outgrowth. (B) Images of nuclei stained with Hoechst dye and visualized under
epifluorescence illumination (a, at the edge of the outgrowth; c, distant from
the outgrowth periphery). Trajectories of 20 randomly selected nuclei
(indicated with a white dots in a and c) were quantified in each area (b, at
the edge of the outgrowth; d, distant from the outgrowth periphery). Scale
bars: 2.35 mm in A; 80 µm in B.
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Fig. 2. Differential expression of MMPs mRNA in migratory cultures of MCF10A cells.
RT-PCR analyses for MT1-MMP, MMP-2, MMP-9, MMP-1, MMP-3 and MMP-11 were
performed on total RNA extracted from migratory cultures of MCF10A cells.
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Fig. 3. Specific overexpression and subcellular organization of MT1-MMP in
migratory MCF10A cells at the periphery of the outgrowth. (A) In situ
hybridization on a migratory culture of MCF10A cells performed with a MT1-MMP
antisense probe 72 hours after the removal of the ring. (B) MT1-MMP
immunolabelling on a migratory culture of MCF10A cells. MT1-MMP labelling is
in red and DAPI staining is in blue. (C) MT1-MMP immunolabelling (in red) on a
migratory culture of MCF10A cells (a). Phase-contrast microscopy analysis of
the corresponding area (b). (D) Confocal microscopy analyses of MT1-MMP in
migratory MCF10A cells 72 hours after the removal of the ring. Twenty-four
successive optical sections were taken from the apical (section 2) to the
basal (section 22) surface of the cells (sections 2, 12, 15, 16, 20 and 22 are
shown). MT1-MMP labelling was mainly found in the lamellipodia at the leading
edge of migratory cells (arrows) as well as at the basal surface of the cells
in contact with the substrate (section 16 and 20). Scale bars: 60 µm in
A,B; 20µm in C; 10 µm in D.
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Fig. 4. Inhibitory effect of BB94, TIMP-2 and MT1-MMP antisense oligonucleotides on
MCF10A cell migration. 72 hours after the removal of the ring, BB-94 (at
5x10-6M) and TIMP-2 (1 µg/ml) were added for 1 hour before
the quantification of migration speed of cells at the periphery of the
outgrowth. MT1-MMP oligonucleotides antisense (+) or scrambled control
oligonucleotides (-) were added to the medium immediately after the ring
removal for 144 hours before the quantification of the cell migration speed at
the periphery of the outgrowth. *P<0.05.
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© The Company of Biologists Ltd 2001
3 and 
2 chain degradation in migratory cultures of MCF10A cells and
cleavage of Ln-5